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猪细小病毒衣壳蛋白的高病毒进化率。

High rate of viral evolution in the capsid protein of porcine parvovirus.

机构信息

Institute for Animal Hygiene and Veterinary Public Health, Faculty of Veterinary Medicine, University of Leipzig, An den Tierkliniken 1, 04103 Leipzig, Germany.

Laboratório de Biologia Genômica e Molecular, Pontifícia Universidade Católica, Av. Ipiranga 6681, Prédio12, bloco C, sala 172, 90619-900 Porto Alegre, Brazil.

出版信息

J Gen Virol. 2011 Nov;92(Pt 11):2628-2636. doi: 10.1099/vir.0.033662-0. Epub 2011 Jul 27.

Abstract

In recent years, it has been shown that some parvoviruses exhibit high substitution rates, close to those of RNA viruses. In order to monitor and determine new mutations in porcine parvovirus (PPV), recent PPV field isolates from Austria, Brazil, Germany and Switzerland were sequenced and analysed. These samples, together with sequences retrieved from GenBank, were included in three datasets, consisting of the complete NS1 and VP1 genes and a partial VP1 gene. For each dataset, the nucleotide substitution rate and the molecular clock were determined. Analysis of the PPV field isolates revealed that a recently described amino acid substitution, S436T, appeared to be common in the VP2 protein in the Austrian, Brazilian and German virus populations. Furthermore, new amino acid substitutions were identified, located mainly in the viral capsid loops. By inferring the evolutionary dynamics of the PPV sequences, nucleotide substitution rates of approximately 10(-5) substitutions per site per year for the non-structural protein gene and 10(-4) substitutions per site per year for the capsid protein gene (for both viral protein datasets) were found. The latter rate is similar to those commonly found in RNA viruses. An association of the phylogenetic tree with the molecular clock analysis revealed that the mutations on which the divergence for both capsid proteins was based occurred in the past 30 years. Based on these findings, it was concluded that PPV variants are continuously evolving and that vaccines, which are based mainly on strains isolated about 30 years ago, should perhaps be updated.

摘要

近年来,已经表明一些细小病毒表现出高取代率,接近 RNA 病毒的取代率。为了监测和确定猪细小病毒 (PPV) 的新突变,对来自奥地利、巴西、德国和瑞士的最近的 PPV 田间分离株进行了测序和分析。这些样本与从 GenBank 中检索到的序列一起包含在三个数据集,包括完整的 NS1 和 VP1 基因和部分 VP1 基因。对于每个数据集,确定了核苷酸取代率和分子钟。对 PPV 田间分离株的分析表明,最近描述的氨基酸取代 S436T 似乎在奥地利、巴西和德国病毒群体的 VP2 蛋白中很常见。此外,还鉴定了新的氨基酸取代,主要位于病毒衣壳环中。通过推断 PPV 序列的进化动态,发现非结构蛋白基因的核苷酸取代率约为每年每个位点 10(-5) 个取代,衣壳蛋白基因的核苷酸取代率为每年每个位点 10(-4) 个取代(对于两个病毒蛋白数据集)。后者的速率与 RNA 病毒中常见的速率相似。与分子钟分析相关的系统发育树表明,两种衣壳蛋白分歧的突变发生在过去 30 年。基于这些发现,得出结论认为 PPV 变体在不断进化,主要基于大约 30 年前分离的毒株的疫苗可能需要更新。

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