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Identification of a truncated nucleoprotein in avian metapneumovirus-infected cells encoded by a second AUG, in-frame to the full-length gene

机译:鉴定由第二个AUG编码的禽偏肺炎病毒感染细胞中的截短的核蛋白,符合全长基因

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Background Avian metapneumoviruses (aMPV) cause an upper respiratory disease with low mortality, but high morbidity primarily in commercial turkeys. There are three types of aMPV (A, B, C) of which the C type is found only in the United States. Viruses related to aMPV include human, bovine, ovine, and caprine respiratory syncytial viruses and pneumonia virus of mice, as well as the recently identified human metapneumovirus (hMPV). The aMPV and hMPV have become the type viruses of a new genus within the Metapneumovirus. The aMPV nucleoprotein (N) amino acid sequences of serotypes A, B, and C were aligned for comparative analysis. Based on predicted antigenicity of consensus protein sequences, five aMPV-specific N peptides were synthesized for development of peptide-antigens and antisera. Results The presence of two aMPV nucleoprotein (N) gene encoded polypeptides was detected in aMPV/C/US/Co and aMPV/A/UK/3b infected Vero cells. Nucleoprotein 1 (N1) encoded from the first open reading frame (ORF) was predicted to be 394 amino acids in length for aMPV/C/US/Co and 391 amino acids in length for aMPV/A/UK/3b with approximate molecular weights of 43.3 kilodaltons and 42.7 kilodaltons, respectively. Nucleoprotein 2 (N2) was hypothesized to be encoded by a second downstream ORF in-frame with ORF1 and encoded a protein predicted to contain 328 amino acids for aMPV/C/US/Co or 259 amino acids for aMPV/A/UK/3b with approximate molecular weights of 36 kilodaltons and 28.3 kilodaltons, respectively. Peptide antibodies to the N-terminal and C-terminal portions of the aMPV N protein confirmed presence of these products in both aMPV/C/US/Co- and aMPV/A/UK/3b-infected Vero cells. N1 and N2 for aMPV/C/US/Co ORFs were molecularly cloned and expressed in Vero cells utilizing eukaryotic expression vectors to confirm identity of the aMPV encoded proteins. Conclusion This is the first reported identification of potential, accessory in-frame N2 ORF gene products among members of the Paramyxoviridae. Genomic sequence analyses of related members of the Pneumovirinae other than aMPV, including human respiratory syncytial virus and bovine respiratory syncytial virus demonstrated the presence of this second potential ORF among these agents.
机译:背景技术禽偏肺病毒(aMPV)引起上呼吸道疾病,死亡率低,但主要在商业火鸡中发病率高。存在三种类型的aMPV(A,B,C),其中C型仅在美国才能找到。与aMPV有关的病毒包括人,牛,绵羊和山羊的呼吸道合胞病毒和小鼠的肺炎病毒,以及最近鉴定出的人间质肺病毒(hMPV)。 aMPV和hMPV已成为间质肺病毒内新属的类型病毒。对比血清型A,B和C的aMPV核蛋白(N)氨基酸序列进行比较分析。基于共有蛋白序列的预测抗原性,合成了五种aMPV特异性N肽,用于开发肽抗原和抗血清。结果在aMPV / C / US / Co和aMPV / A / UK / 3b感染的Vero细胞中检测到两个编码aMPV核蛋白(N)的多肽。预测从第一个开放阅读框(ORF)编码的核蛋白1(N1)的长度约为394个氨基酸,而aMPV / C / US / Co的长度为391个氨基酸,而aMPV / A / UK / 3b的分子量约为39个氨基酸分别为43.3千吨和42.7千吨。假定蛋白2(N2)由第二个下游ORF与ORF1符合读框地编码,并编码一种蛋白,预测该蛋白包含328个氨基酸的aMPV / C / US / Co或259个氨基酸的aMPV / A / UK / 3b分子量分别约为36道尔顿和28.3道尔顿。针对aMPV N蛋白N端和C端部分的肽抗体证实了这些产物在aMPV / C / US / Co-和aMPV / A / UK / 3b感染的Vero细胞中的存在。使用真核表达载体分子克隆了aMPV / C / US / Co ORF的N1和N2,并在Vero细胞中表达,以确认aMPV编码蛋白的身份。结论这是首次报道了副粘病毒科成员中潜在的框内N2 ORF辅助基因产物的鉴定。除aMPV以外的肺炎链球菌相关成员的基因组序列分析,包括人呼吸道合胞病毒和牛呼吸道合胞病毒,表明在这些药物中存在第二种潜在的ORF。

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