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Analysis of sequence diversity in hypervariable regions of the external glycoprotein of human immunodeficiency virus type 1.

机译:1型人类免疫缺陷病毒外部糖蛋白高变区的序列多样性分析

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摘要

Nucleotide sequences in three hypervariable regions of the human immunodeficiency virus type 1 (HIV-1) env gene were obtained by sequencing provirus present in peripheral blood mononuclear cells of HIV-infected individuals. Single molecules of target sequences were isolated by limiting dilution and amplified in two stages by the polymerase chain reaction, using nested primers. The product was directly sequenced to avoid errors introduced by Taq polymerase during the amplification process. There was extensive variation between sequences from the same individual as well as between sequences from different individuals. Interpatient variability was markedly less in individuals infected from a common source. A high proportion of amino acid substitutions in the hypervariable regions altered the number and positions of potential N-linked glycosylation sites. Sequences in two hypervariable regions frequently contained short (3- to 15-bp) duplications or deletions, and by amplifying peripheral blood mononuclear cell DNA containing 10(2) or 10(3) proviral molecules and analyzing the product by high-resolution electrophoresis, the total number and abundance of distinct length variants within an individual could be estimated, providing a more comprehensive analysis of the variants present than would be obtained by sequencing alone. Sequences from many individuals showed frequent amino acid substitutions at certain key positions for neutralizing-antibody and cytotoxic T-cell recognition in the immunodominant loop. The rates of synonymous and nonsynonymous nucleotide substitution in the region of this and flanking regions indicate that strong positive selection for amino acid change is operating in the generation of antigenic diversity.
机译:通过对存在HIV感染者外周血单个核细胞中的原病毒进行测序,获得了人类1型免疫缺陷病毒(HIV-1)env基因的三个高变区中的核苷酸序列。通过有限稀释分离靶序列的单分子,并使用嵌套引物通过聚合酶链反应分两个阶段进行扩增。将产物直接测序以避免扩增过程中Taq聚合酶引入的错误。同一个人的序列之间以及不同个人的序列之间存在广泛的差异。从共同来源感染的个体中患者之间的变异性明显降低。高变区中高比例的氨基酸取代改变了潜在的N-联糖基化位点的数量和位置。两个高变区中的序列通常包含短(3至15 bp)重复或缺失,并通过扩增包含10(2)或10(3)前病毒分子的外周血单核细胞DNA并通过高分辨率电泳分析产物,可以估算出一个个体中不同长度的变异体的总数和丰度,从而提供了比仅通过测序获得的变异体更全面的分析。来自许多个体的序列显示在某些关键位置频繁出现氨基酸取代,以中和抗体并在免疫优势环中识别出细胞毒性T细胞。在该区域和侧翼区域的同义和非同义核苷酸取代率表明,对氨基酸变化的强阳性选择在抗原多样性的产生中起作用。

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