首页> 美国卫生研究院文献>Nucleic Acids Research >The apical stem–loop of the hepatitis B virus encapsidation signal folds into a stable tri–loop with two underlying pyrimidine bulges
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The apical stem–loop of the hepatitis B virus encapsidation signal folds into a stable tri–loop with two underlying pyrimidine bulges

机译:乙型肝炎病毒衣壳信号的顶端茎环折叠成一个稳定的三环带有两个潜在的嘧啶凸起

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摘要

Reverse transcription of hepatitis B virus (HBV) pregenomic RNA is essential for virus replication. In the first step of this process, HBV reverse transcriptase binds to the highly conserved encapsidation signal, epsilon (ε), situated near the 5′ end of the pregenome. ε has been predicted to form a bulged stem–loop with the apical stem capped by a hexa– loop. After the initial binding to this apical stem– loop, the reverse transcriptase synthesizes a 4 nt primer using the bulge as a template. Here we present mutational and structural data from NMR on the apical stem–loop of ε. Application of new isotope-labeling techniques (13C/15N/2H-U-labeling) allowed resolution of many resonance overlaps and an extensive structural data set could be derived. The NMR data show that, instead of the predicted hexa–loop, the apical stem is capped by a stable UGU tri–loop closed by a C-G base pair, followed by a bulged out C. The apical stem contains therefore two unpaired pyrimidines (C1882 and U1889), rather than one as was predicted, spaced by 6 nt. C1882, the 3′ neighbour to the G of the loop-closing C-G base pair, is completely bulged out, while U1889 is at least partially intercalated into the stem. Analysis of 205 of our own HBV sequences and 1026 strains from the literature, covering all genotypes, reveals a high degree of conservation of ε. In particular, the residues essential for this fold are either totally conserved or show rare non-disruptive mutations. These data strongly indicate that this fold is essential for recognition by the reverse transcriptase.
机译:乙型肝炎病毒(HBV)前基因组RNA的逆转录对于病毒复制至关重要。在该过程的第一步中,HBV逆转录酶与位于前基因组5'末端附近的高度保守的衣壳化信号ε(ε)结合。预计ε会形成一个凸起的茎环,其顶部茎被六环覆盖。最初与该根茎杆环结合后,逆转录酶使用凸出物作为模板合成4 nt引物。在这里,我们介绍了ε的根茎环上NMR的突变和结构数据。同位素标记新技术( 13 C / 15 N / 2 HU标记)的应用可以解决许多共振重叠和广泛的结构可以导出数据集。 NMR数据显示,顶端茎被稳定的UGU三环(由CG碱基对封闭,然后由凸出的C取代)取代了预期的六环,因此,根茎包含两个未配对的嘧啶(C1882和U1889),而不是一个预期的,间隔为6 nt。闭环C-G碱基对的G的3'邻域C1882完全凸出,而U1889至少部分插入茎中。从文献中分析了我们自己的205株HBV序列和1026株,涵盖了所有基因型,揭示了ε的高度保守性。特别地,该折叠必不可少的残基是完全保守的或显示罕见的非破坏性突变。这些数据强烈表明该折叠对于逆转录酶的识别至关重要。

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