首页> 外文OA文献 >Procyclic acidic repetitive protein (PARP) genes located in an unusually small alpha-amanitin-resistant transcription unit: PARP promoter activity assayed by transient DNA transfection of Trypanosoma brucei.
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Procyclic acidic repetitive protein (PARP) genes located in an unusually small alpha-amanitin-resistant transcription unit: PARP promoter activity assayed by transient DNA transfection of Trypanosoma brucei.

机译:脯氨酸酸性重复蛋白(PARP)基因位于一个异常小的α-阿马尼汀抗性转录单位中:通过布鲁氏锥虫的瞬时DNA转染测定PARP启动子活性。

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摘要

At least one of the procyclic acidic repetitive protein (PARP or procyclin) loci of Trypanosoma brucei is a small (5- to 6-kilobase) polycistronic transcription unit which is transcribed in an alpha-amanitin-resistant manner. Its single promoter, as mapped by run-on transcription analysis and UV inactivation of transcription, is located immediately upstream of the first alpha-PARP gene. Transcription termination occurs in a region approximately 3 kilobases downstream of the beta-PARP gene. The location of the promoter was confirmed by its ability to direct transcription of the bacterial chloramphenicol acetyltransferase gene in insect-form (procyclic) T. brucei. The putative PARP promoter is located in the region between the 3' splice acceptor site (nucleotide position 0) and nucleotide position -196 upstream of the alpha-PARP genes. Regulatory regions influencing the levels of PARP expression may be located further upstream. We conclude that a single promoter, which is located very close to the 3' splice acceptor site of the alpha-PARP genes, directs the transcription of a small, polycistronic, and alpha-amanitin-resistant transcription unit.
机译:布氏锥虫的至少一个环酸重复蛋白(PARP或procyclin)基因座是一个小的(5至6千碱基)多顺反子转录单位,以抗α-amanitin的方式转录。通过连续转录分析和转录的UV失活定位的单个启动子位于第一个alpha-PARP基因的紧邻上游。转录终止发生在β-PARP基因下游约3公里的区域。该启动子的位置通过其以细菌形式(前环)布氏螺旋体指导细菌氯霉素乙酰转移酶基因转录的能力得以证实。推定的PARP启动子位于3'剪接受体位点(核苷酸位置0)和α-PARP基因上游核苷酸位置-196之间的区域。影响PARP表达水平的调控区可以位于更上游。我们得出的结论是,单个启动子非常靠近alpha-PARP基因的3'剪接受体位点,指导一个小的,多顺反子和α-amanitin抗性转录单位的转录。

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