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截短和 6 节序列改组产生复制型神经氨酸酶阴性的 H5N1 流感病毒。

Truncation and sequence shuffling of segment 6 generate replication-competent neuraminidase-negative influenza H5N1 viruses.

机构信息

Institutes of Diagnostic Virology.

出版信息

J Virol. 2013 Dec;87(24):13556-68. doi: 10.1128/JVI.02244-13. Epub 2013 Oct 9.

Abstract

Influenza viruses are highly genetically variable and escape from immunogenic pressure by antigenic changes in their surface proteins, referred to as "antigenic drift" and "antigenic shift." To assess the potential genetic plasticity under strong selection pressure, highly pathogenic avian influenza virus (HPAIV) of subtype H5N1 was passaged 50 times in embryonated chicken eggs in the presence of a neutralizing, polyclonal chicken serum. The resulting mutant acquired major alterations in the neuraminidase (NA)-encoding segment. Extensive deletions and rearrangements were detected, in contrast to only 12 amino acid substitutions within all other segments. Interestingly, this new neuraminidase segment resulted from complex sequence shuffling and insertion of a short fragment originating from the PA segment. Characterization of that novel variant revealed a loss of the neuraminidase protein and enzymatic activity, but its replication efficiency remained comparable to that of the wild type. Using reverse genetics, a recombinant virus consisting of the wild-type backbone and the shortened NA segment could be generated; however, generation of this recombinant virus required the polybasic hemagglutinin cleavage site. Two independent repetitions starting with egg passage 30 in the presence of alternative chicken-derived immune sera selected mutants with similar but different large deletions within the NA segment without any neuraminidase activity, indicating a general mechanism. In chicken, these virus variants were avirulent, even though the HPAIV polybasic hemagglutinin cleavage site was still present. Overall, the variants reported here are the first HPAIV H5N1 strains without a functional neuraminidase shown to grow efficiently without any helper factor. These novel HPAIV variants may facilitate future studies shedding light on the role of neuraminidase in virus replication and pathogenicity.

摘要

流感病毒具有高度的遗传变异性,可以通过表面蛋白的抗原变化逃避免疫压力,这种变化被称为“抗原漂移”和“抗原转变”。为了评估在强大选择压力下的潜在遗传可塑性,我们在含有中和性多克隆鸡血清的情况下,将高致病性禽流感病毒(HPAIV)亚型 H5N1 在鸡胚中传代 50 次。结果产生的突变体在神经氨酸酶(NA)编码片段中发生了主要改变。与其他所有片段中仅 12 个氨基酸取代相比,检测到广泛的缺失和重排。有趣的是,这个新的神经氨酸酶片段是由复杂的序列洗牌和来自 PA 片段的短片段插入产生的。对该新型变体的特征分析表明,神经氨酸酶蛋白及其酶活性丧失,但它的复制效率仍与野生型相当。使用反向遗传学,可以生成由野生型骨架和缩短的 NA 片段组成的重组病毒;然而,生成该重组病毒需要多碱性血凝素切割位点。在存在替代鸡源性免疫血清的情况下,从第 30 次鸡胚传代开始进行了两次独立的重复实验,选择了具有类似但不同的 NA 片段内较大缺失的突变体,但没有任何神经氨酸酶活性,这表明存在一种普遍机制。在鸡中,这些病毒变体是无毒的,尽管仍然存在 HPAIV 多碱性血凝素切割位点。总的来说,这里报道的变体是第一个没有功能性神经氨酸酶的 HPAIV H5N1 株,它们能够在没有任何辅助因子的情况下高效生长。这些新型 HPAIV 变体可能有助于未来的研究,阐明神经氨酸酶在病毒复制和致病性中的作用。

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