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US20020164656A1 - Microarrays and uses therefor - Google Patents

Microarrays and uses therefor
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Publication number
US20020164656A1
US20020164656A1US10/035,368US3536801AUS2002164656A1US 20020164656 A1US20020164656 A1US 20020164656A1US 3536801 AUS3536801 AUS 3536801AUS 2002164656 A1US2002164656 A1US 2002164656A1
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United States
Prior art keywords
antibodies
antigen
cells
protein
binding
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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.)
Abandoned
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US10/035,368
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James Hoeffler
Joseph Fernandez
Marc Nasoff
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Individual
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Priority to US10/035,368priorityCriticalpatent/US20020164656A1/en
Publication of US20020164656A1publicationCriticalpatent/US20020164656A1/en
Assigned to BANK OF AMERICA, N.A., AS COLLATERAL AGENTreassignmentBANK OF AMERICA, N.A., AS COLLATERAL AGENTSECURITY AGREEMENTAssignors: Life Technologies Corporation
Priority to US12/490,069prioritypatent/US8012703B2/en
Priority to US13/173,637prioritypatent/US8637264B2/en
Priority to US13/648,169prioritypatent/US20130123127A1/en
Assigned to Life Technologies CorporationreassignmentLife Technologies CorporationLIEN RELEASEAssignors: BANK OF AMERICA, N.A.
Abandonedlegal-statusCriticalCurrent

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Abstract

Methods of using microarrays to simplify analysis and characterization of genes and their function are provided. Such methods can be used to identify and characterize antibodies having binding affinity for a specific target antigen. A method of determining gene expression at the protein level by contacting an array of characterized or uncharacterized antibodies on a solid surface with one or more proteins and identifying the antibodies to which said protein(s) binds also is provided. This method can be used to compare the protein expression in two different populations of cells, such as normal cells and cancer cells or resting cells and stimulated cells. In addition, a method of determining gene expression at the protein level by contacting a microarray of nucleic acid samples derived from a variety of different sources with one or more nucleic acid probes then identifying the sample or samples to which the probe binds is provided.

Description

Claims (50)

That which is claimed is:
1. A method of identifying antibodies having binding affinity for an antigen, said method comprising:
(a) contacting an array of uncharacterized antibodies on a solid surface with at least one antigen; and
(b) identifying the antibodies to which the antigen binds.
2. A method according toclaim 1 wherein the antigen is a protein.
3. A method according toclaim 1 wherein the antigen is an intact cell.
4. A method according toclaim 1 wherein the antigen is a cell lysate.
5. A method according toclaim 2 wherein the protein is recombinant.
6. A method according toclaim 5 wherein the protein is full-length.
7. A method according toclaim 5 wherein the protein is a protein fragment.
8. A method according toclaim 7 wherein the protein fragment is encoded by an EST fragment.
9. A method according toclaim 1 wherein the antibodies are monoclonal antibodies.
10. A method according toclaim 1 wherein the antibodies are polyclonal antibodies.
11. A method according toclaim 1 wherein the antibodies are antibody fragments.
12. A method according toclaim 11 wherein the antibody fragments are single chain antibodies.
13. A method according toclaim 1 wherein the antibodies are recombinant antibodies.
14. A method according toclaim 1 wherein the antigen is detectably labeled.
15. A method according toclaim 14 wherein the detectable label is a fluorescent moiety, avidin, streptavidin, or biotin.
16. A method according toclaim 1 wherein the antigen is a fusion protein comprised of an epitope tag or a fluorescent protein.
17. A method according toclaim 1 wherein the binding affinity of said antibody for said antigen is determined by iterative washing of said solid surface with a suitable diluent and detecting when antigen is no longer released therefrom.
18. A method of comparing protein expression in two or more populations of cells, said method comprising:
(a) contacting an array of antibodies on a solid surface with a cell lysate of a first cell population, generating a first binding pattern;
(b) contacting a duplicate array of antibodies on a solid surface with a cell lysate of a second cell population, generating a second binding pattern; and
(c) comparing the binding pattern of the first cell lysate with the binding pattern of the second cell lysate.
19. A method according toclaim 18 wherein the antibodies are uncharacterized antibodies.
20. A method according toclaim 18 wherein the antibodies are recombinant antibodies.
21. A method according toclaim 18 wherein the first cell lysate is derived from normal cells and the second cell lysate is derived from abnormal cells.
22. A method according toclaim 21 wherein the abnormal cells are cancer cells.
23. A method according toclaim 18 wherein the first cell lysate is derived from normal cells in a resting state and the second cell lysate is derived from normal cells in a stimulated state.
24. A method according toclaim 18 wherein the difference between the first and second set of cells is the presence of a different detectable label.
25. A method for determining the effect of varying binding conditions on the binding affinity of antibodies to a specific antigen, said method comprising:
(a) contacting an array of antibodies on a solid surface with at least one antigen under a first set of binding conditions, generating a first binding pattern;
(b) contacting a duplicate array with the antigen under a second set of binding conditions, generating a second binding pattern;
(c) comparing the first and second binding patterns.
26. A method according toclaim 21 wherein said varying binding conditions comprise varying pH, temperature, salt concentration, and/or duration.
27. A method for characterizing a cell, based on the pattern of protein expression produced thereby, said method comprising:
(a) contacting an array of antibodies on a solid surface with a cell lysate; and
(b) identifying the profile of antibodies to which components of the lysate binds.
28. A method of diagnosing a disorder, said method comprising:
(a) contacting an array of antibodies specific for one or more antigens characteristic of a disorder with a biological sample obtained from a subject under conditions suitable for the formation of an antigen:antibody complex, wherein the presence of the antigens in the biological sample would be indicative of the disorder;
and
(b) detecting the formation of any antibody: antigen complexes.
29. A method according toclaim 28 wherein the biological sample is cerebral spinal fluid, blood, plasma, urine, feces, saliva, tears, or extracted tissue.
30. A method according toclaim 29 wherein the disorder is stroke, cerebral hemorrhage, myocardial infarction, peripheral blood clots, diabetes, cancer, Alzheimer's disease, and sepsis.
31. A kit comprising:
(a) an array of uncharacterized antibodies on a solid surface; and
(b) instructions for using the array.
32. A kit according toclaim 31 wherein the instructions are for identifying antibodies to a specific antigen, comparing protein expression in two or more populations of cells, characterizing a cell based on the pattern of protein expression produced thereby, or determining the effect of varying binding conditions on the binding affinity of the antibodies.
33. A kit according toclaim 31 wherein the antibodies are monoclonal antibodies, polyclonal antibodies or antibody fragments.
34. A kit according toclaim 33 wherein the antibody fragments are single chain antibodies.
35. A kit according toclaim 31 wherein the antibodies are recombinant antibodies.
36. A kit according toclaim 31 further comprising reagents for detecting an antigen and instructions for use thereof.
37. A kit comprising:
(a) an array of antibodies on a solid surface; and
(b) instructions for using the array; wherein the instructions are for diagnosing a disorder, characterizing a cell based on the pattern of protein expression produced thereby, or comparing protein expression in two or more populations of cells.
38. A kit according toclaim 37 further comprising reagents for detecting an antigen and instructions for use thereof.
39. A kit according toclaim 37 wherein the antibodies are recombinant antibodies.
40. A kit according toclaim 37 wherein the antibodies are single chain antibodies.
41. A method of comparing protein expression patterns, said method comprising:
(a) contacting a microarray of nucleic acid samples derived from different sources with one or more nucleic acid probes and
(b) identifying the sample or samples to which the probe(s) binds.
42. A method according toclaim 41 wherein the microarray comprises nucleic acid samples derived from a single tissue type but from different species.
43. A method according toclaim 41 wherein the microarray comprises nucleic acid samples derived from a single species but from different tissue types.
44. A method according toclaim 41 wherein the microarray comprises nucleic acid samples derived from the same tissue type at different developmental stages.
45. A method according toclaim 41 wherein the nucleic acid samples are comprised of mRNA or cDNA.
46. A method according toclaim 41 wherein the probe is detectably labeled.
47. A method according toclaim 46 wherein the detectable label is a fluorescent label.
48. A method according toclaim 18 wherein the first and second cell lysates are derived from cells from a single tissue type but from different species.
49. A method according toclaim 18 wherein the first and second cell lysates are derived from cells from a single species but from different tissue types.
50. A method according toclaim 18 wherein the first and second cell lysates are derived from cells from the same tissue type at different developmental stages.
US10/035,3681998-02-042001-10-26Microarrays and uses thereforAbandonedUS20020164656A1 (en)

Priority Applications (4)

Application NumberPriority DateFiling DateTitle
US10/035,368US20020164656A1 (en)1998-02-042001-10-26Microarrays and uses therefor
US12/490,069US8012703B2 (en)1998-02-042009-06-23Microarrays and uses therefor
US13/173,637US8637264B2 (en)1998-02-042011-06-30Microarrays and uses therefor
US13/648,169US20130123127A1 (en)1998-02-042012-10-09Microarrays and uses thereof

Applications Claiming Priority (3)

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US7360598P1998-02-041998-02-04
US09/245,615US7794946B1 (en)1998-02-041999-02-04Microarray and uses therefor
US10/035,368US20020164656A1 (en)1998-02-042001-10-26Microarrays and uses therefor

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US09/245,615DivisionUS7794946B1 (en)1998-02-041999-02-04Microarray and uses therefor

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US12/490,069ContinuationUS8012703B2 (en)1998-02-042009-06-23Microarrays and uses therefor

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US20020164656A1true US20020164656A1 (en)2002-11-07

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US09/245,615Expired - Fee RelatedUS7794946B1 (en)1998-02-041999-02-04Microarray and uses therefor
US10/035,368AbandonedUS20020164656A1 (en)1998-02-042001-10-26Microarrays and uses therefor
US12/490,069Expired - Fee RelatedUS8012703B2 (en)1998-02-042009-06-23Microarrays and uses therefor
US13/173,637Expired - Fee RelatedUS8637264B2 (en)1998-02-042011-06-30Microarrays and uses therefor
US13/648,169AbandonedUS20130123127A1 (en)1998-02-042012-10-09Microarrays and uses thereof

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US12/490,069Expired - Fee RelatedUS8012703B2 (en)1998-02-042009-06-23Microarrays and uses therefor
US13/173,637Expired - Fee RelatedUS8637264B2 (en)1998-02-042011-06-30Microarrays and uses therefor
US13/648,169AbandonedUS20130123127A1 (en)1998-02-042012-10-09Microarrays and uses thereof

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US (5)US7794946B1 (en)
EP (3)EP1060395B1 (en)
JP (1)JP2002502977A (en)
AT (1)ATE393912T1 (en)
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CA (1)CA2318175A1 (en)
DE (1)DE69938623T2 (en)
WO (1)WO1999040434A1 (en)

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US8637264B2 (en)2014-01-28
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EP2189791A3 (en)2011-03-09
WO1999040434A1 (en)1999-08-12
EP1965213A2 (en)2008-09-03
EP1060395B1 (en)2008-04-30
EP2189791A2 (en)2010-05-26
EP1060395A4 (en)2005-02-09
US7794946B1 (en)2010-09-14
US20100022407A1 (en)2010-01-28
CA2318175A1 (en)1999-08-12
US20120004131A1 (en)2012-01-05
DE69938623T2 (en)2009-05-28
AU2583899A (en)1999-08-23
JP2002502977A (en)2002-01-29
US20130123127A1 (en)2013-05-16
EP1965213A3 (en)2009-07-15
US8012703B2 (en)2011-09-06
ATE393912T1 (en)2008-05-15

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