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IE61705B1 - Aerosol beam microinjector - Google Patents

Aerosol beam microinjector

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Publication number
IE61705B1
IE61705B1 IE250490A IE250490A IE61705B1 IE 61705 B1 IE61705 B1 IE 61705B1 IE 250490 A IE250490 A IE 250490A IE 250490 A IE250490 A IE 250490A IE 61705 B1 IE61705 B1 IE 61705B1
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particles
aerosol
cell
housing
conduit
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IE250490A
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IE902504A1 (en
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Laurens J Mets
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Biotechnology Res & Dev
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    • CCHEMISTRY; METALLURGY
    • C12BIOCHEMISTRY; BEER; SPIRITS; WINE; VINEGAR; MICROBIOLOGY; ENZYMOLOGY; MUTATION OR GENETIC ENGINEERING
    • C12NMICROORGANISMS OR ENZYMES; COMPOSITIONS THEREOF; PROPAGATING, PRESERVING, OR MAINTAINING MICROORGANISMS; MUTATION OR GENETIC ENGINEERING; CULTURE MEDIA
    • C12N15/00Mutation or genetic engineering; DNA or RNA concerning genetic engineering, vectors, e.g. plasmids, or their isolation, preparation or purification; Use of hosts therefor
    • C12N15/09Recombinant DNA-technology
    • C12N15/87Introduction of foreign genetic material using processes not otherwise provided for, e.g. co-transformation
    • CCHEMISTRY; METALLURGY
    • C12BIOCHEMISTRY; BEER; SPIRITS; WINE; VINEGAR; MICROBIOLOGY; ENZYMOLOGY; MUTATION OR GENETIC ENGINEERING
    • C12MAPPARATUS FOR ENZYMOLOGY OR MICROBIOLOGY; APPARATUS FOR CULTURING MICROORGANISMS FOR PRODUCING BIOMASS, FOR GROWING CELLS OR FOR OBTAINING FERMENTATION OR METABOLIC PRODUCTS, i.e. BIOREACTORS OR FERMENTERS
    • C12M35/00Means for application of stress for stimulating the growth of microorganisms or the generation of fermentation or metabolic products; Means for electroporation or cell fusion
    • CCHEMISTRY; METALLURGY
    • C12BIOCHEMISTRY; BEER; SPIRITS; WINE; VINEGAR; MICROBIOLOGY; ENZYMOLOGY; MUTATION OR GENETIC ENGINEERING
    • C12MAPPARATUS FOR ENZYMOLOGY OR MICROBIOLOGY; APPARATUS FOR CULTURING MICROORGANISMS FOR PRODUCING BIOMASS, FOR GROWING CELLS OR FOR OBTAINING FERMENTATION OR METABOLIC PRODUCTS, i.e. BIOREACTORS OR FERMENTERS
    • C12M35/00Means for application of stress for stimulating the growth of microorganisms or the generation of fermentation or metabolic products; Means for electroporation or cell fusion
    • C12M35/04Mechanical means, e.g. sonic waves, stretching forces, pressure or shear stimuli

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Abstract

The present invention uses aerosol beam technology to accelerate either wet or dry aerosol particles to speeds enabling the particles to penetrate living cells. Aerosol particles suspended in an inert gas are accelerated to a very high velocity during the jet expansion of the gas as it passes from a region of higher gas pressure to a region of lower gas pressure through a small orifice. The accelerated particles are positioned to impact a preferred target, for example, a plant or animal cell or bacterial culture. When the droplets include DNA or other macromolecules, the macromolecules are introduced into the cells. The particles are constructed as droplets of a sufficiently small size so that the cells survive the penetration. Once introduced into the target cell the macromolecules can elicit biological effects. Because the method of introduction is a physical one, the biological barriers that restrict the application of other DNA transfer methods to a few plant species and a few cell types are not present. In addition, the method and apparatus of the present invention permit the treatment of a large number of cells in the course of any single treatment. Thus, the inventive method and apparatus should be applicable to a wide range of plant species and cell types that have proved in the past to be quite impervious to standard methods of genetic engineering.

Description

AEROSOL BEAM MICROINJECTOR The present invention relates to the introduction of exogenous material into a living cell, tissue, or species, and more particularly, to apparatus and methods for microinjecting exogenous materials into a living cell, tissue, or species.
The genetic transformation of cells using the techniques of genetic engineering has grown dramatically over the last few years. Generally, genetic engineering involves the introduction of foreign DNA into a host cell to change or ”transform” the host cell. When successfully done, the genes carried by the foreign DNA are expressed in the host cell, and thus, the last cell is transformed.
Genetically transformed cells, tissues, or species are of great commercial value in research, agriculture, and medicine. For example, human insulin is presently being produced by bacteria which have been genetically engineered. Human insulin is now available in commercial quantities, and has benefitted millions of diabetics throughout the world. In addition, several plant species have been genetically engineered to produce more crop, become more resistant to disease, and grow in less hospitable climates and soils.
Because of the commercial and social importance of genetic engineering, a plurality of methods for transferring foreign genes into a recipient call have been -2developed for both procaryotic and eucaryotic calls, These gene transfer techniques are routinely used in laboratories throughout the world to genetically transform living cells, tissues and species. However# despite the existence of these diverse transformation techniques# the effective stable transfer* of genes remains an obstacle in many fields of research. One technique for gene transfer is cell fusion. Cell fusion has been applied to both animal and plant cell cultures. Cell fusion techniques integrate the genetic information of two different cells in one. In plant cell cultures# cell walls are dissolved and the naked protoplasts are fused together# forming a new cell. The descendants of the new fused cell express certain characteristics of both the original (parent) cells. However, researchers have no means of predicting what characteristics will be expressed in the progeny. Thus# the results obtained using cell fusion techniques are unpredictable and are generally not reproducible.
In animal cell cultures, hybridomas are the cell fusion product of antibody-secreting cells and ”immortal” cells (myelomas). Hybridomas are used in medicine and research to produce monoclonal antibodies. Hybridomas# like the plant cell fusion products# may react unpredictably, and are expensive to produce and maintain.
Electroporation is another general method for introducing foreign DNA into cells. This procedure involves the exposure of a suspension of cells and fragments of foreign DNA to a pulsed high-voltage electrical discharge. This electrical discharge creates holes or pores in the cell membrane through which DNA fragments diffuse. Upon cessation of the electrical discharge# the pores in the cell membrane close# capturing any DNA fragments which have diffused into the cell.
However# a major drawback in using electroporation to -3introduce DNA into living cells is the necessity prior to a successful transformation, to determine empirically optimum values for a wide variety of parameters for each cell line in question. These parameters include voltage, capacitance, pulse time composition and resistance of electroporation medium, state of cell growth prior to electroporation, concentration of DNA# temperature, and cell density. Also, present methods for applying electroporation to cells with walls, such as plant cells, require removing the walls prior to electroporation.
These protoplasts must then regenerate their walls before they can divide and be regenerated into intact plants. Since not many plants can yet be regenerated from protoplasts, this requirement limits applicability of electroporation.
Viral infection is also an efficient means of transferring foreign DNA into some cells. However, viruses are difficult to work with, and since a particular virus will only infect certain cells, the technique is not applicable to the broad spectrum of living cells, tissue, or species. Further, some virus may in fact be hazardous to the technicians working with them or to the environment.
The most common and effective method for transferring genes into plant cells involves conjugal transfer from living bacteria, primarily Agrobacterium tumefacient and Agrobacterium rhizogenes. The DNA to be transferred is first engineered into plasmids derived from the bacterial Ti plasmid, and the bacteria are then incubated in culture with the recipient plant cells. The cultured, transformed cells must then be regenerated into genetically homogeneous plants. This method is limited to plants susceptible to Agrobacterium infection (principally dicots) that can be regenerated from cultures. 4Still another technique for gene transfer is micropipette microinjection. In micropipette microinjection» DNA or other exogenous materials, are stably introduced into a living cell by microinjecting the material directing into the nuclei of the cell.
Typically, a glass micropipette having a diameter of from about 0.1 to about o. 5 microns is inserted, directly into the nucleus of the cell. Through the bore of the micropipette exogenous material, such as DNA, is injected. An experienced,, skilled technician can inject from about 500 to about 1000 cells per hour. Presently, however, micropipette microinjection requires some fairly sophisticated and expensive equipment, such as, a micropipette puller for making the needles, and a micromanipulator to position th© needles correctly for injection. Moreover, extensive practice and training is needed for a technician to master this tedious technique» Micropipette microinjection is an effective method of gene transfer, however, because of the relatively small number of cells that may be transformed in any one experiment, the cost of the elaborate equipment necessary, and the level of skill needed to perform the procedure, microinjection using micropipettes is not a method of gene transfer available to th© vast majority of researchers in the field.
Although a number of gene transfer techniques are available; presently, no prior technique provides a safe, fast, effective, inexpensive, and reproducible method for genetically transforming a broad spectrum of living material regardless of cell, tissue or species type. Present methods are either expensive, slow, or yield, results which are not reproducible. Moreover, some methods, such as the use of infectious agents, may even be hazardous to the researcher or the environment. -5» Accordingly, a new apparatus and method for transforming cells, tissue, or species is needed.
Advantages of the invention will become apparent upon reading the following detailed description and upon reference to the drawings in which: FIG. 1 is a schematic illustration of the aerosol beam microinjector; Fig. 2 is a schematic illustration of an aerosol beam microinjector including a drying tube and means for providing sheath flow; and Fig. 3 is a schematic illustration of an aerosol beam microinjector additionally including means for adjusting the diameter of the injected droplet.
The present invention is directed to an apparatus and methods for the introduction of exogenous materials, for example foreign DNA, into a variety of recipient cells.
It is believed that the present invention should have a profound effect upon the variety of plants, and animals, that will become amenable to direct genetic manipulation.
The present invention uses aerosol beam technology to accelerate either wet or dry aerosol particles to speeds enabling the particles to penetrate living cells upon impact therewith. Aerosol particles suspended in a inert gas can be accelerated to a very high velocity during the jet expansion of the gas as it passes from a region of higher gas pressure to a region of lover gas pressure through a small orifice. This acceleration process has been well-studied and used for many years in the field of aerosol physics. The accelerated droplets may be positioned to impact a preferred target, for example, a -δplant or animal cell. When the particles include DNA or other macromolecules, the macromolecules are introduced into the cells. The droplets may be constructed as droplets of a sufficiently small size so that th® cells survive the penetration. Once introduced into the target cell the macromolecules can elicit biological effects.
This effect will depend on th© specific properties of tha macromolecules and the nature of the recipient cells. For example,, DNA may be introduced into the target cell, thereby altering the genetic make-up ox the cell. Because the method of introduction is a physical one, the biological barriers that restx’ict the application of other DNA transfer methods to a few plant species and a few cell types are not present. The size, kinetic energy and beam intensity of the aerosol stream can be precisely controlled over a wide range,, and hence may be successful in penetrating and transforming a wide variety of cell types. In addition, the use of a continuous aerosol beam will permit the treatment of a large number of cells in the course of any single treatment. Thus, the inventive method should be applicable to a wide range of plant species and cell types that have proved in the past to be quite impervious to standard methods of genetic engineering. According to a preferred embodiment, the apparatus and methods of the present invention are utilized to produce a transformed line of plants. Aerosol particles comprising exogenous genetic material are produced and accelerated to a speed enabling them to penetrate and enter into a living plant cell upon impact therewith. The cells are thereafter cultured to grow a plant. The progeny of the plant are subsequently screened using techniques well known to one skilled in the art of plant genetics, for transformed progeny.
According to a preferred embodiment, the apparatus and methods of the present invention are utilised to -7produce transformed maize plants. Cells from an embryogenic culture of an alcohol dehydrogenese-deficient (adh) recipient plant are preferably plated on an agar surface of osmotically supportive medium. They would then be placed in ths chamber on the target positioning device for treatment with aerosol carrying a mild type shd gene on a plasmid. The apparatus shown in FIG. 3 is preferably used. The DNA plasmid would b® adjusted to 3mMMyCl., and rapidly mixed with 3.00% ethanol to yield 95% final ethanol concentration. The concentration of DNA would be such that each droplet of primary aerosol generated in the nebulizer contains an average of 2-3 plasmid molecules (about 1013 molecule per ml of final ethanol solutions). The primary aerosol, generated in the nebulizer would then be dried and the ethanol vapor trapped in the diffusion dryer. The DNA aerosol stream would be humidified with 5xl0”lw g water vapor per primary aerosol particles, and the mixture cooled to 0°c. to generate a 0.5 - 1.0 mm diameter uniform size aerosol droplets. These would be accelerated by the expansion of the N2 inert gas through a 250 mm orifice to strike the target cells 1.5 cm away from the orifice. The injected cells would then be cultured and tested by cytological staining for the presence of adh activity in the cells. An appropriate number of cells would be grown into plants and for the tested for the presence of the transforming DNA and for function of the adh gene.
A further preferred embodiment of the present invention utilizes the apparatus and methods of the present invention genetic transformation of maize pollen. Pollen from a recipient variety deficient in adh would be plated on osmotically supportive agar medium and placed in the device shown in FIG. 3. Transforming DNA would be formed into a primary aerosol of 95% ethanol as described for embryogenic cell transformation, and then dried as set forth, above. In this case, th® aerosol stream would be humidified with perfluorocarbon vapor (3H or Air Products) at a density of 8xl0“12 g per primary aerosol droplet. Condensation at 0°C would then generate 2 micron uniform diameter droplets. These would be accelerated with the inert gas expansion to impact the pollen grains. After 1 hr recovery period, the pollen would be transferred to silks of adh deficient corn plants. The seeds obtained would be planted and transformed plants recognized by the presence of adh-stainable pollen in samples from the mature plants.
Aerosol particles are formed by aerosolizing solutions containing the macromolecule., Preferably, excess solvent is subsequently evaporated from the aerosol particles to reduce projectile size, thus increasing the rate of survival in the impacted target cells. When the aerosol particles are constructed as droplets the density of the final droplets is important, since less dense droplets may cause less damage to some target cells when they penetrate, while, on the other hand, more dense droplets may be required to penetrate certain target cells. Accordingly, the present invention provides means to modify both the size and density of the droplets as required for penetrating different cells. According to one preferred embodiment, the density of the droplets is from about 0.8 to about 8 gram/cc, and most preferably about 2 grams/cc. The density is modified by the addition of solutes, for example colloidal gold, to the solution prior to forming an aerosol or by using solvents, such as perfluorocarbons, that have different densities. Further, the apparatus of the present invention may be modified to include means for removing excess solvent, thus reducing droplet size, or adding additional solvent to the droplet, thus increasing the size of the droplet. -9Figs. 1, 2 and 3, illustrate several embodiments of an aerosol beam microinjector of the present invention. Each Fig. will be discussed in detail when appropriate, otherwise the following discussion is applicable to each FIG. Compressed inert gas is filtered as it passes through a tubing 1 into the inlet 3 of a nebulizer 5 disbursing aerosol particles (a suspension of solvent and solute) into the inert gas to form an aerosol. The source of the compressed gas 6 preferably provides a gas pressure of from about 10 to about 100 psi at the inlet 3.
However, the compressed gas most preferably provides about 30 psi at the inlet 3. Preferably, the projectiles (droplets of solvent and suspended particulate matter) have mass mean diameters of from about 0.l to about 2 microns. The present inventor has determined that projectiles having diameters outside of this range are not preferable in the practice of the present invention. Projectiles having a diameter of greater than about 2 microns were found to cause an unacceptable level of cell death following impact, while projectiles having a diameter of below about 0.1 microns were unable to efficiently penetrate into the target cell.
Th© aerosol exits the nebulizer 5 through an outlet 7. The present inventor has determined that it is preferable to dissipate the pressure of the compressed gas prior to the acceleration of the aerosol. This is accomplished, in one preferred embodiment, by venting the aerosol to the outside atmosphere. As shown in Fig. 1, 2, and 3, the outlet 7 and the inlet 9 of tubing XI do not abut each other, but are rather, positioned in a close proximity to each other. This arrangement allows the pressure of the compressed gas to dissipate, while further allowing the aerosol to enter inlet 9 of tubing 11. According to a further preferred embodiment not shown in the FIGS, the aerosol is discharged from the outlet 7 into “10a non-restrictive enclosure# such as a non-reactive plastic bag. Once the gas pressure from the compressed gas has bean alleviated# a portion of the aerosol is drawn into the inlet 9 of a tubing ll. The aerosol is drawn into th® tubing XI by a negative or low gas pressure (a gas pressure below that of the surrounding atmosphere). This negative pressure is preferably about 1 atmosphere and is created within the tubing ll by a high-volume vacuum pump 13 in communication with an air-tight vacuum housing 15 which is functionally connected to the outlet 16 of the tubing 11. If the aerosol is being discharged into the atmosphere# the inlet 9 of the tubing 11 is preferably positioned in a relatively close proximity fco the nebulizer outlet 7. Preferably# this distance is about one-half inch.
Referring specifically to Fig. 1# Fig. 1 shows the tubing 11 entering the housing 15. Fig- 1 shows the tubing outlet 16 including a nozzle 17 through which the inert gas and the aerosol eventually passes through to reach the vacuum housing 15» Returning# generally# to Figs. 1# 2# and 3# the pressure within the tubing 11 and correspondingly within the vacuum housing 15 may be regulated by the pumping speed of tha pump 13, the flow resistance caused by the nozzle 17# or the evaporation of solvent from samples within the vacuum housing 15. The aerosol is drawn through the length of tubing 11 to the nozzle 17» The nozzle 17 preferably has an aperture diameter of from 100 to 300 microns. The present inventor has determined that the most preferred aperture diameter of nozzle 17 is about 200 microns. The aerosol is thereafter drawn through nozzle 17 and into the vacuum housing 15» “11“ The passage of the aerosol from the relatively high gas pressure area within tubing XI into the relatively low gas pressure area within the vacuum housing 15 causes the inert gas to dramatically expand. The rapid expansion of the inert gas through the nossis 17 causes the aerosol particles to accelerate. For example, when nitrogen is used as the inert gas, it has been determined that the aerosol particles can be accelerated up to speeds of from about 400 to about 800 meters/second. Further, if helium is used as tha inert gas, the aerosol particles may be accelerated up to speeds of about 2000 meters/second. The vacuum housing 15 is continuously evacuated by the pump 13 to remove the inert gas and keep the pressure in the housing below tha gas pressure in the tubing 11» According to one preferred embodiment, the gas pressure in housing 15 is from about 0.01 to ©bout 0.05 atmospheres, and most preferably about 0.01 atmospheres.
When the inert gas is expanded and the aerosol Is accelerated, an aerosol beam is generated. In the vacuum housing 15 the inert gas portion of the aerosol is expanded and removed and accelerated aerosol particles follow straight line trajectories. Aerosol beams are thus composed of accelerated isolated particles and droplets (hereinafter referred to as simply projectiles) moving on well defined, straight line trajectories at speeds up to 2000 meters/seconds.
Referring now to Fig. 2, Fig. 2 illustrates an aerosol beam microinjector including means for manipulating the size of th® projectiles, and means for focusing the aerosol flow through the nozzle 17. As the aerosol is drawn through tubing 11 it is drawn into a drying tube 23. Drying tube 23 contains a desiccant which traps solvent evaporated from the surface of the solute, thus decreasing the diameter of the projectile. The flow rate of the aerosol, the length of the drying tube, the solvent used, and the desiccant contained in the drying tube, may all be modified to remove varying amounts of solvent from the aerosol. According to one preferred embodiment, the drying tube 23 has an internal diameter of about one-half inch and an effective length of about 60 cm. The drying tube 23 contains silica gel as a desiccant. The silica gel surrounds a central channel formed by a cylinder of 20 mesh stainless steel screen.
Commercial drying tubes similar to the drying tube described above and useful in the practice of the present invention are available from TSI, Inc., Model 3062 Diffusion Dryer.
Once treated, the aerosol continues through tubing 11. The aerosol is discharged from outlet 7 of tubing 11 and into the precise center of a laminar flow of dry, filtered inert gas. The aerosol is thus entrained in the center of a gas stream moving up to and through the nozzle 17. This is preferable because it increases the average velocity of the projectiles, focuses the aerosol beam, and prevents nozzle clogging. When a gas flows through a nozzle 17, the velocity profile is never constant over the entire cross section. The particles nearest the nozzle wall will have velocities substantially less than particles traveling in the center of the beam. Further, th© radial expansion of the carrier gas will cause the aerosol beam to expand radially outward. Particles near the beam center are not influenced by this radial expansion but particles at increasing radii obtain an increasing radial velocity component. Accordingly, Fig. 2 illustrates an aerosol beam microinjector which includes means for reducing the radial expansion of the aerosol beam and maintaining a substantially uniform velocity through the cross section of the beam. 13~ Fig. 2 shows a piping 19 drawing filtered inert gas into its length and transporting that gas to the inlet 21 of th® sheath flow piping 24. The inert gas, which accounts for the sheath flow, enters the piping 19 with no positive pressure and is drawn from a non-restrictive reservoir of inert gas or from the outside atmosphere when the inert gas is released from a source 26 in the immediate area of the inlet 25 of piping 19, as shown in Fig. 2» The aerosol is discharged from tubing 11 into the center of the sheath flow piping 24. The aerosol is entrained in the laminar flow of the inert gas in the sheath flow piping 24. The laminar flow focuses the aerosol through the center of the nozzle 17, thus allowing the aerosol to maintain a substantially uniform velocity across its cross section. The laminar flow also reduces beam spreading so that a more focused beam is obtained. According to one preferred embodiment the laminar flow accounts for 50% of the flow through the nozzle 17.
Referring to Fig. 3, Fig. 3 illustrates an aerosol beam microinjector having additional means to control particle size. As in the apparatus illustrated in Fig. 2, the apparatus of Fig. 3 includes a drying tube 23.
However, in the apparatus of Fig. 3 the drying tube removes substantially all the solvent from the aerosol. Thus, the aerosol exiting the drying tube 23 through the tubing 11 is comprised substantially of dry solute. The solute is discharged from the tubing 11 into a channel 27 of a gas reheater 29. In addition to the dry solute solvent, solvent saturated carrier gas is discharged into the channel 27.
The solvent saturated inert gas is produced in the vapor saturator 31 and is transported through the piping to the channel 27 of the reheater 29. Filtered dry inert gas is drawn from a source 26 into the piping 19, as -14discussed for the apparatus of Fig. 2. The inert gas thereafter enters the vapor saturator 31, wherein solvent vapor is added to the inert gas to the point of saturation. The vapor saturator 31 is preferably constructed to contain solvent moistened fibrous material forming a central channel 33- Surrounding the solventmoistened material is preferably an aluminum block. 28 heated to a desired temperature with resistive heaters 30. Preferably, this temperature Is from about 50 to about 100° C. The heat causes the solvent moistened material to release solvent vapor which is entrained by the inert gas. Although this is a preferred construction for the vapor saturator 31, other means to saturate the inert gas with solvent vapor may be utilised in th® practice of the present invention.
The solvent-saturated inert gas is discharged from the vapor saturator 31 into piping 20 which communicates with channel 27 of the reheater 29. The dry aerosol is discharged from tubing 11 also into the reheater 29. The reheater 29 heats the dry aerosol and the solventsaturated inert gas to a constant temperature. This facilitates the diffusion and mixing of the vaporsaturated inert gas and the dry aerosol particles. Preferably, the resulting mixture is heated to about 50 C.
From the channel 27 of the reheater 29 the solventsaturated inert gas and the dry aerosol particles move to a vapor condenser 35. The vapor condenser 35 is preferably constructed as having a central channel 37 wherein by reducing the temperature, the solvent vapor is condensed onto the aerosol particles. Depending on the temperature within the channel 37, the amount of solvent condensed may be controlled. Thus, the projectile size may be precisely controlled. According to one embodiment, th© vapor condenser 35 includes Lapeltier Coolers, “15obtained from Marlow Industries. The vapor condenser outlet 39 includes the nozzle 17, and is positioned within the vacuum housing 15.
Referring again to Figs. 1, 2» and 3, placed in the path of these projectiles is the target support platform 41. The target support platform 41 is a substantially horizontal surface capable of supporting target cells thereon and being preferably moveable along the X, Y and Z axis. According to the most preferred embodiment, the target support platform 19 is provided with, supported by, and affixed to a motorized positioning member which enables it to be positioned either closer or farther away from the nozzle 17. Through experimentation, the inventor has determined that the target support platform 41 is preferably positioned about 1.5 cm from the nozzle 17. However, this distance may be varied depending on the specific application. For example, it has been determined that the greater the distance the target support platform 41 is from the nozzle 17 the slower the impact speed of the projectiles. This is due to the background pressure in the vacuum housing 15 reducing the speed of the projectiles as they travel through the housing 15» According to th© most preferred embodiment, th® target support platform 41 is rotated and is moved by the positioning member along on© linear axis 43. This allows for a biological sample placed on the target support platform 41 to be impacted throughout its entirety by projectiles. The present inventors had determined that an effective rate of rotation about axis 43 is 40 rpm and that an effective rate of simultaneous linear advance along axis 43 is 333 microns per revolution. This allows the entirety of a biological sample of approximately 5x7 centimeters to be impacted (hereinafter referred to as scanned) in three to four minutes.
-ISPreferable inert gases utilised in the practice of the present invention ar® filtered compressed inert gas.
A preferable carrier gas useful in the practice present invention is one gas selected from the group of gases consisting of carbon dioxide, room air, hydrogen, helium, and nitrogen. However, it should be noted, that any compressed gas substantially nontoxic to living materials may be utilised in a practice of the present invention.
The source of the carrier gas 6 is a source of gas capable of generating a gas pressure of 30 pounds per square inch at the inlet 3 of the nebulizer 7. Preferred sources of compressed gas are compressed gas cylinder, and laboratory electrolytic cell gas generators.
The nebulizer 5 utilized in the practice of the present invention may be any nebulizer 5 which produces aerosols having droplet sizes of from 0.X to about 3 microns in diameter. Although ultrasonic nebulizers, such as the LK3 Instruments, model X08 may be used in the practice of the present invention, down draft or respiratory inhalation nebulisers of the Lovelace design are most preferred. The most preferred nebulizers of the present invention is a nebulizer used in inhalation therapy obtained from Inhalation Plastic. Inc., model 4207, of the Lovelace design. These nebulizers are single use, disposable units that generate aerosol droplets with median mass diameters in the range of two microns. They require only a few millimeters of solution to operates efficiently and generate dense mist having up to 10 droplets per liter of gas. -17“ Examples Examples 1-3 are presented, to demonstrate the optimal range of particle sizes effective in transforming target cells in the practice of the present invention.
Examples 4-8 are presented to demonstrate the successful transformation of Ch1amydomonas yeinhardtii cells using the apparatus and methods of the present invention.
Example.! Aerosol Beam Microinjection of Carboxyfluorescein into Chlamvdomonas reinhardtii using 2 micron mass median diameter solute/solvent droplets Chlamvdomonas reinhardtii is a unicellular eucaryotic green alga- Cells of the wild type strain of Chlamvdomonas reinhardtii (Chlamvdomonas) were used as the target cells. The calls were cultured in tris-acetatephosphate (TAP) liquid medium. (Harris# E.H.
Chlamvdomonas Source Book. Academic Press# 1989). The cells were concentrated by centrifugation and resuspended in TAP at a concentration of 107 cells/ml. 100 microliters of the cell suspension were subsequently plated onto an agar medium slab containing TAP and 1.5% by weight agar for consistency. The slab also included an inert layer of Miracloth (Calbiochem, Co.) which was washed and steam autoclaved. Miracloth was included to facilitate the handling of the agar slabs. The slabs were thereafter incubated at 25°C for from 1 to about 4 hours. Following the incubation period tha slabs were chilled at 4°C for about an hour. -18The schematic of the apparatus used in the instant example is shown in Fig. l. The aerosol was produced by a respiratory therapy nebulizer,, model 4207 obtained from Inhalation Plastic, Inc. The mass median diameter of the aerosol droplets produced by the nebulizer was 2 micrometers, according to manufacturer’s literature. The nebulizing solution used was a buffered aqueous solution containing 0.0IM sodium phosphate Ph 7.0 and 10 mg/ml of carboxyfluorescein. Both chemicals were obtained from the sigma Chemical Company. The carrying gas was compressed nitrogen having a flow rate of 4 liters/min to achieve 30 psi in the nebulizer. The positive pressure created by the carrier gas was neutralized by opening the output piping of the nebulizer to the outside atmosphere. The piping leading to the vacuum housing (tubing 11 in Fig. 1) was positioned in close proximity to the open outlet piping of the nebulizer. The negative pressure in the system was created by a high-volume vacuum pump attached to the vacuum chamber. The vacuum pump used was a Marvac model R-10, set at 170 liters/min. The aerosol was accelerated into the vacuum housing through a nozzle having a diameter of 200 microns. Th© agar slab on which the cells were plated was placed on the target support platform, which, in turn, was positioned 1.5cm from the nozzle. The target support platform was rotated, at 40 rpm, and advanced at a rate of 333 micrometers/revolution. The entire slab was scanned (impacted by carrier gas or droplets) in about 3 to 4 minutes. A control group of cells (non-impacted cells) was created on the slab by interrupting the aerosol flow in a regular pattern. Thus, the control cells on the slab are impacted with only carrier gas.
To determine the morphology of the cells impacted, the scanned slab was examined using a 4OX dissection microscope. To determine the pattern of 19carboxyfluorescein impact, the slab was examined using a UV Products model T~33 longwave UV transilluminator. To determine cell survival after impact, the slab was placed on a petri dish containing TAP medium and Incubated for 2 days. To determine if microinjection of carboxyfluorescein had occurred in the impacted cells, the cells were removed from the slab, washed, resuspended in TAP liquid medium, and examined with a Nikon Labophot epifluorescence microscope, using a UV filter cube to observe carboxyfluorescein fluorescence.
Results Following scanning the slab with 2 micron droplets no intact cells were observed in the impact areas. Fluorescence was observed uniformly in all the impact areas. There was no growth in the impact area following a two day incubation. Thus, it was determined that cells impacted by droplets having a mass median diameter of 2 microns or greater would not service the procedure.
Aerosol Beam Microinjection of Carboxyfluorescein into Chlamydomonas reinhardtii usinq. 0.1 micron mass median diameter solute/solvent droplets The protocol set forth in Example 1 was followed in Example 2 with the following exception. A drying tube was included in the apparatus. The drying tube was located in close proximity to the nebulizer, as shown in Fig. 2. The drying tube had an internal diameter of 1/2 inch and was 60 cm long. It contained silica gel which, surrounded a central channel formed by a cylinder of 20 mesh stainless steel screening. The drying tube of the instant example was prepared by the inventor; however, similar drying tubes are available from TSI, Inc. (model 3062 Diffusion -20Dryer). The solvent was completely removed by the drying tube so that only a dry aerosol of the solutes remained to be accelerated and impact the cells. Based on the mean masses of the solutes it is estimated that the impacting projectiles had a mass median diameter of about 0,1 microns„ Results Following scanning the slab with 0.1 micron projectiles, visual examination with the 4OX dissection microscope revealed that all the cells in the impacted area were intact. Further, the distribution of carboxyfluorescein on the slab was uniform throughout the impact areas. Thus, demonstrating that the cells has ben impacted. There was 100% cell survival after a 2 day incubation. However, no fluorescence was observed in the washed and resuspended impacted cells. This suggested that no carboxyfluorescein was successfully injected into the cells.
Example 3 Aerosol Beam Microinjection of Carboxyfluorescein into Chlamydomonas reinhardtii on sorbitol containing medium using 2.0 micron mass median diameter solute/solvent droplets Example 3 followed the protocol set forth in Example 1 with the following exceptions: the agar slab included 0.5M sorbitol to help osmotically stabilize the impacted cells; and the cells were immediately washed and resuspended following microscopic and UV inspection of the slab. Thus, the incubation step, which determined cell survival was postponed until it was determined if carboxyfluorescein had been successfully mieroinjeeted into th® cells. -21Results Following scanning the slab with 2 micron droplets th® cells were inspected with the 4OX dissection microscope and substantially all the cells in the impact area appeared intact. Following washing and resuspension, substantially all of the impacted cells contained florescent carboxyfluorescein. Thus, carboxyfluor©seein was successfully microinjected into the cells. However, following subsequent replating of the impacted cells, no cell survival was below 0.1%.
Example 4 Transformation of Chlamydomonas reinhardtli Mutant D15 through the microinjection of DNA olasmid. p71.
The target cells were wild type Chlamydomonas relnhardtii Mutant D15 which are incapable of growing on minimal media because of a deletion of th© chloroplast tscA gen© that renders them defective in photosynthesis.
Mo spontaneous reversion of this deletion has been observed. The DNA plasmid p71 used as th© genetic transforming agent carries the Chlamydomonas reinhardtii chloroplast DNA fragment Ecol8 (Harris, E.H. Chlamydomonas Source Book. Academic Press, 1989) cloned in E. coli in the pUC8 cloning vector. It was obtained from Dr. Jane Aldrich, BP America. This fragment has the intact tscA gene that was deleted from the D15 mutant chloroplast DNA.
The nebulising solution included lOmM tris-Cl pH 8.0, ImM disodium EDTA, 3mM magnesium chloride, O.lmg/ml plasmid p71, 10% polyethylene glycol 5000, and distilled water. All reagents were obtained from the Sigma Chemical Company. Polyethylene glycol and magnesium chloride are included in the solvent mixture to cause the tight condensation of the DNA, which protects it from shear -22“ degradation during aerosol formation. The effectiveness of this treatment was verified in preliminary experiments in which the aerosol generated from this solvent was recovered and the DNA analysed by electrophoresis for intactness. In addition, it was tested for biological function by transformation of £. coli.
The target cells were grown in TAP liguid medium and concentrated by centrifugation. The cells were plated on an agar slab and incubated as described in Example 1. Before scanning, the agar slab was placed onto a petri plate containing solidified TAP medium containing 0.5M sorbitol for two hours at room temperature and for an additional one hour at 4* C. It is believed that the presence of the sorbitol in the medium helps the cells to maintain their integrity during an osmotically sensitive period during recovery after being impacted by the projectiles.
The apparatus used in Example 4 is illustrated schematically in Fig. 2. The drying tube utilised was the same drying tube as used in Example 2- The laminar flow accounted for 50% of the total flow through the nozzle.
The nozzle was 200 microns in diameter. The target cells were positioned 1.. 5cm from the nozzle and the procedure used for scanning the surface of the agar slab was the same as was used in Examples 1-3. The carrier gas was nitrogen and the flow rate through the drying tube was set at 160 ml/minute.
Following the scanning of the surface of the agar slab, the impacted cells wer® screened for the presence of transformants. The slab was transferred to tris-minimal medium (Harris, Ξ.Η., Chlamvdomonas Source Book. Academic Press, 1989) and incubated in light. Thus, only those cells which had been transformed could phofcosynthesize In the presence of light and survive. Following incubation -23“ for two days, two colonies were observed on the minimal medium. These colonies were removed and streaked onto petri dishes containing tris-minimal medium.
Subsequently, a plurality of colonies grew. This growth test was repeated a second time after seven days.
Total cell DNA was isolated from the transformed chlamvdomonas reinhardtii cells. The cells were grown to a concentration of 3 X 10S cells/ml in TAP liquid medium.
They were harvested by centrifugation at 5000 Xg for five 8 minutes and resuspended to a final concentration of 10 cells per ml in ice water buffer I (lOmM sodium chloride, XOmM tris-Cl, iOmM sodium EDTA, pH 8.0). This suspension was incubated with an equal volume of ice cold 4H lithium chloride and incubated for thirty minutes. The cells were then harvested by centrifugation as before and then washed twice with ice cold buffer I. The cell pellet obtained in the final wash was weighed and then the cells resuspended in 10 ml per gram pellet of ice cold buffer I. One third volume of 10% (w-v) sodium dodecyl sulfate detergent was added along with 0.1 mg/ml of Pronase (Sigma). This mixture was incubated at 37° C for three hours or longer until the chlorophyll was entirely converted to pheophvtin (olive-green in color). This solution was then cooled to room temperature and extracted twice with freshly distilled phenol (the phenol was distilled, washed with one half volume of 0.5M tris base and equilibrated before use with one volume of IOmM tris-Cl pH 8.0, ImM disodium EDTA, 50mM sodium chloride ). The aqueous phase separated from the second phenol extraction was mixed with one half volume of 7.5H ammonium acetate and then centrifuged in a micro centrifuge (Eppendorf) for one minute. The supernatant was thereafter mixed with two volumes of ethanol and placed in -70® C freezer for ten minutes. The precipitated nucleic acids were collected by centrifugation in the micro centrifuge for one minute and -24 — the supernatant discarded. The pellet was resuspended in one tenth of TS buffer (XOmM tris-Cl, imM disodium EDTA, pH 8.0). This ammonium acetate precipitation step was repeated once more.
The DNA obtained from the transformants was thereafter analyzed. One aliquot of the DNA obtained as set forth above from one of transformants was digested with restriction enzyme EcoRI, one with a combination of BamHI and Bglll and one with Smal, using the enzymes according the manufacturer’s instructions (BoehringerMannheim). A similar digestion was performed on DNA from wild-type cells, DNA from the D15 mutant cells, and DNA from the p7l plasmid used in th© transformation experiment. The DNA fragments were separated by electrophoresis in 0.7% agarose gels using trxs-faorateEDTA buffer according to standard procedures. The DNA was transferred to Nytran membranes (Schleicher and Schuell) using the standard Southern blot procedure. DNA for use as probes to detect specific fragments on the membrane was radioactively labeled by random priming, using a kit according to the manufacturer’s instructions (BoehringerMannheim). Probes were prepared from pUC18 plasmid DNA and from fragments of the Eco-18 chloroplast DNA isolated from the p71 plasmid.
The hybridization with the pUC probe reveals the presence of an intact puC vector sequence in transformants. No reactivity was seen in the wild type or D15 strain DNA samples. These results demonstrate that the DNA was microinjected into the target mutant cells to produce transformants in th® experiment.
While the invention is susceptible to various modifications and alternative forms, specific embodiments thereof have been shown by way of example in the drawings -25and have been described in detail. It should be understood# however, that it is not intended to limit the invention to th® particular forms disclosed, but on th© contrary, the intention is to cover all modifications, equivalents, and alternatives falling within the spirit and scope of the invention as defined by the appended claims.

Claims (4)

  1. CLAIMS: 1. A method of introducing exogenous material into a living cell, the method including the steps of: a) producing aerosol particles comprising said exogenous material; b) accelerating said particles to a speed enabling them to penetrate and enter into said cell upon impact therewith; and c) impacting said living cell with said accelerated aerosol particles.
  2. 2. The method of is DNA.
  3. 3. The method of include a solvent.
  4. 4. The method of based. claim 1 wherein said claim l wherein said claim 3 wherein said exogenous material aerosol particles solvent is alcohol 5. The method of have a diameter of claim 3 wherein said aerosol particles from about 0.1 to about 2 microns. 6. The method of claim 1 wherein said aerosol particles are accelerated by passing said aerosol particles from sn area of higher gas pressure through an aperture having a -27diameter of from about 100 to about 300 microns and into an area of lower gas pressure. 7. The method of claim 6 wherein the gas pressure in said high gas pressure area is about 1 atmosphere and the gas pressure in said low gas pressure area is about 0.01 atmospheres. 8. The method further defined of claim 6 wherein said aperture is as having a diameter of about 200 microns. 9. The method of claim 1 wherein said speed is from about 400 to about 2000 meters/second. 10. The method of claim 2 wherein said aerosol particles are produced from a solution including condensed fragments of foreign DNA in an alcohol solution. 11. The method of claim 10 wherein said condensed fragments of DNA are produced by adding to said solution one DNA condensing agent selected from the group of DNA condensing agents consisting of polyvalent cationic agents, polyethylene glycol, spermidine, and polylysine. 12. The method of claim 11 wherein said solution is further defined as including colloidal gold, said colloidal gold being included to adjust the density of the resulting aerosol particles. -2813- A method of introducing exogenous DNA into a living plant cell, the method including the steps of: a) solubilizing said exogenous DNA in an alcohol solution including one DNA condensing agent selected from the group of DNA condensing agents consisting of polyvalent cationic agents# polyethylene glycol# spermidine and polylysine# under conditions to condense said exogenous DNA to protect it from shear degradation; b) producing aerosol droplet particles from said solution having a diameter of from about 0..1 to about 2 microns# said droplets consisting essentially of said solvent and said exogenous DNA# c) accelerating said droplets to a speed enabling said droplets to penetrate and enter into said living plant cell upon impact therewith# said droplets being accelerated by passing from an area of high gas pressure through an aperture having a diameter of about 200 microns and into an area of low gas pressure# said area of low gas pressure having an atmospheric pressure of about 0,01 atmospheres and said area of high gas pressure having an atmospheric pressure of about 1 atmosphere# said living cell being positioned in said area of low gas pressure such that it is impacted by a plurality of the accelerated droplets# and d) impacting said living plant cells with said accelerated droplets# said droplets penetrating and entering into said cells. -2914. A method of introducing exogenous genetic material into a living cell, the method including the steps of: a) producing aerosol particles comprising said exogenous genetic material; b) accelerating said aerosol particles to a speed enabling them to penetrate and enter into said living cell without substantial damage to the cell upon impact therewith; and c) impacting said living cell with said accelerated aerosol particles. 13. 15. The method of claim 14 wherein said exogenous material is DNA. IS. The method have a diameter of claim 14 wherein said aerosol particles of from about 0.1 to about 2 microns. 14. 17. The method of claim 14 wherein said aerosol particles are accelerated by passing said aerosol particles from an area of higher gas pressure through an aperture having a diameter of from about 100 to about 300 microns and into an area of lower gas pressure. 15. 18. The method of claim 17 wherein the gas pressure in said high gas pressure area is about 1 atmosphere and the gas pressure in said low gas pressure area is about 0.01 atmospheres. -30“ 16. 19» The method of claim 17 wherein said aperture is further defined as having a diameter of about 200 microns. 17. 20. The method of claim 14 wherein said speed is from about 400 to about 2000 meters/second. 18. 21. The method of claim 15 wherein said aerosol particles are produced from a solution including condensed fragments of foreign DNA in an alcohol solution. 19. 22. The method of claim 21 wherein said solution is further defined as including colloidal gold, said colloidal gold being included to adjust the density of the resulting aerosol particles. 20. 23. The method of claim 21 wherein said condensed fragments of DNA are produced by adding to said solution one DNA condensing agent selected from the group of DNA condensing agents consisting of a polyvalent cationic agent, polyethylene glycol, spermidine, and polylysine. 21. 24. A method of genetically transforming a living plant cell, the method comprising the steps of: a) producing aerosol particles comprising exogenous genetic material and a solvent; b) accelerating said aerosol particles to a speed enabling them to penetrate and enter into said living plant cell upon impact therewith; -31c) impacting said living plant call with said aerosol particle, and d) screening the progeny of said impacted living plant cells for transformed progeny. 25. The method of claim 24 wherein said exogenous material is DNA. 26. The method of claim 24 wherein said aerosol particles include ethanol as said solvent. 27. The method of claim 24 wherein said solvent is aqueous based. 28. The method of claim 26 wherein said aerosol particles have a diameter of from about 0.1 to about 2 microns. 29. The method of claim 24 wherein said aerosol particles are accelerated by passing said aerosol particles from an area of higher gas pressure through an aperture having a diameter of from about 100 to about 300 microns and into an area of lower gas pressure. 30. The method of claim 29 wherein the gas pressure in said high gas pressure area is about 1 atmosphere and the gas pressure in said low gas pressure area is about 0.01 atmospheres. -3231. The method of claim 29 wherein said aperture is further defined as having a diameter of about 200 microns. 32. The method of claim 24 wherein said speed is from about 400 to about 2000 meters/second. 33. The method of claim 25 wherein said aerosol particles are produced from a solution including condensed fragments of foreign DNA in an aqueous solution. 34. The method of claim 33 wherein said solution is further defined as including colloidal gold, said colloidal gold being included to adjust th® density of the resulting aerosol particles. 35. The method of claim 33 wherein said condensed fragments of DNA are produced by adding to said solution one DNA. condensing agent selected from the group of DNA condensing agents consisting of a polyvalent cationic agent, polyethylene glycol, spermidine, and polylysine. 36. A method for making a genetically transformed line of plants, the method comprising the steps of: a) producing aerosol particles comprising exogenous genetic material; b) accelerating said particles to a speed enabling them to penetrate and enter into living plant cells upon impact therewith; “33 c) impacting said living plant cells with said aerosol particles; d) culturing said impacted living plant cells to grow a plant; and e) screening among the progeny of said plant for transformed progeny. 37. The method material is DNA. of claim 35 wherein said exogenous 38» The method of include a solvent. claim 35 wherein said aerosol particles 39» The method alcohol based. of claim 38 wherein said solvent is 4 0» The method of claim 38 wherein said aerosol particles have a diameter of from about 0.1 to about 2 microns. 41. The method of claim 35 wherein said aerosol particles are accelerated by passing said aerosol particles from an area of higher gas pressure through an aperture having a diameter of from about 100 to about 300 microns and into an area of lower gas pressure. 42. The method of claim 41 wherein the gas pressure in said high gas pressure area is about 1 atmosphere and the -34” gas pressure in said low gas pressure area is about 0,01 atmospheres. 43. The method of claim 41 wherein said aperture is further defined as having a diameter of about 200 microns. 44. The method of claim 35 wherein said speed is from about 400 to about 2000 meters/second. 45. The method of claim 37 wherein said aerosol particles are produced from a solution including condensed fragments of foreign DNA in an alcohol solution. 45. The method of claim 45 wherein said solution is further defined as including colloidal gold, said colloidal gold being included to adjust the density of the resulting aerosol particles. 47. The method of claim 45 wherein said condensed fragments of DNA are produced by adding to said solution one DNA condensing agent selected from the group of DNA condensing agents consisting of a polyvalent cationic agent, polyethylene glycol, spermidine, and polylysine. 48. An apparatus for introducing exogenous material into a living cell, comprising: a) a first assembly for producing aerosol particles, said aerosol particles including a solvent and said exogenous material; -35b) a second assembly for accelerating said aerosol particles to a speed enabling said particles to penetrate and enter into said living cell upon impact therewith; and c) a target support platform member mounted in said second assembly for supporting said cells such that said accelerated exogenous material impacts said cells. 49. An apparatus for introducing exogenous material into a living cell comprising: an airtight housing; -36a means for creating a partial vacuum within said housing, said means being in communication with said housing to continuously remove atmosphere from said housing to create a partial vacuum therein; a target support platform mounted within said housing for supporting and positioning said living cells thereon within said housing, said target support platform including a substantially planar surface supported by and affixed to a positioning member# said positioning member being mounted within said housing# said positioning member including a motor driven gear assembly capable of rotationally# vertically and horizontally moving said target support platform within said housing; a conduit having a central bore of a predetermined diameter# said conduit having a first end portion and a second end portion# said first end portion is connected to said housing such that said central bore communicates with the partial vacuum therein# said first end portion including an aperture said aperture having a substantially smaller diameter than said conduit# said aperture having a diameter of from about 100 to about 300 microns# said conduit second end portion including an opening which communicates with said central channel# said opening having the same diameter as said central bore# said partial vacuum in said housing creating a partial vacuum within said conduit central bore; and 37means an assembly for producing aerosol particles from a solution comprising a solvent and said exogenous material, said assembly including an exit piping, said exit piping having one end positioned in close proximity to said conduit second end portion opening, said aerosol particles exit said assembly through said exit piping into the outside atmosphere whereby said aerosol particles are influenced into said central bore of said conduit second end portion by said partial vacuum therein, whereby said aerosol particles are accelerated from said conduit central bore, through said aperture and into said housing, to impact and penetrate said living cells positioned on said target support platform. 50 o The apparatus of claim 48 wherein said first assembly includes a nebuliser member and a source of compressed gas adapted to supply gas to the nebulizer member, said nebulizer member being capable of interacting said compressed gas entering said nebulizer member with a solution including a solvent and said exogenous material to produce aerosol particles. 51. The apparatus of claim 48 wherein said second assembly is further defined as including: an airtight housing; means for creating a partial vacuum within said housing; -38a conduit having a central bore of a predetermined diameter, said conduit having a first end portion and a second end portion, said first end portion connected to said housing such that said central bore communicates with the partial vacuum therein, said first end portion including an aperture having a substantially smaller diameter than said conduit, said aperture having a diameter of from about 100 to about 300 microns, said conduit second end portion including an opening which communicates with said central bore, said opening having the same diameter as said central bore, said impartial vacuum in said housing creating a partial vacuum within said conduit central bore. 52. The apparatus of claim 48 wherein said assembly comprises a housing and said target support platform is capable of rotational, vertical and horizontal movement within said housing. 53. Tha apparatus of claim 51, wherein said aperture is further defined as having a diameter of from about 100 to about 300 microns. 54. The apparatus of claim 51 wherein said aperture is further defined as having a diameter of about 100 microns. 5 5 Apparatus for introducing exogenous material into living cells comprising: an airtight housing; -39“ means for creating a partial vacuum within said housing, said means connected to said housing by a tube to continuously remove atmosphere from said housing to create a partial vacuum therein; a target support platform mounted within said housing for supporting and positioning living cells thereon, said target support platform including a substantially planar surface supported by and affixed to a positioning member, said positioning member being mounted in the interior of said housing, said positioning member including a motor driven gear assembly capable of rotationally, vertically and horizontally moving said target support platform with said housing; a conduit having a central bore of a predetermined diameter, said conduit having a first end portion and a second end portion, said first end portion is connected to said housing such that said central bore communicates with the partial vacuum therein, said first end portion of said central bore including a laminar flow assembly and an aperture at the terminus of said central bore, said aperture having a substantially smaller diameter than said central bore, said conduit second end portion including an inlet which is connected to a drying assembly, said drying assembly is connected to and communicates with said central bore, said inlet having the same diameter as said central bore, said partial vacuum in said housing creating a partial vacuum within said conduit central bore; and -40an assembly for producing aerosol particles therein,, said aerosol particles including a solvent and said exogenous material, said assembly including an exit piping, said exit piping having one end 5 positioned in close proximity to said conduit second end portion inlet, wherein said aerosol particles exit said assembly through said exit piping into the outside atmosphere and are influenced into said inlet by said partial 10 vacuum therein, said aerosol particles being accelerated by the transition from said conduit central bore, through said aperture and into said housing, said accelerated aerosol particles impact and penetrate said living cells 15 positioned on said target support platform. 56. The apparatus of claim 55 wherein said drying assembly includes a central bore formed by a cylinder of 20 non-reactive metal mesh surrounded by a desiccant. 57. The apparatus of claim 56 wherein said non-reactive metal mesh is further defined as stainless steel. 58. The apparatus of claim 56 wherein said desiccant is further defined as silica gal. 59. - The apparatus of claim 55 wherein said laminar flow assembly includes a first and second piping, said, first piping communicating with said means for producing aerosol particles, said second piping forming a sheath about said 35 first piping, said partial vacuum in said housing drawing inert gas in a laminar flow through said second piping, —41 said second piping communicating with a non-pressurized inert gas source through a tubing, said aerosol particles discharging from said first piping into the center of the inert gas laminar flow, said laminar flow channeling said aerosol particles through said aperture and into said housing. 60. An apparatus for introducing exogenous genetic material into a living cell, comprising: an air-tight housing; means for continuously evacuating said housing; a target support platform mounted within said housing for supporting and positioning said living cells thereon within said housing; a vapor condenser, including a central bore which is connected to and communicates with said housing, said vapor condenser central bore including an aperture at one end proximate said housing, a vapor reheater, including a central bore which is connected to said vapor condenser central bore; a drying assembly, including a central bore having one end connected to and communicating with the central bore of the vapor reheater, and the other end open to the surrounding atmosphere; a vapor saturator assembly, including a central bore which communicates with the central bore of the vapor reheater; and -42an assembly for producing an aerosol comprising aerosol particles including solvent and said exogenous material, said assembly including an exit end positioned in close proximity to said other end of the drying assembly central bore. 61 e . The apparatus of claim go wherein said drying assembly includes a central bore formed by a cylinder of non-reactive metal mesh surrounded by a desiccant. 62. The apparatus of claim 61 wherein said non-reactive metal mesh is further defined as stainless steel. 63. The apparatus further defined as of claim 61 silica gel. wherein said desiccant is 64. The apparatus of claim 60 wherein said target support platform is further defined as including a substantially planar surface supported by and affixed to a positioning member. 65. The apparatus of claim 64 wherein said positioning member is capable of rotationally, vertically and horizontally moving said target support platform within said housing. 66. The apparatus of claim 60 wherein said aperture is further defined as having a diameter of about 100 to about 300 microns. -43~ 67θ The apparatus of claim 66 wherein said aperture is further defined as having a diameter of about 100 microns. gg_ The apparatus of claim 67 wherein said vapor condenser includes a cooling member, said cooling member lowering the temperature within th® central bore of said vapor condenser sufficient to cause the precipitation of the solvent included in said solvent saturated vapor to precipitate onto the surface of aerosol particle within said central bore. θ 9 » The apparatus of claim 68 wherein the temperature within said vapor condenser central bore is from about 0 to about 10°C. 70. The apparatus of claim 60 wherein said vapor reheater includes a heating member, said heating member heating said solvent saturated vapor and said aerosol particles to a uniform temperature within its central bore. 71. The apparatus of claim 70 wherein said vapor reheater heats said aerosol particles and said solvent saturated vapor to a temperature of from SO to about 100 degrees C. 72» The apparatus of claim 60 wherein said vapor saturator assembly is further defined as including a solvent reservoir and means for vaporizing solvent contained therein. -4473. The apparatus of claim 72 wherein said solvent reservoir is further defined as matted# layered# fibrous material disposed about said central bore and wetted with a solvent. 74 The apparatus of claim 73 wherein said means for vaporizing solvent is further defined as a heating unit# said heating unit supplying sufficient thermal energy to produce solvent saturated vapor. 75 Apparatus for injecting genetic particles into a live cell# which comprises: a) a first conduit adapted to pass pressurized gas from an inlet end through an outlet end; b) a second conduit having an inlet end exterior of the first conduit adapted to receive aerosol particles# and an outlet end terminating within the first conduit such that gas flowing through the first conduit aspirates aerosol particles into the flowing gas; c) a discharge jet at the outlet end of tha first conduit adapted to accelerate and discharge the flowing gas and aspirated particles in an aerosol beam; d) a vacuum housing enclosing the outlet end of the first conduit and adapted to receive flowing gas discharged through th® discharge jet; e) a target support platform mounted in the vacuum housing and adapted to support a live cell in a -45position to be impacted by an aerosol beam from the discharge jet. 76. The apparatus of claim 75 wherein the outlet end of the second conduit is positioned to discharge the aspirated aerosol particles above the center of the gas flow in the first conduit. 77. The apparatus of claim 75 which further comprises a nebulizer capable of generating an aerosol and delivering the aerosol to the inlet end of the second conduit. 78. The apparatus of claim 77 which further comprises a drying tube operable to dry an aerosol passed through the second conduit. 79. The apparatus of claim 77 which further comprises a heater operable to heat gas flowing through the first conduit. I 80. The apparatus of claim 75 which further comprises a vapor saturator operable to increase the vapor content of pressurized gas passed to the first conduit. 81 - The apparatus of claim 75 wherein the platform is adapted to position a live cell about 1.5 cm from the discharge jet. -46“ 82. The apparatus of claim 75 wherein the platform is movable relative to the jet» 83. The apparatus of claim 7.7 wherein the nebulizer is capable of generating an aerosol having particles between about 0.5 and 2 micrometers in sise. 24 Tha apparatus of claim 77 which further comprises means to control the sise of the particles. 22. 25 s Apparatus for injecting genetic particles into a live cell, which comprises: a) a conduit having an inlet end and an outlet end; b) a jet at the outlet end of the conduit capable of accelerating gas flowing through the jet; c) a vacuum housing enclosing the outlet end of the conduit and adapted to receive gas discharged by the jet; d) a vacuum generator operable to evacuate the vacuum housing at a rate sufficient to aspirate an aerosol containing genetic particles through the conduit and to accelerate th© particles through the jet; and e) a target support platform mounted in the vacuum housing and adapted to support a live cell in a position to be impacted by accelerated particles discharged by the jet. -47“ 86o The apparatus of claim 85 wherein the target platform is capable of movement relative to the jet. 87. The apparatus of claim 85 wherein the target platform is capable of movement in three orthogonal directions relative to the jet. θθ· . The apparatus of claim 87 wherein the target platform is further capable of rotational movement. 89« . The apparatus of claim 85 wherein the target support platform is adapted to support a live cell about 1.5 cm. from the jet. 90. The apparatus of claim 85 which further comprises a nebulizer adapted to generate an aerosol and to discharge the aerosol sufficiently proximate the inlet end of the conduit such that the aerosol may be aspirated by the vacuum generator through the conduit. 91 . . The apparatus of claim 85 wherein the vacuum generator is operable to maintain a pressure in the range between about 0.01 and 0.05 atmosphere in the vacuum housing. 92. The apparatus of claim90 wherein the nebulizer is operable to generate an aerosol of genetic particles wherein the particles have a size between about 0.1 and about 2 microns. -4893. The apparatus of claim 91 wherein the vacuum generator is further capable of maintaining a laminar flow of gas in the conduit. 94. A method of introducing genetic material into a live cell which comprises the following steps: a) generating an aerosol from the genetic material and a liquid to form an aerosol of particles comprising the genetic material and the liquid; b) adjusting the size of the particles, as may be necessary, to between about 0.1 and about 2 microns; and c) accelerating the particles and impacting the accelerated particles against the live cell at a velocity sufficient for the particles to penetrate the cell without fatal damage to the cell. 95. Ths method of claim 94 wherein th® size of the particles is adjusted in step (b) by adjusting the content of said liquid in the particles. 96. The method of claim 95 which further comprises heating the aerosol to vaporize liquid from the cell. 97. The method of claim 94 wherein th® particles are accelerated in step (c) by generating a stream of non49toxic gas and aspirating the aerosol particles into the stream. 98. The method of claim wherein the stream of non toxic gas is generated by releasing a pressurised supply of ths gas. gg The method of claim 97 wherein the stream of nontoxic gas is generated by evacuating a sone containing the live cell and drawing the gas into the sone. 103 o The method of claim 99 wherein the gas comprises an inert gas. 101. & method of introducing exogenous material into a living cell, which comprises the steps of: a) aerosolizing a solution of the exogenous material; b) removing at least a portion ox the solvent from the aerosol to dry the particles of exogenous material in the aerosol; c) aspirating the dried aerosol particles into a carrier stream of an inert gas; and d) accelerating the carrier stream and the aspirated aerosol particles against the living cell at a velocity sufficient for the particles to penetrate the cell and for the cell to survive the impact. 102. A method of introducing exogenous material into a living cell, which comprises the steps of: a) nebulizing a solution of the exogenous material with a solvent to form an aerosol of particles of the exogenous material; b) adjusting the size of the particles to a size between about 0.1 and 2 microns; c) entraining the adjusted particles in a stream of a gas inert to the cell; and d) accelerating th® resulting stream of said gas and entrained particles cigainst the cell at a velocity sufficient for th© particles to penetrate the cell and for the cell to survive the impact. 103„ The method of claim 102 wherein the accelerating is obtained by aspirating the stream of said gas and entrained particles into a chamber containing the cell, and wherein the pressure in the chamber is less than the pressure in the stream. 104_„- The method of claim 102 wherein the size of the particles in step (b) is adjusted by removing solvent from the particles. -51105„ The method of claim 102 which further comprises the step of drying the particles in the aerosol by removing solvent from the particles; and wherein the sise of the dried particles is adjusted in step (b) by humidifying the dried particles with a vapor inert to the cell. 106. The method of claim 102 which further comprises adjusting the density of the particles by adding a solute of greater density than the particles to the solution of step (a). 107. A method of introducing exogenous material into a living cell which comprises the steps of: a) dissolving the exogenous material in solvent to form a solution; b) nebulising the solution to form an aerosol containing particles of th® material having a sise in the range between about 0.1 and 2.0 microns; c) removing solvent, if any, from the aerosol to dry the particles; d) aspirating the dried aerosol particles into a stream of a gas inert to the cell; and e) aspirating the stream of gas containing the dried aerosol particles into an evacuated zone containing the cell and accelerating the aspirated stream to impact the cell at a velocity such that said dried aerosol particles penetrate the cell while enabling th® cell to survive.. »52108. A method of introducing materials into a living cell substantially as described herein with refernece to the accompanying drawings and/or the Examples. 109. A living cell comprising material introduced therein by a method as claimed in any of claims 1 to 23 or 94 to 108. 110. A method of genetically transforming a plant cell substantially as described herein with reference to the accompanying drawings and/or the Examples. 111. A plant cell transformed by a method as claimed in any of claims 24 to 47 or 110, 112. An apparatus of introducing material into a living cell substantially as described herein with reference to the accompanying drawings and/or the Examples.
IE250490A 1989-07-11 1990-07-10 Aerosol beam microinjector IE61705B1 (en)

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Families Citing this family (82)

* Cited by examiner, † Cited by third party
Publication number Priority date Publication date Assignee Title
US5141131A (en) * 1989-06-30 1992-08-25 Dowelanco Method and apparatus for the acceleration of a propellable matter
ES2079467T3 (en) * 1989-12-19 1996-01-16 Ciba Geigy Ag PROCEDURE AND DEVICE FOR THE GENETIC TRANSFORMATION OF CELLS.
WO1992004439A1 (en) * 1990-08-30 1992-03-19 Brian John Bellhouse Ballistic apparatus
ATE174631T1 (en) * 1991-03-06 1999-01-15 Agracetus PARTICLE TRIGGERING TRANSFORMATION OF COTTON
AU2781892A (en) * 1991-10-07 1993-05-03 Ciba-Geigy Ag Particle gun for introducing dna into intact cells
WO1993023552A1 (en) 1992-05-21 1993-11-25 Government Of The United States As Represented By Secretary Department Of Health And Human Services Targeting gene expression to living tissue using jet injection
DE4418965A1 (en) * 1994-05-31 1995-12-07 Boehringer Ingelheim Int Transfection of eukaryotic cells with nucleic acid
GB9416663D0 (en) * 1994-08-17 1994-10-12 Oxford Bioscience Limited Particle delivery
US6433154B1 (en) 1997-06-12 2002-08-13 Bristol-Myers Squibb Company Functional receptor/kinase chimera in yeast cells
WO2001005994A2 (en) * 1999-07-21 2001-01-25 Immunoporation Ltd. Method for introducing a substance into a cell
US7314969B2 (en) 1999-11-29 2008-01-01 Midwest Oilseeds, Inc. Methods and compositions for the introduction of molecules into cells
ATE538205T1 (en) * 1999-11-29 2012-01-15 Midwest Oilseeds Inc METHOD, MEDIA AND DEVICE FOR INTRODUCING MOLECULES INTO PLANT CELLS AND BACTERIA USING AEROSOL JETS
CN1247314C (en) 2000-05-16 2006-03-29 明尼苏达大学评议会 High mass throughput particle generation using multiple nozzle spraying
EP1337140B1 (en) * 2000-11-28 2010-07-21 Midwest Oilseeds, Inc. Methods for the introduction of molecules into cells
US7247338B2 (en) 2001-05-16 2007-07-24 Regents Of The University Of Minnesota Coating medical devices
PT1444999E (en) 2003-02-03 2010-11-11 Bioware Technology Co Ltd Low pressure gas accelerated gene gun
ATE412054T1 (en) 2003-02-20 2008-11-15 Athenix Corp DELTA-ENDOTOXIN GENES AND METHODS OF USE THEREOF
NZ577786A (en) 2005-04-01 2010-10-29 Athenix Corp AXMI-027, a delta-endotoxin genes and methods for its use
DE102005061371A1 (en) 2005-12-14 2007-06-28 Eberhard-Karls-Universität Tübingen Generation of biological material using a nebulisation process in combination with cell-affecting biological and physical stimuli
US20070173470A1 (en) * 2006-01-23 2007-07-26 Chi-Hung Lin Methods for delivering extracellular target into cells
WO2007089881A2 (en) 2006-01-31 2007-08-09 Regents Of The University Of Minnesota Electrospray coating of objects
EP1988941A2 (en) 2006-01-31 2008-11-12 Nanocopoeia, Inc. Nanoparticle coating of surfaces
US9108217B2 (en) 2006-01-31 2015-08-18 Nanocopoeia, Inc. Nanoparticle coating of surfaces
EP2455391A3 (en) 2006-06-15 2012-08-22 Athenix Corporation A family of pesticidal proteins and methods for their use
US9040816B2 (en) 2006-12-08 2015-05-26 Nanocopoeia, Inc. Methods and apparatus for forming photovoltaic cells using electrospray
RU2495935C2 (en) * 2007-10-05 2013-10-20 ДАУ АГРОСАЙЕНСИЗ ЭлЭлСи Method of transferring molecular substances in plant cells
WO2009049126A2 (en) 2007-10-10 2009-04-16 Athenix Corporation Synthetic genes encoding cry1ac
AU2008312468B2 (en) 2007-10-16 2014-07-31 BASF Agricultural Solutions Seed US LLC AXMI-066 and AXMI-076: delta-endotoxin proteins and methods for their use
BRPI0914780B8 (en) 2008-06-25 2022-07-05 Athenix Corp ISOLATED NUCLEIC ACID MOLECULE, VECTOR, HOST CELL, COMPOSITION, AND METHODS FOR CONTROLLING A PEST POPULATION, KILLING A PEST PROTECTION OF A PLANT FROM A PEST AND PRODUCTION OF A POLYPEPTIDE WITH PESTICIDE ACTIVITY
EA035103B1 (en) 2008-07-02 2020-04-28 Атеникс Корпорейшн Insecticidal polypeptide axmi-115 of delta-endotoxin and use thereof
CA2746766C (en) 2008-12-15 2018-01-23 Cheryl L. Peters Genes encoding nematode toxins
CA2747812A1 (en) 2008-12-22 2010-07-01 Athenix Corporation Pesticidal genes from brevibacillus and methods for their use
US8084416B2 (en) 2008-12-23 2011-12-27 Athenix Corp. AXMI-150 delta-endotoxin gene and methods for its use
HUE032178T2 (en) 2009-02-05 2017-09-28 Athenix Corp Variant Axmi-R1 delta-endotoxin genes and methods for their use
EP2957638B1 (en) 2009-02-27 2018-12-12 Athenix Corporation Pesticidal proteins and methods for their use
US7919272B2 (en) 2009-03-06 2011-04-05 Athenix Corp. Methods and compositions for controlling plant pests
CN102421792B (en) 2009-03-11 2015-11-25 阿森尼克斯公司 AXMI-001, AXMI-002, AXMI-030, AXMI-035 and AXMI-045: from the insecticidal proteins and using method thereof of bacillus thuringiensis
ES2609332T3 (en) 2009-07-02 2017-04-19 Athenix Corporation AXMI-205 pesticide gene and methods for its use
AR077344A1 (en) 2009-07-31 2011-08-17 Athenix Corp FAMILY OF PESTICIATED GENES AXMI-192 AND METHODS FOR USE
BR112012020921A2 (en) 2010-02-18 2015-09-08 Athenix Corp delta-endotoxin genes axmi218, axmi219, axmi220, axmi226, axmi227, axmi228, axmi229, axmi230 and axmi231 and methods for their use
EP2536267B1 (en) 2010-02-18 2015-07-22 Athenix Corp. AXMI221z, AXMI222z, AXMI223z, AXMI224z, AND AXMI225z DELTA-ENDOTOXIN GENES AND METHODS FOR THEIR USE
WO2012135501A2 (en) 2011-03-30 2012-10-04 Athenix Corp. Axmi232, axmi233, and axmi249 toxin genes and methods for their use
WO2012135436A1 (en) 2011-03-30 2012-10-04 Athenix Corp. Axmi238 toxin gene and methods for its use
PL2694659T3 (en) 2011-04-05 2019-11-29 BASF Agricultural Solutions Seed US LLC Axmi115 variant insecticidal gene and methods for its use
CN103597082B (en) 2011-06-06 2017-09-15 拜尔作物科学公司 For the ways and means in preselected site modified plant genome
US9862965B2 (en) 2011-07-28 2018-01-09 Athenix Corp. AXMI205 variant proteins and methods of use
RU2014107672A (en) 2011-07-28 2015-09-10 Атеникс Корп. AXMI270 GENE AND WAYS OF ITS APPLICATION
BR112014002027A8 (en) 2011-07-29 2022-07-05 Athenix Corp AXMI279 PESTICIDE GENE AND METHODS FOR ITS USE
MX348003B (en) 2011-08-22 2017-03-08 Bayer Cropscience Nv Methods and means to modify a plant genome.
MX362999B (en) 2012-03-08 2019-03-01 Athenix Corp Axmi345 delta-endotoxin gene and methods for its use.
AR090274A1 (en) 2012-03-08 2014-10-29 Athenix Corp GENE OF TOXIN AXMI335 OF BACILLUS THURINGIENSIS AND ITS METHODS OF USE
KR20240116574A (en) 2012-03-09 2024-07-29 베스타론 코포레이션 Toxic peptide production, peptide expression in plants and combinations of cysteine rich peptides
US11692016B2 (en) 2012-03-09 2023-07-04 Vestaron Corporation High gene expression yeast strain
CN103998610B (en) 2012-06-29 2020-03-17 阿森尼克斯公司 AXMI277 nematode toxins and methods of use thereof
WO2014036238A1 (en) 2012-08-30 2014-03-06 Athenix Corp. Axmi-234 and axmi-235 toxin genes and methods for their use
US20150376243A1 (en) 2013-02-13 2015-12-31 Athenix Corp. Use of AXMI184 for the Control of Rootworm Insects
CN105247054B (en) 2013-03-07 2019-06-18 阿则耐克斯公司 Toxin gene and its application method
CN105102474B (en) 2013-03-15 2019-11-12 拜耳作物科学有限合伙公司 Composing type soybean promoter
UY35696A (en) 2013-08-09 2015-03-27 Athenix Corp ? RECOMBINANT DNA MOLECULE THAT INCLUDES AXMI440 TOXIN GENE, VECTOR, GUEST CELL, PLANTS, COMPOSITIONS AND RELATED METHODS ?.
US9862967B2 (en) 2013-08-09 2018-01-09 Athenix Corp. AXMI281 toxin gene and methods for its use
CN105764343B (en) 2013-11-25 2020-04-17 拜耳作物科学有限合伙公司 Control of hemipteran insects using AXMI-011
UA120843C2 (en) 2013-12-09 2020-02-25 Атенікс Корп. Axmi477, axmi482, axmi486 and axmi525 toxin genes from bacillus thuringiensis and methods for their use
CA3021682A1 (en) 2016-05-25 2017-11-30 Cargill Incorporated Engineered nucleases to generate deletion mutants in plants
AU2017347761C1 (en) 2016-10-21 2024-03-28 Vestaron Corporation Cleavable peptides and insecticidal and nematicidal proteins comprising same
CA3234859A1 (en) 2016-11-23 2018-05-31 BASF Agricultural Solutions Seed US LLC Axmi669 and axmi991 toxin genes and methods for their use
KR20190095411A (en) 2016-12-22 2019-08-14 바스프 아그리컬쳐럴 솔루션즈 시드 유에스 엘엘씨 Use of CR14 for the control of nematode pests
AR110756A1 (en) 2017-01-18 2019-05-02 Bayer Cropscience Lp USE OF BP005 FOR PLANT PATHOGEN CONTROL
EP3571303A1 (en) 2017-01-18 2019-11-27 Basf Agricultural Solutions Seed Us Llc Bp005 toxin gene and methods for its use
CN107303538B (en) * 2017-05-23 2019-05-31 东南大学 A kind of biology molecule separating equipment and separation method
AR114734A1 (en) 2018-09-14 2020-10-07 Vestaron Corp Av3 MUTANT INSECTICIDE POLYPEPTIDES AND METHODS TO PRODUCE AND USE THEM
US12173299B2 (en) 2019-01-04 2024-12-24 Pioneer Hi-Bred International, Inc. Engineered nucleases to generate mutations in plants
WO2021058659A1 (en) 2019-09-26 2021-04-01 Bayer Aktiengesellschaft Rnai-mediated pest control
CN114787360A (en) 2019-10-14 2022-07-22 巴斯夫农业种子解决方案美国有限责任公司 Novel insect resistance genes and methods of use
MX2022004465A (en) 2019-10-14 2022-07-21 BASF Agricultural Solutions Seed US LLC NEW INSECT RESISTANCE GENES AND METHODS OF USE.
PE20231212A1 (en) 2020-04-20 2023-08-17 Vestaron Corp PROTEOLITICALLY STABLE VARIANT POLYPEPTIDES OF U1-AGATOXIN-TA1B FOR PEST CONTROL
CA3181913A1 (en) 2020-05-01 2021-11-04 Vestaron Corporation Insecticidal combinations
KR20230078719A (en) 2020-09-28 2023-06-02 베스타론 코포레이션 Mu-diguetoxin-Dc1a mutant polypeptide for pest control
MX2023011579A (en) 2021-04-01 2023-10-10 Vestaron Corp Av3 mutant polypeptides for pest control.
WO2023245100A1 (en) 2022-06-17 2023-12-21 Vestaron Corporation Antimicrobial ncr13 variant peptides
WO2024137438A2 (en) 2022-12-19 2024-06-27 BASF Agricultural Solutions Seed US LLC Insect toxin genes and methods for their use
WO2024259306A2 (en) 2023-06-16 2024-12-19 Vestaron Corporation Pvd1 variant polypeptides for pest control
WO2025034576A1 (en) 2023-08-04 2025-02-13 Vestaron Corporation Delta-amaurobitoxin pl1c variant polypeptides for pest control

Family Cites Families (1)

* Cited by examiner, † Cited by third party
Publication number Priority date Publication date Assignee Title
US5015580A (en) * 1987-07-29 1991-05-14 Agracetus Particle-mediated transformation of soybean plants and lines

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WO1991000915A1 (en) 1991-01-24
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IE902504A1 (en) 1991-03-13
AU5950090A (en) 1991-02-06

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