鉴定水痘-带状疱疹病毒早期蛋白 ORF63 的磷酸化残基。
Identification of phosphorylated residues on varicella-zoster virus immediate-early protein ORF63.
机构信息
Department of Neurology, University of Colorado Denver School of Medicine, Denver, USA.
出版信息
J Gen Virol. 2010 May;91(Pt 5):1133-7. doi: 10.1099/vir.0.019067-0. Epub 2010 Jan 20.
Abstract
Efficient replication of varicella-zoster virus (VZV) in cell culture requires expression of protein encoded by VZV open reading frame 63 (ORF63p). Two-dimensional gel analysis demonstrates that ORF63p is extensively modified. Mass spectroscopy analysis of ORF63p isolated from transiently transfected HEK 293 and stably transfected MeWo cells identified 10 phosphorylated residues. In VZV-infected MeWo cells, only six phosphorylated residues were detected. This report identifies phosphorylation of two previously uncharacterized residues (Ser5 and Ser31) in ORF63p extracted from cells infected with VZV or transfected with an ORF63p expression plasmid. Computational analysis of ORF63p for known kinase substrates did not identify Ser5 or Ser31 as candidate phosphorylation sites, suggesting that either atypical recognition sequences or novel cellular kinases are involved in ORF63p post-translational modification.
摘要
水痘带状疱疹病毒(VZV)在细胞培养中的高效复制需要 VZV 开放阅读框 63(ORF63p)编码的蛋白表达。二维凝胶分析表明 ORF63p 广泛修饰。从瞬时转染的 HEK 293 和稳定转染的 MeWo 细胞中分离的 ORF63p 的质谱分析鉴定了 10 个磷酸化残基。在 VZV 感染的 MeWo 细胞中,仅检测到六个磷酸化残基。本报告鉴定了从 VZV 感染的细胞或转染 ORF63p 表达质粒中提取的 ORF63p 中的两个以前未表征的残基(Ser5 和 Ser31)的磷酸化。对 ORF63p 进行已知激酶底物的计算分析并未将 Ser5 或 Ser31 鉴定为候选磷酸化位点,这表明 ORF63p 的翻译后修饰涉及非典型识别序列或新型细胞激酶。
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