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Reverse Transcription in the Saccharomyces cerevisiae Long-Terminal Repeat Retrotransposon Ty3

机译:酿酒酵母长期重复反转录转座子Ty3中的逆转录。

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Converting the single-stranded retroviral RNA into integration-competent double-stranded DNA is achieved through a multi-step process mediated by the virus-coded reverse transcriptase (RT). With the exception that it is restricted to an intracellular life cycle, replication of the Saccharomyces cerevisiae long terminal repeat (LTR)-retrotransposon Ty3 genome is guided by equivalent events that, while generally similar, show many unique and subtle differences relative to the retroviral counterparts. Until only recently, our knowledge of RT structure and function was guided by a vast body of literature on the human immunodeficiency virus (HIV) enzyme. Although the recently-solved structure of Ty3 RT in the presence of an RNA/DNA hybrid adds little in terms of novelty to the mechanistic basis underlying DNA polymerase and ribonuclease H activity, it highlights quite remarkable topological differences between retroviral and LTR-retrotransposon RTs. The theme of overall similarity but distinct differences extends to the priming mechanisms used by Ty3 RT to initiate (?) and (+) strand DNA synthesis. The unique structural organization of the retrotransposon enzyme and interaction with its nucleic acid substrates, with emphasis on polypurine tract (PPT)-primed initiation of (+) strand synthesis, is the subject of this review.
机译:通过由病毒编码的逆转录酶(RT)介导的多步骤过程,可以将单链逆转录病毒RNA转化为具有整合能力的双链DNA。除限于细胞内生命周期外,酿酒酵母长末端重复(LTR)-反转录转座子Ty3基因组的复制受等价事件的指导,尽管它们通常相似,但相对于逆转录病毒对应物显示出许多独特而细微的差异。直到最近,我们对RT结构和功能的了解还受到有关人类免疫缺陷病毒(HIV)酶的大量文献的指导。尽管在RNA / DNA杂合体存在下,Ty3 RT的最近解析结构在DNA聚合酶和核糖核酸酶H活性的基础基础上几乎没有增加新颖性,但它突出了逆转录病毒和LTR-逆转录转座子RT之间的显着拓扑差异。总体相似但截然不同的主题扩展到Ty3 RT用于引发(?)和(+)链DNA合成的启动机制。逆转座子酶的独特结构组织及其与核酸底物的相互作用,重点是由聚嘌呤束(PPT)引发的(+)链合成引发,是本综述的主题。

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