Literature DB >> 17948236

Optimization of flow cytometric measurement of ZAP-70 in chronic lymphocytic leukemia.

Sergey N Preobrazhensky1, David W Bahler.   

Abstract

BACKGROUND: The goal of this study was to optimize a cell staining procedure for flow cytometric detection of zeta-chain associated protein-70 (ZAP-70). Our specific objectives were to improve antibody selection criteria, identify a cell permeabilization procedure better tailored to ZAP-70 analysis, as well as to establish objective criteria to control antigen stability.
METHODS: Sequentially titrated 2F3.2-FITC, 1E7.2-FITC, and 1E7.2-Alexa Fluor 488 anti-ZAP-70 antibodies were used to stain normal B and T cells and Scatchard analysis was applied to calculate K(d) and B(max) values from saturation curves of specific binding. ZAP-70 staining was compared in cells permeabilized with two commercially available kits, Triton X-100, and a custom saponin procedure.
RESULTS: Normal B-cells were found to provide an excellent measure of nonspecific staining while varying ZAP-70 antibodies and concentrations. Comparing Scatchard analyses of specific T-cell binding revealed that 1E7.2-Alexa Fluor 488 had the highest binding affinity of the tested anti-ZAP-70 antibodies and was the best choice. The highest levels of ZAP-70 fluorescence occurred when cells were permeabilized using a noncommercial saponin procedure. Decrease of chronic lymphocytic leukemia cell viability correlated with diminished ZAP-70 expression; when viability was lower than 95% the percentage of bright positive samples was significantly decreased, indicating a possibility of false-negative results.
CONCLUSIONS: The efficiency and reliability of flow cytometric detection of ZAP-70 can be optimized by using Scatchard analysis to help select the most effective antibodies and antibody concentrations that maximize specific to nonspecific binding, by using a "custom" ZAP-70 permeabilization procedure, and by better controlling antigen stability by measuring cell viability. (c) 2007 Clinical Cytometry Society

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Year:  2008        PMID: 17948236     DOI: 10.1002/cyto.b.20378

Source DB:  PubMed          Journal:  Cytometry B Clin Cytom        ISSN: 1552-4949            Impact factor:   3.058


  7 in total

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2.  Methodological comparison of two anti-ZAP-70 antibodies.

Authors:  Heba A Degheidy; David J Venzon; Mohammed Z H Farooqui; Fatima Abbasi; Diane C Arthur; Wyndham H Wilson; Adrian Wiestner; M A Stetler-Stevenson; Gerald E Marti
Journal:  Cytometry B Clin Cytom       Date:  2011-04-06       Impact factor: 3.058

3.  Immunomagnetic bead separation of mononuclear cells from contaminating granulocytes in cryopreserved blood samples.

Authors:  Sergey N Preobrazhensky; David W Bahler
Journal:  Cryobiology       Date:  2009-09-18       Impact factor: 2.487

4.  Quantitative detection of zeta-chain-associated protein 70 expression in chronic lymphocytic leukemia.

Authors:  Peixuan Zhu; Heba A Degheidy; Gerald E Marti; Shuhong Li; Fatima Abbasi; Adrian Wiestner; Platte Amstutz; Cha-Mei Tang
Journal:  Leuk Lymphoma       Date:  2012-08-14

5.  Smudge cell percentage as a surrogate marker for ZAP-70 expression in patients with chronic lymphocytic leukemia.

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Journal:  Blood Res       Date:  2018-09-28

6.  Assessment of different permeabilization methods of minimizing damage to the adherent cells for detection of intracellular RNA by flow cytometry.

Authors:  Zahra Amidzadeh; Abbas Behzad Behbahani; Nasrollah Erfani; Sedigheh Sharifzadeh; Reza Ranjbaran; Leili Moezi; Farzaneh Aboualizadeh; Mohammad Ali Okhovat; Parniyan Alavi; Negar Azarpira
Journal:  Avicenna J Med Biotechnol       Date:  2014-01

7.  Using the geometric mean fluorescence intensity index method to measure ZAP-70 expression in patients with chronic lymphocytic leukemia.

Authors:  Yu-Jie Wu; Hui Wang; Jian-Hua Liang; Yi Miao; Lu Liu; Hai-Rong Qiu; Chun Qiao; Rong Wang; Jian-Yong Li
Journal:  Onco Targets Ther       Date:  2016-02-18       Impact factor: 4.147

  7 in total

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