首页> 美国卫生研究院文献>Nucleic Acids Research >A sequence immediately upstream of the plus-strand primer is essential for plus-strand DNA synthesis of the Saccharomyces cerevisiae Ty1 retrotransposon.
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A sequence immediately upstream of the plus-strand primer is essential for plus-strand DNA synthesis of the Saccharomyces cerevisiae Ty1 retrotransposon.

机译:正链引物正上游的序列对于酿酒酵母Ty1反转录转座子的正链DNA合成至关重要。

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摘要

Priming of plus-strand DNA is a critical step in reverse transcription of retroviruses and retrotransposons. All retroelements use an RNase H-resistant oligoribonucleotide spanning a purine-rich sequence (the polypurine tract or PPT) to prime plus-strand DNA synthesis. Plus-strand DNA synthesis of the yeast Saccharomyces cerevisiae Ty1-H3 retrotransposon is initiated at two sites, PPT1 and PPT2, located at the upstream boundary of the 3'-long terminal repeat and near the middle of the pol gene in the integrase coding region. The two plus-strand primers have the same purine-rich sequence GGGTGGTA. This sequence is not sufficient by itself to generate a plus-strand origin since two identical sequences located upstream of PPT2 in the integrase coding region are not used efficiently as primers for plus-strand DNA synthesis. Thus, other factors must be involved in the formation of a specific plus-strand DNA primer. We show here that mutations upstream of the PPT in a highly conserved T-rich region severely alters plus-strand DNA priming of Ty1. Our results demonstrate the importance of sequences or structural elements upstream of the PPT for initiation of plus-strand DNA synthesis.
机译:正链DNA的引物是逆转录病毒和逆转座子逆转录的关键步骤。所有的逆转录元件都使用跨越富嘌呤序列(多嘌呤区或PPT)的RNase H耐药寡核苷酸来引发正链DNA合成。酵母酿酒酵母Ty1-H3逆转座子的正链DNA合成起始于两个位点PPT1和PPT2,位于3'长末端重复序列的上游边界且位于整合酶编码区中pol基因的中间附近。两条正链引物具有相同的富嘌呤序列GGGTGGTA。该序列本身不足以产生正链起源,因为位于整合酶编码区中PPT2上游的两个相同序列不能有效地用作正链DNA合成的引物。因此,其他因素必须与特异性正链DNA引物的形成有关。我们在这里显示,高度保守的T富集区域中PPT上游的突变严重改变Ty1的正链DNA引发。我们的结果证明了PPT上游序列或结构元件对于启动正链DNA合成的重要性。

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