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对人类免疫球蛋白重链向所有同种型类别转换重组的可量化分析。

Quantifiable analysis of human immunoglobulin heavy chain class-switch recombination to all isotypes.

作者信息

Weckert H A, Hughes J A, Benson E M, Dunn I S

机构信息

Institute for Immunology and Allergy Research, PO Box 145, Westmead, Sydney, Australia.

出版信息

J Immunol Methods. 2000 Jan 13;233(1-2):141-58. doi: 10.1016/s0022-1759(99)00132-5.

Abstract

Somatic recombinational events, including the immunoglobulin heavy chain class-switch, are a normal feature of B-cell maturation. To enable comprehensive and sensitive class-switch analysis in ex vivo human B cells, we have developed multiple digestion-circularization PCR (DC-PCR) techniques for quantifiable detection of switching to all immunoglobulin isotypes. This technology was validated by extensive sequencing of PCR products, tests with control non-lymphoid cells and B-cell lines of known isotypic specificities, and by demonstrating DC-PCR selectivity in a model system. With tonsillar B-cell DNA, switching to gamma 3, gamma 1, alpha1, gamma 2, gamma 4 and alpha2 isotypes was reproducibly detectable among different individuals. Levels of epsilon switching were relatively low and usually required higher total amounts of template DNAs for detection. Quantitation of alpha1 class switching in a panel of human tonsillar whole B cells was performed by the internal-competitor approach, and showed a pattern consistent with previous studies on IgA+ tonsillar cells. We demonstrate that these assays can rapidly show germline status or specific switch rearrangements in B lymphoid cell lines.

摘要

体细胞重组事件,包括免疫球蛋白重链类别转换,是B细胞成熟的正常特征。为了能够对体外人B细胞进行全面且灵敏的类别转换分析,我们开发了多种消化-环化PCR(DC-PCR)技术,用于可量化检测向所有免疫球蛋白同种型的转换。该技术通过对PCR产物进行广泛测序、用已知同种型特异性的对照非淋巴细胞和B细胞系进行测试,以及在模型系统中证明DC-PCR的选择性来验证。对于扁桃体B细胞DNA,在不同个体中可重复检测到向γ3、γ1、α1、γ2、γ4和α2同种型的转换。ε转换水平相对较低,通常需要更高总量的模板DNA进行检测。通过内部竞争法对一组人扁桃体全B细胞中的α1类别转换进行定量,结果显示的模式与先前关于IgA+扁桃体细胞的研究一致。我们证明这些检测方法能够快速显示B淋巴细胞系中的种系状态或特定的转换重排。

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