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The RNA polymerase III terminator used by a B1-Alu element can modulate 3 processing of the intermediate RNA product.

机译:B1-Alu元件使用的RNA聚合酶III终止子可以调节中间RNA产物的3加工。

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摘要

The dispersion of short interspersed elements (SINEs) probably occurred through an RNA intermediate. B1 is a murine homolog of the human SINE Alu; these elements are composed of 5' G + C-rich regions juxtaposed to A-rich tracts and are flanked by direct repeats. Internal promoters direct RNA polymerase III to transcribe B1 and Alu elements and proceed into the 3' flanking DNA until it reaches a (dT)4 termination signal. The resulting transcripts contain 3'-terminal oligo(U) tracts which can presumably base pair with the A-rich tract to form self-primed templates for reverse transcriptase and retrotransposition. Nuclear extracts from mouse tissue culture cells contain an RNA processing activity that removes the A-rich and 3'-terminal regions from purified B1 RNAs (R. Maraia, Nucleic Acids Res. 19:5695-5702, 1991). In this study, we examined transcription and RNA processing in these nuclear extracts. In contrast to results with use of purified RNA, nascent transcripts synthesized in nuclear extract by RNA polymerase III are not processed, suggesting that the transposition-intermediate-like RNA is shielded from processing by a protein(s). Alteration of an AATTTT TAA termination signal to a GCTTTTGC signal activated processing by greater than 100-fold in coupled transcription/processing reactions. A similar difference was found when expression was compared in frog oocytes. No difference in processing was found if the transcripts were made by T7 RNA polymerase in the presence of the nuclear extract, indicating that the different processing effects of the two terminators were dependent on synthesis by polymerase III. The modulation of processing of B1-Alu transcripts and the potential for retrotransposition of B1 and Alu DNA sequences are discussed.
机译:短分散元素(SINE)的分散可能是通过RNA中间体发生的。 B1是人SINE Alu的鼠同源物;这些元素由与富含A的区域并列的5'G + C丰富的区域组成,并且两侧是直接重复。内部启动子指导RNA聚合酶III转录B1和Alu元素,并进入3'侧翼DNA,直到达到(dT)4终止信号。产生的转录本包含3'-末端oligo(U)片段,大概可以与富含A的片段进行碱基配对,从而形成用于逆转录酶和逆转座子的自引模板。小鼠组织培养细胞的核提取物具有RNA加工活性,该RNA加工活性从纯化的B1 RNA中去除了富含A和3'端的区域(R. Maraia,Nucleic Acids Res。19:5695-5702,1991)。在这项研究中,我们检查了这些核提取物中的转录和RNA加工。与使用纯化的RNA的结果相反,未处理通过RNA聚合酶III在核提取物中合成的新生转录物,表明类似转座中间体的RNA被蛋白质屏蔽。在偶联的转录/加工反应中,AATTTT TAA终止信号向GCTTTTGC信号的改变激活了超过100倍的加工过程。当在青蛙卵母细胞中比较表达时,发现类似的差异。如果转录本是由T7 RNA聚合酶在核提取物的存在下制成的,则在加工中没有发现差异,这表明两个终止子的不同加工效果取决于聚合酶III的合成。讨论了B1-Alu转录物加工的调控以及B1和Alu DNA序列逆转位的潜力。

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