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T细胞受体β可变基因启动子是高效Vβ重排所必需的,但不是等位基因排斥所必需的。

The T-cell receptor beta variable gene promoter is required for efficient V beta rearrangement but not allelic exclusion.

作者信息

Ryu Chun Jeih, Haines Brian B, Lee Hye Ran, Kang Yun Hee, Draganov Dobrin D, Lee Minhui, Whitehurst Charles E, Hong Hyo Jeong, Chen Jianzhu

机构信息

Center for Cancer Research and Department of Biology, Massachusetts Institute for Technology, Cambridge, MA 02139, USA.

出版信息

Mol Cell Biol. 2004 Aug;24(16):7015-23. doi: 10.1128/MCB.24.16.7015-7023.2004.

Abstract

To investigate the role of promoters in regulating variable gene rearrangement and allelic exclusion, we constructed mutant mice in which a 1.2-kb region of the V beta 13 promoter was either deleted (P13(-/-)) or replaced with the simian virus 40 minimal promoter plus five copies of Gal4 DNA sequences (P13(R/R)). In P13(-/-) mice, cleavage, rearrangement, and transcription of V beta 13, but not the flanking V beta gene segments, were significantly inhibited. In P13(R/R) mice, inhibition of V beta 13 rearrangement was less severe and was not associated with any apparent reduction in V beta 13 cleavage. Expression of a T-cell receptor (TCR) transgene blocked cleavages at the normal V beta 13-recombination signal sequence junction and V beta 13 coding joint formation of both wild-type and mutant V beta 13 alleles. However, a low level of aberrant V beta 13 cleavage was consistently detected, especially in TCR transgenic P13(R/R) mice. These findings suggest that the variable gene promoter is required for promoting local recombination accessibility of the associated V beta gene segment. Although the promoter is dispensable for allelic exclusion, it appears to suppress aberrant V beta cleavages during allelic exclusion.

摘要

为了研究启动子在调节可变基因重排和等位基因排斥中的作用,我们构建了突变小鼠,其中Vβ13启动子的1.2 kb区域要么被删除(P13(-/-)),要么被猿猴病毒40最小启动子加五个Gal4 DNA序列拷贝所取代(P13(R/R))。在P13(-/-)小鼠中,Vβ13的切割、重排和转录受到显著抑制,但侧翼Vβ基因片段不受影响。在P13(R/R)小鼠中,Vβ13重排的抑制作用较轻,且与Vβ13切割的任何明显减少无关。T细胞受体(TCR)转基因的表达阻断了野生型和突变型Vβ13等位基因在正常Vβ-13重组信号序列连接处的切割以及Vβ13编码接头的形成。然而,始终检测到低水平的异常Vβ13切割,尤其是在TCR转基因P13(R/R)小鼠中。这些发现表明,可变基因启动子是促进相关Vβ基因片段局部重组可及性所必需的。虽然启动子对于等位基因排斥是可有可无的,但它似乎在等位基因排斥过程中抑制了异常的Vβ切割。

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