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The Nucleotide Sequence and Spliced pol mRNA Levels of the Nonprimate Spumavirus Bovine Foamy Virus

机译:非灵长类Spumavirus牛泡沫病毒的核苷酸序列和剪接的pol mRNA水平

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摘要

We have determined the complete nucleotide sequence of a replication-competent clone of bovine foamy virus (BFV) and have quantitated the amount of splice pol mRNA processed early in infection. The 544-amino-acid Gag protein precursor has little sequence similarity with its primate foamy virus homologs, but the putative nucleocapsid (NC) protein, like the primate NCs, contains the three glycine-arginine-rich regions that are postulated to bind genomic RNA during virion assembly. The BFV gag and pol open reading frames overlap, with pro and pol in the same translational frame. As with the human foamy virus (HFV) and feline foamy virus, we have detected a spliced pol mRNA by PCR. Quantitatively, this mRNA approximates the level of full-length genomic RNA early in infection. The integrase (IN) domain of reverse transcriptase does not contain the canonical HH-CC zinc finger motif present in all characterized retroviral INs, but it does contain a nearby histidine residue that could conceivably participate as a member of the zinc finger. The env gene encodes a protein that is over 40% identical in sequence to the HFV Env. By comparison, the Gag precursor of BFV is predicted to be only 28% identical to the HFV protein.
机译:我们已经确定了牛泡沫病毒(BFV)具有复制能力的克隆的完整核苷酸序列,并定量了感染初期加工的剪接pol mRNA的数量。 544个氨基酸的Gag蛋白前体与其灵长类泡沫病毒同源物几乎没有序列相似性,但是推定的核衣壳(NC)蛋白像灵长类NC一样,包含三个富含甘氨酸和精氨酸的区域,这些区域被假定与基因组RNA结合。在病毒体组装期间。 BFV gag和pol开放阅读框重叠,pro和pol位于同一翻译框中。与人类泡沫病毒(HFV)和猫泡沫病毒一样,我们已经通过PCR检测到剪接的pol mRNA。从数量上讲,该mRNA接近感染早期全长基因组RNA的水平。逆转录酶的整合酶(IN)域不包含存在于所有特征性逆转录病毒IN中的典型HH-CC锌指基序,但确实包含附近的组氨酸残基,可以想象作为锌指的成员参与。 env基因编码的蛋白质与HFV Env的序列具有40%以上的同一性。相比之下,预计BFV的Gag前体与HFV蛋白只有28%的同一性。

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