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细小病毒LuIII在同步培养系统中的增殖。IV. 病毒结构多肽与宿主细胞染色质的关联

Multiplication of parvovirus LuIII in a synchronized culture system. IV. Association of viral structural polypeptides with the host cell chromatin.

作者信息

Gautschi M, Siegl G, Kronauer G

出版信息

J Virol. 1976 Oct;20(1):29-38. doi: 10.1128/JVI.20.1.29-38.1976.

Abstract

Newly synthesized structural polypeptides of parvovirus LuIII, VP1 (62,000 daltons) and VP2 (74,000 daltons), were detected in nuclei of synchronized, infected HeLa cells at 11 to 12 h postinfection, i.e., after cells had passed through the S phase of the cell cycle. At this time, most of intranuclear viral polypeptides were associated with the chromatin acidic proteins. However, 13 to 14 h postinfection, about one-third of intranuclear VP1 and VP2 also could be extracted in the fraction containing nuclear sap proteins. According to pulse-chase experiments, VP1 and VP2 accumulated in the chromatin with a time lag of 20 to 30 min. About 90% of these chromatin-associated viral polypeptides represented empty viral capsids. In addition, chromatin prepared at 14 h postinfection contained 90 to 95% of the total intranuclear viral 16S replicative-form DNA. Since viral replicative-form DNA and empty viral capsids seem to be associated specifically with cellular chromatin, we assume that this subnuclear structure is the site of the synthesis of progeny viral DNA and the formation of complete virions.

摘要

细小病毒LuIII新合成的结构多肽VP1(62,000道尔顿)和VP2(74,000道尔顿),在同步化感染的HeLa细胞的细胞核中于感染后11至12小时被检测到,即细胞经过细胞周期的S期之后。此时,大多数核内病毒多肽与染色质酸性蛋白相关。然而,在感染后13至14小时,约三分之一的核内VP1和VP2也能在含有核液蛋白的组分中被提取出来。根据脉冲追踪实验,VP1和VP2在染色质中积累存在20至30分钟的时间滞后。这些与染色质相关的病毒多肽中约90%代表空病毒衣壳。此外,感染后14小时制备的染色质含有核内病毒16S复制型DNA总量的90%至95%。由于病毒复制型DNA和空病毒衣壳似乎与细胞染色质特异性相关,我们推测这种亚核结构是子代病毒DNA合成和完整病毒粒子形成的场所。

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