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Sequences of complete human cytomegalovirus genomes from infected cell cultures and clinical specimens.从感染细胞培养物和临床标本中获得的完整人类巨细胞病毒基因组序列。
J Gen Virol. 2010 Mar;91(Pt 3):605-15. doi: 10.1099/vir.0.015891-0. Epub 2009 Nov 11.
2
Sense from sequence reads: methods for alignment and assembly.从序列读取中获取意义:比对和组装方法
Nat Methods. 2009 Nov;6(11 Suppl):S6-S12. doi: 10.1038/nmeth.1376.
3
Genomics. Genome project standards in a new era of sequencing.基因组学。测序新时代的基因组计划标准。
Science. 2009 Oct 9;326(5950):236-7. doi: 10.1126/science.1180614.
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Detection of novel sequences related to african Swine Fever virus in human serum and sewage.在人血清和污水中检测与非洲猪瘟病毒相关的新序列。
J Virol. 2009 Dec;83(24):13019-25. doi: 10.1128/JVI.00638-09. Epub 2009 Oct 7.
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Divergence and genotyping of human alpha-herpesviruses: an overview.人类α疱疹病毒的分化与基因分型:概述。
Infect Genet Evol. 2010 Jan;10(1):14-25. doi: 10.1016/j.meegid.2009.09.004. Epub 2009 Sep 20.
6
Insertional mutations in herpes simplex virus type 1 gL identify functional domains for association with gH and for membrane fusion.1型单纯疱疹病毒gL中的插入突变鉴定了与gH结合及膜融合的功能结构域。
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J Virol. 2009 Nov;83(22):11599-606. doi: 10.1128/JVI.00677-09. Epub 2009 Sep 2.
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High-throughput sequencing reveals suppressors of Vibrio cholerae rpoE mutations: one fewer porin is enough.高通量测序揭示霍乱弧菌rpoE突变的抑制因子:少一个孔蛋白就足够了。
Nucleic Acids Res. 2009 Sep;37(17):5757-67. doi: 10.1093/nar/gkp568. Epub 2009 Jul 20.
9
Characterization of the herpes simplex virus (HSV)-1 tegument protein VP1-2 during infection with the HSV temperature-sensitive mutant tsB7.单纯疱疹病毒1型(HSV-1)温度敏感突变体tsB7感染期间病毒被膜蛋白VP1-2的特性分析
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10
Disruption of LANA in rhesus rhadinovirus generates a highly lytic recombinant virus.恒河猴疱疹病毒中LANA的破坏产生了一种高度裂解性的重组病毒。
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单纯疱疹病毒 1 临床和实验室分离株的序列变异揭示了新的突变。

Sequence variability in clinical and laboratory isolates of herpes simplex virus 1 reveals new mutations.

机构信息

Department of Molecular Biology, Princeton University, Princeton, New Jersey 08544, USA.

出版信息

J Virol. 2010 May;84(10):5303-13. doi: 10.1128/JVI.00312-10. Epub 2010 Mar 10.

DOI:10.1128/JVI.00312-10
PMID:20219902
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC2863834/
Abstract

Herpes simplex virus 1 (HSV-1) is a well-adapted human pathogen that can invade the peripheral nervous system and persist there as a lifelong latent infection. Despite their ubiquity, only one natural isolate of HSV-1 (strain 17) has been sequenced. Using Illumina high-throughput sequencing of viral DNA, we obtained the genome sequences of both a laboratory strain (F) and a low-passage clinical isolate (H129). These data demonstrated the extent of interstrain variation across the entire genome of HSV-1 in both coding and noncoding regions. We found many amino acid differences distributed across the proteome of the new strain F sequence and the previously known strain 17, demonstrating the spectrum of variability among wild-type HSV-1 proteins. The clinical isolate, strain H129, displays a unique anterograde spread phenotype for which the causal mutations were completely unknown. We have defined the sequence differences in H129 and propose a number of potentially causal genes, including the neurovirulence protein ICP34.5 (RL1). Further studies will be required to demonstrate which change(s) is sufficient to recapitulate the spread defect of strain H129. Unexpectedly, these data also revealed a frameshift mutation in the UL13 kinase in our strain F isolate, demonstrating how deep genome sequencing can reveal the full complement of background mutations in any given strain, particularly those passaged or plaque purified in a laboratory setting. These data increase our knowledge of sequence variation in large DNA viruses and demonstrate the potential of deep sequencing to yield insight into DNA genome evolution and the variation among different pathogen isolates.

摘要

单纯疱疹病毒 1(HSV-1)是一种适应良好的人类病原体,能够侵入外周神经系统并作为终身潜伏感染存在。尽管它们无处不在,但只有一种 HSV-1 的天然分离株(株 17)被测序。我们使用 Illumina 高通量测序病毒 DNA,获得了实验室株(F)和低传代临床分离株(H129)的基因组序列。这些数据表明,在 HSV-1 的整个基因组中,无论是编码区还是非编码区,株间变异程度很大。我们发现,新株 F 序列和以前已知的株 17 的整个蛋白质组中分布着许多氨基酸差异,表明野生型 HSV-1 蛋白的变异性谱。临床分离株 H129 表现出独特的顺行传播表型,其因果突变完全未知。我们已经定义了 H129 的序列差异,并提出了一些潜在的因果基因,包括神经毒蛋白 ICP34.5(RL1)。需要进一步的研究来证明哪些变化足以重现 H129 株的传播缺陷。出乎意料的是,这些数据还揭示了我们株 F 分离株 UL13 激酶中的一个移码突变,表明深度基因组测序如何能够揭示任何给定菌株的完整背景突变,特别是那些在实验室环境中传代或斑块纯化的菌株。这些数据增加了我们对大 DNA 病毒序列变异的认识,并展示了深度测序在深入了解 DNA 基因组进化和不同病原体分离株之间的变异方面的潜力。