Potential regulatory elements in the Trypanosoma cruzi rRNA gene promoter

Elisa Figueroa-Angulo , Ana María Cevallos , Alejandro Zentella , Imelda López-Villaseñor , Roberto Hernández
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引用次数: 9

Abstract

The Trypanosoma cruzi rRNA gene promoter was characterized by deletion and point mutation analyses. A core of 89 bp was identified as the minimal region with full promoter activity. This core region is flanked upstream by a control element that stimulates its activity, and downstream by a novel down regulating region of about 200 bp. A point mutation analysis of the transcription start region evidenced 7 contiguous nucleotides where individual substitutions produced in all cases a defective promoter. It is generally accepted that the anciently speciated trypanosomatids lack strict promoters for protein coding genes transcribed by RNA polymerase II. The occurrence of a well structured rRNA gene promoter in these species suggests an early appearance of the RNA polymerase I promoters in the evolution of eukaryotic cells.

克氏锥虫rRNA基因启动子的潜在调控元件
对克氏锥虫rRNA基因启动子进行了缺失和点突变分析。一个89 bp的核心被确定为具有完全启动子活性的最小区域。这个核心区域的上游有一个刺激其活性的控制元件,下游有一个大约200 bp的新下调区域。转录起始区域的点突变分析证实了7个连续的核苷酸,其中单个替换在所有情况下产生有缺陷的启动子。人们普遍认为,古老的锥虫缺乏RNA聚合酶II转录的蛋白质编码基因的严格启动子。在这些物种中,结构良好的rRNA基因启动子的出现表明,RNA聚合酶I启动子在真核细胞的进化中早期出现。
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