Analysis of circulating tumor cells, fragments, and debris

US 7,863,012 B2
Filed: 02/17/2004
Issued: 01/04/2011
Est. Priority Date: 02/17/2004
Status: Expired due to Fees

First Claim

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1. A method for monitoring malignancy in a test subject comprising:

a. obtaining a blood sample from a test subject, said sample comprising a mixed cell population suspected of containing intact malignant cancer cells of epithelial cell origin and further comprising;

i. cell fragments derived from said malignant cells, and/orii. cellular debris derived from said malignant cells;

b. preparing a sample with magnetically-labeled said intact malignant cells, said cell fragments and said cellular debris wherein said blood sample is mixed with colloidal magnetic particles, having a size range between 90 to 150 nm and a bovine serum albumin coating using high temperature, coupled to a first biospecific ligand which reacts and binds specifically to an epitope present in each of said intact malignant cells, said cell fragments and said cellular debris to form specific binding complexes with said colloidal magnetic particles and first biospecific ligand;

c. exposing said specific binding complexes formed in step b) to an externally-applied high gradient magnetic field to the substantial exclusion of other specimen components;

d. contacting said specific binding complexes in step c) with at least one additional biospecific ligand forming a specific binding pair with a receptor of said intact malignant cells, said cell fragments and said cellular debris, to the substantial exclusion of other specimen components, wherein the receptor is present in malignant tumor cells of epithelial cell origin;

e. differentially analyzing amounts of said labeled malignant cells, said labeled cell fragments and said labeled cellular debris in step d) over time, a change in the numerical proportions of said labeled malignant cells, said labeled cell fragments, and said labeled cellular debris indicating a change of malignancy.

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Abstract

The methods and reagents described in this invention are used to analyze circulating tumor cells, clusters, fragments, and debris. Analysis is performed with a number of platforms, including flow cytometry and the CellSpotter® fluorescent microscopy imaging system. Analyzing damaged cells has shown to be important. However, there are two sources of damage: in vivo and in vitro. Damage in vivo occurs by apoptosis, necrosis, or immune response. Damage in vitro occurs during sample acquisition, handling, transport, processing, or analysis. It is therefore desirable to confine, reduce, eliminate, or at least qualify in vitro damage to prevent it from interfering in analysis. Described herein are methods to diagnose, monitor, and screen disease based on circulating rare cells, including malignancy as determined by CTC, clusters, fragments, and debris. Also provided are kits for assaying biological specimens using these methods.

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16 Claims

1. A method for monitoring malignancy in a test subject comprising:
- a. obtaining a blood sample from a test subject, said sample comprising a mixed cell population suspected of containing intact malignant cancer cells of epithelial cell origin and further comprising;
  
  i. cell fragments derived from said malignant cells, and/orii. cellular debris derived from said malignant cells;
  
  b. preparing a sample with magnetically-labeled said intact malignant cells, said cell fragments and said cellular debris wherein said blood sample is mixed with colloidal magnetic particles, having a size range between 90 to 150 nm and a bovine serum albumin coating using high temperature, coupled to a first biospecific ligand which reacts and binds specifically to an epitope present in each of said intact malignant cells, said cell fragments and said cellular debris to form specific binding complexes with said colloidal magnetic particles and first biospecific ligand;
  
  c. exposing said specific binding complexes formed in step b) to an externally-applied high gradient magnetic field to the substantial exclusion of other specimen components;
  
  d. contacting said specific binding complexes in step c) with at least one additional biospecific ligand forming a specific binding pair with a receptor of said intact malignant cells, said cell fragments and said cellular debris, to the substantial exclusion of other specimen components, wherein the receptor is present in malignant tumor cells of epithelial cell origin;
  
  e. differentially analyzing amounts of said labeled malignant cells, said labeled cell fragments and said labeled cellular debris in step d) over time, a change in the numerical proportions of said labeled malignant cells, said labeled cell fragments, and said labeled cellular debris indicating a change of malignancy.
- View Dependent Claims (2, 3, 4, 5, 6, 7, 8)
- - 2. The method of claim 1, wherein said is blood sample is whole blood sample.
  - 3. The method of claim 2, wherein after said blood sample is obtained, it is contacted with an agent capable of stabilizing said blood sample.
  - 4. The method of claim 1, wherein after the step of preparing said magnetically-labeled sample, said sample is subjected to a high gradient magnetic field to produce a separated magnetically-labeled fraction which is enriched for said intact malignant cells, and said cell fragments and said cellular debris.
  - 5. The method of claim 1, wherein said analysis is selected from the group consisting of:
    - multiparameter flow cytometry, immunofluorescent microscopy, laser scanning cytometry, bright field base image analysis, capillary volumetry, spectral imaging analysis, manual cell analysis, and automated cell analysis.
  - 6. The method of claim 1, wherein said analysis further comprises classifying cell fragments or said cellular debris based on their origin as caused by apoptosis or necrosis and wherein said additional biospecific ligand is directed against cytokeratin.
  - 7. The method of claim 6, wherein analysis further comprises classifying cell fragments or said cellular debris based on their origin as caused by mechanical damage, drug-induced damage, or immunological damage and wherein said additional biospecific ligand is directed against cytokeratin.
  - 8. The method of claim 6, wherein said classification is based on at least one of the group consisting of:
    - morphologic analysis and epitopic analysis.

9. A method for monitoring malignancy in a test subject comprising:
- a. obtaining a blood sample from a test subject, said sample comprising a mixed cell population suspected of containing intact malignant cancer cells of epithelial cell origin and clusters of said malignant cells;
  
  b. preparing a sample with magnetically-labeled said intact malignant cells and said clusters of malignant cells wherein said blood sample is mixed with colloidal magnetic particles, having a size range between 90 to 150 nm and a bovine serum albumin coating using high temperature, coupled to a first biospecific ligand which reacts and binds specifically to an epitope present in each of said intact malignant cells and said clusters of malignant cells to form specific binding complexes with said colloidal magnetic particles and first biospecific ligand;
  
  c. exposing said specific binding complexes formed in step b) to an externally-applied high gradient magnetic field to the substantial exclusion of other specimen components;
  
  d. contacting said specific binding complexes in step c) with at least one additional biospecific ligand forming a specific binding pair with a receptor of said intact malignant cells and said clusters of malignant cells, to the substantial exclusion of other specimen components, wherein the receptor is present in malignant tumor cells of epithelial cell origin;
  
  e. differentially analyzing amounts of said labeled malignant cells and said labeled clusters of malignant cells in step d) over time, a change in the numerical proportions of said labeled malignant cells and said labeled clusters of malignant cells indicating a change of malignancy.
- View Dependent Claims (10, 11, 12, 13)
- - 10. The method of claim 9, wherein said is blood sample is whole blood sample.
  - 11. The method of claim 10, wherein after said blood sample is obtained, it is contacted with an agent capable of stabilizing said blood sample.
  - 12. The method of claim 9, wherein after the step of preparing said magnetically-labeled sample, said sample is subjected to a high gradient magnetic field to produce a separated magnetically-labeled fraction which is enriched for said intact malignant cells and said clusters of malignant cells.
  - 13. The method of claim 9, wherein said analysis is selected from the group consisting of:
    - multiparameter flow cytometry, immunofluorescent microscopy, laser, scanning cytometry, bright field base image analysis, capillary volumetry, spectral imaging analysis, manual cell analysis, and automated cell analysis.

14. A kit for assaying a blood sample suspected of containing intact malignant cancer cells of epithelial cell origin for the presence of malignant cells, cell fragments derived from malignant cells and cellular debris derived from malignant cells, comprising:
- a. coated colloidal magnetic nanoparticles comprising;
  
  i. a magnetic core material having a size range between 90 to 150 nm;
  
  ii. a protein base coating comprising bovine serum albumin applied using high temperature; and
  
  iii. an antibody that binds specifically to an epitope present in each of said intact malignant cells, said cell fragments and said cellular debris, wherein said antibody is coupled to said protein base coating on the colloidal magnetic nanoparticle;
  
  b. at least one antibody having binding specificity for a receptor of said malignant cell, said cell fragments and said cellular debris, and wherein the receptor is present in malignant tumor cells of epithelial cell origin; and
  
  c. an agent capable of staining further morphological features of said malignant cells, said cell fragments and said cellular debris.
- View Dependent Claims (15, 16)
- - 15. The kit of claim 14, further comprising a panel of antibodies each specific for a different characteristic determinant.
  - 16. The kit of claim 14, further comprising a specific agent capable of labeling non-target entities.

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Current Assignee
Menarini Silicon Biosystems S.P.A
Original Assignee
Veridex LLC (Johnson & Johnson)
Inventors
O'Hara, Shawn Mark, Rao, Galla Chandra, Repollet, Madeline, Rutner, Herman, Larson, Christopher, Gross, Steven, Terstappen, Leon W. M. M.
Primary Examiner(s)
GABEL, GAILENE

Application Number

US10/780,399
Publication Number

US 20050181463A1
Time in Patent Office

2,513 Days
Field of Search

435/2, 435/7.21, 435/7.23, 435/7.24, 435/287.2, 435/962, 435/7.94, 436/526, 436/518, 436/64, 436/164, 436/175, 436/177, 436/813, 436/824, 436/825, 436/501, 436/538, 436/10, 530/388.8, 530/389.7, 530/413, 422/61, 422/73, 422/101
US Class Current

435/7.23
CPC Class Codes

G01N 33/54326   Magnetic particles

G01N 33/574   for cancer

Y10S 436/813   Cancer

Y10T 436/101666   Particle count or volume st...

Y10T 436/25125   Digestion or removing inter...

Y10T 436/25375   Liberation or purification ...

Analysis of circulating tumor cells, fragments, and debris

First Claim

4 Assignments

0 Petitions

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Abstract

144 Citations

16 Claims

Specification

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Analysis of circulating tumor cells, fragments, and debris

First Claim

4 Assignments

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0 Petitions

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Accused Products

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Abstract

144 Citations

16 Claims

Specification

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Solutions

Use Cases

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