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大鼠和小鼠前脑啡肽原基因的转录在生精细胞和体细胞的不同位点起始。

Transcription of the rat and mouse proenkephalin genes is initiated at distinct sites in spermatogenic and somatic cells.

作者信息

Kilpatrick D L, Zinn S A, Fitzgerald M, Higuchi H, Sabol S L, Meyerhardt J

机构信息

Neurobiology Group, Worcester Foundation for Experimental Biology, Shrewsbury, Massachusetts 01545.

出版信息

Mol Cell Biol. 1990 Jul;10(7):3717-26. doi: 10.1128/mcb.10.7.3717-3726.1990.

Abstract

During spermatogenesis, several genes are expressed in a germ cell-specific manner. Previous studies have demonstrated that rat and mouse spermatogenic cells produce a 1,700-nucleotide proenkephalin RNA, while somatic cells that express the proenkephalin gene contain a 1,450-nucleotide transcript. Using cDNA cloning, RNA protection, and primer extension analyses, we showed that transcription of the rat and mouse spermatogenic-cell RNAs is initiated downstream from the proenkephalin somatic promoter in the first somatic intron (intron As). In both species, the germ cell cap site region consists of multiple start sites distributed over a length of approximately 30 base pairs. Within rat and mouse intron As, the region upstream of the germ cell cap sites is GC rich and lacks TATA sequences. A consensus binding site for the transcription factor SP1 was identified in intron As downstream of the proenkephalin germ cell cap site region. These features are characteristic of several previously described promoters that lack TATA sequences. Homologies were also identified between the proenkephalin and rat cytochrome c spermatogenic-cell promoters, including the absence of a TATA box, a multiple start site region, and several common sequences. This promoter motif thus may be shared with other genes expressed in male germ cells.

摘要

在精子发生过程中,有几个基因以生殖细胞特异性方式表达。先前的研究表明,大鼠和小鼠的生精细胞产生一种1700个核苷酸的前脑啡肽RNA,而表达前脑啡肽基因的体细胞含有一种1450个核苷酸的转录本。通过cDNA克隆、RNA保护和引物延伸分析,我们发现大鼠和小鼠生精细胞RNA的转录起始于前脑啡肽体细胞启动子下游的第一个体细胞内含子(内含子As)。在这两个物种中,生殖细胞帽位点区域由分布在大约30个碱基对长度上的多个起始位点组成。在大鼠和小鼠的内含子As内,生殖细胞帽位点上游区域富含GC且缺乏TATA序列。在前脑啡肽生殖细胞帽位点区域下游的内含子As中鉴定出了转录因子SP1的共有结合位点。这些特征是几个先前描述的缺乏TATA序列的启动子所具有的特点。在前脑啡肽和大鼠细胞色素c生精细胞启动子之间也发现了同源性,包括没有TATA框、多个起始位点区域以及几个共同序列。因此,这种启动子基序可能与在雄性生殖细胞中表达的其他基因共有。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/2b9b/360821/87f47db2998c/molcellb00043-0444-a.jpg

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