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在免疫球蛋白重链基因座(IgH)的V(D)J重排过程中产生的倒位。

Inversions produced during V(D)J rearrangement at IgH, the immunoglobulin heavy-chain locus.

作者信息

Sollbach A E, Wu G E

机构信息

Department of Immunology, University of Toronto, Canada.

出版信息

Mol Cell Biol. 1995 Feb;15(2):671-81. doi: 10.1128/MCB.15.2.671.

Abstract

Diversity in immunoglobulin antigen receptors is generated in part by V(D)J recombination. In this process, different combinations of gene elements are joined in various configurations. Products of V(D)J recombination are coding joints, signal joints, and hybrid junctions, which are generated by deletion or inversion. To determine their role in the generation of diversity, we have examined two sorts of recombination products, coding joints and hybrid junctions, that have formed by inversion at the mouse immunoglobulin heavy-chain locus. We developed a PCR assay for quantification and characterization of inverted rearrangements of DH and JH gene elements. In primary cells from adult mice, inverted DJH rearrangements are detectable but they are rare. There were approximately 1,100 to 2,200 inverted DJH coding joints and inverted DJH hybrid junctions in the marrow of one adult mouse femur. On day 16 of gestation, inverted DJH rearrangements are more abundant. There are approximately 20,000 inverted DJH coding joints and inverted DJH hybrid junctions per day 16 fetal liver. In fetal liver cells, the number of inverted DJH rearrangements remains relatively constant from day 14 to day 16 of gestation. Inverted DJH rearrangements to JH4, the most 3' JH element, are more frequently detected than inverted DJH rearrangements to other JH elements. We compare the frequencies of inverted DJH rearrangements to previously determined frequencies of uninverted DJH rearrangements (DJH rearrangements formed by deletion). We suggest that inverted DJH rearrangements are influenced by V(D)J recombination mechanistic constraints and cellular selection.

摘要

免疫球蛋白抗原受体的多样性部分是由V(D)J重组产生的。在这个过程中,基因元件的不同组合以各种构型连接在一起。V(D)J重组的产物是编码连接、信号连接和杂合连接,它们是通过缺失或倒位产生的。为了确定它们在多样性产生中的作用,我们研究了两种重组产物,即编码连接和杂合连接,它们是在小鼠免疫球蛋白重链基因座处通过倒位形成的。我们开发了一种PCR检测方法,用于定量和表征DH和JH基因元件的倒位重排。在成年小鼠的原代细胞中,可检测到倒位的DJH重排,但它们很少见。一只成年小鼠股骨骨髓中大约有1100到2200个倒位的DJH编码连接和倒位的DJH杂合连接。在妊娠第16天,倒位的DJH重排更为丰富。妊娠第16天的胎儿肝脏中每天大约有20000个倒位的DJH编码连接和倒位的DJH杂合连接。在胎儿肝细胞中,从妊娠第14天到第16天,倒位的DJH重排数量保持相对恒定。与其他JH元件相比,向最3'的JH元件JH4的倒位DJH重排更频繁地被检测到。我们将倒位DJH重排的频率与先前确定的未倒位DJH重排(通过缺失形成的DJH重排)的频率进行比较。我们认为倒位的DJH重排受V(D)J重组机制限制和细胞选择的影响。

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