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在小鼠成纤维细胞克隆亚系(L2p.176细胞)中培养的原型和野生型大鼠冠状病毒分离株的生长特性和蛋白质谱。

Growth characteristics and protein profiles of prototype and wild-type rat coronavirus isolates grown in a cloned subline of mouse fibroblasts (L2p.176 cells).

作者信息

Gaertner D J, Compton S R, Winograd D F, Smith A L

机构信息

Section of Comparative Medicine, Yale University School of Medicine, New Haven, CT 06520-8016, USA.

出版信息

Virus Res. 1996 Mar;41(1):55-68. doi: 10.1016/0168-1702(95)01274-5.

DOI:10.1016/0168-1702(95)01274-5
PMID:8725102
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC7134090/
Abstract

Rat coronaviruses (RCVs) infect laboratory rats and confound biomedical research results. In vitro systems developed so far have limited the growth in knowledge about RCVs by not permitting generation of plaque-cloned virus stocks, reliable isolation of RCVs from rat tissues, or growth of high titered stocks of all isolates. Due to the fact that less than 20% of L2(Percy) cells were becoming infected, sublines were produced and selected for maximal growth of RCVs. Screening of 238 cell sublines yielded L2p.176 cells which were highly susceptible to all RCVs tested; however, susceptibility declined after 30 passages in vitro. Low-passaged L2p.176 cells were used to isolate virus from natural outbreaks and to propagate individual RCV plaques into high titered stocks. Proteins from six RCV isolates were immunoblotted using polyclonal rat and mouse antibodies to sialodacryoadenitis virus and polyclonal monospecific rabbit and goat antibodies against the peplomer (S) and nucleocapsid (N) proteins of mouse hepatitis virus (MHV). Proteins of two prototype, one Japanese and three wild type RCVs were examined and found to be similar to those of MHV, although the exact sizes and ratios of protein forms were unique for most RCV isolates. This study reports the development of a continuous cell line which reliably supports RCVs opening an opportunity for further in vivo studies of the biology of these agents. As a first step in the characterization of RCVs, we have shown that RCV proteins are very similar to those of MHV.

摘要

大鼠冠状病毒(RCV)可感染实验大鼠并干扰生物医学研究结果。迄今为止开发的体外系统由于无法产生空斑克隆病毒株、无法从大鼠组织中可靠分离出RCV或无法培养所有分离株的高滴度病毒株,限制了对RCV的了解。由于不到20%的L2(珀西)细胞被感染,因此产生了亚系并选择用于RCV的最大生长。对238个细胞亚系进行筛选后得到了L2p.176细胞,该细胞对所有测试的RCV都高度敏感;然而,在体外传代30次后敏感性下降。低代的L2p.176细胞被用于从自然爆发中分离病毒,并将单个RCV空斑繁殖成高滴度病毒株。使用抗涎泪腺炎病毒的多克隆大鼠和小鼠抗体以及抗小鼠肝炎病毒(MHV)的纤突(S)蛋白和核衣壳(N)蛋白的多克隆单特异性兔和山羊抗体,对六种RCV分离株的蛋白进行免疫印迹分析。对两种原型、一种日本和三种野生型RCV的蛋白进行了检测,发现它们与MHV的蛋白相似,尽管大多数RCV分离株的蛋白的确切大小和比例是独特的。本研究报告了一种连续细胞系的开发,该细胞系可可靠地支持RCV,为进一步对这些病原体的生物学进行体内研究提供了机会。作为RCV特性鉴定的第一步,我们已经表明RCV蛋白与MHV的蛋白非常相似。

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本文引用的文献

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Preliminary characterization of the structural proteins of the coronaviruses, sialodacryoadenitis virus and Parker's rat coronavirus.冠状病毒、涎泪腺炎病毒和帕克大鼠冠状病毒结构蛋白的初步特征分析
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Molecular characterization of the S proteins of two enterotropic murine coronavirus strains.两种嗜肠性小鼠冠状病毒株S蛋白的分子特征分析
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