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The Genome of Fowlpox Virus

机译:禽痘病毒的基因组

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摘要

Here we present the genomic sequence, with analysis, of a pathogenic fowlpox virus (FPV). The 288-kbp FPV genome consists of a central coding region bounded by identical 9.5-kbp inverted terminal repeats and contains 260 open reading frames, of which 101 exhibit similarity to genes of known function. Comparison of the FPV genome with those of other chordopoxviruses (ChPVs) revealed 65 conserved gene homologues, encoding proteins involved in transcription and mRNA biogenesis, nucleotide metabolism, DNA replication and repair, protein processing, and virion structure. Comparison of the FPV genome with those of other ChPVs revealed extensive genome colinearity which is interrupted in FPV by a translocation and a major inversion, the presence of multiple and in some cases large gene families, and novel cellular homologues. Large numbers of cellular homologues together with 10 multigene families largely account for the marked size difference between the FPV genome (260 to 309 kbp) and other known ChPV genomes (178 to 191 kbp). Predicted proteins with putative functions involving immune evasion included eight natural killer cell receptors, four CC chemokines, three G-protein-coupled receptors, two β nerve growth factors, transforming growth factor β, interleukin-18-binding protein, semaphorin, and five serine proteinase inhibitors (serpins). Other potential FPV host range proteins included homologues of those involved in apoptosis (e.g., Bcl-2 protein), cell growth (e.g., epidermal growth factor domain protein), tissue tropism (e.g., ankyrin repeat-containing gene family, N1R/p28 gene family, and a T10 homologue), and avian host range (e.g., a protein present in both fowl adenovirus and Marek's disease virus). The presence of homologues of genes encoding proteins involved in steroid biogenesis (e.g., hydroxysteroid dehydrogenase), antioxidant functions (e.g., glutathione peroxidase), vesicle trafficking (e.g., two α-type soluble NSF attachment proteins), and other, unknown conserved cellular processes (e.g., Hal3 domain protein and GSN1/SUR4) suggests that significant modification of host cell function occurs upon viral infection. The presence of a cyclobutane pyrimidine dimer photolyase homologue in FPV suggests the presence of a photoreactivation DNA repair pathway. This diverse complement of genes with likely host range functions in FPV suggests significant viral adaptation to the avian host.
机译:在这里,我们通过分析介绍了致病性禽痘病毒(FPV)的基因组序列。 288 kbp FPV基因组由一个由相同的9.5 kbp反向末端重复序列界定的中央编码区组成,并包含260个开放阅读框,其中101个与已知功能的基因相似。将FPV基因组与其他脊索病毒(ChPV)的基因组进行比较,发现65个保守的基因同源物,编码参与转录和mRNA生物发生,核苷酸代谢,DNA复制和修复,蛋白质加工以及病毒体结构的蛋白质。将FPV基因组与其他ChPV的基因组进行比较,发现广泛的基因组共线性在FPV中被易位和主要倒转,多个基因家族(在某些情况下是大型基因家族)的存在以及新颖的细胞同源物所中断。大量的细胞同源物以及10个多基因家族在很大程度上解释了FPV基因组(260至309 kbp)和其他已知的ChPV基因组(178至191 kbp)之间明显的大小差异。具有推定功能的涉及免疫逃逸的预测蛋白包括八个自然杀伤细胞受体,四个CC趋化因子,三个G蛋白偶联受体,两个β神经生长因子,转化生长因子β,白介素18结合蛋白,信号蛋白和五个丝氨酸蛋白酶抑制剂(丝氨酸蛋白酶抑制剂)。其他潜在的FPV宿主范围蛋白包括与细胞凋亡相关的同源物(例如Bcl-2蛋白),细胞生长(例如表皮生长因子域蛋白),组织嗜性(例如锚蛋白重复序列​​基因家族,N1R / p28基因)家族,T10同源物和禽类宿主范围(例如禽腺病毒和马立克氏病病毒中都存在一种蛋白质)。存在与类固醇生物发生有关的蛋白质的编码基因的同源物(例如,羟基类固醇脱氢酶),抗氧化剂功能(例如,谷胱甘肽过氧化物酶),囊泡运输(例如,两种α型可溶性NSF附着蛋白)以及其他未知的保守细胞过程(例如,Hal3结构域蛋白和GSN1 / SUR4)表明病毒感染后宿主细胞功能发生了显着改变。 FPV中环丁烷嘧啶二聚体光解酶同系物的存在表明存在光活化DNA修复途径。 FPV中可能具有宿主范围功能的基因的这种多样化补体表明病毒对禽类宿主的适应性强。

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