Detection of True IgE-expressing Mouse B Lineage Cells |
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Authors: | Michael P Gallagher Akritee Shrestha Jennifer M Magee Duane R Wesemann |
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Institution: | 1.Department of Medicine, Division of Rheumatology, Immunology and Allergy, Brigham and Women''s Hospital and Harvard Medical School |
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Abstract: | B lymphocyte immunoglobulin heavy chain (IgH) class switch recombination (CSR) is a process wherein initially expressed IgM switches to other IgH isotypes, such as IgA, IgE and IgG. Measurement of IgH CSR in vitro is a key method for the study of a number of biologic processes ranging from DNA recombination and repair to aspects of molecular and cellular immunology. In vitro CSR assay involves the flow cytometric measurement surface Ig expression on activated B cells. While measurement of IgA and IgG subclasses is straightforward, measurement of IgE by this method is problematic due to soluble IgE binding to FcεRII/CD23 expressed on the surface of activated B cells. Here we describe a unique procedure for accurate measurement of IgE-producing mouse B cells that have undergone CSR in culture. The method is based on trypsin-mediated cleavage of IgE-CD23 complexes on cell surfaces, allowing for detection of IgE-producing B lineage cells by cytoplasmic staining. This procedure offers a convenient solution for flow cytometric analysis of CSR to IgE. |
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Keywords: | Immunology Issue 94 Class switch recombination AID B cell activation IgE IgG1 CD23/Fcε RII flow cytometry trypsin cytosolic staining |
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