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在健康供体和荨麻疹患者中均检测到一种VH抗体序列。

Detection of one VH antibody sequence in both healthy donors and urticaria patients.

作者信息

Fux Michaela, Vogel Monique, Stadler Michael B, Stadler Beda M, Miescher Sylvia M

机构信息

Institute of Immunology, University of Bern, Inselspital, Switzerland.

出版信息

J Immunol Methods. 2005 Dec 20;307(1-2):107-17. doi: 10.1016/j.jim.2005.09.014. Epub 2005 Oct 25.

Abstract

We have previously isolated anti-FcepsilonRIalpha autoantibodies from phage libraries of healthy donors and urticaria patients. Strikingly, the same antibody, LTMalpha15, was isolated from both libraries. Sequence analysis revealed a germline configuration of the LTMalpha15 variable heavy (V(H)) chain with a slightly mutated variable light (V(L)) chain supporting its classification as a natural autoantibody. Distribution analysis of anti-FcepsilonRIalpha autoantibodies by functional or serological tests delivered conflicting data. For this reason we have developed a new real-time PCR to analyse the distribution of LTMalpha15V(H) in healthy donors and urticaria patients. Our new bioinformatic program permitted the design of a minor groove binder (MGB) TaqMan probe that specifically detected the LTMalpha15V(H). We were able to demonstrate a broad range of rearranged V(H) gene copy number without any correlation to the state of health. Monitoring LTMalpha15V(H) gene copy number in a single donor over a period of 70 days revealed a time-related fluctuation of circulating B cells carrying LTMalpha15V(H). We propose that our real-time PCR may serve as a model for the quantification of natural antibody sequences at a monoclonal level.

摘要

我们之前从健康供体和荨麻疹患者的噬菌体文库中分离出了抗FcepsilonRIalpha自身抗体。令人惊讶的是,从两个文库中都分离出了相同的抗体LTMalpha15。序列分析显示,LTMalpha15可变重链(V(H))具有种系构型,可变轻链(V(L))略有突变,这支持了将其归类为天然自身抗体。通过功能或血清学检测对抗FcepsilonRIalpha自身抗体进行的分布分析得出了相互矛盾的数据。因此,我们开发了一种新的实时PCR方法来分析健康供体和荨麻疹患者中LTMalpha15V(H)的分布。我们新的生物信息学程序允许设计一种小沟结合剂(MGB)TaqMan探针,该探针能特异性检测LTMalpha15V(H)。我们能够证明重排的V(H)基因拷贝数范围很广,且与健康状况无任何关联。在70天的时间里对单个供体的LTMalpha15V(H)基因拷贝数进行监测,结果显示携带LTMalpha15V(H)的循环B细胞存在与时间相关的波动。我们认为,我们的实时PCR可作为在单克隆水平上定量天然抗体序列的模型。

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