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US20080254489A1 - Methods and compositions for risk stratification - Google Patents

Methods and compositions for risk stratification
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Publication number
US20080254489A1
US20080254489A1US12/061,565US6156508AUS2008254489A1US 20080254489 A1US20080254489 A1US 20080254489A1US 6156508 AUS6156508 AUS 6156508AUS 2008254489 A1US2008254489 A1US 2008254489A1
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marker
cells
activation
cell
sample
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US12/061,565
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Omar D. Perez
Garry P. Nolan
Jonathan M. Irish
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Leland Stanford Junior University
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Assigned to THE BOARD OF TRUSTEES OF THE LELAND STANFORD JUNIOR UNIVERSITYreassignmentTHE BOARD OF TRUSTEES OF THE LELAND STANFORD JUNIOR UNIVERSITYASSIGNMENT OF ASSIGNORS INTEREST (SEE DOCUMENT FOR DETAILS).Assignors: IRISH, JONATHAN M., NOLAN, GARRY P., PEREZ, OMAR D.
Publication of US20080254489A1publicationCriticalpatent/US20080254489A1/en
Priority to US13/082,306prioritypatent/US20110269634A1/en
Abandonedlegal-statusCriticalCurrent

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Abstract

The present invention provides an approach for the simultaneous determination of the activation states of a plurality of proteins in single cells. This approach permits the rapid detection of heterogeneity in a complex cell population based on activation states, and the identification of cellular subsets that exhibit correlated changes in activation within the cell population. Moreover, this approach allows the correlation of cellular activities or properties. In addition, the use of potentiators of cellular activation allows for characterization of such pathways and cell populations.

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Claims (39)

14. A method for establishing a composite marker profile for a sample derived from an individual suspected having a neoplastic condition, the method comprising the steps of: (a) reacting the biological sample with a collection of binding molecules, wherein the collection of binding molecules contains two or more groups of binding molecules specific for distinct cell population associated markers, wherein marker levels and marker combinations identify normal and neoplastic cell populations internal to the sample, (b) identifying the presence of normal and neoplastic cell populations internal to the sample by detecting the marker levels and marker combinations that identify the normal and neoplastic cell populations internal to the sample, and (c) correlating the marker levels across each of the normal and neoplastic cell populations with the presence of a target protein to establish a composite marker profile for a sample derived from an individual suspected having a neoplastic condition.
29. A method for predicting the clinical course of Ig-unmutated B-cell Chronic Lymphocytic Leukemia (CLL) in an individual, the method comprising the steps of: (a) providing a biological sample derived from the individual; (b) reacting the biological sample with a collection of binding molecules, wherein the collection of binding molecules contains two or more groups of binding molecules specific for distinct cell population associated markers, wherein marker levels and marker combinations identify normal and neoplastic cell populations internal to the sample, (c) identifying the presence of normal and neoplastic cell populations internal to the sample by detecting the marker levels and marker combinations that identify the normal and neoplastic cell populations internal to the sample, (d) correlating the marker levels across each of the normal and neoplastic cell populations with the presence of at least one signal transduction protein to establish a composite marker profile for a sample derived from an individual suspected having B-Cell Chronic Lymphocytic Leukemia (B-CLL), wherein the composite profile represents a relative quantification of levels of said signal transduction protein; and (e) comparing the composite profile to one or more reference composite profiles, wherein the comparison allows for predicting the clinical course of Ig-unmutated B-cell Chronic Lymphocytic Leukemia (CLL).
30. A method for establishing a composite marker profile for a sample derived from an individual suspected having Chronic Myelogenous Leukemia (CML), the method comprising the steps of: (a) reacting the biological sample with a collection of binding molecules, wherein the collection of binding molecules contains two or more groups of binding molecules specific for distinct cell population associated markers, wherein marker levels and marker combinations identify normal and neoplastic cell populations internal to the sample, (b) identifying the presence of normal and neoplastic cell populations internal to the sample by detecting the marker levels and marker combinations that identify the normal and neoplastic cell populations internal to the sample, and (c) correlating the marker levels across each of the normal and neoplastic cell populations with the presence of at least one target protein selected from the group consisting of activation-phosphorylated signal transduction proteins, proliferation markers, differentiation markers and apoptosis markers to establish a composite marker profile for a sample derived from an individual suspected having Chronic Myelogenous Leukemia (CML).
37. A method for predicting the clinical course of Chronic Myelogenous Leukemia (CML) in an individual, the method comprising the steps of: (a) providing a biological sample derived from the individual; (b) reacting the biological sample with a collection of binding molecules, wherein the collection of binding molecules contains two or more groups of binding molecules specific for distinct cell population associated markers, wherein marker levels and marker combinations identify normal and neoplastic cell populations internal to the sample, (c) identifying the presence of normal and neoplastic cell populations internal to the sample by detecting the marker levels and marker combinations that identify the normal and neoplastic cell populations internal to the sample, (d) correlating the marker levels across each of the normal and neoplastic cell populations with the presence of at least one target protein selected from the group consisting of activation-phosphorylated signal transduction proteins, proliferation markers and apoptosis markers to establish a composite marker profile for a sample derived from an individual suspected having Chronic Myelogenous Leukemia (CML), and (e) comparing the composite profile to one or more reference composite profiles, wherein the comparison allows for predicting the clinical course of Chronic Myelogenous Leukemia (CML).
38. A method for establishing a composite marker profile for a sample derived from an individual suspected having Acute Myelogenous Leukemia (AML), the method comprising the steps of: (a) reacting the biological sample with a collection of binding molecules, wherein the collection of binding molecules contains two or more groups of binding molecules specific for distinct cell population associated markers, wherein marker levels and marker combinations identify normal and neoplastic cell populations internal to the sample, (b) identifying the presence of normal and neoplastic cell populations internal to the sample by detecting the marker levels and marker combinations that identify the normal and neoplastic cell populations internal to the sample, and (c) correlating the marker levels across each of the normal and neoplastic cell populations with the presence of at least one target protein selected from the group consisting of activation-phosphorylated signal transduction proteins, proliferation markers and apoptosis markers to establish a composite marker profile for a sample derived from an individual suspected having Acute Myelogenous Leukemia (AML).
46. A method for predicting the clinical course of Acute Myelogenous Leukemia (AML) in an individual, the method comprising the steps of: (b) reacting the biological sample obtained from the individual with a collection of binding molecules, wherein the collection of binding molecules contains two or more groups of binding molecules specific for distinct cell population associated markers, wherein marker levels and marker combinations identify normal and neoplastic cell populations internal to the sample, (c) identifying the presence of normal and neoplastic cell populations internal to the sample by detecting the marker levels and marker combinations that identify the normal and neoplastic cell populations internal to the sample, (d) correlating the marker levels across each of the normal and neoplastic cell populations with the presence of at least one target protein selected from the group consisting of activation-phosphorylated signal transduction proteins, proliferation markers and apoptosis markers to establish a composite marker profile for a sample derived from an individual suspected having Acute Myelogenous Leukemia (AML); and (e) comparing the composite profile to one or more reference composite profiles, wherein the comparison allows for predicting the clinical course of Acute Myelogenous Leukemia (AML).
US12/061,5652001-07-102008-04-02Methods and compositions for risk stratificationAbandonedUS20080254489A1 (en)

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US12/061,565US20080254489A1 (en)2004-07-212008-04-02Methods and compositions for risk stratification
US13/082,306US20110269634A1 (en)2001-07-102011-04-07Methods and Compositions for Risk Stratification

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US10/898,734US7393656B2 (en)2001-07-102004-07-21Methods and compositions for risk stratification
US12/061,565US20080254489A1 (en)2004-07-212008-04-02Methods and compositions for risk stratification

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US10/898,734ContinuationUS7393656B2 (en)2001-07-102004-07-21Methods and compositions for risk stratification

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US10/898,734Expired - Fee RelatedUS7393656B2 (en)2001-07-102004-07-21Methods and compositions for risk stratification
US12/016,174Expired - Fee RelatedUS7939278B2 (en)2004-07-212008-01-17Methods and compositions for risk stratification
US12/061,565AbandonedUS20080254489A1 (en)2001-07-102008-04-02Methods and compositions for risk stratification
US12/125,763Expired - Fee RelatedUS8865420B2 (en)2004-07-212008-05-22Methods and compositions for risk stratification
US12/125,759AbandonedUS20090068681A1 (en)2004-07-212008-05-22Methods and compositions for risk stratification
US12/778,847Expired - Fee RelatedUS8394599B2 (en)2004-07-212010-05-12Methods and compositions for risk stratification
US13/082,306AbandonedUS20110269634A1 (en)2001-07-102011-04-07Methods and Compositions for Risk Stratification
US13/094,731Expired - Fee RelatedUS8309316B2 (en)2004-07-212011-04-26Methods and compositions for risk stratification
US13/098,912Expired - Fee RelatedUS8206939B2 (en)2004-07-212011-05-02Methods and compositions for risk stratification
US13/098,902AbandonedUS20120070849A1 (en)2004-07-212011-05-02Methods and compositions for risk stratification

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US12/125,759AbandonedUS20090068681A1 (en)2004-07-212008-05-22Methods and compositions for risk stratification
US12/778,847Expired - Fee RelatedUS8394599B2 (en)2004-07-212010-05-12Methods and compositions for risk stratification
US13/082,306AbandonedUS20110269634A1 (en)2001-07-102011-04-07Methods and Compositions for Risk Stratification
US13/094,731Expired - Fee RelatedUS8309316B2 (en)2004-07-212011-04-26Methods and compositions for risk stratification
US13/098,912Expired - Fee RelatedUS8206939B2 (en)2004-07-212011-05-02Methods and compositions for risk stratification
US13/098,902AbandonedUS20120070849A1 (en)2004-07-212011-05-02Methods and compositions for risk stratification

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US7393656B2 (en)2008-07-01
US20110201018A1 (en)2011-08-18
CN101023353B (en)2015-08-12
EP1771728A2 (en)2007-04-11
US7939278B2 (en)2011-05-10
US20090081699A1 (en)2009-03-26
US20100221750A1 (en)2010-09-02
JP2008507286A (en)2008-03-13
US8206939B2 (en)2012-06-26
WO2006012507A3 (en)2006-10-12
US20110269634A1 (en)2011-11-03
US20110207149A1 (en)2011-08-25
US8865420B2 (en)2014-10-21
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US20050112700A1 (en)2005-05-26
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US20120070849A1 (en)2012-03-22
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JP2014055964A (en)2014-03-27
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US20080182262A1 (en)2008-07-31
US8394599B2 (en)2013-03-12

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