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布氏锥虫热休克蛋白70(hsp70)基因座中的RNA聚合酶II启动子。

An RNA polymerase II promoter in the hsp70 locus of Trypanosoma brucei.

作者信息

Lee M G

机构信息

Department of Pathology, New York University Medical Center 10016, USA.

出版信息

Mol Cell Biol. 1996 Mar;16(3):1220-30. doi: 10.1128/MCB.16.3.1220.

Abstract

To study of structure of RNA polymerase (pol) II transcription units a nd the influence of temperature on the regulation of gene expression in Trypanosoma brucei, and hsp70 intergenic region promoter was characterized. In T. brucei, the hsp70 locus contains, from 5' to 3', a cognate hsp70-related gene (gene 1) which is separated by about 6 kb of DNA from a cluster of five identical hsp70 genes (genes 2 to 6). Transcription proceeds on the entire 23-kb locus, and polycistronic transcription occurs in hsp70 genes 2 to 6. Transcription of hsp70 genes 2 to 6 is only moderately sensitive to UV irradiation, indicating that it cannot be driven by a single far-upstream promoter, which suggests that promoters could be located in the region close to the hsp70 coding region. Transient transformations demonstrated that sequences located upstream of hsp70 gene 2 and in the intergenic region between hsp70 genes 2 and 3 are able to direct transcription of the reporter gene, the chloramphenicol acetyltransferase (CAT) gene. The plasmid DNA driven by the hsp70 intergenic region promoter gave CAT activity approximately 85-fold above to background level. This is equivalent to approximately 1% of that derived from a CAT plasmid driven by the procyclic acidic repetitive protein gene promoter, which is controlled by RNA pol I. The hsp70 intergenic region promoter can drive alpha-amanitin-sensitive transcription at an internal position of the chromosome as well as an episome, suggesting that it is controlled by RNA pol II. However, this hsp70 intergenic region promoter, along with the 3' splice site and the 5' untranslated region of the hsp70 genes that controls the transcription of the reporter gene, cannot up-regulate the expression of the reporter gene during heat shock. This result is consistent with the previous observation that expression of the hsp70 genes in T. brucei is mainly controlled at the posttranscriptional level.

摘要

为研究布氏锥虫RNA聚合酶(pol)II转录单元的结构以及温度对基因表达调控的影响,对hsp70基因间隔区启动子进行了表征。在布氏锥虫中,hsp70基因座从5'到3'包含一个同源的hsp70相关基因(基因1),该基因与一组五个相同的hsp70基因(基因2至6)被约6 kb的DNA隔开。转录在整个23 kb的基因座上进行,多顺反子转录发生在hsp70基因2至6中。hsp70基因2至6的转录对紫外线照射仅中度敏感,这表明它不能由单个远上游启动子驱动,这表明启动子可能位于靠近hsp70编码区的区域。瞬时转化表明,位于hsp70基因2上游和hsp70基因2与3之间的基因间隔区的序列能够指导报告基因氯霉素乙酰转移酶(CAT)基因的转录。由hsp70基因间隔区启动子驱动的质粒DNA产生的CAT活性比背景水平高约85倍。这相当于由受RNA聚合酶I控制的前循环酸性重复蛋白基因启动子驱动的CAT质粒产生的活性的约1%。hsp70基因间隔区启动子可以在染色体内部位置以及附加体上驱动α-鹅膏蕈碱敏感的转录,这表明它受RNA聚合酶II控制。然而,这个hsp70基因间隔区启动子,连同控制报告基因转录的hsp70基因的3'剪接位点和5'非翻译区,在热休克期间不能上调报告基因的表达。这一结果与之前关于布氏锥虫中hsp70基因表达主要在转录后水平受到控制的观察结果一致。

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