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人类T细胞γ基因含有N片段,且具有明显的连接多样性。

Human T-cell gamma genes contain N segments and have marked junctional variability.

作者信息

Quertermous T, Strauss W, Murre C, Dialynas D P, Strominger J L, Seidman J G

出版信息

Nature. 1986;322(6075):184-7. doi: 10.1038/322184a0.

Abstract

The gamma-chain genes are encoded by immunoglobulin-like gene segments in germline DNA which rearrange during the somatic development of T cells to form an active gene. The protein produced by these genes has not been identified and the diversity of the proteins that the genes can express has not been determined. We expect that the diversity of expressed gamma-chains is produced by the same three mechanisms that produce diversity of other immunoglobulin-like genes: (1) germline variable (V) and joining (J) region repertoires; (2) somatic mutation; and (3) junctional diversity. To define the contribution of each of these mechanisms to the generation of gamma-chain diversity, several gamma-chain complementary clones and rearranged gamma-chain genes have been characterized. Most of these clones seem to encode a defective gamma-chain, the variable- and constant-region portions being joined such that they would not be translated in the same reading frame. Here we report that the germline J-region diversity of the human T-cell gamma-chain is very limited and that somatic mutation does not contribute to the diversity of the gamma-chains encoded by the cloned segments. However, the junctional diversity of these gamma-chain genes is extensive. We suggest that N sequences (template-independent sequences) have been inserted enzymatically into all of the gamma-chain genes characterized.

摘要

γ链基因由种系DNA中的免疫球蛋白样基因片段编码,这些片段在T细胞的体细胞发育过程中发生重排以形成一个活性基因。这些基因产生的蛋白质尚未被鉴定,并且这些基因能够表达的蛋白质的多样性也尚未确定。我们预计,表达的γ链的多样性是由产生其他免疫球蛋白样基因多样性的相同三种机制产生的:(1)种系可变(V)区和连接(J)区基因库;(2)体细胞突变;以及(3)连接多样性。为了确定这些机制中的每一种对γ链多样性产生的贡献,已经对几个γ链互补克隆和重排的γ链基因进行了表征。这些克隆中的大多数似乎编码一种有缺陷的γ链,可变区和恒定区部分连接在一起,以至于它们不会在相同的阅读框中被翻译。在此我们报告,人类T细胞γ链的种系J区多样性非常有限,并且体细胞突变对克隆片段编码的γ链的多样性没有贡献。然而,这些γ链基因的连接多样性是广泛的。我们认为,N序列(与模板无关的序列)已通过酶促方式插入到所有已表征的γ链基因中。

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