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布氏锥虫中的信使核糖核酸加工位点

Messenger RNA processing sites in Trypanosoma brucei.

作者信息

Benz Corinna, Nilsson Daniel, Andersson Björn, Clayton Christine, Guilbride D Lys

机构信息

Zentrum für Molekulare Biologie, Im Neuenheimer Feld 282, D69120 Heidelberg, Germany.

出版信息

Mol Biochem Parasitol. 2005 Oct;143(2):125-34. doi: 10.1016/j.molbiopara.2005.05.008.

Abstract

In Kinetoplastids, protein-coding genes are transcribed polycistronically by RNA polymerase II. Individual mature mRNAs are generated from polycistronic precursors by 5' trans splicing of a 39-nt capped leader RNA and 3' polyadenylation. It was previously known that trans splicing generally occurs at an AG dinucleotide downstream of a polypyrimidine tract, and that polyadenylation is coupled to downstream trans splicing. The few polyadenylation sites that had been examined were 100-400 nt upstream of the polypyrimidine tract which marked the adjacent trans splice site. We wished to define the sequence requirements for trypanosome mRNA processing more tightly and to generate a predictive algorithm. By scanning all available Trypanosoma brucei cDNAs for splicing and polyadenylation sites, we found that trans splicing generally occurs at the first AG following a polypyrimidine tract of 8-25 nt, giving rise to 5'-UTRs of a median length of 68 nt. We also found that in general, polyadenylation occurs at a position with one or more A residues located between 80 and 140 nt from the downstream polypyrimidine tract. These data were used to calibrate free parameters in a grammar model with distance constraints, enabling prediction of polyadenylation and trans splice sites for most protein-coding genes in the trypanosome genome. The data from the genome analysis and the program are available from: .

摘要

在动质体中,蛋白质编码基因由RNA聚合酶II进行多顺反子转录。单个成熟mRNA通过39个核苷酸的带帽前导RNA的5'反式剪接和3'聚腺苷酸化从多顺反子前体产生。此前已知反式剪接通常发生在多嘧啶序列下游的AG二核苷酸处,并且聚腺苷酸化与下游反式剪接偶联。少数已检测的聚腺苷酸化位点位于标记相邻反式剪接位点的多嘧啶序列上游100 - 400 nt处。我们希望更精确地定义锥虫mRNA加工的序列要求并生成一种预测算法。通过扫描所有可用的布氏锥虫cDNA中的剪接和聚腺苷酸化位点,我们发现反式剪接通常发生在8 - 25 nt的多嘧啶序列之后的第一个AG处,产生的5'非翻译区(5'-UTR)的中位数长度为68 nt。我们还发现,一般来说,聚腺苷酸化发生在距离下游多嘧啶序列80至140 nt之间有一个或多个A残基的位置。这些数据用于校准具有距离约束的语法模型中的自由参数,从而能够预测锥虫基因组中大多数蛋白质编码基因的聚腺苷酸化和反式剪接位点。基因组分析的数据和该程序可从以下网址获取: 。

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