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小鼠bcl-x基因的基因组结构、启动子区域分析及染色体定位

Genomic organization, promoter region analysis, and chromosome localization of the mouse bcl-x gene.

作者信息

Grillot D A, González-García M, Ekhterae D, Duan L, Inohara N, Ohta S, Seldin M F, Nuñez G

机构信息

Department of Pathology, University of Michigan Medical School, Ann Arbor 48109, USA.

出版信息

J Immunol. 1997 May 15;158(10):4750-7.

PMID:9144489
Abstract

The bcl-x gene, a bcl-2 family member, is highly regulated during lymphoid development, and its expression modulates apoptosis in lymphoid and other cell populations. Several forms of bcl-x mRNAs with different biologic functions have been described in rodents and humans. In this study, we have determined the organization and promoter region of the mouse bcl-x gene in an effort to understand the molecular basis for the different bcl-x mRNA species identified in tissues. We show that mouse bcl-x maps to the distal mouse chromosome 2 at approximately 89 cM, and exhibits a three-exon structure with an untranslated first exon and a facultative first intron. The coding region of bcl-xL is generated by the juncture of exons II and III through a splicing reaction, whereas bcl-xS is generated by an alternatively utilized donor splice site located within exon II. Analysis of multiple cDNAs and primer extension experiments revealed major transcription initiation sites in brain and thymus within a GC-rich region, with multiple Sp1-binding motifs located upstream of exon I. Another promoter was mapped to a 57-bp region localized upstream of the translation initiation codon by transfection of reporter constructs into FL5.12 and K562 cell lines. The remarkable similarity between the genomic regions of bcl-2 and bcl-x suggests that these genes have evolved from a common ancestral gene or through gene duplication.

摘要

bcl-x基因是bcl-2家族成员,在淋巴细胞发育过程中受到高度调控,其表达可调节淋巴细胞及其他细胞群体中的细胞凋亡。在啮齿动物和人类中已描述了几种具有不同生物学功能的bcl-x mRNA形式。在本研究中,我们确定了小鼠bcl-x基因的结构和启动子区域,以了解在组织中鉴定出的不同bcl-x mRNA种类的分子基础。我们发现小鼠bcl-x基因定位于小鼠2号染色体远端约89 cM处,具有三外显子结构,其中第一个外显子为非编码外显子,且有一个选择性的第一内含子。bcl-xL的编码区是通过外显子II和III通过剪接反应连接产生的,而bcl-xS则是由外显子II内一个选择性使用的供体剪接位点产生的。对多个cDNA的分析和引物延伸实验揭示了在富含GC的区域中脑和胸腺中的主要转录起始位点,在外显子I上游有多个Sp1结合基序。通过将报告基因构建体转染到FL5.12和K562细胞系中,另一个启动子定位于翻译起始密码子上游的一个57 bp区域。bcl-2和bcl-x基因区域之间的显著相似性表明这些基因是由一个共同的祖先基因进化而来或通过基因复制产生的。

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