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人巨细胞病毒对细胞胸苷激酶的刺激作用。

Stimulation of cellular thymidine kinases by human cytomegalovirus.

作者信息

Estes J E, Huang E S

出版信息

J Virol. 1977 Oct;24(1):13-21. doi: 10.1128/JVI.24.1.13-21.1977.

Abstract

Thymidine kinase (TK) activity in WI-38 and MRC-5 human fibroblasts was analyzed by discontinuous polyacrylamide gel electrophoresis (disc-PAGE) and discontinuous glycerol gradient electrophoresis (disc-GEP) after subculture or human cytomegalovirus (HCMV) infection. Two peaks of TK activity with different relative fraction-of-migration (R(f)) values were resolved by disc-PAGE or disc-GEP in extracts from log-phase and infected cells. Growing WI-38 cells expressed a slowly migrating (R(f) = 0.14 PAGE, R(f) = 0.4 GEP) peak of TK activity, which was partially inhibited by 1.0 mM dCTP, but which retained little activity at pH 4.5. Growing MRC cells also displayed a slowly migrating peak (R(f) = 0.10 PAGE) with similar properties. Both cell types expressed a faster-migrating TK activity (R(f) = 0.45 PAGE, R(f) = 0.7 GEP) in the growing and resting state that was strongly inhibited by 1 mM dCTP but retained 50% activity at pH 4.5. When either cell type was infected with HCMV, there was a rapid and high-level stimulation of the slowly migrating form of TK and a slight stimulation of the faster-migrating form. Two strains of HCMV (AD169 and Town) failed to produce an electrophoretically distinct virus TK in either cell type after infection. TK enzymes were partially purified by disc-GEP from extracts of log-phase WI-38 or AD169-infected WI-38 cells. Characterization of these enzymes with respect to phosphate donor specificity, pH optima, thermostability, and salt inhibition showed the HCMV-stimulated TKs to be of cellular origin.

摘要

在传代培养或人巨细胞病毒(HCMV)感染后,通过不连续聚丙烯酰胺凝胶电泳(disc-PAGE)和不连续甘油梯度电泳(disc-GEP)分析WI-38和MRC-5人成纤维细胞中的胸苷激酶(TK)活性。在对数期细胞和感染细胞的提取物中,通过disc-PAGE或disc-GEP分离出两个具有不同相对迁移率(R(f))值的TK活性峰。生长中的WI-38细胞表达一个迁移缓慢的(R(f) = 0.14,PAGE;R(f) = 0.4,GEP)TK活性峰,该峰被1.0 mM dCTP部分抑制,但在pH 4.5时活性很低。生长中的MRC细胞也显示出一个具有相似特性的迁移缓慢的峰(R(f) = 0.10,PAGE)。两种细胞类型在生长和静止状态下均表达一种迁移较快的TK活性(R(f) = 0.45,PAGE;R(f) = 0.7,GEP),该活性被1 mM dCTP强烈抑制,但在pH 4.5时保留50%的活性。当任何一种细胞类型感染HCMV时,迁移缓慢的TK形式会迅速受到高水平刺激,而迁移较快的形式受到轻微刺激。两株HCMV(AD169和Town)感染后,在任何一种细胞类型中均未产生电泳上明显不同的病毒TK。通过disc-GEP从对数期WI-38或AD169感染的WI-38细胞提取物中部分纯化TK酶。对这些酶在磷酸供体特异性、最适pH、热稳定性和盐抑制方面的特性进行表征,结果表明HCMV刺激的TK是细胞来源的。

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