US2591927A - Obtaining tumor tissue specimen - Google Patents

Obtaining tumor tissue specimen Download PDF

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Publication number: US2591927A
Authority: US; United States
Prior art keywords: sponge; tissue; tumor; specimen; tumor tissue
Prior art date: 1948-10-06
Legal status (The legal status is an assumption and is not a legal conclusion. Google has not performed a legal analysis and makes no representation as to the accuracy of the status listed.): Expired - Lifetime

Application number

US53131A

Inventor

Sidney A Gladstone

Current Assignee (The listed assignees may be inaccurate. Google has not performed a legal analysis and makes no representation or warranty as to the accuracy of the list.)

Individual

Original Assignee

Individual

Priority date (The priority date is an assumption and is not a legal conclusion. Google has not performed a legal analysis and makes no representation as to the accuracy of the date listed.)

1948-10-06

Filing date

1948-10-06

Publication date

1952-04-08

1948-10-06 Application filed by Individual filed Critical Individual

1948-10-06 Priority to US53131A priority Critical patent/US2591927A/en

1952-04-08 Application granted granted Critical

1952-04-08 Publication of US2591927A publication Critical patent/US2591927A/en

1969-04-08 Anticipated expiration legal-status Critical

Status Expired - Lifetime legal-status Critical Current

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Classifications

- A—HUMAN NECESSITIES
- A61—MEDICAL OR VETERINARY SCIENCE; HYGIENE
- A61B—DIAGNOSIS; SURGERY; IDENTIFICATION
- A61B10/00—Instruments for taking body samples for diagnostic purposes; Other methods or instruments for diagnosis, e.g. for vaccination diagnosis, sex determination or ovulation-period determination; Throat striking implements
- A61B10/02—Instruments for taking cell samples or for biopsy

Definitions

This-invention is concerned with the "problem of obtaining tissue from a tumor carried bya patient. Pathologists require such tissue .ior their determinations of whether tumors :are
One object of the present invention is to obtain living tissue from a tumor for examination by a pathologist without excising a specimen from the tumor. Another object is 'toprovide a new means for removing the tissue and permitting its processing and examination in a manner easily followed by pathologists. Other objects may be inferred from the following.
the present invention is based on the discovery that when a sponge is rubbed over :a tumor of the type that might be suspected as being malignant, the interstices or pores, or cavities of the sponge pick up or absorb small particles of tissue which are retained or held with the sponge functioning as a carrier.
the sponge may be processed for microscopic examination by a pathologist in the same fashion he would process a tissue specimen excised from a tumor.
the appearance of the tissue carried or absorbed by the sponge, under the microscope, has been found to be such that a pathologist has no seri-v ous di'fficulty in diagnosing the tumor type or condition.
the sponge may be of the type commercially known as a fine pore cellulose sponge.
the cavities or pores are provided by blown cellulose bubbles and these have blown-but ruptures providing entrancestoithem. Thus the cavities or pores are able to pick up, absorb or entrap the tissue when the sponge is rubbed .on the tumor.
the above described sponge in a dry condition is rubbed over the tumor carried by the patient. Judgment is needed in determining the rubbing pressure. However, no great amount of skill is required since a rubbing pressure light enough to avoid hurting or I materially annoying the patient or aggravating his condition, is sufficient to entrap or absorb the tissue in the pores ofthe sponge.
the sponge carrying the tissue may then be processed just as though it were a piece or tissue excised from the patient. That is to say the sponge may be promptly immersed in formaldehyde to stop any further growth and to harden the tissue. Then, usually at a subsequent time in the laboratory, the sponge may .be immersed in a dehydrating agent, impregnated with parafiin, sliced .by amicrotome and .placed on a microscope glass for microscopic examination by the pathologist. Selective acting stains may be used in the-usual fashion to visually develop or contrast the tissue structure.
Fig. 1 shows the rubbing step
Fig. 2 shows the immersion in formaldehyde
Fig. 4 the impregnation with or immersion in paraffin
Fig. 5 shows the sponge after solidification of the paraffin
Fig. 6 represents the piece from the microtome on the microscope glass
Fig. 7 shows the structure of the sponge and tissue as it appears under the microscope.
a sponge l is shown being held by forceps 2 and rubbed on a tumor 3 with a generally circular motion accompanied :by downward pressure as indicated by the arrows. Reciprocatory motion may also be used. As previously indicated the amount of pressure used depends on judgment. Ver light pressure might be used if the rubbing time is long enough and the maximum pressure used need not be sufli- .cient :to hurt or annoy the patient unduly.
Fig. 2 the sponge is shown immersed in a 7 bottle of formaldehyde. This step may be carried out promptly after the absorbing step and isfor the purpose or killing the tissue and hardening its structure. .It may be the same type .of fixing that is done in the case of an excised specimen.
Fig. 3 the sponge is shown immersed in a dehydrating agent which may be alcohol, acetone or the like.
a dehydrating agent which may be alcohol, acetone or the like.
the sponge is immersed in heated molten paraflin 4 in a pan 5 with the side of the sponge that was rubbed on the tumor down on the bottom of the pan.
the parafiin solidifies into a cake embodying the sponge as generally indicated by Fig. 5.
This cake may be easily handled by a microtome for slicing, as represented by the broken line shown, in the same manner that an excised tumor specimen is sliced to produce tissue thin enough for microscopic examination by transmitted light.
the usual practice of staining with various stains for developing the tissue structure may be followed after the slice of tissue has been floated on the microscope glass.
the final result is the microscope glass 6 carrying the microtome slice 'l' ready for microscopic examination by a pathologist.
Various kinds of sponges have been used in practicing the invention, as exemplified by cotton gauze, synthetic rubber sponge, natural sea sponge, blotting and tissue paper sponge, gelatin sponge and cellulose sponges of various pore sizes.
Cellulose sponge has the advantage that particles do not break oiT easily during the rubbing step and no diificulties are introduced during subsequent processing.
Cellulose sponge is not soluble in any of the materials customarily used to process an excised specimen and such as may be used in practicing this invention, and no operational difliculties are introduced during the operation of the microtome.
the color of the sponge should preferably be white since it permits easy visual determination of when the sponge has absorbed or picked up an adequate amount of matter from the tumor.
Fig. '7 shows, as well as can be done with pen and ink, the microscopic structure of the sponge and tissue at about 400 x magnification.
the cellular structure of the sponge l is easily distinguished from the characteristic appearance of the tissue 3, shown as cancerous.
a competent pathologist has no material difficulty in examining the tissue entrapped or absorbed in the pores or cavities of the sponge. It is to be emphasized that the tissue represents living tissue obtained directly from the tumor. Therefore, it has the characteristic appearance of living tissue obtained by excising a specimen from the tumor.
a method for examining a tumor to determine its type or condition comprising rubbing a sponge on the surface of the tumor to absorb tissue in the interstices of the sponge, treating said sponge to condition it for slicing, and slicing said sponge after said conditioning to'form a specimen adapted for microscopic examination thereof.
a sponge adapted to collect tissue from a tumor by contact therewith and which is sterile and insuiilated with a powdered agent for coagulating blood and serum, said sponge being a fine pore cellulose sponge.
a device for obtaining tumor tissue for mi croscopic-examination comprising a spongy mass of sterile elastic material containing a large number of pores or cavities for absorbing and retaining the tissue when rubbed on the tumor, with said material having adequate structural strength to resist material disintegration or fragmentation when rubbed on the tumor and having a composition insoluble in the agents used to process excised tissue specimens for microscopic examination and having physical properties permitting clean severance by a microtome, and with a substantial number of said pores or cavities ranging from .01 to .10 of an inch in size and dispersed throughout at least one surface of said mass, said mass bein adapted to be rubbed on a tumor and thereafter processed for microscopic examination in the manner of an excised tumor specimen.
a sponge adapted to collect tissue from a tumor by contact therewith and which is sterile and insuiilated with a powdered agent for coagulating blood and serum, said sponge being a fine pore cellulose sponge having a structure providing an average cavity size ranging from .01 to .10 of an inch.
a sponge adapted to collect tissue from a tumor by contact therewith and which is sterile and insuiilated with a powdered agent for coagulating blood and serum, said sponge being a fine pore cellulose sponge having a structure providing an average cavity size ranging from .01 to .10 of an inch and provided by blown cellulose bubbles with blown-out ruptures providing entrances thereto.
a method for examining a tumor to determine its type or condition comprising rubbing a sponge on the surface of the tumor to absorb tissue in the interstices of the sponge, and dehydrating said sponge, impregnating said sponge with molten paraflin and allowing the par-v afiin to solidify and form the sponge into a solid cake, and slicing said cake to form a specimen adapted for microscopic examination thereof.

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Health & Medical Sciences (AREA)
Life Sciences & Earth Sciences (AREA)
Medical Informatics (AREA)
Engineering & Computer Science (AREA)
Biomedical Technology (AREA)
Heart & Thoracic Surgery (AREA)
Pathology (AREA)
Molecular Biology (AREA)
Surgery (AREA)
Animal Behavior & Ethology (AREA)
General Health & Medical Sciences (AREA)
Public Health (AREA)
Veterinary Medicine (AREA)
Investigating Or Analysing Biological Materials (AREA)

Description

April 8, 1952 s. A. GLADSTONE 2,591,927

OBTAINING TUMOR TISSUE SPECIMEN Filed Oct. 6, 1948 2 SHEETSSHEET l INVENTOR. 5/04 51 ,4. z/lasm/vf A TTO/Q/VEVS April 8, 1952 s. A. GLADSTONE OBTAINING TUMOR TISSUE SPECIMEN '2 SHEETS-SHEET 2 Filed Oct. 6, 1948 INVENTOR. 670/1 51 A. GZAwm/VE A 7 f K Arum Ens Patented Apr. 8, 1952 UNITED STATES: PATENT OFF-ICE 9 Claims. 1

This-invention is concerned with the "problem of obtaining tissue from a tumor carried bya patient. Pathologists require such tissue .ior their determinations of whether tumors :are

malignant.

Hereto'fore, it has been usual to excise a'specimen from the tumor. This is very painfulior the patient and in many instances is extremely dangerous, such as when bleeding cannot be stopped or sterile conditions cannot be satisfactorily maintained. No other practice heretofore existed forobtaining living tissue fro-m'a tumor.

One object of the present invention is to obtain living tissue from a tumor for examination by a pathologist without excising a specimen from the tumor. Another object is 'toprovide a new means for removing the tissue and permitting its processing and examination in a manner easily followed by pathologists. Other objects may be inferred from the following.

The present invention is based on the discovery that when a sponge is rubbed over :a tumor of the type that might be suspected as being malignant, the interstices or pores, or cavities of the sponge pick up or absorb small particles of tissue which are retained or held with the sponge functioning as a carrier. The sponge 'may be processed for microscopic examination by a pathologist in the same fashion he would process a tissue specimen excised from a tumor. The appearance of the tissue carried or absorbed by the sponge, under the microscope, has been found to be such that a pathologist has no seri-v ous di'fficulty in diagnosing the tumor type or condition.

Although many kinds of sponges may be used with varying degrees of success, a new form of sponge has been developed in connection with .is sterile and which is insufiiated with a powdered agent for coagulating blood and serum which is normally absorbed with the tissue. The sponge dimensions depend on the location and accessibility of the tumor. The sponge may be of the type commercially known as a fine pore cellulose sponge. The cavities or poresare provided by blown cellulose bubbles and these have blown-but ruptures providing entrancestoithem. Thus the cavities or pores are able to pick up, absorb or entrap the tissue when the sponge is rubbed .on the tumor.

In practicing the invention in its presently preferred form the above described sponge in a dry condition is rubbed over the tumor carried by the patient. Judgment is needed in determining the rubbing pressure. However, no great amount of skill is required since a rubbing pressure light enough to avoid hurting or I materially annoying the patient or aggravating his condition, is sufficient to entrap or absorb the tissue in the pores ofthe sponge.

The sponge carrying the tissue may then be processed just as though it were a piece or tissue excised from the patient. That is to say the sponge may be promptly immersed in formaldehyde to stop any further growth and to harden the tissue. Then, usually at a subsequent time in the laboratory, the sponge may .be immersed in a dehydrating agent, impregnated with parafiin, sliced .by amicrotome and .placed on a microscope glass for microscopic examination by the pathologist. Selective acting stains may be used in the-usual fashion to visually develop or contrast the tissue structure.

The accompanying drawings illustrate the foregoing as follows:

Fig. 1 shows the rubbing step;

Fig. 2 shows the immersion in formaldehyde;

Fig. 3 the dehydrating;

Fig. 4 the impregnation with or immersion in paraffin;

Fig. 5 shows the sponge after solidification of the paraffin;

Fig. 6 represents the piece from the microtome on the microscope glass; and

Fig. 7 shows the structure of the sponge and tissue as it appears under the microscope.

In Fig. 1 a sponge l is shown being held by forceps 2 and rubbed on a tumor 3 with a generally circular motion accompanied :by downward pressure as indicated by the arrows. Reciprocatory motion may also be used. As previously indicated the amount of pressure used depends on judgment. Ver light pressure might be used if the rubbing time is long enough and the maximum pressure used need not be sufli- .cient :to hurt or annoy the patient unduly.

carried withor actually carrying the tissue :into

vthesponge. The sponge being sterile, there, :is little chance for infection since the amount "of tissue removed is extremely slight. No incision is made at all.

In Fig. 2 the sponge is shown immersed in a 7 bottle of formaldehyde. This step may be carried out promptly after the absorbing step and isfor the purpose or killing the tissue and hardening its structure. .It may be the same type .of fixing that is done in the case of an excised specimen.

Thereafter. usually .in the laboratory, the .re-

mainder of the processing is carried out. In Fig. 3 the sponge is shown immersed in a dehydrating agent which may be alcohol, acetone or the like. Next the sponge is immersed in heated molten paraflin 4 in a pan 5 with the side of the sponge that was rubbed on the tumor down on the bottom of the pan. After cooling the parafiin solidifies into a cake embodying the sponge as generally indicated by Fig. 5. This cake may be easily handled by a microtome for slicing, as represented by the broken line shown, in the same manner that an excised tumor specimen is sliced to produce tissue thin enough for microscopic examination by transmitted light. The usual practice of staining with various stains for developing the tissue structure may be followed after the slice of tissue has been floated on the microscope glass.

The final result is the microscope glass 6 carrying the microtome slice 'l' ready for microscopic examination by a pathologist.

It is important to note that all of the foregoing steps are familiar to pathologists excepting for the fact that instead of using an excised specimen, with its attendant pain and dangers to the patient, a suitable sponge is simply rubbed firmly on the tumor and then handled in the manner of an excised specimen.

Various kinds of sponges have been used in practicing the invention, as exemplified by cotton gauze, synthetic rubber sponge, natural sea sponge, blotting and tissue paper sponge, gelatin sponge and cellulose sponges of various pore sizes. Cellulose sponge has the advantage that particles do not break oiT easily during the rubbing step and no diificulties are introduced during subsequent processing. Cellulose sponge is not soluble in any of the materials customarily used to process an excised specimen and such as may be used in practicing this invention, and no operational difliculties are introduced during the operation of the microtome. For practical reasons the color of the sponge should preferably be white since it permits easy visual determination of when the sponge has absorbed or picked up an adequate amount of matter from the tumor.

Fig. '7 shows, as well as can be done with pen and ink, the microscopic structure of the sponge and tissue at about 400 x magnification. The cellular structure of the sponge l is easily distinguished from the characteristic appearance of the tissue 3, shown as cancerous. A competent pathologist has no material difficulty in examining the tissue entrapped or absorbed in the pores or cavities of the sponge. It is to be emphasized that the tissue represents living tissue obtained directly from the tumor. Therefore, it has the characteristic appearance of living tissue obtained by excising a specimen from the tumor.

blood and serum, prior to said rubbing, and with said sponge comprising a fine pore cellulose sponge.

3. A method for examining a tumor to determine its type or condition, said method comprising rubbing a sponge on the surface of the tumor to absorb tissue in the interstices of the sponge, treating said sponge to condition it for slicing, and slicing said sponge after said conditioning to'form a specimen adapted for microscopic examination thereof.

4. A method as defined by claim 3 wherein said sponge is insufflated with a powdered agent for coagulating blood and serum, prior to said rubbing.

5. A sponge adapted to collect tissue from a tumor by contact therewith and which is sterile and insuiilated with a powdered agent for coagulating blood and serum, said sponge being a fine pore cellulose sponge.

6. A device for obtaining tumor tissue for mi croscopic-examination, said device comprising a spongy mass of sterile elastic material containing a large number of pores or cavities for absorbing and retaining the tissue when rubbed on the tumor, with said material having adequate structural strength to resist material disintegration or fragmentation when rubbed on the tumor and having a composition insoluble in the agents used to process excised tissue specimens for microscopic examination and having physical properties permitting clean severance by a microtome, and with a substantial number of said pores or cavities ranging from .01 to .10 of an inch in size and dispersed throughout at least one surface of said mass, said mass bein adapted to be rubbed on a tumor and thereafter processed for microscopic examination in the manner of an excised tumor specimen.

'7. A sponge adapted to collect tissue from a tumor by contact therewith and which is sterile and insuiilated with a powdered agent for coagulating blood and serum, said sponge being a fine pore cellulose sponge having a structure providing an average cavity size ranging from .01 to .10 of an inch. 1

8. A sponge adapted to collect tissue from a tumor by contact therewith and which is sterile and insuiilated with a powdered agent for coagulating blood and serum, said sponge being a fine pore cellulose sponge having a structure providing an average cavity size ranging from .01 to .10 of an inch and provided by blown cellulose bubbles with blown-out ruptures providing entrances thereto.

9. A method for examining a tumor to determine its type or condition, said method comprising rubbing a sponge on the surface of the tumor to absorb tissue in the interstices of the sponge, and dehydrating said sponge, impregnating said sponge with molten paraflin and allowing the par-v afiin to solidify and form the sponge into a solid cake, and slicing said cake to form a specimen adapted for microscopic examination thereof.

SIDNEY A. GLADSTONE.

Name Date Correll Mar. 29, 1949 OTHER REFERENCES Pages 539-541 of Standard Methods by Wadsworth, published in 1947 by Williams and Wilkins Co., Baltimore, Md. (A copy is available in Div. 43 of the U. S. Patent Office.)

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US53131A 1948-10-06 1948-10-06 Obtaining tumor tissue specimen Expired - Lifetime US2591927A (en)

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US53131A US2591927A (en)	1948-10-06	1948-10-06	Obtaining tumor tissue specimen

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US53131A US2591927A (en)	1948-10-06	1948-10-06	Obtaining tumor tissue specimen

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Cited By (10)

* Cited by examiner, † Cited by third party
Publication number	Priority date	Publication date	Assignee	Title
US3037495A (en) *	1959-07-17	1962-06-05	John F Naz	Biopsy device
US3815580A (en) *	1972-08-31	1974-06-11	C Oster	Apparatus for and method of collecting and preserving cytologic samples
US3945372A (en) *	1973-06-01	1976-03-23	Milan Albert R	Medical tissue-obtaining system
US4175439A (en) *	1977-05-13	1979-11-27	Laker Thomas L	Apparatus and method for collecting, storage and transporting liquid samples for diagnostic examination
US5031635A (en) *	1982-03-01	1991-07-16	Accu-Med Corporation	Plastic molded biological sample collection swab
US5103836A (en) *	1990-02-28	1992-04-14	Epitope, Inc.	Oral collection device and kit for immunoassay
US5858781A (en) *	1994-05-13	1999-01-12	Matyas; John R.	Method of tissue transfer and retrieval
US5968746A (en) *	1997-11-26	1999-10-19	Schneider; David R.	Method and apparatus for preserving human saliva for testing
US20040087874A1 (en) *	2002-10-28	2004-05-06	David Schneider	Saliva collection system
US20080139962A1 (en) *	2004-12-14	2008-06-12	Ahmed Jehanli	Analyte Collection Apparatus and Method

Citations (1)

* Cited by examiner, † Cited by third party
Publication number	Priority date	Publication date	Assignee	Title
US2465357A (en) *	1944-08-14	1949-03-29	Upjohn Co	Therapeutic sponge and method of making

1948
- 1948-10-06 US US53131A patent/US2591927A/en not_active Expired - Lifetime

Patent Citations (1)

* Cited by examiner, † Cited by third party
Publication number	Priority date	Publication date	Assignee	Title
US2465357A (en) *	1944-08-14	1949-03-29	Upjohn Co	Therapeutic sponge and method of making

Cited By (12)

* Cited by examiner, † Cited by third party
Publication number	Priority date	Publication date	Assignee	Title
US3037495A (en) *	1959-07-17	1962-06-05	John F Naz	Biopsy device
US3815580A (en) *	1972-08-31	1974-06-11	C Oster	Apparatus for and method of collecting and preserving cytologic samples
US3945372A (en) *	1973-06-01	1976-03-23	Milan Albert R	Medical tissue-obtaining system
US4175439A (en) *	1977-05-13	1979-11-27	Laker Thomas L	Apparatus and method for collecting, storage and transporting liquid samples for diagnostic examination
US5031635A (en) *	1982-03-01	1991-07-16	Accu-Med Corporation	Plastic molded biological sample collection swab
US5103836A (en) *	1990-02-28	1992-04-14	Epitope, Inc.	Oral collection device and kit for immunoassay
US5858781A (en) *	1994-05-13	1999-01-12	Matyas; John R.	Method of tissue transfer and retrieval
US5866417A (en) *	1994-05-13	1999-02-02	Matyas; John R.	Method of tissue transfer
US5968746A (en) *	1997-11-26	1999-10-19	Schneider; David R.	Method and apparatus for preserving human saliva for testing
US6291178B1 (en)	1997-11-26	2001-09-18	David R. Schneider	Method and apparatus for preserving human saliva for testing
US20040087874A1 (en) *	2002-10-28	2004-05-06	David Schneider	Saliva collection system
US20080139962A1 (en) *	2004-12-14	2008-06-12	Ahmed Jehanli	Analyte Collection Apparatus and Method

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Schneider et al.	1950	Nuclei from normal and leukemic mouse spleen: I. The isolation of nuclei in neutral medium
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Guyer	1917	Animal micrology
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US3870789A (en)	1975-03-11	Enhancement of morphologic detail in tissue
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US20190178761A1 (en)	2019-06-13	Method and apparatus for cell block preparation of cytology specimens
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Teesdale et al.	1976	A simple thick-smear technique for the diagnosis of Schistosoma mansoni infection
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Wetzel	1961	Sodium permanganate fixation for electron microscopy
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