2003
DOI: 10.1002/cyto.a.10063
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Immunoreactivity of Stat5 phosphorylated on tyrosine as a cell‐based measure of Bcr/Abl kinase activity

Abstract: Background: Stat5 1 (Signal Transducer and Activator of Transcription 5) is normally phosphorylated and activated by Janus kinases. In cells transformed with BCR/ABL, Stat5 is constitutively activated by promiscuous phosphorylation. Cytometry of intracellular antigens can be used to evaluate cell treatments affecting gene expression, because it precisely provides the fraction of affected cells and the quantitative change in expression. Here, we asked whether we could measure a phosphorylated epitope on Stat5 b… Show more

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Cited by 52 publications
(42 citation statements)
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“…However, although we do not have evidence that our original technique provides biologically relevant measurements, we do know that the signal is equivalent to western blot analysis. In general, our experience indicates that fluorescence-based cytometric measurements are more precise but less sensitive than western blots (5,16). Further, by comparing western blotting with cytometry for samples that have been extracted with various solutions (Frisa and Jacobberger, unpublished data), we have come to the expected conclusion that we detect only a fraction of the intracellular epitope by cytometry, i.e., a significant portion of the epitope is not available for staining after alcohol fixation/permeabilization and staining at antibody saturation.…”
Section: Discussionmentioning
confidence: 99%
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“…However, although we do not have evidence that our original technique provides biologically relevant measurements, we do know that the signal is equivalent to western blot analysis. In general, our experience indicates that fluorescence-based cytometric measurements are more precise but less sensitive than western blots (5,16). Further, by comparing western blotting with cytometry for samples that have been extracted with various solutions (Frisa and Jacobberger, unpublished data), we have come to the expected conclusion that we detect only a fraction of the intracellular epitope by cytometry, i.e., a significant portion of the epitope is not available for staining after alcohol fixation/permeabilization and staining at antibody saturation.…”
Section: Discussionmentioning
confidence: 99%
“…Thus, different anticoagulants, overnight storage and shipment, whole blood staining, and several erythrocyte lysis techniques result in reproducible, convenient, and flexible assays. Recently, interest has been stimulated in potentially less robust assays of cell signaling components based on the relatively recent availability of phosphorylation state-specific antibodies (1)(2)(3)(4)(5)(6). Because of the quantitative and correlative natures of cytometry, this represents a novel and potentially powerful approach to classification of hematologic malignancies including the selection of patients for molecular targeted therapies and monitoring drug effects in individual patients (1,(6)(7)(8).…”
mentioning
confidence: 99%
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“…In this study, we present the development and validation of a multiparameter fluorescence-activated cell sorting (FACS) method for the quantification of pERK, and the detection of nucleated CTCs isolated from peripheral human blood. Phosphorylation state-specific antibodies (19)(20)(21)(22)(23)(24) have recently become available and were used for the quantification of pERK. The applicability of the method was demonstrated in peripheral blood from patients with advanced metastatic breast, colon, lung, ovarian, and urothelial cancer.…”
mentioning
confidence: 99%
“…Many of these early and successful targeted therapies, such as the bcr:abl kinase inhibitor therapy, to mention only one, are kinase inhibitors. Cytometric assays to monitor kinase activity are rapidly being developed (1)(2)(3) and are a part of most clinical trials of these new generations of targeted therapies as key analyses to help understand drug action, emergence of drug resistance, and interactions with other therapies used in combination with these targeted therapies. It is clear that these cell-based cytometric assays are going to move to the clinical laboratory in the near future, thus ensuring a growing role of clinical cytometry in patient therapeutic decisions and monitoring.…”
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confidence: 99%