NZ747901B2 - Solid inspection apparatus and method of use - Google Patents
Solid inspection apparatus and method of use Download PDFInfo
- Publication number
- NZ747901B2 NZ747901B2 NZ747901A NZ74790117A NZ747901B2 NZ 747901 B2 NZ747901 B2 NZ 747901B2 NZ 747901 A NZ747901 A NZ 747901A NZ 74790117 A NZ74790117 A NZ 74790117A NZ 747901 B2 NZ747901 B2 NZ 747901B2
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- New Zealand
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- energy level
- optical target
- optical
- energy
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Links
- 238000007689 inspection Methods 0.000 title claims abstract description 142
- 239000007787 solid Substances 0.000 title claims abstract description 110
- 238000000034 method Methods 0.000 title claims abstract description 48
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- ORUIBWPALBXDOA-UHFFFAOYSA-L magnesium fluoride Chemical compound [F-].[F-].[Mg+2] ORUIBWPALBXDOA-UHFFFAOYSA-L 0.000 description 1
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Classifications
-
- G—PHYSICS
- G01—MEASURING; TESTING
- G01J—MEASUREMENT OF INTENSITY, VELOCITY, SPECTRAL CONTENT, POLARISATION, PHASE OR PULSE CHARACTERISTICS OF INFRARED, VISIBLE OR ULTRAVIOLET LIGHT; COLORIMETRY; RADIATION PYROMETRY
- G01J3/00—Spectrometry; Spectrophotometry; Monochromators; Measuring colours
- G01J3/12—Generating the spectrum; Monochromators
- G01J3/18—Generating the spectrum; Monochromators using diffraction elements, e.g. grating
- G01J2003/1842—Types of grating
- G01J2003/1861—Transmission gratings
-
- G—PHYSICS
- G01—MEASURING; TESTING
- G01J—MEASUREMENT OF INTENSITY, VELOCITY, SPECTRAL CONTENT, POLARISATION, PHASE OR PULSE CHARACTERISTICS OF INFRARED, VISIBLE OR ULTRAVIOLET LIGHT; COLORIMETRY; RADIATION PYROMETRY
- G01J3/00—Spectrometry; Spectrophotometry; Monochromators; Measuring colours
- G01J3/02—Details
- G01J3/0289—Field-of-view determination; Aiming or pointing of a spectrometer; Adjusting alignment; Encoding angular position; Size of measurement area; Position tracking
-
- G—PHYSICS
- G01—MEASURING; TESTING
- G01J—MEASUREMENT OF INTENSITY, VELOCITY, SPECTRAL CONTENT, POLARISATION, PHASE OR PULSE CHARACTERISTICS OF INFRARED, VISIBLE OR ULTRAVIOLET LIGHT; COLORIMETRY; RADIATION PYROMETRY
- G01J3/00—Spectrometry; Spectrophotometry; Monochromators; Measuring colours
- G01J3/12—Generating the spectrum; Monochromators
- G01J3/18—Generating the spectrum; Monochromators using diffraction elements, e.g. grating
-
- G—PHYSICS
- G01—MEASURING; TESTING
- G01J—MEASUREMENT OF INTENSITY, VELOCITY, SPECTRAL CONTENT, POLARISATION, PHASE OR PULSE CHARACTERISTICS OF INFRARED, VISIBLE OR ULTRAVIOLET LIGHT; COLORIMETRY; RADIATION PYROMETRY
- G01J3/00—Spectrometry; Spectrophotometry; Monochromators; Measuring colours
- G01J3/28—Investigating the spectrum
- G01J3/44—Raman spectrometry; Scattering spectrometry ; Fluorescence spectrometry
- G01J3/4406—Fluorescence spectrometry
-
- G—PHYSICS
- G01—MEASURING; TESTING
- G01N—INVESTIGATING OR ANALYSING MATERIALS BY DETERMINING THEIR CHEMICAL OR PHYSICAL PROPERTIES
- G01N21/00—Investigating or analysing materials by the use of optical means, i.e. using sub-millimetre waves, infrared, visible or ultraviolet light
- G01N21/62—Systems in which the material investigated is excited whereby it emits light or causes a change in wavelength of the incident light
- G01N21/63—Systems in which the material investigated is excited whereby it emits light or causes a change in wavelength of the incident light optically excited
- G01N21/64—Fluorescence; Phosphorescence
- G01N2021/6417—Spectrofluorimetric devices
- G01N2021/6419—Excitation at two or more wavelengths
-
- G—PHYSICS
- G01—MEASURING; TESTING
- G01N—INVESTIGATING OR ANALYSING MATERIALS BY DETERMINING THEIR CHEMICAL OR PHYSICAL PROPERTIES
- G01N21/00—Investigating or analysing materials by the use of optical means, i.e. using sub-millimetre waves, infrared, visible or ultraviolet light
- G01N21/62—Systems in which the material investigated is excited whereby it emits light or causes a change in wavelength of the incident light
- G01N21/63—Systems in which the material investigated is excited whereby it emits light or causes a change in wavelength of the incident light optically excited
- G01N21/64—Fluorescence; Phosphorescence
- G01N21/6428—Measuring fluorescence of fluorescent products of reactions or of fluorochrome labelled reactive substances, e.g. measuring quenching effects, using measuring "optrodes"
- G01N2021/6439—Measuring fluorescence of fluorescent products of reactions or of fluorochrome labelled reactive substances, e.g. measuring quenching effects, using measuring "optrodes" with indicators, stains, dyes, tags, labels, marks
-
- G—PHYSICS
- G01—MEASURING; TESTING
- G01N—INVESTIGATING OR ANALYSING MATERIALS BY DETERMINING THEIR CHEMICAL OR PHYSICAL PROPERTIES
- G01N21/00—Investigating or analysing materials by the use of optical means, i.e. using sub-millimetre waves, infrared, visible or ultraviolet light
- G01N21/17—Systems in which incident light is modified in accordance with the properties of the material investigated
- G01N21/25—Colour; Spectral properties, i.e. comparison of effect of material on the light at two or more different wavelengths or wavelength bands
- G01N21/27—Colour; Spectral properties, i.e. comparison of effect of material on the light at two or more different wavelengths or wavelength bands using photo-electric detection ; circuits for computing concentration
- G01N21/274—Calibration, base line adjustment, drift correction
- G01N21/278—Constitution of standards
-
- G—PHYSICS
- G01—MEASURING; TESTING
- G01N—INVESTIGATING OR ANALYSING MATERIALS BY DETERMINING THEIR CHEMICAL OR PHYSICAL PROPERTIES
- G01N21/00—Investigating or analysing materials by the use of optical means, i.e. using sub-millimetre waves, infrared, visible or ultraviolet light
- G01N21/62—Systems in which the material investigated is excited whereby it emits light or causes a change in wavelength of the incident light
- G01N21/63—Systems in which the material investigated is excited whereby it emits light or causes a change in wavelength of the incident light optically excited
- G01N21/64—Fluorescence; Phosphorescence
-
- G—PHYSICS
- G01—MEASURING; TESTING
- G01N—INVESTIGATING OR ANALYSING MATERIALS BY DETERMINING THEIR CHEMICAL OR PHYSICAL PROPERTIES
- G01N21/00—Investigating or analysing materials by the use of optical means, i.e. using sub-millimetre waves, infrared, visible or ultraviolet light
- G01N21/62—Systems in which the material investigated is excited whereby it emits light or causes a change in wavelength of the incident light
- G01N21/63—Systems in which the material investigated is excited whereby it emits light or causes a change in wavelength of the incident light optically excited
- G01N21/64—Fluorescence; Phosphorescence
- G01N21/6428—Measuring fluorescence of fluorescent products of reactions or of fluorochrome labelled reactive substances, e.g. measuring quenching effects, using measuring "optrodes"
-
- G—PHYSICS
- G01—MEASURING; TESTING
- G01N—INVESTIGATING OR ANALYSING MATERIALS BY DETERMINING THEIR CHEMICAL OR PHYSICAL PROPERTIES
- G01N21/00—Investigating or analysing materials by the use of optical means, i.e. using sub-millimetre waves, infrared, visible or ultraviolet light
- G01N21/62—Systems in which the material investigated is excited whereby it emits light or causes a change in wavelength of the incident light
- G01N21/63—Systems in which the material investigated is excited whereby it emits light or causes a change in wavelength of the incident light optically excited
- G01N21/64—Fluorescence; Phosphorescence
- G01N21/6428—Measuring fluorescence of fluorescent products of reactions or of fluorochrome labelled reactive substances, e.g. measuring quenching effects, using measuring "optrodes"
- G01N21/643—Measuring fluorescence of fluorescent products of reactions or of fluorochrome labelled reactive substances, e.g. measuring quenching effects, using measuring "optrodes" non-biological material
-
- G—PHYSICS
- G01—MEASURING; TESTING
- G01N—INVESTIGATING OR ANALYSING MATERIALS BY DETERMINING THEIR CHEMICAL OR PHYSICAL PROPERTIES
- G01N21/00—Investigating or analysing materials by the use of optical means, i.e. using sub-millimetre waves, infrared, visible or ultraviolet light
- G01N21/62—Systems in which the material investigated is excited whereby it emits light or causes a change in wavelength of the incident light
- G01N21/63—Systems in which the material investigated is excited whereby it emits light or causes a change in wavelength of the incident light optically excited
- G01N21/64—Fluorescence; Phosphorescence
- G01N21/645—Specially adapted constructive features of fluorimeters
- G01N21/6456—Spatial resolved fluorescence measurements; Imaging
-
- G—PHYSICS
- G01—MEASURING; TESTING
- G01N—INVESTIGATING OR ANALYSING MATERIALS BY DETERMINING THEIR CHEMICAL OR PHYSICAL PROPERTIES
- G01N21/00—Investigating or analysing materials by the use of optical means, i.e. using sub-millimetre waves, infrared, visible or ultraviolet light
- G01N21/62—Systems in which the material investigated is excited whereby it emits light or causes a change in wavelength of the incident light
- G01N21/63—Systems in which the material investigated is excited whereby it emits light or causes a change in wavelength of the incident light optically excited
- G01N21/64—Fluorescence; Phosphorescence
- G01N21/6489—Photoluminescence of semiconductors
-
- G—PHYSICS
- G01—MEASURING; TESTING
- G01N—INVESTIGATING OR ANALYSING MATERIALS BY DETERMINING THEIR CHEMICAL OR PHYSICAL PROPERTIES
- G01N21/00—Investigating or analysing materials by the use of optical means, i.e. using sub-millimetre waves, infrared, visible or ultraviolet light
- G01N21/84—Systems specially adapted for particular applications
- G01N21/88—Investigating the presence of flaws or contamination
- G01N21/95—Investigating the presence of flaws or contamination characterised by the material or shape of the object to be examined
- G01N21/9515—Objects of complex shape, e.g. examined with use of a surface follower device
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- G—PHYSICS
- G01—MEASURING; TESTING
- G01N—INVESTIGATING OR ANALYSING MATERIALS BY DETERMINING THEIR CHEMICAL OR PHYSICAL PROPERTIES
- G01N2201/00—Features of devices classified in G01N21/00
- G01N2201/02—Mechanical
- G01N2201/022—Casings
- G01N2201/0227—Sealable enclosure
-
- G—PHYSICS
- G01—MEASURING; TESTING
- G01N—INVESTIGATING OR ANALYSING MATERIALS BY DETERMINING THEIR CHEMICAL OR PHYSICAL PROPERTIES
- G01N2201/00—Features of devices classified in G01N21/00
- G01N2201/02—Mechanical
- G01N2201/024—Modular construction
- G01N2201/0245—Modular construction with insertable-removable part
-
- G—PHYSICS
- G01—MEASURING; TESTING
- G01N—INVESTIGATING OR ANALYSING MATERIALS BY DETERMINING THEIR CHEMICAL OR PHYSICAL PROPERTIES
- G01N2201/00—Features of devices classified in G01N21/00
- G01N2201/12—Circuits of general importance; Signal processing
- G01N2201/127—Calibration; base line adjustment; drift compensation
Abstract
inspection apparatus may comprise: an optical target including a solid host material and a fluorescing material embedded in the solid host material, the solid host material having a predetermined phonon energy HOSTPE; a body having a pocket to receive the optical target, wherein the body includes an inset region located at a top surface and surrounding the pocket; and a transparent layer mounted in the inset region and positioned above the optical target; wherein the body includes a channel at least partially surrounding the pocket, the channel to receive an adhesive to bond to a grating layer, wherein the channel includes a series of pressure relief pockets distributed about the channel, the pressure relief pockets to relieve stress induced onto the grating layer by the adhesive during a curing process; wherein the fluorescing material exhibits a select ground energy level and a target excitation (TE) energy level separated from the ground energy level by a first energy gap corresponding to a fluorescence emission wavelength of interest (FEWI), the fluorescing material having a next lower lying (NLL) energy level relative to the TE energy level, the NLL energy level spaced a second energy gap FMEG2 below the TE energy level wherein a ratio of the FMEG2/HOSTPE is three or more. an inset region located at a top surface and surrounding the pocket; and a transparent layer mounted in the inset region and positioned above the optical target; wherein the body includes a channel at least partially surrounding the pocket, the channel to receive an adhesive to bond to a grating layer, wherein the channel includes a series of pressure relief pockets distributed about the channel, the pressure relief pockets to relieve stress induced onto the grating layer by the adhesive during a curing process; wherein the fluorescing material exhibits a select ground energy level and a target excitation (TE) energy level separated from the ground energy level by a first energy gap corresponding to a fluorescence emission wavelength of interest (FEWI), the fluorescing material having a next lower lying (NLL) energy level relative to the TE energy level, the NLL energy level spaced a second energy gap FMEG2 below the TE energy level wherein a ratio of the FMEG2/HOSTPE is three or more.
Description
SOLID INSPECTION APPARATUS AND METHOD OF USE
CROSS-REFERENCE TO RELATED APPLICATIONS
This application claims the benefit of U.S. provisional application Serial Number
62/443,675, filed January 7, 2017, the contents of which is incorporated by reference herein in its
entirety.
BACKGROUND
Optical targets are frequently used in calibration, alignment and measurement in
optical systems. The optical targets are utilized, among other things, when determining accuracy
and performance of the optical system. By way of example, the optical target affords a basis,
with respect to which the system may quantify optical resolution, depth of focus, optical and
mechanical drift, distortion, lens-based aberration, chromatism and the like.
However, some pre-existing optical targets have experienced certain limitations.
For example, some pre-existing optical targets include channels that convey liquids that have a
fluorescing dye provided therein, where the dye emits fluorescence in a desired emission spectra.
Some pre-existing optical targets include inlet and outlet ports to allow the liquid dye within the
channels to be replaced, which allows different dye materials to be utilized in a common optical
target at different points in time. However, the use of channels and inlet and outlet ports
increases the fluidic complexity of the optical target. In addition, particular operations may have
to be followed in order to avoid the introduction of air bubbles into the channel of the optical
target when liquid dye materials are changed or passed through the channels.
There is a need for tools that facilitate accurate calibration of alignment and
validation of optical detection systems.
DEFINITIONS
All literature and similar material cited in this application, including, but not
limited to, patents, patent applications, articles, books, treatises, and web pages, regardless of the
format of such literature and similar materials, are expressly incorporated by reference in their
entirety. In the event that one or more of the incorporated literature and similar materials differs
from or contradicts this application, including but not limited to defined terms, term usage,
described techniques, or the like, this application controls.
As used herein, the following terms have the meanings indicated.
The term “solid host material” refers to materials that have an atomic or
molecular structure arranged in a lattice or other matrix such that the solid host material exhibits
a predetermined phonon energy HOST . Solid host materials may comprise any crystalline,
semi-crystalline or amorphous material capable of being doped or otherwise embedded with a
fluorescing material as described herein. For example, ceramic represents one example of a
crystalline material. Glass and some polymers may represent non-crystalline or semi-crystalline
materials that may be doped/embedded with fluorescing materials of interest. The choice of the
solid host material is determined (at least in part) by the application in which the solid host
material is to be used. For example, in many applications, the solid host material choice is based
on its mechanical properties (e.g., hardness), chemical stability/inertness, thermal properties
and/or optical properties. Microscopic properties such as lattice arrangement, chemical structure
and phonon spectrum may also be relevant when choosing the solid host material. For example,
lattice and chemical structure play a role in terms of specific dopant type and concentration,
while the optical phonon spectrum affects the quantum efficiency of a specific transition via non-
radiative decay.
The term “fluorescing material” refers to one or more chemical elements,
combinations of chemical elements or other materials that are added to the solid host material
and that fluoresce, alone or in cooperation with the solid host material, when excited. For
example, the solid host material may be infused or doped with one or more chemical elements,
such as transition metal ions, rare-earth lanthanide ions, and/or actinide ions. The fluorescing
material may be referred to as a dopant, such as when transition metal ions, rare-earth lanthanide
ions, and/or actinide ion are added to a solid host material. The fluorescing material may
comprise a single element or may comprise a combination of elements (e.g., co-dopants). It is
recognized that, while the term “fluorescing material” refers to the one or more elements that are
added to the solid host material, in at least some examples, the element(s) added to the solid host
material may not fluoresce independent of the solid host material. Instead, the one or more
elements form a fluorescing material when cooperating with the solid host material. Optionally,
in alternative examples, the element(s) added to the solid host material may fluoresce
independent of the solid host material. Optionally, the fluorescent material may represent a
fluorescent dye embedded within epoxy. As another example, a fluorescent film may be coated
on top of an optical target in addition to or in place of doping fluorescent material within a solid
host material.
The term “quantum dots” (QD) refers to very small semiconductor particles (e.g.,
several nanometers in size) that have optical and electronic properties that differ from the
properties of larger particles. The quantum dots are designed to emit light of specific frequencies
of interest in response to electricity or light applied thereto. The emission frequencies may be
tuned by changing the dot size, shape and/or material. In some examples, nanoscale
semiconductor materials tightly confine either electrons or electron holes. By way of example,
quantum dots may also be referred to as artificial atoms, a term that emphasizes that a quantum
dot is a single object with bound, discrete electronic states, as is the case with naturally occurring
atoms or molecules. Quantum dots have optoelectronic properties that change as a function of
both size and shape. Larger QDs (radius of 5–6 nm, for example) emit longer wavelengths
resulting in emission colors such as orange or red. Smaller QDs (radius of 2–3 nm, for example)
emit shorter wavelengths resulting in emission colors like blue and green, although the specific
colors and sizes vary depending on the exact composition of the QD.
The term “solid body” includes any non-liquid, non-gaseous substrate that is
utilized to enclose fluorescing material. One example of a solid body is a solid host material that
has one or more fluorescing materials doped or otherwise embedded within the solid host
material. Another example of a solid body includes a non-liquid, non-gaseous substrate to
enclose quantum dots.
As used herein, relative or spatial terms such as “top,” “bottom,” “front,” “rear,”
“first,” “second,” “upper,” and “lower” are used as terms of direction with respect to a reference
object, point or axis. In accordance with examples disclosed herein, the relative or spatial terms
are used relative to the objective in the instrument when positioned adjacent to the inspection
apparatus. For example, structures, portions, and/or surfaces of the inspection apparatus that are
proximate/closest to the objective may be referred to as “top”, “upper”, etc. Similarly,
structures, portions, and/or surfaces of the inspection apparatus that are remote/further from the
objective may be referred to as “bottom”, “lower”, etc.
SUMMARY
According to a first principal aspect, there is provided an inspection apparatus,
comprising:
an optical target including a solid host material and a fluorescing material
embedded in the solid host material, the solid host material having a predetermined phonon
energy HOST ;
a body having a pocket to receive the optical target, wherein the body includes an
inset region located at a top surface and surrounding the pocket; and
a transparent layer mounted in the inset region and positioned above the optical
target;
wherein the body includes a channel at least partially surrounding the pocket, the
channel to receive an adhesive to bond to a grating layer, wherein the channel includes a series of
pressure relief pockets distributed about the channel, the pressure relief pockets to relieve stress
induced onto the grating layer by the adhesive during a curing process;
wherein the fluorescing material exhibits a select ground energy level and a target
excitation (TE) energy level separated from the ground energy level by a first energy gap
corresponding to a fluorescence emission wavelength of interest (FEWI), the fluorescing
material having a next lower lying (NLL) energy level relative to the TE energy level, the NLL
energy level spaced a second energy gap FM below the TE energy level wherein a ratio of the
FM /HOST is three or more.
EG2 PE
Optionally, the ratio of the FM /HOST equals or is between four and ten.
EG2 PE
Optionally, the solid host material includes at least one of glass, amorphous
polymers, crystalline materials, semi-crystalline polymers, metallic glass, or ceramic.
Optionally, the fluorescing material represents an ion of at least one of a rare-
earth element or a transition metal element.
Optionally, the solid host material has a maximum phonon energy less than or
equal to 580 cm .
Optionally, the fluorescence emission wavelength of interest has a center
wavelength at or below about 1000nm.
Optionally, the body further includes a diffusion well located below the pocket,
the diffusion well to receive excitation light passing through the optical target, the diffusion well
including a well bottom having a surface finish that exhibits a reflectively of no more than about
.0%.
Optionally, the apparatus comprises microstructures formed on a surface of at
least one of the transparent layer or the optical target to form the grating layer.
Optionally, the apparatus further comprises an anti-reflective coating formed on a
surface of at least one of the transparent layer or the optical target.
In accordance with examples disclosed herein, an inspection apparatus is provided
that comprises an optical target including a solid host material and a fluorescing material
embedded in the solid host material. The solid host material has a predetermined phonon energy
HOST . The fluorescing material exhibits a select ground energy level and a target excitation
(TE) energy level separated from the ground energy level by a first energy gap corresponding to
a fluorescence emission wavelength of interest. The fluorescing material has a next lower lying
(NLL) energy level relative to the TE energy level. The NLL energy level is spaced a second
energy gap FM below the TE energy level, wherein a ratio of the FM / HOST is three or
EG2 EG2 PE
more.
In accordance with examples disclosed herein, an inspection apparatus is provided
that comprises an optical target including a solid host material and a fluorescing material
embedded in the solid host material. The solid host material has a predetermined phonon energy
HOST . The fluorescing material exhibits a select ground energy level and a target excitation
(TE) energy level separated from the ground energy level by a first energy gap corresponding to
a fluorescence emission wavelength of interest (FEWI). The fluorescing material has a next
lower lying (NLL) energy level relative to the TE energy level. The NLL energy level is spaced
a second energy gap FM below the TE energy level, wherein a ratio of the FM /HOST is
EG2 EG2 PE
three or more.
Optionally, the ratio of the FM /HOST equals or is between four and ten.
EG2 PE
Optionally, the solid host material includes at least one of glass, amorphous polymers, crystalline
materials, semi-crystalline polymers, metallic glass, or ceramic. Optionally, the fluorescing
material represents an ion of at least one of a rare-earth element or a transition metal element.
Optionally, the solid host material has a maximum phonon energy less than or equal to 580 cm .
Optionally, the fluorescence emission wavelength of interest has a center wavelength at or below
1000 nm.
Optionally, the apparatus may further comprise a body having a pocket to receive
the optical target, wherein the body includes an inset region located at a top surface and
surrounding the pocket; and a transparent layer mounted in the inset region and positioned above
the optical target. Optionally, the body includes a channel at least partially surrounding the
pocket, the channel to receive an adhesive to bond to a grating layer. The channel includes a
series of pressure relief pockets distributed about the channel. The pressure relief pockets are to
relieve stress induced onto the grating layer by the adhesive during a curing process. Optionally,
the body may further comprise microstructures formed on a surface of at least one of the
transparent layer or the optical target to form a grating layer. Optionally, the apparatus may
further comprise an optical target retention body having a pocket to receive the optical target.
The body may be formed of aluminum that includes a surface having a reflectivity of no more
than about 20%. The body may include an inset region located at the top surface and
surrounding the pocket. The apparatus may further comprise a transparent grating layer mounted
in the inset region and that may be positioned above the optical target and spaced apart from the
optical target by a fringe gap. As mentioned above, the body may include a pocket to receive the
optical target. The body may include a diffusion well located below the pocket. The diffusion
well may receive excitation light passing through the optical target. The diffusion well may
include a well bottom having a surface finish that exhibits a reflectively of no more than about
.0%. The apparatus may further comprise an anti-reflective coating formed on a surface of at
least one of the transparent layer or the optical target.
Optionally, in accordance with an alternative example, the inspection apparatus
may include an optical target and a transparent layer directly bonded onto one another without
any additional supporting body structure. Microstructures may be provided at the interface
between the optical target and transparent layer. The microstructures may represent one or more
chrome patterns formed on a top surface of the optical target and/or on a bottom surface of the
transparent layer. Optionally, in accordance with an alternative example, the inspection
apparatus may be utilized as an inspection apparatus located directly on a flow cell, instead of
being mounted into an instrument. Optionally, the transparent layer may be omitted entirely.
Optionally, the optical target may be utilized as a stand-alone inspection apparatus without a
transparent layer or any other supporting structures, such as the body.
It is to be understood that any features of the inspection apparatus may be
combined together in any desirable manner and/or configuration.
In accordance with examples herein, an optical detection device is provided. The
optical detection device includes an optical target, which includes a solid body that encloses a
fluorescing material. An objective directs excitation light toward the optical target and receives
fluorescence emission from the optical target. A driver moves the objective to a region of
interest proximate to the optical target. A memory to store program instructions is also part of
the optical detection device. A processor executes the program instructions for detecting
fluorescence emission from the optical target in connection with at least one of optical alignment
or calibration of an instrument.
Optionally, the objective may direct excitation light onto the optical target. The
processor may derive reference information from the fluorescence emission. The processor may
utilize the reference information in connection with the at least one of optical alignment or
calibration of the instrument. The optical target may be permanently mounted at a calibration
location proximate to the objective. The calibration location may be separate from flow cell
channels within the instrument. Optionally, the optical target includes a solid host material and a
fluorescing material embedded in the solid host material, the solid host material having a
predetermined phonon energy HOST . The fluorescing material exhibits a select ground energy
level, a target excitation (TE) energy level and a next lower lying (NLL) energy level spaced an
energy gap FM below the TE energy level, wherein a ratio of the FM /HOST is three or
EG2 EG2 PE
more.
The solid body may represent a substrate comprising a solid host material with the
fluorescing material embedded in the solid host material. The solid body may represent at least
one of an epoxy or polymer that encloses quantum dots that emit fluorescence in one or more
predetermined emission bands of interest when irradiated by the excitation light.
In an example, the optical detection device further comprises an anti-reflective
coating formed on the optical target.
It is to be understood that any features of the optical detection device may be
combined together in any desirable manner. Moreover, it is to be understood that any
combination of features of the optical detection device and/or of the inspection apparatus may be
used together, and/or that any features from either or both of these aspects may be combined
with any of the examples disclosed herein.
In accordance with examples disclosed herein, a method is provided. The method
aligns an objective of an instrument with an optical target that includes a solid body that encloses
a fluorescing material. The method directs excitation light onto the optical target, detects
fluorescence emission from the optical target as reference information and utilizes the reference
information in connection with at least one of optical alignment or calibration of the instrument.
Optionally, the method may further comprise focusing the excitation light to a
focal point that may be below an upper surface of the optical target.
The aligning operation may comprise aligning the objective with a grating region
that includes a microstructure located above the optical target and focusing the excitation light to
a first focal point at the microstructure, and aligning the objective with a non-grating region that
is void of the microstructure and focusing the excitation light to a second focal point that is
below an upper surface of the optical target. Optionally, the fluorescing material may comprise a
chemical element that comprises an ion of at least one of erbium, holmium or praseodymium and
the solid host material comprises at least one of Silicate, Germanate, InF , or ZBLAN (i.e., heavy
metal fluoride glasses, such as ZrF -BaF -LaF -AlF -NaF).
4 2 3 3
It is to be understood that any features of the method may be combined together
in any desirable manner. Moreover, it is to be understood that any combination of features from
the method and/or the optical detection device and/or the inspection apparatus may be used
together, and/or that any features from any or all of these aspects may be combined with any of
the features of the examples disclosed herein.
BRIEF DESCRIPTIONS OF THE DRAWINGS
Figure 1A illustrates a perspective view of an inspection apparatus formed in
accordance with an example herein, where an optical target is shown separate from a body that is
to receive the optical target.
Figure 1B illustrates a top plan view of a body formed in accordance with an
alternative example.
Figure 1C illustrates a perspective view of an inspection apparatus formed in
accordance with an alternative example, where an optical target and a grating layer are shown
separate from a body that is to receive the optical target and the grating layer.
Figure 2A illustrates a side sectional view of the inspection apparatus of Figure
1A along line 2A-2A in Figure 1A, with the optical target installed in accordance with examples
herein.
Figure 2B illustrates a side view of a model of the optical target with an objective
positioned at a first measurement position in accordance with an example herein.
Figure 2C illustrates a side view of a model of the optical target with the objective
positioned at a second measurement position in accordance with an example herein.
Figure 2D illustrates a top plan view of the inspection apparatus formed in
accordance with an example.
Figure 2E illustrates a side sectional view of an inspection apparatus formed in
accordance with an alternative example.
Figure 2F illustrates a side sectional view of an inspection apparatus formed in
accordance with an alternative example.
Figure 3A illustrates an energy band diagram in connection with a trivalent
erbium ion (Er ) utilized in accordance with examples herein.
Figure 3B illustrates an ion energy level diagram associated with a trivalent
praseodymium ion (Pr ) in accordance with examples herein.
Figure 3C illustrates an ion energy level diagram associated with a trivalent
holmium ion (Ho ) in accordance with examples herein.
Figure 4 illustrates example intensity test measurements corresponding to
different fluorescence emission colors collected in connection with various optical targets in
accordance with examples herein.
Figure 5 illustrates test results of a solid host material that was formed by doping
a metal fluoride glass (ZBLAN) with predetermined concentrations of a trivalent erbium ion in
accordance with examples herein.
Figure 6A illustrates a side sectional view of an inspection apparatus formed in
accordance with an alternative example.
Figure 6B illustrates a side view of a portion of an inspection apparatus formed in
accordance with an alternative example.
Figure 6C illustrates a side view of a portion of an inspection apparatus formed in
accordance with an alternative example.
Figure 7 illustrates a block diagram of an optical detection device formed in
accordance with an example.
Figure 8 shows an exploded view of an example microfluorometer for purposes of
demonstrating functional arrangement for various optical components in accordance with
examples herein.
Figure 9 illustrates a block diagram for a detection apparatus that may utilize an
inspection apparatus in accordance with examples herein.
Figure 10 illustrates an example automated process flow that may be run utilizing
an inspection apparatus in accordance with examples herein.
DETAILED DESCRIPTION
Examples disclosed herein describe optical targets that utilize solid bodies with
fluorescing material therein. The optical target may be used to calibrate the optics of
fluorescence-based optical systems with a predetermined level of precision and accuracy, such as
in a nanometer scale, or a micrometer scale, etc., depending upon the optical property being
measured. One or more of the examples disclosed herein afford significant benefits. For
example, a solid body target system is relatively easy to fabricate as compared to conventional
liquid die based targets and fluidic counterpart targets. A solid body target system exhibits a
relatively long shelf life, as the parts do not leak or photo-degrade over time. Also, the solid
body target system does not require custom in-house processes and hence can be readily
outsourced to suppliers. Also, the solid body target system enables fluorescence emission that is
constant over time without photo-degradation at a given optical power, which provides the
potential that a solid body target system can be used for power metering and power calibration of
instrument illumination sources while in the field. Integrating the foregoing functionalities
permanently into a sequencing system enables remote system monitoring to improve instrument
up time.
Figure 1A illustrates a perspective view of an inspection apparatus 100 formed in
accordance with an example disclosed herein. The inspection apparatus 100 includes a body 102
having top and bottom surfaces 104, 106 that extend generally planar to one another. The body
102 may include rounded corners that transition between lateral sides 108 and front and back
ends 110, 112. In the present example, the body 102 is rectangular in shape, although alternative
shapes may be utilized. The inspection apparatus 100 is shaped and dimensioned to be mounted
within an instrument that performs optical measurements and analysis. By way of example, the
instrument may be a fluidics instrument, although the examples disclosed herein may be utilized
with non-fluidic optical instruments. As examples, the inspection apparatus 100 described herein
may be utilized in connection with micro-fluidics, semiconductors, biotechnology and consumer
industry instruments. For example, the inspection apparatus 100 may be utilized for alignment
of a semiconductor tool, such as mask aligners and steppers, for calibration of a machine vision
system, for optical stages in applications such as optical coherence tomography and
fluorescence-based biological imaging. As another example, the inspection apparatus 100 may
be utilized in connection with calibration of standard consumer optical tools such as fluorescence
microscopes.
Examples herein may be utilized in connection with next generation sequencing
systems that utilize various fluorescence methods. For example, the inspection apparatus 100
may be utilized in connection with the MINISEQ® instrument, HISEQ® instrument,
NEXTSEQ® instrument and MISEQ® instrument offered by Illumina Inc. (San Diego, CA)
and/or in connection with instruments offered by other companies. In accordance with at least
some examples, the inspection apparatus 100 enables the optical calibration of an instrument
without a need for fluorescent reference particles or fluorescent dies (as conventionally used).
Conventional fluorescent reference particles and dies provide calibration for a few of the more
frequently used fluorophores (e.g., Fluorescein and Phycoerythin). However, conventional
fluorescent reference particles and dyes suffer from thermal and photo-stability, leakage and/or
mechanical failure.
In accordance with the examples provided herein, the inspection apparatus 100
may be utilized as a built-in remote diagnostic optical target. The inspection apparatus 100 may
be permanently mounted within an instrument and positioned to enable a detector within the
instrument to perform optical measurements without having to manually load any additional tool.
The inspection apparatus 100 may be used, by the instrument, to provide remote diagnostic
information in connection with various activities. For example, the instrument may utilize the
inspection apparatus 100 to perform data trending such as trends in a point spread function of an
instrument, laser alignment, optical calibration, and optical transmission efficiency over the life
of the instrument. Data can be collected automatically with no user intervention and uploaded to
the cloud in order to perform remote debugging, perform predictive diagnostics, and trend across
multiple instruments. The inspection apparatus 100 may be utilized to evaluate various aspects
of the instrument’s optical system, as well as aspects of the XYZ stages. For example, if the
laser alignments are found to be off, software can automatically actuate the pointing mirrors to
bring the laser into alignment.
In accordance with some examples, an inspection apparatus 100 may be
assembled and shipped with each instrument, where the instrument includes a current software
release of an inspection application that controls the instrument to carry out various tests with the
inspection apparatus 100. When the inspection apparatus 100 is dimensioned to be loaded and
unloaded, the inspection apparatus 100 may be configured as a full-sized inspection apparatus
that may be used for measuring optical metrics. The full-sized inspection apparatus will mate
with a flow cell holder and be utilized to evaluate flow cell holder alignment. The full-size
inspection apparatus will extend the full length of a sequencing flow cell to enable a simulation
of a sequencing run. Optionally, the inspection apparatus 100 may be reduced in size and
mounted within the instrument at a staging location, adjacent to the flow cell lanes. When the
inspection apparatus 100 is permanently mounted within the instrument (at a reduced footprint),
the instrument may perform inspection operations without a need to load and unload the
inspection apparatus 100. The reduced footprint inspection apparatus may be utilized to perform
optical metrics.
An optical target 120 includes top and bottom target surfaces 107, 109 that are
generally planar and oriented parallel to one another. A sidewall 105 extends about the optical
target 120. In the present example, the optical target 120 generally has a rectangular cubical
shape, although it is recognized that alternative shapes may be utilized based upon a particular
application. As explained herein, the optical target 120 represents a solid body structure that
includes a solid host material and a fluorescing material embedded within the solid host material.
The solid host material may be entirely or at least partially transparent. For example, a degree of
transparency in the solid host material may be based, in part, on a desired intensity of fluorescing
emissions that are emitted from the optical target 120. By way of example, the solid host
material of the solid body structure or substrate may represent a glass substrate or another solid
host material having desired mechanical and optical properties as described herein.
As one example, the host solid material may be indium-fluoride glass. For
example, the solid host material may include at least one of glass, amorphous polymers,
crystalline materials, semi-crystalline polymers, metallic glass, ceramic and the like. Table 1
below illustrates examples of solid host materials that may be utilized within the solid body
structure or substrate. As illustrated in Table 1, the solid host material may represent heavy
metal fluoride glasses (e.g., ZBLAN). ZBLAN glass may utilize various combinations with
fluoride, such as ZrF , BaF , LaF , AlF , and NaF. Optionally, the solid host material may be
4 2 3 3
CaF . The solid host materials exhibit low maximum phonon energy levels. In accordance with
some examples, the solid host material may exhibit a maximum phonon energy of less than or
equal to a predetermined wave number. As a further example, the solid host material may
-1 -1
exhibit a maximum phonon energy of or between about 370 cm and about 525 cm . The solid
host material may be formed of other materials that include low maximum phonon energy and
exhibit available energy bands at locations of interest to obtain fluorescing within emission
bands that correspond to optical channels of interest.
Table 1
Glass Former Maximum phonon energy
(cm )
ZrF 580
HfF 580
GaF 525
InF 510
CdF /CdCl 370
The fluorescing material may be a rare-earth element such as rare earth ions: Tm
3+ 3+ 3+ 3+ 3+
(455 nm), Ho (550 nm), Tb (540 nm), Eu (611 nm), Sm (550 nm), Pr (488, 590 nm),
3+ 3+
Dy (480 nm & 575 nm), or Er (550 nm & 660 nm); an element from the Actinide series: U;
3+ 2+/ 3+
transition metal ions: Ti , Cr , etc. The fluorescing material may be distributed in an even
and homogeneous fixed manner throughout the solid host material, such as to form Er-InF glass.
The fluorescing material emits in one or more emission channels of interest. For example, the
fluorescing material may emit at a wavelength shorter than 1000 nm.
The fluorescence material may be provided in various concentrations within the
solid host material, where the concentration of the fluorescing material is managed based, in part,
on a desired intensity of fluorescence emission to be obtained in response to an expected
excitation light intensity. In the above example, when the host substrate is indium-fluoride
(InF ) glass doped with trivalent erbium ions, the trivalent erbium ions may be provided at a
dopant concentration at or between about 0.1% and about 10.0% and, for example, at or between
about 0.5% and about 6% by atomic fraction. As another example, the dopant concentration of
trivalent erbium ions may range from about 1.0% to 3.0% +/- 0.01% by atomic fraction. The
fluorescing material exhibits a select emission intensity that may be tuned by adjusting the
composition. For example, the emission intensity and/or color may be varied by adjusting the
concentration of the fluorescing material, by adding a secondary dopant (e.g., co-dopant), and/or
by adjusting the composition of the solid host material. For example, a first dopant may
represent a primary dopant or activator ion, while a secondary dopant may be added to increase
or decrease the emission intensity of the primary dopant. The secondary dopant represents a
sensitizer ion. Combining more than one dopant may enhance fluorescent intensity. By co-
doping with an additional sensitizer ion, the emission intensity can be increased by energy
3+ 3+
transfer between the sensitizer ion and the activator ion (e.g., Er). For example, Yb or Tm
may be used as a sensitizer ion when Er is used as the activator ion. As other examples, Yb,
Ho and YF may be used as sensitizer ions.
Optionally, combining more than one dopant may be used to decrease fluorescent
intensity of one or more emission bands. By co-doping with an additional sensitizer ion, the
emission intensity can be decreased by energy transfer between the sensitizer ion and the
activator (e.g., Er). For example, Tb/Eu may be co-doped in Yb O , where the energy transfer
from Tb to Eu results in emission changes from red to green. As another example, Tm may be
co-doped with Tb or Ho to promote continuous wave (cw) lasing at 1.5 microns (µm). Examples
of combinations for co-doping are described in: “Properties of the 1.5 and 2.3 um laser emissions
of various Tm doped fluoride crystals codoped with Tb or Yb ions” published in OSA TOPS
Vol. 26 Advanced Solid-State Lasers; “Ultraviolet and visible emissions of Er in KY(WO )
single crystals co-doped with Yb ions” published in Journal of Luminescence 115 (2005) 131-
3+ 3+
137; “Color-tunable properties of Eu - and Dy -codoped Y O phosphor particles published in
Nanoscale Res Lett. 2012; 7(1):556; and the book “Current Trends in Optical Amplifiers and
Their Applications” edited by Tien-Pei Lee, the complete subject matter of which are
incorporated by reference in their entirety.
The solid host material and the dopant may be chosen such that the combination
exhibits a desired energy level ratio. For example, the combination may exhibit an energy level
ratio of HOST /FM , where the HOST represents the maximum phonon energy of the solid
PE ET PE
host material and FM represents the energy transition between a target emission energy level
and a nearest neighbor energy level of the fluorescing material.
In accordance with examples disclosed herein, the solid host material and the
fluorescing material exhibit an energy level ratio of FM /HOST >= (≥) 4, where the HOST
EG2 PE PE
represents the phonon energy of the solid host material and FM represents the energy
transition between a target excitation energy level and a next lower lying (NLL) energy level of
the fluorescing material. By way of example, Table 2 is provided below to show a relationship
for an example fluorescing material energy gap FM with various solid host materials. For
example, the fluorescing material may represent a trivalent erbium ion (Er ) element where the
TE energy level is the F energy level and the NLL energy level is the I energy level. The
9/2 9/2
4 4 -1
energy gap between the F and I energy levels is a wave number of 2900 cm . In Table 2,
9/2 9/2
example solid host materials include silicate, germanate and ZBLAN which have maximum
-1 -1 -1
phonon energies of 1100 cm , 900 cm , and 500 cm , respectively. The energy level ratio for
trivalent erbium ion (Er ) and the solid host materials silicate, germanate and ZBLAN
(FM /HOST ) are 3, 4 and 6, respectively, while the quantum efficiencies are about 0.22%,
EG2 PE
14% and 90%, respectively. The "quantum efficiency" (Q.E.) is a ratio of the number of emitted
fluorescing photons to a number of incident excitation light photons. As evident in Table 2,
ZBLAN exhibits a high degree of quantum efficiency as compared to silicate and germanate for
the particular fluorescing material Er . Optionally, silicate and germanate may be afforded a
higher quantum efficient than illustrated in Table 2 when a different fluorescing material is
utilized as a dopant. For InF glass doped with Er , the energy level ratio is 6, corresponding to
a quantum efficiency of about 90%. It is recognized that other fluorescing materials will exhibit
different quantum efficiencies with the listed solid host materials.
Table 2
Host material Maximum Energy Level Ratio Quantum
phonon energy (FM /HOST ) Efficiency
EG2 PE
for Er3
Silicate 1100 cm 3 0.22%
Germanate 900 cm 4 14%
ZBLAN 580 cm 5 85%
InF3 500 cm 6 90%
With continued reference to Figure 1A, the body 102 may comprise aluminum or
another material having similar mechanical and optical properties. The body 102 may be formed
through a milling process or another manufacturing process that affords desired tolerances for
the various ledges, walls, wells, etc. discussed herein. The body 102 includes an inset region 118
provided across the top surface 104. A central pocket 114 and channels 116 are provided within
an interior area of the inset region 118. The central pocket 114 is configured to receive the
optical target 120. The optical target 120 may be secured within the pocket 114 in various
manners, such as with an adhesive. Optionally, the pocket 114 may be formed with peripheral
features that securely engage with peripheral walls of the optical target 120 (e.g., in a press fit
manner). The inset region 118 is configured to receive a glass layer (not shown in Figure 1A) or
other transparent material (i.e., transparent layer) that covers the optical target 120 into the
pocket 114. The channels 116 receive an adhesive that bonds to the glass layer and the body
102, thereby covering and hermetically sealing the optical target 120 from the external
environment. In accordance with at least some examples, the layer of glass may have
microstructures formed thereon, thereby defining a grating layer (e.g., 122 in Figure 2A).
Optionally, the glass layer may be omitted entirely and the optical target 120 may be exposed
from the top surface 104 of the body 102.
In the example of Figure 1A, the central pocket 114 is elongated and positioned to
extend in a longitudinal direction along a length of the body 102. The channels 116 are formed
along opposite sides of the pocket 114. The channels 116 include one or more inlet/outlet ports
117 in the bottom thereof that extend from the bottom of the channels 116 to the bottom surface
106 of the body 102. The inlet/outlet ports 117 may be used to inject the adhesive into the
channels 116 after the top glass has been inserted into the inset region 118.
Optionally, the optical target 120 may be utilized as a stand-alone inspection
apparatus with no microstructures or other patterns formed thereon or provided proximate
thereto. For example, the optical target 120 may simply be mounted directly on a flow cell
and/or within an instrument without any other supporting structures.
Figure 1B illustrates a top plan view of a body 202 formed in accordance with an
alternative example. The body 202 includes a top surface 204 that includes an inset region 218
formed therein. The inset region 218 is shallow and extends a depth downward into the body
202, where the depth generally corresponds to the thickness of a glass layer (e.g., grating layer)
to be received in the insert region 218. In the example of Figure 1B, the inset region 218 is
generally square or rectangular, although alternative shapes may be utilized. Further, in the
example of Figure 1B, the inset region 218 has a generally even/common depth corresponding to
the thickness of the glass layer. However, the inset region 218 may have varied depths in
different regions thereof, such as when it is desirable to utilize a glass layer with portions having
different thicknesses and/or separate pieces to form the glass layer.
The body 202 also includes a pocket 214 generally centered within the inset
region 218. The pocket 214 is shaped and dimensioned to receive the optical target 120. The
pocket 214 extends a predetermined depth below a depth of the inset region 218. A channel 216
is provided within the inset region 218 and positioned to substantially surround of the pocket
214. The channel 216 generally corresponds to the channel 116 in Figure 1A, except that the
channel 216 is continuous to surround the pocket 214. The channel 216 includes inlet/outlet
ports 217 that represent holes extending through the body 202 to the bottom surface thereof. The
inlet/outlet ports 217 may be utilized to access the interior of the glass layer once inserted and to
insert an adhesive into the channel 216.
In an example, the channel 216 also includes a series of pressure relief pockets
221 distributed about the channel 216. As explained below in more detail, the pressure relief
pockets 221 relieve stress induced on the glass layer by the adhesive silicone added to the
channel 216. More specifically, when silicone is introduced into the channel 216 through the
inlet/outlet ports 217, the silicone at least partially bridges over the pockets 221, thereby trapping
small amounts of air in each of the pockets 221. As the silicone cures, the silicone contracts,
thereby introducing a drawing/shrinking force on to the grating layer and surrounding walls of
the channel 216. The air trapped in the pockets 221 form a first region of relief for the silicone,
thereby reducing the drawing force applied by the silicone onto the grating layer.
The pocket 214 and channel 216 are separated by an interior ledge 215 that, in the
example of Figure 1B, is also rectangular. It is recognized that any of the square or rectangular
geometries illustrated in Figure 1B may be modified to resemble numerous alternative shapes.
The channel 216 is surrounded on an outer perimeter thereof by an exterior ledge 219. The
interior and exterior ledges 215 and 219 form a shelf that receives the glass layer.
When assembled, the optical target 120 is inserted into the pocket 214 and may be
retained therein with an adhesive, by frictional interference between the walls of the pocket 214
and the sides of the optical target 120, and the like. Once the optical target 120 is inserted into
the pocket 214, the glass layer is inserted into the inset region 218 until resting on the interior
and exterior ledges 215, 219. In accordance with some examples disclosed herein, the inset
region 218 receives a transparent layer (e.g., formed of glass and thus also referred to as the glass
layer) that functions as a grating layer (e.g., see 122 in Figure 2A). The grating layer is sealed
into the inset region 218 to prevent contaminants from getting into the pocket 214 after assembly
is complete. For example, end users may wipe the inspection apparatus periodically with
cleaners (e.g., alcohol) to clean it. Examples herein utilize an alcohol resistant adhesive that is
injected into the channel 216 to attach the grating layer to the body 202, where the adhesive will
hold up well to alcohol exposure. For example, the adhesive may be silicone which is highly
stable in alcohol, whereas UV cure adhesives tend to break down in alcohol. The silicone is
injected until the channels 116 are filled. However, silicone may exhibit “outgassing” when
curing.
Examples disclosed herein isolate the pocket 214 and optical target 120 from the
byproducts of the outgassing process. To do so, once the grating layer is inserted into the inset
region 218 and resting on the interior and exterior ledges 215, 219, an outgassing barrier 213 is
formed about the interface between the grating layer and the interior ledge 215. An outgassing
barrier 211 is also formed about the interface between the grating layer and the exterior ledge
219. The outgassing barriers 213, 215 may be formed by injecting a tool through one or more of
the inlet/outlet ports 217 and depositing a predetermined volume of a barrier adhesive along the
edge of the interface between the grating layer and the interior ledge 215, and along the edge of
the interface between the grating layer and the exterior ledge 219. For example, the barrier
adhesive may be a low-viscosity (e.g., 300 cp) UV cure adhesive. After waiting a predetermined
period of time, the barrier adhesive wicks across the interior and exterior ledges 215 and 219 to
form thin bonding layers between the interior ledge 215, exterior ledge 219 and the grating layer
(denoted by the dashed lines 211, 213 as outgassing barriers). The grating layer will be in a
stress-free state and pulled down to the interior and exterior ledges 215, 219. UV curing in this
state maintains the grating layer flat and properly positioned without using any clamping fixtures
which could bend the grating layer. Additionally the outgassing barrier 213 at the interior ledge
215 prevents any silicone outgassing from getting into the pocket 214.
Figure 1C illustrates a perspective view of an inspection apparatus 250 formed in
accordance with an alternative example. The inspection apparatus 250 includes a body 252, an
optical target 270, and a grating layer 272. The body 252 includes a pocket 264 generally
centered within an inset region 268. The pocket 264 is shaped and dimensioned to receive the
optical target 270. A channel 266 is provided within the inset region 268 and positioned to
substantially surround of the pocket 264. The channel 266 includes inlet/outlet ports 267. The
inset region 268 includes an interior ledge 265 and an exterior ledge 269 that are arranged in a
coplanar manner and positioned to receive a lower surface of the grating layer 272. The body
252 is formed in a manner to maintain a desired amount of flatness in grating layer 272.
Maintaining a desired amount of flatness in the grating layer 272 is beneficial as some optical
calibrations utilize a flat region of the chrome pattern. When silicone cures, it may shrink which
may pull the grating layer 272 down into the channel 266, unless otherwise corrected. If the
grating layer 272 is pulled into the channels 266, a central portion of the grating layer 272 may
bow upward in the region over the optical target 270. Also, clamping the top glass (grating layer
272) in position during adhesive curing may bend the grating layer 272 in a manner that becomes
permanent when the adhesive cures in this state.
In accordance with examples herein, the top surface of the grating layer 272 is
maintained with a desired amount of flatness/planar geometry. To do so, the channel 266 is
provided with a series of pressure relief pockets 271 distributed about the channel 266. The
pressure relief pockets 271 relieve stress induced on to the grating layer 272 by the adhesive
silicone added to the channel 266 during the curing process. Some of the examples disclosed
herein prevent the silicone, when curing, from pulling the grating layer 272 down into the
channel 266. The UV cure adhesive (barriers 211, 213 in Figure 1B) holds the grating layer 272
down on both sides of the channel 266, thereby avoiding bending (or at least substantially
reducing bending) of the grating layer 272. The potential for bending of the grating layer 272 is
further reduced by leaving part of the channel 266 unconstrained so that the silicone can shrink
without pulling on the grating layer 272. This may be achieved by making periodic pockets 271
(holes) in the bottom of the channel 266. When silicone is flowed through the channel 266, air is
trapped inside the pockets 271. When the silicone cures, air bubbles are free to expand up into
the channel 266 as the silicone shrinks. It is much easier to pull the air bubble up into the
channel 266 than it is to pull the grating layer 272 down into the channel 266, so the grating layer
272 does not deform during curing.
Optionally, the body 252 may include one or more mounting features 251, such as
openings provided at opposite ends thereof. The mounting features 251 receive a mating
component on the instrument to position the inspection apparatus 250 at a desired location. In
the example of Figure 1C, the mounting features 251 represent holes that receive corresponding
pins. Alternative or additional mounting features may be utilized.
A general process for assembling the inspection apparatus 250 will be described.
The optical target 270 is inserted into the pocket 264. In the example of Figure 1C, opposite
ends of the pocket 264 include cavities 263 that facilitate introduction of an adhesive. For
example, a tool (e.g., a syringe) loaded with adhesive may be inserted into the cavities 263 at the
ends of the optical target 270. Adhesive is introduced from the tool and allowed to wick/flow,
through capillary force, along the bottom surface of the optical target 270 at least partially across
bottom pocket ledges 259. Capillary forces pull the optical target 270 against the bottom of the
pocket ledges 259, thereby maintaining the optical target 270 at a desired depth within the pocket
264. Optionally, when the adhesive represents a UV cured adhesive, UV light may be
introduced at this point to cure the adhesive.
The grating layer 272 is loaded into the inset region 268, with a perimeter of the
inset region 268 abutting against an exterior perimeter of the grating layer 272. The body 252
includes one or more cavities 249 about the perimeter of the inset region 268 such that, once the
grating layer 272 is positioned in place, the cavities 249 are distributed about a perimeter of the
grating layer 272. Once the grating layer 272 is mounted into the inset region 268, an adhesive
dispensing tool (e.g., a pneumatic adhesive dispenser loaded with a syringe) may be utilized to
introduce a controlled amount of adhesive at one or more points about the perimeter of the
grating layer 272. For example, a tip of a syringe may be inserted into the cavities 249 at corners
of the grating layer 272. A predetermined amount of adhesive is introduced. The adhesive is
pulled, through capillary forces, along the interface between the grating layer 272 and the
exterior ledge 269. The capillary force causes the adhesive to wick/flow along the outer edge
269, without flowing over the portion of the grating layer 272 proximate to the optical target 270.
The capillary forces pull the grating layer 272 against the exterior ledge 269, thereby maintaining
the grating layer 272 at a desired depth within the inset region 268. Optionally, when the
adhesive represents a UV cured adhesive, UV light may be introduced at this point to cure the
adhesive.
Additionally or alternatively, adhesive may be introduced onto the interior ledge
265. The adhesive may be introduced to the interior ledge 265 before or after the grating layer
272 is inserted into the inset region 268. For example, one or more drops of adhesive may be
located on the interior ledge 268 before the grating layer 272 is inserted. Optionally, an adhesive
dispensing tool may be utilized to introduce adhesive to the interior ledge 265 after insertion of
the grating layer 272. For example, a tip of a syringe may be inserted through one or more of the
inlet/outlet ports 267, and the syringe may introduce a predetermined amount of adhesive. The
adhesive is pulled, through capillary forces, along the interface between the grating layer 272 and
the interior ledge 265. The capillary force causes the adhesive to wick/flow along the interior
ledge 265, without flowing over the portion of the grating layer 272 proximate to the optical
target 270. The capillary forces pull the grating layer 272 against the interior ledge 265, thereby
maintaining the grating layer 272 at a desired depth within the inset region 268. Optionally,
when the adhesive represents a UV cured adhesive, UV light may be introduced at this point to
cure the adhesive.
An adhesive (e.g., silicone) is introduced into the channel 266 through one or
more of the inlet/outlet ports 267. For example, the inlet/outlet ports 267 at one or more corners
of the channel 266 may be utilized as an inlet to introduce adhesive, while the inlet/outlet ports
267 at one or more other corners of the channel 266 form an outlet to allow air to discharge from
the channel 266. As explained above, as the adhesive flows through the channel 266, and the
adhesive bridges over the pockets 271. The pockets 271 later provide an air relief for shrinkage
as the adhesive is cured.
Figure 2A illustrates a side sectional view of the inspection apparatus 100 of
Figure 1A along line 2A-2A in Figure 1, with the optical target 120 installed. Figure 2A
illustrates the optical target 120 installed in the pocket 114, and a transparent layer, representing
a grating layer 122, mounted in the inset region 118. The grating layer 122 may have different
regions to be used in connection with different types of alignment operations and/or calibration
tests. For example, as discussed below in connection with Figure 2D, the grating layer 122 may
include one or more “tiles”, representing regions at which the objective (200 in Figure 2D) is
positioned to collect information in connection with various operations. By way of example, the
grating layer 122 may include one or more image quality tiles, distortion tiles, clear tiles,
fiducials and the like. The objective is positioned relative to various tiles to collect information
in connection with performing various tests. The grating layer 122 may also be used to monitor
the uniformity and position of the excitation spatial profile. The grating layer 122 may be
formed from a clear carrier substrate (e.g., glass) with various microstructures 123 provided
thereon and shaped in one or more predetermined patterns. The microstructures 123 are
provided in one or more tiles/areas, at which the objective is positioned in connection with
corresponding calibration operations and tests. Examples of various calibration operations and
tests are described below in connection with Figure 10. For example, the microstructure 123
may comprise chromium or another opaque composition, where the composition exhibits a
desired amount of opacity (e.g., partially or entirely opaque) to excitation light and/or one or
more fluorescence emission bands of interest. For example, a layer of chromium may be
deposited through various techniques onto the surface of the grating layer 122, with different
regions of the chromium forming different patterns (also referred to as “chrome” or a “chrome
pattern”) to be utilized in connection with different alignment and/or calibration operations as
described herein. The microstructure 123 may be shaped with various patterns, such as strips,
dots, pinholes and the like. Optionally, the microstructure 123 may be provided as a solid layer
with the predetermined pattern represented by opening or gaps through the microstructure 123
that form channels, pin holes, and the like. The microstructure 123 may be provided on an upper
and/or lower surface of the grating layer 122, where the upper and lower surfaces are designated
relative to the objective of the instrument. For example, the upper surface represents the surface
that is proximate to the objective, while the lower surface represents the surface that is distal
from the objective. Alternately, the grating structure may be patterned directly on the solid
fluorescing substrate (e.g., see Figure 2E) to form a monolithic structure. In this example, the
grating structure is in contact with the optical target 120 which increases the coupling of the
excitation illumination to the optical target and likewise increases the coupling of the
fluorescence of the optical target 120 to the grating structure such that the light intensity emitted
achieves a desired level (e.g., is maximized). Optionally, the grating layer 122 may be omitted
entirely. Optionally, a spacing between the grating layer 122 and optical target 120 may be
adjusted to provide for spherical aberrations.
In the example shown in Figure 2A, the microstructure 123 includes first and
second grating regions 115, 117 that are separated by a central region 119. The central region
119 is void of microstructures 123.
As shown in Figure 2A, an anti-reflective coating 121 may be formed on a surface
of at least one of the transparent layer (grating layer 122) or the optical target 120. The anti-
reflective coating 121 may be formed on any surface that faces a fringe gap between the grating
layer 122 and the optical target 120. In one example, the anti-reflective coating 121 is positioned
on the surface of the optical target 120. In another example, the anti-reflective coating 121 is
positioned on the surface of the grating layer 122, including on the microstructures 123. In yet
another example, the anti-reflective coating 121 is positioned on the surface of the optical target
120 and on the surface of the grating layer 122, including on the microstructures 123.
To form one example of the anti-reflective coating 121, an anti-reflective material
may be applied to the surface of the optical target 120 that is to face the fringe gap 124 when the
optical target 120 is positioned in the pocket 114. To form another example of the anti-reflective
coating 121, the microstructures 123 may be formed on the surface of the transparent layer (i.e.,
grating layer 122), and then the anti-reflective material may be applied to the surface.
The anti-reflective coating(s) 121 may be included to reduce or eliminate optical
interference that may occur from light reflecting between the surface of the optical target 120
and the grating layer 122 in the fringe gap 124. As a result, optical interference patterns or
fringes may be reduced or eliminated from images that are obtained when using the apparatus
and device disclosed herein.
While the anti-reflective coatings 121 are shown as single layers, it is to be
understood that a single layer may be used or multiple layers may be used to achieve the
desirable anti-reflective effect. For example, multiple layers may be stacked up in order to
achieve minimal or no reflection at the emission band/wavelength(s) of interest. For example, a
multi-layer anti-reflective coating 121 may exhibit from 0% reflectance to 1% reflectance at
wavelengths ranging from about 520 nm to about 700 nm, and may exhibit from 0% reflectance
to about 5% reflectance at wavelengths ranging from about 500 nm to about 520 nm, and may
also exhibit from 0% reflectance to about 9% reflectance at wavelengths ranging from about 700
nm to about 1000 nm. As such, the anti-reflective properties of the anti-reflective coating(s) 121
may not be the same for different wavelengths, and may be varied depending upon the
application in which the apparatus or device is being used.
Examples of suitable anti-reflective materials that may be used to form the anti-
reflective coating(s) 121 include any transparent material having a refractive index equal to the
square root of the refractive index of the substrate (e.g., optical target 120 or grating layer 122)
on which the material is placed. Some examples of anti-reflective materials include magnesium
fluoride (MgF ), fluoropolymers, mesoporous silica nanoparticles, alternating layers of silica and
a higher refractive index material, or other anti-reflective materials that exhibit the desirable ant-
reflective property within the desirable emission band/wavelengths being used.
In the present example, the inset region 118 is formed with an inset ledge 126 and
inset wall 127 that are formed in the body 102. The inset ledge 126 is spaced a predetermined
distance below the top surface 104 of the body 102 and extends inward by a predetermined
distance. The inset ledge 126 defines a depth of the inset region 118, where the depth
corresponds to a thickness of the grating layer 122. For example, the inset ledge 126 may extend
inward by a distance sufficient to support the grating layer 122. As one example, an adhesive
may be applied along the inset ledge 126 to retain the grating layer 122 in a desired position.
The inset ledge 126 may have a length that is determined in part to allow the adhesive to spread
across the inset ledge 126 without overflowing into the pocket 114. The ledge wall 127 is
shaped and dimensioned to extend about a perimeter of the inset region 118. The inset region
118 is formed continuous with the pocket 114.
The pocket 114 is bordered and defined by a pocket ledge 128 and a pocket wall
129. The pocket ledge 128 is spaced a predetermined distance below the inset ledge 126 and
extends inward by a predetermined distance. For example, the pocket ledge 128 may extend
inward by a distance sufficient to support the optical target 120. As one example, an adhesive
may be applied along the pocket ledge 128 to retain the optical target 120 in a desired position.
The pocket ledge 128 may extend inward by a length that is determined in part to allow the
adhesive to spread across the pocket ledge 128 without overflowing into a diffusion well 130.
The pocket 114 is spaced apart inward within the body 102 such that the pocket 114 is centered
in the body 102 to prevent the adhesive from getting under the central region 119 of the optical
target 120.
The pocket wall 129 is shaped and dimensioned to correspond to a shape of the
optical target 120. The pocket wall 129 has a height that extends from the pocket ledge 128 to
the inset ledge 126. The height 129A of the pocket wall 129 is a predetermined distance greater
than a height 120A of the optical target 120 such that, when the optical target 120 is inserted and
firmly rests against the pocket ledge 128, a top surface of the optical target 120 is located below
a plane of the inset ledge 126. The top surface of the optical target 120 is located below the
plane of the inset ledge 126 by a thickness of a fringe gap 124. The fringe gap 124 corresponds
to a distance between the top surface of the optical target 120 (or an anti-reflective coating 121
thereon) and a bottom surface of the grating layer 122 (or an anti-reflective coating 121 thereon).
The fringe gap 124 is large enough to avoid interference fringes. Interference fringes may occur
when the grating layer 122 and the optical target 120 directly contact one another at one or more
points. The fringe gap 124 is sufficiently large to avoid direct contact between the optical target
120 and the grating layer 122. The fringe gap 124 is small enough to avoid introducing adverse
optical properties as light passes between the grating layer 122 and the optical target 120. For
example, if the fringe gap 124 were made unduly large, an excessive amount of light may be lost
while passing through the fringe gap 124. The fringe gap 124 avoids undue loss of light within
the fringe gap 124 as the light passed between the grating layer 122 and optical target 120. For
example, the fringe gap 124 may have a thickness of or between about 10 µm and about 100 µm,
and, in an example, a thickness of about 30 µm (+/- 20 µm). Optionally, the fringe gap 124 may
have a different thickness provided that an amount of light loss remains within a predetermined
light loss limit (e.g., less than or equal to about 20% of the incoming light intensity). Optionally,
the grating layer 122 and the optical target 120 may experience a controlled minimal amount of
contact which may introduce small interference fringes that do not unduly affect use of the
optical target 120. As mentioned above, the interference fringes may be further reduced or
eliminated by including the anti-reflective coating 121 on one or both of the optical target 120
and the grating layer 122.
Optionally, an index matching fluid or index matching epoxy may be provided to
fill the fringe gap 124 to reduce the potential for movement between the grating layer 122 and
the optical target 120 over time. At least certain index matching epoxies may experience slight
changes in color (e.g., discoloration) over time which may be undesirable in at least certain
applications. Also, a potential exists that an index matching fluid may leak out of the fringe gap
124 over time. Consequently, the potential exists that, at least certain index matching fluids
and/or epoxies may cause the intensity of the fluorescence emission to change over time. For
example, over time the matching fluid or epoxy may slightly diminish the excitation light
intensity impinging upon the optical target 120 and/or the intensity of the fluorescent emission
that crosses the fringe gap 124. Accordingly, in at least certain examples, utilizing air within the
fringe gap 124 may represent at least one aspect for maintaining a constant intensity of the
fluorescence emitted from the inspection apparatus 100. Further, the addition of an index
matching fluid or epoxy may introduce an extra step/complexity to the manufacturing process
that is not otherwise present when the fringe gap 124 is filled with air.
The pocket 114 is joined with a diffusion well 130 located below the pocket 114
(distal from the objective 200, shown in Figure 2B), and below the optical target 120 when
inserted in the pocket 114. The diffusion well 130 is located below the pocket 114 and is
centered within the optical target 120. The diffusion well 130 is configured to receive light that
passes through the optical target 120. The light progressively becomes defocused or diffused as
the light traverses the diffusion well 130 until contacting a well base 132. When the light
engages the well base 132, the light has diffused to a desired degree sufficient to avoid photo
bleaching of the well base 132.
The pocket 114 has a height that is dimensioned to provide a desired distance
(e.g., a maximum distance) between a focal point of the light (within the optical target 120) and a
bottom portion of the body 120. The diffusion well 130 includes a well bottom 132 that may be
provided with a pigment-based black finish or coating to facilitate avoidance of photo bleaching
and to manage reflectivity to within a desired level (e.g., less than or equal to about 6%). For
example, the pigment-based black finish may represent an electrolytic blackening using
inorganic metallic salts such as ANOBLACK™ EC offered by Anoplate Corp. of Syracuse, N.Y.
In accordance with examples disclosed herein, the black finish is provided utilizing a pigment,
and not a dye, as black dyes have large molecules (relative to the molecule size for pigments)
that are more susceptible to being broken down over time with exposure to the excitation light.
The pigments, utilized to form the black finish, in accordance with at least some examples, are
formed from smaller molecules that are less susceptible to the excitation light and are not broken
down over time. As one example, the pigment may be phosphorous enriched black nickel oxide
which forms a black finish, has a relatively small molecule size that is not susceptible to being
broken down by excitation light and thus maintains a relatively constant reflectivity. Also, the
pigment may be chosen to afford low fluorescence in the coating because a low initial
fluorescence in the coating will mean that the coating fluorescence will not drop by much over
time.
Optionally, various other portions of the surface of the body 102 (e.g., the top
and/or bottom surfaces 104, 106, the lateral sides 108 and/or front and back ends 110, 112 may
be covered with the finish or coating.
Figure 2B illustrates a side view of a model of the optical target 120 with an
objective 200 positioned at a first measurement position in accordance with an example herein.
Figure 2C illustrates a side view of a model of the optical target 120 with the objective 200
positioned at a second measurement position in accordance with an example herein. Figures 2B
and 2C illustrate the objective 200 positioned at first and second measurement locations,
respectively, relative to the inspection apparatus 100. The models of Figures 2B and 2C
illustrate the body 102, optical target 120, grating layer 122, and diffusion well 130, among other
structures, although to simplify the illustration, the fringe gap 124 and other features of Figure
2A are not illustrated in detail.
In Figure 2B, the inspection apparatus 200 is positioned proximate the central
region 119 of the grating layer 122, such as in connection with performing excitation
measurement operations. When the objective 200 is positioned within the central region 119, the
excitation light 202 avoids the microstructures 123 in the grating regions 115, 117. The
objective 200 directs excitation light 202 into the inspection apparatus 100, where the excitation
light 202 is focused to different focal points based upon the particular measurement being
performed. For example, in connection with the frame measurement operation (corresponding to
Figure 2B), the objective 200 focuses the excitation light 202 to a focal point 204 that is below
the upper surface 107 of the optical target 120 (e.g., 50 µm). The objective 200 manages an
angular aperture 208 to obtain a desired degree of focus at the focal point 204 and to obtain a
desired degree of diffusion/defocus at greater depths within the optical target 120 and thereafter.
The objective 200 receives fluorescence emission that is emitted from the upper surface 107 of
the optical target 120 within the central region 119.
During operation, non-grating-based measurements (e.g., an optical intensity
measurement) may be obtained by positioning the objective 200 above the region 119. For
example, the non-grating-based measurement may be performed in connection with imaging the
position of the excitation light illumination relative to a field of view of a detection camera. The
focal point 204 is located below the upper surface 107 in order to remove scratches, dust,
fingerprints and the like from the focal plane, such as debris, scratches and defects in the surface
of the optical target 120, so that these potentially interfering effects will have no or relatively
little affect on the measurement. Other operations are discussed in connection with Figure 10
that may utilize images obtained from the region 119.
Excitation light is emitted from the objective 200, and travels through the grating
layer 122 and into the optical target 120 without passing through the microstructures 123. In
response, the optical target 120 produces fluorescence emissions from within the optical target
120 that return through the region 119 and impinge upon the objective 200, where the
fluorescence emissions are redirected through internal optics to one or more detectors. The
objective 200 focuses the excitation light at a focal point that is located below a surface of the
optical target 120 by a predetermined distance. For example, the focal point 204 may be located
from about 20 µm to about 100 µm below the surface 107 of the optical target 120. As another
example, the focal point 204 may be located at about 50 µm below the surface 107 of the optical
target 120. The excitation light is diffused within a lower portion of the optical target 120 below
the focal point 204 to cause fluorescence emission across a relatively large area within the
optical target 120, thereby affording a relatively uniform scan. At least some examples eliminate
or substantially reduce negative effects of scratches, debris, fingerprints and the like on the
surface 107 of the optical target 120 and/or grating layer 122 by locating the focal point 204
below the surface 107 of the optical target 120 and managing the angular aperture 208.
In Figure 2C, the inspection apparatus 200 is positioned proximate to one of the
grating regions 115, 117, such as in connection with performing a grating measurement
operation. When the objective 200 is positioned proximate to one of the grating regions 115,
117, the excitation light 202 impinges upon the microstructures 123, passing through gaps or
apertures therebetween. The objective 200 focuses the excitation light 202 to a focal point 206
that corresponds to the bottom surface of the grating layer 122. The objective 200 manages an
angular aperture 210 to obtain a desired degree of focus at the focal point 206 and to obtain a
desired degree of diffusion/defocus at greater depths within the optical target 120 and thereafter.
The focal point 206 also corresponds to the position of the microstructures 123. The objective
200 receives fluorescence emission that is emitted from the optical target 120 within a
corresponding grating region 115, 117. In accordance with at least some examples, all or a
portion of the emission may come from a top volume of the optical target 120, while none or a
lesser portion of the emission comes from the remaining volume of the optical target 120.
During operation, grating-based measurements are obtained by positioning the
objective 200 above one or both of the first and second grating regions 115 and 117. Excitation
light is emitted from the objective 200, travels through the grating regions 115, 117 and into the
optical target 120. The excitation light diffuses or defocuses beyond the focal point 206 at a rate
determined by the angular aperture 210 at greater depths within the optical target 120. In
response to the excitation light, the corresponding region of the optical target 120 produces
fluorescence emissions that emit from the upper surface 107 and impinge upon the lower surface
(and microstructures 123) of the grating layer 122. The fluorescence emissions pass between the
microstructures 123 on the grating layer 122 and pass upward until impinging upon the objective
200. The fluorescence emissions are redirected through internal optics to one or more detectors
and are processed accordingly. To the extent that excitation light passes through the optical
target 120, the excitation light exhibits a desired degree of defocus when passing through the
diffusion well 130 before contacting the well bottom 132. The intensity of the excitation light
that contacts the well bottom 132 is below a predetermined threshold and as such, avoids a
potential of changing the optical characteristics of the well bottom 132 over time.
As the excitation light passes beyond the microstructures 132, the laser light
diverges into a larger area which causes a relatively large portion of the optical target 120 to
glow when emitting fluorescence. Accordingly, cameras within the instrument are able to collect
chrome pattern measurements from portions of the microstructures 132 that may be positioned
laterally to either side of the focal point 206, thereby affording improved illumination uniformity
for the chrome pattern measurements.
The objective 200 may be provided with a large numerical aperture, such that, the
further the objective 200 is moved away from the surface of the grating layer 122, the more out
of focus the excitation source becomes. The excitation laser diverges as the excitation light
moves away from the focal point 206. The rate, at which the excitation light diverges/focuses, is
dependent in part on the numerical aperture of the objective 200. In accordance with at least
some examples, the excitation light is substantially defocused by the time the excitation light
exits the bottom surface of the optical target 120. The excitation light continues to further
diverge (become more unfocused) as the excitation light passes the diffusion well 130. By the
time the excitation light impinges upon the well bottom 132, the excitation light is
defocused/divergent to a desired degree to limit the intensity of energy impinged upon any point
on the well bottom 132 to below a desired intensity threshold.
In accordance with the examples herein, the objective 200 and inspection
apparatus 100 avoid undue photo degradation of the body 102 (e.g., minimize the photo
bleaching) by spreading the excitation laser lines over a large area (e.g., 2.3 mm in X and 0.53
mm in Y). In addition, some examples avoid undue auto-fluorescence (e.g., minimize) of
structures on the body 102, in part, by managing focus of the excitation light such that the
excitation light is defocused by a desired amount (measured at less than about 1.5% of the Er-
InF signal) when the excitation light impinges upon surfaces of the body 102.
In addition, the diffusion well 130, and the distance between the focal point 206
and the well bottom 132, reduce a potential for auto-fluorescence. Auto-fluorescence may result
from the well bottom 132 in response to reception of excitation light. To the extent that the well
bottom 132 emits any fluorescent energy, such fluorescent energy becomes substantially
dispersed while traveling through the diffusion well 130 without impacting the characteristics of
interest from the optical target 120.
Optionally, in accordance with at least some examples, a length of the optical
target 120 may be dimensioned in a desired manner relative to the microstructures 123 within the
grating regions 115, 117. For example, it may be desirable to manage the position of the
objective 200 such that, when performing the measurements over the grating (corresponding to
Figure 2C), the excitation light within the numerical aperture 210 does not impact the pocket
wall 129.
In accordance with examples herein, the inspection apparatus 100 affords a
fluorescent source that substantially remains constant over a large period of time. For example,
the inspection apparatus 100 does not exhibit notable loss of fluorescence intensity and remains
substantially stable over at least 10,000 inspection operations (where each inspection operation
corresponds to at least one illumination operation of the optical target by excitation light). As
another example, the inspection apparatus 100 may exhibit no more than about a 3% change in
fluorescence emission intensity over at least 10,000 inspection operations. More generally, the
inspection apparatus 100, when formed in accordance with examples described herein, exhibits
no more than about a 2% reduction in fluorescence emission intensity over a useful life of a
corresponding instrument with which the inspection apparatus 100 is utilized.
Figure 2D illustrates a top plan view of the inspection apparatus formed in
accordance with an example. The grating layer (122 in Figure 2A) and microstructures are
arranged in various tiles/areas to be utilized in connection with different types of test. The
regions within the boxes labeled 281 and 283 in Figure 2D (including any sub-regions identified
within boxes 281 and 283) correspond to areas where chrome/microstructures is/are provided on
the grating layer. It is to be understood that these areas may also be chrome with pinholes. Any
region outside of the regions marked 281 or 283 (e.g., the region between 281 or 283 and the
perimeter, or between 281 and 283) represent clear areas where no chrome/microstructures are
positioned. It is to be understood that the area within the plus signs may also be clear areas
where no chrome/microstructures are positioned.
The inspection apparatus includes top and bottom auto centering fiducials 280,
282 that are utilized in connection with an automated centering operation for an imaging
apparatus. An image quality tile 284 is provided for use with an image quality test. A distortion
tile 286 is provided to be utilized in connection with a distortion test. A clear tile 288 is provided
for use with an illumination uniformity and flat field correction operation. A clear area 290 is
provided for use with laser line measurements. A horizontal knife edge 292 and a vertical knife
edge 294 are provided in connection with laser spot position checks. A pattern of clear holes is
provided at tile 296 to be utilized in connection with measuring a modulation transfer function.
Optionally, additional, fewer or alternative tile areas may be provided.
Figure 2E illustrates a side sectional view of an inspection apparatus 300 formed
in accordance with an alternative example. The inspection apparatus 300 resembles the
inspection apparatus 100 of Figure 2A in various manners, with the differences discussed
hereafter. The inspection apparatus 300 includes a body 302 that receives an optical target 320
in a pocket 314. The pocket 314 includes a pocket ledge 328 that maintains the optical target
320 above a diffusion well 330 and at a predetermined depth within the body 302. A transparent
layer 322 (e.g., formed of glass) is inserted into an inset region 318 defined in the body 302. An
exterior ledge 326 maintains the transparent layer 322 a predetermined distance above the optical
target 320, with a fringe gap 324 therebetween. The optical target 320 includes microstructures
323 formed on the top surface thereof. The microstructures 323 are separated from the
transparent layer 322 by the fringe gap 324. The microstructures 323 form a grating layer on a
surface of the optical target 320 that is separate and distinct from the transparent layer 322.
Optionally, the transparent layer 322 may be omitted entirely. Optionally, a spacing between the
transparent layer 322 and optical target 320 may be adjusted to provide for spherical aberrations.
Accordingly, the inspection apparatus 300 be made by printing the chrome pattern
(microstructure 323) directly onto the top surface of the optical target 320 instead of on the
bottom of the transparent layer 322.
While not shown, the example shown in Figure 2E may also include the anti-
reflective coating 121 on the surface of the transparent layer 322 that faces the fringe gap 324
and/or on the surface of the optical target 320 and on the microstructures 323 formed on the
optical target 320. Any examples of the anti-reflective material(s) disclosed herein may be used
in this example.
The thickness of the transparent layer 322 is set to compensate for spherical
aberration in the imaging system. If the imaging system is designed with zero spherical
aberration, then the transparent layer 322 may be omitted entirely and the chrome pattern would
be printed on top of the optical target 320. If the imaging system has spherical aberration (since
it is designed to look through a certain thickness of glass), then the transparent layer 322 would
be used even if the chrome pattern is printed on the optical target 320. Optionally, the fringe gap
324 may be omitted entirely, such that the optical target 320 directly rest on and abuts against a
top surface of the optical target 320.
Figure 2F illustrates a side sectional view of an inspection apparatus 350 formed
in accordance with an alternative example. The inspection apparatus 350 does not include a
separate body (such as the body 302 or body 102, described above). The inspection apparatus
350 includes an optical target 356 and a transparent layer 352 directly bonded onto one another.
Microstructures 353 are provided at the interface between the optical target 356 and transparent
layer 352. The microstructures 353 may represent one or more chrome patterns formed on a top
surface of the optical target 356 and/or on a bottom surface of the transparent layer 352. By way
of example, the inspection apparatus 350 may be utilized in examples in which the inspection
apparatus 350 is located directly on a flow cell, instead of being mounted into an instrument.
Additionally or alternatively, the inspection apparatus 350 may also be mounted within an
instrument.
Optionally, the transparent layer 352 may be omitted entirely. For example, any
of the optical targets 120, 320, 356 described herein may be utilized as a stand-alone inspection
apparatus with no additional body components or transparent layers provided therewith.
Optionally, the optical targets 120, 320 and 356 may be utilized as a stand-alone inspection
apparatus with no microstructures or other patterns formed thereon or provided proximate
thereto. For example, the optical targets 120, 320 and 356 may simply be mounted directly on a
flow cell and/or within an instrument without any other supporting structures.
Figure 3A illustrates an energy level diagram in connection with a fluorescing
material utilized in accordance with examples herein. The energy level diagram illustrates
energy (cm ) along the vertical axis and alternative transitions distributed across the horizontal
axis. A ground energy level 302 is illustrated, along with elevated energy levels 304 – 309, to
which an electron of the trivalent erbium ion may be raised when excited. For example, an
electron of the erbium ion may absorb an energy of about 18,800 cm , causing the electron to
move from the I ground energy level 302 to a S target excitation (TE) energy level 308.
/2 3/2
As another example, an electron of an erbium ion may absorb an energy of about 15,000 cm ,
causing the electron to move from the I ground energy level 302 to a different F TE energy
/2 9/2
level 307. The electrons of the erbium ion absorb energy from the excitation light and then move
to the corresponding TE energy level 307, 308. Once the ions have moved to a corresponding
elevated TE energy level, the ions then discharge the absorbed energy, in the form of a photon,
and return to the ground energy level 302. The TE energy level is separated from the ground
energy level by a first energy gap FM corresponding to a fluorescence emission wavelength
of interest (FEWI). For example, the FEWI may be a red, green, blue or other emission
wavelength. The discharged photon is then received by the objective as fluorescence emission.
The color of the fluorescence emission is dependent upon the energy of the photon which
corresponds to the first energy gap FM . When an ion transitions from the target excitation
energy level 307 to the ground energy level 302, the corresponding discharged photon has an
energy of about 15000 cm which is detectable as a fluorescence emission wavelength of interest
of 650 nm (visible as a red fluorescence emission). When an ion transitions from the target
excitation energy level 308 to the ground energy level 302, the corresponding discharged photon
has an energy of about 18,800cm which is detectable as a fluorescence wavelength emission of
interest about 532 nm (visible as a green fluorescence emission).
Figure 3A also illustrates additional energy level transitions that may be exhibited
by a trivalent erbium ion. Each of the energy levels 304-308 has one corresponding next lower
lying energy level. In accordance with examples herein, the solid host material and fluorescing
material are chosen based in part on the energy gap between one or more target excitation energy
levels (e.g., 308) and the next lower lying energy level (e.g., 307). The F energy level 307
represents a next lower lying (NLL) energy level relative to the S energy level 308. The I
3/2 9/2
energy level 306 represents the NLL energy level relative to the S energy level 307.
Electrons may be elevated to the energy levels 304, 305 and 306, and when
returning to the ground energy level 302 discharge photons having a corresponding amount of
energy. The photons discharged during transitions from the energy levels 304 – 306 have
corresponding wavelengths of 1520 nm, 975 nm and 800 nm, respectively. In addition, an
electron may transition between intermediate elevated energy levels 304 – 308. When an
electron transitions between adjacent or intermediate elevated energy levels, a photon is
discharge with a corresponding amount of energy, which corresponds to the difference between
the starting and ending elevated energy levels. Figure 3A illustrates example wavelengths that
may be visible in connection with photons emitted when electrons transition between different
elevated energy levels. For example, an electron at the energy level 308 may transition to any of
energy levels 307, 306, 305 and 304, in which case a discharged photon would have a
wavelength of 3230 nm, 1670 nm, 1210 nm, and 840 nm, respectively. As a further example,
when an electron at the energy level 307 transitions to another intermediate elevated energy level
306 – 304, the corresponding discharged photon will have a wavelength of 3450 nm, 1940 nm,
and 1132 nm, respectively. The discharged photon will emit fluorescence at a color
corresponding to the photon wavelength.
Several, but not all, examples described herein contemplate use of an inspection
apparatus in connection with a fluidics system that utilizes fluorescence emissions in
predetermined emission bands of interest. By way of example, the emission bands may be
centered at a wavelength corresponding to a green fluorescence emission and/or corresponding to
a red fluorescence emission. When the emission bands of interest are centered about
wavelengths corresponding to red or green emissions, the corresponding portion of the energy
diagram of Figure 3A is of interest. More specifically, when green emission is of interest, it is
desirable to transition between target excitation and ground energy levels 308 and 302. When
red emission is of interest, it is desirable to transition between target excitation and ground
energy levels 307 and 302. In the present example, transitions between other energy level
combinations in the diagram of Figure 3A are not of interest in connection with an instrument
that utilizes red and/or green emission bands of interest.
It is recognized that the foregoing discussion is one example, and that other
examples are contemplated as being within the purview of the instant disclosure. Additionally or
alternatively, other emission bands may be of interest. For example, an instrument may utilize
the emission band associated with 800 nm and/or 975 nm. When an emission band of interest
has a wavelength centered about 800 nm and/or 975 nm, energy transitions between levels 306
and 302, and levels 305 and 302 are of interest. In general, energy bands above 1000 nm may
typically not be of interest in connection with fluidics instruments, as the fluorescence emitted in
connection with performing a sequencing analysis typically does not utilize energy bands above
1000 nm. Accordingly, the transition between the first elevated energy level 304 and the ground
energy level 302 may not be of interest or useful in connection with a fluidics instrument.
In accordance with examples herein, fluorescence from the fluorescing material is
achieved by optical excitation to an upper-lying energy level (also referred to as a target
excitation energy level) by means of a laser or light emitting diode (LED) source. Following the
optical excitation process, decay to lower lying energy levels within the impurity ion occurs via
two competing energy transfer processes: radiative decay, with the corresponding emission of
photons (fluorescence) and non-radiative decay, by means of optical phonon emission to the
surrounding lattice structure. The non-radiative decay rate depends on the coupling interaction
between the surrounding lattice and the impurity ion, dropping exponentially with the number of
emitted phonons. Consequently, non-radiative processes involving a large number of emitted
phonons have a low probability of occurrence. The non-radiative transition probability between
two energy levels is adequately described by an exponential decaying function: W = Cexp(-
αΔE)[n(T)+1] , where C and α are constants specific to the solid host material, ΔE is the energy
gap separating the two energy levels, n(T) is the Bose-Einstein occupation number at
temperature, T, and p is the minimum number of phonons required to span the energy gap. In
general, non-radiative decay via multi-phonon processes can be minimized by selecting hosts
with low maximum phonon energies. For example, to observe visible fluorescence at about 660
3+ 4 4
nm from the Er F – I transition, it is necessary to minimize non-radiative decay between
9/2 15/2
4 4 4
the F level to the next lower lying state, I . Since the energy separation between the F –
9/2 9/2 9/2
4 -1
I levels is ~ 2900 cm , it is advantageous to select a host material with a maximum phonon
energy less than or equal to about 580 cm (corresponding to the simultaneous emission of 5 or
more phonons). In addition to favoring emission in the red wavelength region, selection of a low
3+ 4
phonon host material also enhances green emission from the Er S excited state, for which
4 -1
the next lower lying energy level ( F ) lies at about 3100 cm therebelow.
The solid host material has a predetermined phonon energy HOST , while the
fluorescing material exhibits a select ground energy level and a target excitation energy level
separated from the ground energy level by a first energy gap corresponding to a fluorescence
emission wavelength of interest (FEWI). In the example of Figure 3A, the FEWI is the green
and/or red emission wavelength. The fluorescing material has a next lower lying (NLL) energy
level relative to the TE energy level. The NLL energy level is spaced a second energy gap
FM below the TE energy level wherein a ratio of the FM /HOST is three or more.
EG2 EG2 PE
Optionally, the ratio of the FM /HOST is at or between four and ten.
EG2 PE
It is recognized that Figure 3A represents one example of an energy level diagram
associated with a potential fluorescing material that may be doped within a solid host material.
As discussed herein, alternative fluorescing materials may be utilized as dopants. As examples,
Figure 3B illustrates an ion energy level diagram associated with a trivalent praseodymium ion
(Pr3+), and Figure 3C illustrates an ion energy level diagram associated with a trivalent holmium
ion (Ho3+). The diagrams in Figures 3B and 3C illustrate ground energy levels, target excitation
energy levels and intermediate elevated energy levels, as well as wavelengths associated with
photons emitted by an electron when transitioning between the corresponding designated energy
levels. Continuing with the foregoing example, the subset of the energy level transitions that is
of interest is based on the emission band of interest.
With respect to Pr3+ (Figure 3B), a transition between a target excitation energy
level P0 and ground energy level H will emit a photon having a wavelength between 515 and
548 nm (which includes the band of interest at 532 nm). With respect to Pr , a transition
between target excitation energy level P and intermediate energy level F will emit a photon
having a wavelength between 597 nm and 737 nm (which includes the band of interest at 660
nm). Accordingly, Pr may represent a potential candidate for a fluorescing material to be
doped into a solid host material. In the example of Figure 3B, when the target excitation energy
level is P , the next lower lying energy level is D .
With respect to Ho (Figure 3C), a transition between a target excitation energy
level F and ground energy level I will emit a photon having a wavelength of about 544 nm
(which is proximate to the wavelength band of interest at 532 nm). A transition between the
target excitation energy level S and intermediate energy level I will emit a photon having a
wavelength of about 656 nm (which is proximate to the band of interest at 660 nm).
Accordingly, Ho may represent a potential candidate for a fluorescing material to be doped into
a solid host material. In the example of Figure 3C, when the target excitation energy level is S ,
the next lower lying energy level is F .
Figure 4 illustrates an example of intensities that were exhibited for different
fluorescence emission colors. The vertical axis plots energy intensity, while the horizontal axis
plots a concentration (in percentage) of a fluorescing material doped into a solid host material.
As reference points, data point 402 corresponds to an intensity measured upon excitation of a
liquid green dye, while data point 404 corresponds to an intensity measured upon excitation of a
liquid red dye. When the liquid green dye was illuminated with an excitation laser, the liquid
green dye emitted fluorescence in the green energy spectrum with an intensity of about 1650
counts. When the liquid red dye was illuminated with an excitation laser, the liquid red dye
emitted fluorescence in the red energy spectrum with an intensity of about 1150 counts.
Figure 4 also illustrates data measurements performed in connection with solid-
state optical targets, namely data points 410 – 416. Data points 410 and 414 correspond to the
intensity measured upon excitation of a solid-state optical target in which a host indium fluoride
glass was doped with a trivalent erbium ion at a concentration of 2.5%. Data points 412, 416
correspond to the intensity measured upon excitation of a solid-state optical target in which a
host indium fluoride glass was doped with a trivalent erbium ion at a concentration of about 4%.
As evident from Figure 4, the 2.5% doped solid-state optical target emitted fluorescence in the
green energy spectrum at about 650 counts and emitted fluorescence in the red energy spectrum
at about 1300 counts. The 4.0% doped solid-state optical target emitted fluorescence in the
green energy spectrum at about 500 counts and emitted fluorescence in the red energy spectrum
at about 2350 counts. From the foregoing test data, concentrations of a trivalent erbium dopant
can be determined, based upon the desired intensity of fluorescence. For example, when it is
desirable for the optical target to emit fluorescence in the red energy spectrum, it may be
desirable to increase the concentration of trivalent erbium ion dopant to 3.5% or more (e.g., 4%,
4.5%). When it is desirable for the optical target to emit fluorescence in the green energy
spectrum, it may be desirable to decrease the concentration of trivalent erbium ion dopant to
between about 1.5% and about 2%.
Further, from the foregoing test data, concentrations of a trivalent erbium dopant
may be determined when it is desirable for the optical target to emit fluorescence in two or more
energy spectrums with equal intensity (e.g., in the green and red energy spectrums). For
example, it may be desirable to maintain the trivalent erbium ion dopant concentration between
about 1.25% and about 2%. As a further example, a trivalent erbium ion dopant concentration
may be between about 1.3% and about 1.5% within indium fluoride glass. Figure 5 illustrates
test results of a solid host material that was formed by doping a metal fluoride glass (ZBLAN)
with about a 2% concentration and about a 5% concentration of a trivalent erbium ion. Figure 5
plots an intensity along the vertical axis of fluorescence emissions and emission wavelength
along the horizontal axis. The 2% concentration and the 5% concentration of erbium ions
exhibited an intensity spike centered about 550 nm. The 2% and 5% erbium concentrations also
exhibited a secondary intensity spike at about 660 nm.
In the example of Figure 4, trivalent erbium ions represent an active fluorescing
material. Optionally, one or more additional elements may be added as a co-dopant to the solid
host material. The co-dopant may be utilized to increase or decrease the emission intensity of
the active fluorescing material (e.g., erbium).
Figure 6A illustrates a side sectional view of an inspection apparatus 600 formed
in accordance with an alternative example. The inspection apparatus 600 includes a body 602
that holds an optical target 620 in a pocket 614. A grating layer 622 is positioned above the
optical target 620 proximate to an objective (not shown). The grating layer 622 includes
microstructures 623 formed in predetermined patterns on a bottom surface of the grating layer
622.
The optical target 620 may be separated from the grating layer 622 by a fringe
gap 624. The optical target 620 includes top and bottom target surfaces 607, 609 that are
generally planar and oriented parallel to one another. The optical target 620 comprises a solid
body that includes a plurality of quantum dots 621 embedded therein. The solid body may be
formed of epoxy, polymers and other materials that may enclose a plurality of discrete bodies
(e.g., the quantum dots 621) and hold the discrete bodies in a fixed arrangement. The quantum
dots 621 are distributed substantially evenly throughout the optical target 620, such that, when
irradiated by an excitation light, the quantum dots 621 emit fluorescence in one or more
predetermined emission bands of interest. The inspection apparatus 600 may be utilized in the
same manner as any other inspection apparatus described herein.
Optionally, the quantum dots 621 may be formed as silicon (Si) quantum dots,
such as to enable the wavelength to be tuned.
Figure 6B illustrates a portion of an inspection apparatus 640 formed in
accordance with an alternative example. The inspection apparatus 640 includes a grating layer
662 and a body 642. An optical target 660 is held within the body 642 and directly engages the
grating layer 662. The grating layer 662 includes microstructures 663 formed on a back or
bottom surface thereof (relative to an objective). The optical target 660 surrounds and
hermetically seals with the microstructures 663. The optical target 660 includes quantum dots
661 distributed throughout. The quantum dots 661 are also provided within regions 665 between
the microstructures 663. By way of example, the optical target 660 may be formed from epoxy,
a polymer or other composition that will flow into and fill the gap(s) 665 between the
microstructures 663 and that will hermetically enclose therein a distributed group of the quantum
dots 661.
Figure 6C illustrates a portion of an inspection apparatus 670 formed in
accordance with an alternative example. The inspection apparatus 670 includes a grating layer
682 and a body 672 and an optical target 680 that is held within the body 672. The optical target
680 directly engages the grating layer 682 and fills gaps 685 between the microstructures 683
formed on the back/bottom side of the grating layer 682. In the example of Figure 6C, quantum
dots 681 are held within the gaps 685 and clustered to be located proximate to and surrounding
the microstructures 683. A portion of the optical target 680 that is remote from the
microstructures 683 is substantially void of quantum dots 681.
In the examples of Figures 6A – 6C, the quantum dots 621, 661, 681 may be
constructed to emit fluorescence centered about one or more wavelengths of interest depending
upon the emission band or emission bands of interest. For example, a portion of the quantum
dots 621, 661, 681 may be constructed to emit fluorescence at a wavelength of about 532 nm,
while another portion of the quantum dots 621, 661, 681 may be constructed to emit fluorescence
at a wavelength of about 660 nm. Optionally, the quantum dots 621, 661, 681 may be
constructed to emit at other wavelengths instead of or in addition to the foregoing examples.
Optionally, the fluorescent material may be provided as an organo-polymer.
Optionally, the fluorescent material may represent a fluorescent dye embedded within epoxy. As
another example, a fluorescent film may be coated on top of an optical target in addition to or in
place of doping fluorescent material within a solid host material.
Applications
Examples herein may be used in connection with instruments used for biological
or chemical research, including the execution of a large number of controlled reactions. The
reactions may be carried out in accordance with a predetermined protocol by automated systems
that have, for example, suitable fluidics, optics, and electronics. The systems may be used, for
example, to generate a biological or chemical product for subsequent use or to analyze a sample
to detect certain properties/characteristics of the sample. When analyzing a sample in some
cases, a chemical moiety that includes an identifiable label (e.g., fluorescent label) may be
delivered to a chamber where the sample is located and selectively bind to another chemical
moiety of the sample. These chemical reactions may be observed or confirmed by exciting the
labels with radiation and detecting light emissions from the labels. Such light emissions may
also be provided through other means, such as chemiluminescence.
Some known systems use a fluidic device, such as a flow cell, that includes a flow
channel (e.g., interior chamber) defined by one or more interior surfaces of the flow cell. The
reactions may be carried out along the interior surfaces. The flow cell is typically positioned
proximate to an optical assembly that includes a device for imaging the sample within the flow
channel. The optical assembly may include an objective lens and/or a solid body imaging device
(e.g., charge-coupled device (CCD) or complementary metal-oxide-semiconductor (CMOS)). In
some cases, an objective lens is not used and the solid body imaging device is positioned
immediately adjacent to the flow cell for imaging the flow channel.
Any example of the inspection apparatus described herein may be used with
various systems, methods, assemblies, and apparatuses that detect desired reactions in a sample
for biological or chemical analysis. For example, in one sequencing-by-synthesis (SBS)
technique, one or more surfaces of the flow channel have arrays of nucleic acid clusters (e.g.,
clonal amplicons) that are formed through bridge PCR. After generating the clusters, the nucleic
acids are "linearized" to provide single stranded DNA (sstDNA). To complete a cycle of
sequencing, a number of reaction components are flowed into the flow channel according to a
predetermined schedule. For example, each sequencing cycle includes flowing one or more
nucleotides (e.g., A, T, G, C) into the flow channel for extending the sstDNA by a single base. A
reversible terminator attached to the nucleotides may ensure that only a single nucleotide is
incorporated by the sstDNA per cycle. Each nucleotide has a unique fluorescent label that emits
a color when excited (e.g., red, green, blue, and the like) that is used to detect the corresponding
nucleotide. With the newly-incorporated nucleotides, an image of numerous clusters is taken in
four channels (i.e., one for each fluorescent label). After imaging, another reaction component is
flowed into the flow channel to chemically cleave the fluorescent label and the reversible
terminator from the sstDNA. The sstDNA is then ready for another cycle. Accordingly, a
number of different reaction components are provided to the flow channel for each cycle. A
single sequencing session may include numerous cycles, such as 100, 300, or more. The
inspection apparatus may be constructed to emit fluorescence at the colors utilized by the
fluorescent labels in the analysis. The inspection apparatus may be utilized at various points
before and/or during the sequencing session.
In some examples, the desired reactions provide optical signals that are detected
by an optical assembly. The inspection apparatus may be used to verify, validate, calibrate, etc.
the optical assembly. The optical signals may be light emissions from labels or may be
transmission light that has been reflected or refracted by the sample. For example, the optical
assembly may be used to perform or facilitate performing a sequencing protocol in which
sstDNA is sequenced in a flow cell.
In accordance with examples herein, the inspection apparatus may be used with
an optical scanning device and a fluidic cartridge that can be used to provide a sample and
reagents to the device. The fluidic cartridge may include a housing that protects various fluidic
components such as reservoirs, fluidic connections, pumps, valves and the like. A flow cell may
be integrated into the fluidic cartridge in a position where it is in fluid communication with
reagents within the housing. For example, the housing may have an opening through which a
face of the flow cell is exposed such that it can interact optically with the optical scanning device
when the fluidic cartridge is placed in the cartridge receptacle. The device includes one or more
microfluorometers.
Figure 7 illustrates a block diagram of an optical detection device 700 (also
referred to as a detector) formed in accordance with an example. The detector 700 includes one
or more processors 730 that execute program instructions stored in memory 732 to perform the
operations described herein. The processor 730 directs one or more drivers 734 to move the
objective 701 in the Z direction and to move the detector 700 in the XY direction. The detector
700 is positioned proximate to a flow cell 770 having an upper layer 771 and a lower layer 773
that are separated by a fluid filled channel 775. In the configuration shown, the upper layer 771
is optically transparent and the detector 700 is focused to an area 776 on the inner surface 772 of
the upper layer 771. In an alternative configuration, the detector 700 can be focused on the inner
surface 774 of the lower layer 773. One or both of the surfaces 772, 774 can include array
features that are to be detected by the detector 700.
The detector 700 includes an objective 701 that is configured to direct excitation
radiation from a radiation source 702 to the flow cell 770 and to direct emission from the flow
cell 770 to a detector 708. In the example layout, excitation radiation from the radiation source
702 passes through a lens 705 then though a beam splitter 706 and then through the objective on
its way to the flow cell 770. In the example shown, the radiation source 702 includes two light
emitting diodes (LEDs) 703 and 704, which produce radiation at different wavelengths from
each other. The emission radiation from the flow cell 770 is captured by the objective 701 and is
reflected by the beam splitter 706 through conditioning optics 707 and to the detector 708 (e.g., a
CMOS sensor). The beam splitter 706 functions to direct the emission radiation in a direction
that is orthogonal to the path of the excitation radiation. The position of the objective 701 can be
moved in the Z direction to alter focus of the microfluorometer. The detector 700 can be moved
back and forth in the Y direction to capture images of several areas of the inner surface 772 of
the upper layer 771 of the flow cell 770.
The inspection apparatus of Figures 1A-1C, 2A-2F, and 6A-6C may be located at
a predefined position within the flow cell 770. Optionally, the inspection apparatus may be
positioned at a predefined position adjacent to the flow cell 770 within a range of the objective
701. The objective 701 may be moved to the inspection apparatus before, during and/or after a
sequencing session, in connection with various types of tests.
Figure 8 shows an exploded view of an example microfluorometer for purposes of
demonstrating the functional arrangement for various optical components. Two excitation
sources are shown, including a green LED (LEDG) and a red LED (LEDR). Excitation
light/radiation from each passes through a green LED collector lens (L6) and red LED collector
lens (L7), respectively. An LED fold mirror (M1) reflects the green excitation radiation to a
combiner dichroic (F5) which reflects the green excitation radiation through an excitation filter
(F2), then through a laser diode beam splitter (F3), then through an excitation field stop (FS),
then through an excitation projection lens group (L2) to an excitation/emission dichroic (F4)
which reflects the green excitation radiation through a stationary objective lens group (L3) and a
translating objective lens group (L4) to the surface of a flow cell (FC). The red excitation
radiation passes from the red LED collector lens (L7) to the combiner dichroic (F5) after which
the red excitation radiation follows the same path as the green excitation radiation to the surface
of the flow cell (FC). As shown in Figure 8, focusing is actuated by moving the translating
objective lens group (L4) up and down (i.e., along the Z direction). Emission from the flow cell
(FC) surface passes back through the translating objective lens group (L4), and then through the
stationary objective lens group (L3) to the excitation/emission dichroic (F4) which passes the
emission radiation to the emission projection les group (L1) through to the emission filter (F1)
and then to the CMOS image sensor (S1). A laser diode (LD) is also directed via a laser diode
coupling lens group (L5) to the laser diode beam splitter (F3) which reflects the laser diode
radiation through the excitation field stop (FS), the excitation projection lens group (L2), the
excitation/emission dichroic (F4), the stationary objective lens group (L3) and the translating
objective lens group (L4) to the flow cell (FC).
The inspection apparatus of Figures 1A-1C, 2A-2F, and 6A-6C may be located at
a predefined position within the flow cell (FC). Optionally, the inspection apparatus may be
positioned at a predefined position adjacent to the flow cell (FC) within a range of the
microfluorometer. The microfluorometer may be moved to the inspection apparatus before,
during and/or after a sequencing session, in connection with various types of tests.
Figure 9 illustrates a block diagram for a detection apparatus that may utilize an
inspection apparatus in accordance with examples disclosed herein. A readout printed circuit
board (PCB) is present in a read head and is connected to a main PCB that is typically contained
within the detection apparatus housing. In alternative examples, the main PCB can be located
exterior to the instrument. Data can be communicated between the readout PCB and main PCB
via the LVDS line. The LVDS line can be configured to communicate image data from the
readout PCB to the main PCB, and instructions for camera control from the main PCB to the
readout PCB.
In the example of Figure 9, the main PCB is also connected to an exterior primary
analysis personal computer (PC) via USB 3.0 SS I/F connectors or other suitable connectors. In
some examples the primary analysis computer can be located within the housing of the detection
apparatus. However, placing the primary analysis computer off-instrument allows for
interchangeable use of a variety of computers to be used for different applications, convenient
maintenance of the primary analysis computer by replacement without having to interrupt the
activity of the detection apparatus and small footprint for the detection apparatus. Any of a
variety of computers, can be used including, for example, a desktop computer, laptop computer,
or server containing a processor in operational communication with accessible memory and
instructions for implementation of the computer implemented methods described herein. The
main PCB is also connected to a liquid crystal display (LCD) for communication to a human
user. Other user interfaces can be used as well.
In some examples, a user interface may include a display (e.g., an LCD) to
display or request information from a user and a user input device (e.g., a keyboard) to receive
user inputs. In some examples, the display and the user input device are the same device. For
example, the user interface may include a touch-sensitive display configured to detect the
presence of an individual's touch and also identify a location of the touch on the display.
However, other user input devices may be used, such as a mouse, touchpad, keyboard, keypad,
handheld scanner, voice-recognition system, motion-recognition system, and the like.
The readout PCB includes transmitters for transferring data from individual
sensors (i.e., detectors) to the LVDS line, 3.3 volt switching regulator, a 5 volt switching
regulator, and LED buck drives for the LED excitation radiation sources. The main PCB
includes an FPGA processor configured to accept image data from the LVDS. A DDR3 DIMM
frame buffer is electronically connected to the FPGA processor. The main PCB also includes a
thermal control regulator and control circuitry for various drive motors such as a Y-axis motor,
cartridge motor, valve motor, and pump motor.
The inspection apparatus of Figures 1A-1C, 2A-2F, and 6A-6C may be located at
a predefined position relative to the detection apparatus of Figure 9. The detection apparatus
may be moved to the inspection apparatus before, during and/or after a sequencing session, in
connection with various types of tests.
Any of a variety of characteristics of an image module can be evaluated using the
inspection apparatus described herein. Several examples are set forth below in the context of
testing a sequencer instrument with an inspection apparatus. It will be understood that similar
tests can be carried out for other analytical systems using a different inspection apparatus.
Furthermore, details of each test need not be necessary in all applications as will be evident to
those skilled in the art when applying the principles exemplified below to alternative analytical
systems and inspection apparatus.
Figure 10 illustrates an example of various measurements and tests that may be
performed utilizing an inspection apparatus formed in accordance with the examples disclosed
herein. In accordance with the examples herein, the method of Figure 10 aligns an objective of
an instrument with an optical target that includes a solid body that encloses a fluorescing
material. The method of Figure 10 directs excitation light onto the optical target, detects
fluorescence emission from the optical target as reference information and utilizes the reference
information in connection with at least one of optical alignment or calibration of the instrument.
Various types of reference information are discussed herein. Non-limiting examples of reference
information include the information recorded at each of the operations in Figure 10 (as discussed
hereafter).
While the operations of Figure 10 are described in an order, it is understood that
the operations may be performed in alternative orders. Also, it is understood that one or more of
the operations of Figure 10 may be omitted entirely. At 1002, one or more processors of the
instrument direct motors to adjust the tilt of the flow cell deck that holds the optical target and
sequencing flow cells to perform an auto tilt operation. During the auto tilt operation, the
instrument determines and records the final tilt motor coordinates. At 1004, the one or more
processors of the instrument direct motors to adjust the XY position of the flow cell deck to
perform an auto centering operation. During the auto centering operation, the instrument records
the XY stage position of fiducial(s) on the inspection apparatus. The positions of the fiducials
are used to monitor drift in the XY stage of the instrument and/or the flow cell deck position
when a flow cell is inserted into the instrument.
At 1006, the instrument obtains one or more frame-mode images of the laser lines
and adjusts the laser line XY positions accordingly. In connection therewith, the objective is
moved to a clear area upon the inspection instrument and adjusted to focus a predetermined
depth into the optical target (e.g., 100 µm below the surface of the optical target). Frame-mode
images are captured that include laser lines. The XY position of the laser lines is adjusted and
additional frame-mode images are captured. The process is repeated until achieving a desired
XY position for the laser lines.
At 1008, the instrument collects a time delay and integration (TDI) image of a
clear area on the inspection apparatus and adjusts a beam expander of the instrument to achieve
uniform illumination. For example, the TDI image may be obtained at a clear tile upon the
inspection apparatus with the objective focused a predetermined depth into the optical target.
The laser zoom beam expander may be adjusted until a select illumination uniformity is
obtained. At 1010, one or more processors of the instrument determine whether the illumination
uniformity and laser line position meet predetermined thresholds or specifications. When the
illumination uniformity and laser line position do not meet the threshold/specification, flow
returns to 1006 where the operations at 1006 and 1008 are repeated. Alternatively, when the
illumination uniformity and laser line position meets the thresholds/specifications, flow
continues to 1012. Following the operations at 1006 and 1008, the instrument records the final
positions of the laser XY pointing actuators and zoom beam expander actuators. The instrument
also records the final illumination uniformity, the laser line positions in the X and Y directions,
the laser line width and the camera rotation relative to the laser lines.
At 1012, the one or more processors of the instrument measure focus model
repeatability. In connection therewith, the objective is moved to an image quality tile on the
inspection apparatus, and the instrument obtains focus models and tests the autofocus position
repeatability. At 1012, the instrument records the autofocus spot position at the best focus Z
position, autofocus laser intensities, autofocus capture range, autofocus gain, autofocus stray
light and autofocus Z position repeatability.
At 1014, one or more processors of the instrument measure image quality and
optical alignment and save camera tilt offset calibrations. When an instrument auto tilts a
sequencing flow cell, the system adjusts certain tilt motors to set the flow cells imaging surfaces
parallel to the direction of travel of the X stage. The direction of travel for the XY stage is
intended to be perpendicular to the optical axis of the objective. However, slight variations may
occur. During manufacturing, the objective and camera may be tilted so that the imaging surface
is coplanar to the image of a properly de-tilted flow cell. However, adjustments may occur over
time and drift may be introduced. The inspection apparatus may be utilized to measure the
camera tilt. To do so, the one or more processors collect a through focus stack of images of a
pinhole array and analyze the images to determine the tilt of the chrome layer (microstructures)
relative to the camera tilt. The instrument measures the tilt of the chrome layer utilizing one or
both of autofocus spots and/or through focus stacks. An error is identified between the camera
tilt and the tilt of the chrome layer and corrected by measuring an angle of the chrome layer. By
way of example, the angle of the chrome layer may be measured by doing multiple through focus
stacks at different X coordinates and comparing the best-focus Z position at each X-coordinate.
Additionally or alternatively, the angle of the chrome layer may be measured by detecting the Z
position of the chrome layer at multiple X locations using an instrument autofocus system. The
camera tilt calibration may be performed at the beginning of each sequencing run, with the tilt
motors adjusted to compensate based on the results thereof.
When measuring image quality and optical alignment, the instrument positions
the objective over an image quality tile provided on the inspection apparatus. The image quality
tile is formed with an array of pinholes through chrome or another microstructure (e.g., 1 µm
pinholes on a 3 µm pitch hex pattern). The imaging system within the instrument collects a
series of images where the objective is adjusted in the Z position between one or more of the
images. As the objective is moved in the Z position between images, the pinholes come into and
go out of focus. The series of images with different objective positions are analyzed to identify
the image having a desired focus quality (e.g., best focus). For example, the system may
determine how tightly the pinholes focus between the series of stacked images, which affords an
indication of image quality (e.g., full width at half maximum). As another example, by
determining the Z position at which the pinholes come into best focus at various points across the
field of view, the system may evaluate axial chromatic shift between different emission colors
(e.g., red and green), field curvature, camera tilt and a usable depth of field. At 1014, the
instrument records image quality (FWHM), axial chromatism, field curvature and usable depth
of field. The instrument also records best focus Z position. The instrument also records camera
tilt relative to the X stage and tilt motor offsets to compensate for the camera tilt.
At 1016, one or more processors of the instrument perform a distortion correction
calibration by measuring distortion and saving distortion correction coefficients. When imaging
pattern flow cells, where each cluster is at a known location, it may be advantageous to
compensate for optical distortion in the imaging system in order that the instrument will know
where the clusters should appear within the image. The inspection apparatus may be utilized to
calibrate for distortion correction at the start of a sequencing run. To do so, the objective is
positioned over the distortion correction tile. The distortion correction tile includes pinholes
positioned with a predetermined position tolerance across the entire field of view (e.g., 10 nm),
thereby providing a pinhole array with a consistent predetermined pinhole spacing. The image is
analyzed to identify shifts between the positions of adjacent pinholes across the field of view.
The shift is then analyzed, such as by fitting a polynomial to the pinhole shift, where the
polynomial indicates where clusters should appear in subsequent images obtained during a
sequencing process. At 1016, the instrument records coefficients for distortion correction
polynomials, optical magnification, rotation of the flow cell deck and rotation of the Y stage.
At 1018, one or more processors of the instrument performs an autofocus laser
spot measurement for the position of one or more lasers in the Y direction. In connection with
checking the autofocus laser spot position, the objective is positioned at best focus over the
horizontal knife edge which exhibit sharp transitions between clear areas and chrome areas. The
autofocus laser spot is bright over chrome areas and very dim over clear areas. A TDI scan is
taken using the red and/or green cameras. The images are utilized to identify where the camera
fields of view for each emission band of interest are positioned relative to the horizontal knife
edge. The objective is then initially positioned over the chrome area and then slowly stepped
down in the Y direction until the laser spot disappears, which happens when the laser spot is no
longer directed onto a portion of the chrome and instead is entirely directed onto the clear area
proximate to the horizontal knife edge. The system may then identify an autofocus spot position
in the Y direction relative to the red and green camera’s field of view. At 1018, the instrument
records the autofocus laser spot position in the Y direction relative to fields of view for emission
bands of interest (e.g., relative to red and green fields of view).
At 1020, one or more processors of the instrument performs an autofocus laser
spot measurement for the position of one or more lasers in the X direction. In connection with
checking the autofocus laser spot position, the objective is positioned over the vertical knife edge
which exhibit sharp transitions between clear areas and chrome areas. The autofocus laser spot
is bright over chrome areas and very dim over clear areas. A TDI scan is taken using the red
and/or green cameras. The images are utilized to identify where the camera fields of view for
each emission band of interest are positioned relative to the vertical knife edge. The objective is
then initially positioned over the chrome area and then slowly stepped down in the X direction
until the laser spot disappears, which happens when the laser spot is no longer directed onto a
portion of the chrome and instead is entirely directed onto the clear area proximate to the vertical
knife edge. The system may then identify an autofocus spot position in the X direction relative
to the red and green camera’s field of view. At 1020, the instrument records the autofocus laser
spot position in the X direction relative to fields of view for emission bands of interest (e.g.,
relative to red and green fields of view).
At 1022, one or more processors of the instrument may perform a flat-field
correction calibration. In connection therewith, the instrument moves the objective to a clear tile
and focuses the objective a predetermined distance below the surface of the optical target, when
performing the flat-field correction calibration. The flat-field correction calibration includes
obtaining flat field correction images. The one or more processors calculates optical transmission
efficiency of the imaging system and saves flat-field correction coefficients in connection
therewith. Base calling operations during sequencing is based on intensity of clusters within
images. Intensity non-uniformities across a field of view can impact base calling. The
instrument would uniformly illuminate clusters within a flow cell to minimize errors, however, it
is not always practical to achieve perfectly uniform illumination. A gain and offset of the pixels
in the camera are calibrated during manufacturing, however the potential exists that the
calibration of camera pixels may change over time and/or with temperature. To perform flat-
field correction calibration, the objective is positioned over a clear area of the inspection
instrument and focused at a predetermined depth into the optical target (e.g., 100 µm). A
measurement is obtained to provide a uniformity baseline for image intensity. Thereafter, at the
start of one or more sequencing runs, the instrument may compensate for illumination non-
uniformity and camera pixels gain and offset changes by performing the flat-field correction
calibration.
The flat-field correction calibration includes obtaining images of the clear area of
the inspection apparatus focused to a predetermined depth within the optical target with the
lasers shutter closed (to produce a dark image) and with the lasers on at multiple laser powers to
get images at different counts of intensity (e.g., about 500, about 1000, about 1500, about 2000,
about 2500, about 3000, and about 3500 counts of intensity) in the images. By way of example,
and image may be about 1.4 mm long so that the impact of dust, fingerprints, etc. can be
averaged out by averaging all pixels in the scanning (Y) dimension. For each of the 3200 pixels
(in the non-scanning dimension of the camera), the instrument uses the dark reading and the
different intensity readings and fits a polynomial to the data to characterize the response of that
pixel (combination of how much light it is exposed to combined with the photo response of that
pixel of the camera). When taking images of clusters during sequencing, the instrument uses the
measured polynomial response of each pixel and adjusts the intensity of that pixel in the cluster
image to make the whole image equivalent to what would be obtained with perfectly uniform
illumination and perfectly uniform pixel gain and offsets. At 1022, the instrument records the
optical transmission efficiency and the flat-field correction polynomial coefficients for all or at
least a portion of the pixels in one or both of the X and Y directions.
At 1024, one or more processors of the instrument checks filter breakthrough and
background light. In connection therewith, the instrument moves the objective to a solid chrome
tile on the inspection apparatus and performs the filter breakthrough test. For example, a filter
breakthrough tile may be formed as a solid chrome region which appears as a mirror. The
instrument imaging system is designed to filter out all laser light from hitting the camera.
Therefore, when the objective is positioned over a filter breakthrough tile, the system would
expect to detect no light at the camera. When light is detected at the camera, the source may be
from various factors. For example, the optical filters may not properly filter out all of the laser
light. Additionally or alternatively, contaminants in the optical path may be excited by the laser
excitation light and fluoresce in the emission band of interest (e.g., red or green). When the
optical filter is not properly operating or contaminants exist in the optical path, both
circumstances may result in a high background level being detected by the camera. Various
corrective measures may be taken. At 1024, the instrument records the filter breakthrough
information, background light information and the like.
At 1026, the one or more processors measure the XY stage position repeatability.
In connection therewith, the instrument moves the objective to the auto centering fiducial and
performs an XY stage position repeatability test. The instrument moves the X and Y stage
multiple times from each direction to the auto centering fiducial and after each move it takes an
image of the auto centering fiducial. Ideally, the auto centering fiducial would show up at
exactly the same position in the image after every move. Movements of the fiducial in the image
indicate imperfect positioning of the XY stage. The instrument records the position repeatability
in the X and Y directions. The instrument also records the hysteresis exhibited in the X and Y
directions. At 1028, the one or more processors records all of the results collected in the
foregoing process at a remote diagnostics site. Thereafter, the instrument continues with a
sequencing operation.
In connection with the foregoing operations, the instrument may be directed to
perform remote diagnostics. By collecting and analyzing images of the inspection apparatus
periodically (e.g., at the start of every sequencing run), the instrument may monitor the
performance of the imaging system over time. Results can be stored on a local hard drive and/or
uploaded to a remote server or cloud server. The diagnostic information may be monitored to
monitor the health of the instrument’s imaging system and to identify trends in the instrument’s
performance over time. If any aspect of the imaging system is trending towards failure, repairs
may be scheduled before the instrument actually fails. This will increase customer up time.
Also, when questions arise as to whether an instrument is experiencing problems with the
imaging system, the alignment data may be collected to determine if any aspect of the image
system has changed. This will quickly eliminate the imaging system as potential root cause of
many issues or may point to a specific issue with the imaging system. If the instrument is not
uploading information to the cloud, a field service engineer will be able to trend the data over
time by reviewing the historical results stored on the local hard drive.
Further, fluorescent intensity is proportional to dopant concentration. By
controlling the dopant concentration (e.g., about 1.1% +/- 0.01%), the inspection apparatus can
control the measured fluorescence to a desired tolerance (e.g., +/- 0.6% in red and +/- 0.1% in
green). Measuring intensity of the inspection apparatus at a certain scan speed and laser power
on one instrument will provide measurement information indicative of an intensity to expect on
substantially all similar instruments. The fluorescent intensity measurement from the inspection
apparatus can be utilized to indicate whether the instrument is behaving properly (e.g., providing
proper laser power delivered to the flow cell, proper amount of fluorescent light collected and
delivered to the camera, etc.). Given that the emission characteristics of the inspection apparatus
will not change over time, any change in measured fluorescent intensity over the life of the
instrument will indicate that either the proper laser power is not being delivered to the flow cell
or not all the fluorescent light is being delivered to the camera.
It is recognized that the above operations are non-limiting examples of various
operations that may be performed utilizing an inspection apparatus. The above discussed
operations maybe performed entirely independent of one another and at different points in time.
A non-limiting example of remote diagnostics and metrics that may be performed automatically
utilizing an inspection apparatus include: Optical transmission efficiency, Image quality (Full-
Width-Half-Maximum), Camera tilt, Axial chromatism, Field curvature, Usable depth of field,
Distortion, Magnification, Laser line XY positions and line widths, Illumination uniformity,
Camera rotation relative to laser lines, Flat field correction coefficients Autofocus Z position
repeatability, Autofocus spot position at best focus, Autofocus spot position relative to red and
green field of view, Autofocus laser intensity, Autofocus capture range, Autofocus gain,
Autofocus stray light, Best-focus Z position , Autotilt motor coordinates after autotilt, Hysteresis
in X and Y, Position repeatability in X and Y, Rotation of the flow cell deck, Y stage direction of
travel, XY stage position of BIRD fiducial, Positions of the laser pointing actuators, and
Positions of the laser zoom beam expander actuators.
In accordance with examples herein, an inspection method may include a routine
for setting excitation source currents for proper image intensity. The routine can include
sequential steps of positioning the inspection apparatus in an imaging module such that an open
area of the channel (i.e., with no microstructures) is detected, setting the camera exposure to 1
ms and LED currents to 30%, capturing a dark image with 1 ms exposure and no LEDs on,
capturing an image in red and green optical channels with 1 ms exposure, calculating mean
intensity of the images, and adjusting LED currents to hit a desired intensity of 2500 counts with
1 ms exposure. LED currents are kept at these values for the remainder of the tests. All
subsequent tests can use different exposure times based on the geometry of the microstructure
pattern. For example, fiducial tiles and uniformity tiles (lacking microstructures) can be detected
with a 1 ms exposure, autofocus tiles can be detected with a 4 ms exposure, image quality tiles
can be detected with a 150 ms exposure, and filter breakthrough tiles (fully coated with metal on
the interior surface of the upper glass) can be detected with a 500 ms exposure.
In accordance with examples herein, an inspection method can include a routine
for excitation source calibration. The routine can be carried out as follows. The XY stage of an
instrument is moved to an autofocus tile. A through-focus stack is generated in red and a best-
focus Z height is calculated (e.g., step size is 6 µm, exposure time is 4 ms and sweep range is
108 µm). Then the XY stage is moved to a neighboring tile to collect laser images. This is done
to mitigate the risk of a manufacturing defect in the inspection apparatus where not all the
chrome is removed from inside the 500 micron square opening in the autofocus tile. This defect
would make the laser spot intensity too bright at the autofocus tile. The process then collects
laser through-focus images (using standard settings for focus model generation) and the laser
spot intensity is checked. The step size during these measurements is 2 microns with a Z range
that is +/-18 microns. Then the laser exposure time is adjusted until the AF spots are 2000+/-200
counts for "brightest spot" (within +/-18 microns of red best focus). If "save calibrations" is
selected on the user interface, then the laser exposure time to use for sequencing is stored.
In accordance with examples herein, a method may include a detector calibration
test. As one example, the test can be carried out as follows. Images of an inspection apparatus
are obtained at 4 different LED intensities: (1) Dark (LEDs off), (2) Middle low intensity, (3)
Middle high intensity, and (4) Bright intensity (about 3000 counts). When taking these images,
the XY stage is moved between each image. All tiles in select lanes are used to average out any
non-uniform fluorescence (due to debris or fingerprints on top of the inspection). Camera
corrections need not be applied to any subsequent tests that were selected.
Closing Statements
It will be appreciated that various aspects of the present disclosure may be
embodied as a method, system, computer readable medium, and/or computer program product.
Aspects of the present disclosure may take the form of hardware examples, software examples
(including firmware, resident software, micro-code, etc.), or examples combining software and
hardware aspects that may all generally be referred to herein as a “circuit,” “module,” or
“system.” Furthermore, the methods of the present disclosure may take the form of a computer
program product on a computer-usable storage medium having computer-usable program code
embodied in the medium.
Any suitable computer useable medium may be utilized for software aspects of
the present disclosure. The computer-usable or computer-readable medium may be, for example
but not limited to, an electronic, magnetic, optical, electromagnetic, infrared, or semiconductor
system, apparatus, device, or propagation medium. The computer readable medium may include
transitory examples. More specific examples (a non-exhaustive list) of the computer-readable
medium would include some or all of the following: an electrical connection having one or more
wires, a portable computer diskette, a hard disk, a random access memory (RAM), a read-only
memory (ROM), an erasable programmable read-only memory (EPROM or Flash memory), an
optical fiber, a portable compact disc read-only memory (CD-ROM), an optical storage device, a
transmission medium such as those supporting the Internet or an intranet, or a magnetic storage
device. Note that the computer-usable or computer-readable medium could even be paper or
another suitable medium upon which the program is printed, as the program can be electronically
captured, via, for instance, optical scanning of the paper or other medium, then compiled,
interpreted, or otherwise processed in a suitable manner, if necessary, and then stored in a
computer memory. In the context of this document, a computer-usable or computer-readable
medium may be any medium that can contain, store, communicate, propagate, or transport the
program for use by or in connection with the instruction execution system, apparatus, or device.
Program code for carrying out operations of the methods and apparatus set forth
herein may be written in an object oriented programming language such as Java, Smalltalk, C++
or the like. However, the program code for carrying out operations of the methods and apparatus
set forth herein may also be written in conventional procedural programming languages, such as
the “C” programming language or similar programming languages. The program code may be
executed by a processor, application specific integrated circuit (ASIC), or other component that
executes the program code. The program code may be simply referred to as a software
application that is stored in memory (such as the computer readable medium discussed above).
The program code may cause the processor (or any processor-controlled device) to produce a
graphical user interface (“GUI”). The graphical user interface may be visually produced on a
display device, yet the graphical user interface may also have audible features. The program
code, however, may operate in any processor-controlled device, such as a computer, server,
personal digital assistant, phone, television, or any processor-controlled device utilizing the
processor and/or a digital signal processor.
The program code may be locally and/or remotely executed. The program code,
for example, may be entirely or partially stored in local memory of the processor-controlled
device. The program code, however, may also be at least partially remotely stored, accessed, and
downloaded to the processor-controlled device. A user’s computer, for example, may entirely
execute the program code or only partly execute the program code. The program code may be a
stand-alone software package that is at least partly on the user’s computer and/or partly executed
on a remote computer or entirely on a remote computer or server. In the latter scenario, the
remote computer may be connected to the user’s computer through a communications network.
The methods and apparatus set forth herein may be applied regardless of
networking environment. The communications network may be a cable network operating in the
radio-frequency domain and/or the Internet Protocol (IP) domain. The communications network,
however, may also include a distributed computing network, such as the Internet (sometimes
alternatively known as the “World Wide Web”), an intranet, a local-area network (LAN), and/or
a wide-area network (WAN). The communications network may include coaxial cables, copper
wires, fiber optic lines, and/or hybrid-coaxial lines. The communications network may even
include wireless portions utilizing any portion of the electromagnetic spectrum and any signaling
standard (such as the IEEE 802 family of standards, GSM/CDMA/TDMA or any cellular
standard, and/or the ISM band). The communications network may even include powerline
portions, in which signals are communicated via electrical wiring. The methods and apparatus
set forth herein may be applied to any wireless/wireline communications network, regardless of
physical componentry, physical configuration, or communications standard(s).
Certain aspects of present disclosure are described with reference to various
methods and method steps. It will be understood that each method step can be implemented by
the program code and/or by machine instructions. The program code and/or the machine
instructions may create means for implementing the functions/acts specified in the methods.
The program code may also be stored in a computer-readable memory that can
direct the processor, computer, or other programmable data processing apparatus to function in a
particular manner, such that the program code stored in the computer-readable memory produce
or transform an article of manufacture including instruction means which implement various
aspects of the method steps.
The program code may also be loaded onto a computer or other programmable
data processing apparatus to cause a series of operational steps to be performed to produce a
processor/computer implemented process such that the program code provides steps for
implementing various functions/acts specified in the methods of the present disclosure.
The terms “substantially” and “about” used throughout this disclosure, including
the claims, are used to describe and account for small fluctuations, such as due to variations in
processing. For example, they can refer to less than or equal to ±5%, such as less than or equal
to ±2%, such as less than or equal to ±1%, such as less than or equal to ±0.5%, such as less than
or equal to ±0.2%, such as less than or equal to ±0.1%, such as less than or equal to ±0.05%.
The terms “comprise,” “include,” “contain,” etc., and variations thereof, that are
used in the specification and claims herein are intended to be open-ended, including not only the
recited elements, but further encompassing any additional elements. Reference throughout the
specification to “one example”, “another example”, “an example”, and so forth, means that a
particular element (e.g., feature, structure, and/or characteristic) described in connection with the
example is included in at least one example described herein, and may or may not be present in
other examples. In addition, it is to be understood that the described elements for any example
may be combined in any suitable manner in the various examples unless the context clearly
dictates otherwise.
It should be appreciated that all combinations of the foregoing concepts and
additional concepts discussed in greater detail below (provided such concepts are not mutually
inconsistent) are contemplated as being part of the inventive subject matter disclosed herein. In
particular, all combinations of claimed subject matter appearing at the end of this disclosure are
contemplated as being part of the inventive subject matter disclosed herein. It should also be
appreciated that terminology explicitly employed herein that also may appear in any disclosure
incorporated by reference should be accorded a meaning most consistent with the particular
concepts disclosed herein.
It is to be understood that the ranges provided herein include the stated range and
any value or sub-range within the stated range. For example, a range represented by equals or is
between four and ten (4 to 10), should be interpreted to include not only the explicitly recited
limits of from 4 to 10, but also to include individual values, such as about 6, 7.5, 9, etc., and sub-
ranges, such as from about 5 to about 8, etc.
While several examples have been described in detail, it is to be understood that
the disclosed examples may be modified. Therefore, the foregoing description is to be
considered non-limiting.
Claims (9)
1. An inspection apparatus, comprising: an optical target including a solid host material and a fluorescing material embedded in the solid host material, the solid host material having a predetermined phonon energy HOST ; a body having a pocket to receive the optical target, wherein the body includes an inset region located at a top surface and surrounding the pocket; and a transparent layer mounted in the inset region and positioned above the optical target; wherein the body includes a channel at least partially surrounding the pocket, the channel to receive an adhesive to bond to a grating layer, wherein the channel includes a series of pressure relief pockets distributed about the channel, the pressure relief pockets to relieve stress induced onto the grating layer by the adhesive during a curing process; wherein the fluorescing material exhibits a select ground energy level and a target excitation (TE) energy level separated from the ground energy level by a first energy gap corresponding to a fluorescence emission wavelength of interest (FEWI), the fluorescing material having a next lower lying (NLL) energy level relative to the TE energy level, the NLL energy level spaced a second energy gap FM below the TE energy level wherein a ratio of the FM /HOST is three or more. EG2 PE
2. The apparatus of claim 1, wherein the ratio of the FM /HOST equals or is EG2 PE between four and ten.
3. The apparatus of claim 1, wherein the solid host material includes at least one of glass, amorphous polymers, crystalline materials, semi-crystalline polymers, metallic glass, or ceramic.
4. The apparatus of claim 1, wherein the fluorescing material represents an ion of at least one of a rare-earth element or a transition metal element.
5. The apparatus of claim 1, wherein the solid host material has a maximum phonon energy less than or equal to 580 cm .
6. The apparatus of claim 1, wherein the fluorescence emission wavelength of interest has a center wavelength at or below about 1000nm.
7. The apparatus of claim 1, wherein the body further includes a diffusion well located below the pocket, the diffusion well to receive excitation light passing through the optical target, the diffusion well including a well bottom having a surface finish that exhibits a reflectively of no more than about 20.0%.
8. The apparatus of claim 1, further comprising microstructures formed on a surface of at least one of the transparent layer or the optical target to form the grating layer.
9. The apparatus of claim 1, further comprising an anti-reflective coating formed on a surface of at least one of the transparent layer or the optical target.
Priority Applications (1)
| Application Number | Priority Date | Filing Date | Title |
|---|---|---|---|
| NZ767004A NZ767004B2 (en) | 2017-12-11 | Solid Inspection Apparatus and Method of Use |
Applications Claiming Priority (3)
| Application Number | Priority Date | Filing Date | Title |
|---|---|---|---|
| US201762443675P | 2017-01-07 | 2017-01-07 | |
| US62/443,675 | 2017-01-07 | ||
| PCT/US2017/065606 WO2018128753A1 (en) | 2017-01-07 | 2017-12-11 | Solid inspection apparatus and method of use |
Publications (2)
| Publication Number | Publication Date |
|---|---|
| NZ747901A NZ747901A (en) | 2021-02-26 |
| NZ747901B2 true NZ747901B2 (en) | 2021-05-27 |
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