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KU812Ep6细胞中细小病毒B19 2型的特征分析

Characterization of Parvovirus B19 genotype 2 in KU812Ep6 cells.

作者信息

Blümel Johannes, Eis-Hübinger Anna Maria, Stühler Albert, Bönsch Claudia, Gessner Matthias, Löwer Johannes

机构信息

Paul-Ehrlich-Institut, Langen, Germany.

出版信息

J Virol. 2005 Nov;79(22):14197-206. doi: 10.1128/JVI.79.22.14197-14206.2005.

DOI:10.1128/JVI.79.22.14197-14206.2005
PMID:16254355
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC1280213/
Abstract

An infectious parvovirus B19 (B19V) genotype 2 variant was identified as a high-titer contaminant in a human plasma donation. Genome analysis revealed a 138-bp insertion within the p6 promoter. The inserted sequence was represented by an additional 30 bp from the end of the inverted terminal repeat adjacent to a 108-bp element found also, in inverted orientation, at the extreme right end of the unique sequence of the genome. However, despite the profound variations in the promoter region, the pattern of gene expression and DNA replication did not differ between genotype 1 and genotype 2 in permissive erythroid KU812Ep6 cells. Capsid proteins of both genotypes differ in their amino acid sequences. However, equivalent kinetics of virus inactivation at 56 degrees C or pH 4 indicated a comparable physicochemical stability of virus capsids. Sera from six individuals infected by B19V genotype 1 were investigated on cross-neutralization of B19V genotype 2 in vitro. Similar neutralization of both B19V genotypes was observed in sera from three individuals, while the sera from three other individuals showed weaker cross-neutralization for genotype 2. In conclusion, the in vitro replication characteristics and physical stability of B19V capsids are very similar between human parvovirus B19 genotypes 1 and 2, and cross-neutralization indicates a close antigenic relation of genotypes 1 and 2.

摘要

一种传染性细小病毒B19(B19V)基因型2变体在一份人类血浆捐献物中被鉴定为高滴度污染物。基因组分析显示在p6启动子内有一个138碱基对的插入。插入序列由来自反向末端重复序列末端的另外30个碱基对以及一个108碱基对的元件组成,该元件也以反向方向存在于基因组独特序列的最右端。然而,尽管启动子区域存在显著差异,但在允许性红系KU812Ep6细胞中,1型和2型的基因表达模式和DNA复制并无不同。两种基因型的衣壳蛋白氨基酸序列不同。然而,在56℃或pH 4条件下病毒灭活的等效动力学表明病毒衣壳具有相当的物理化学稳定性。对6名感染B19V基因型1的个体的血清进行了体外对B19V基因型2交叉中和作用的研究。在3名个体的血清中观察到对两种B19V基因型的类似中和作用,而另外3名个体的血清对2型的交叉中和作用较弱。总之,人细小病毒B19的1型和2型之间,B19V衣壳的体外复制特性和物理稳定性非常相似,交叉中和表明1型和2型之间存在密切的抗原关系。

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