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两种腺病毒早期E1A蛋白的功能及其保守结构域在大鼠细胞周期改变、肌动蛋白重组和基因激活中的作用。

Functions of the two adenovirus early E1A proteins and their conserved domains in cell cycle alteration, actin reorganization, and gene activation in rat cells.

作者信息

Bellett A J, Jackson P, David E T, Bennett E J, Cronin B

机构信息

Department of Microbiology, John Curtin School of Medical Research, Canberra, Australia.

出版信息

J Virol. 1989 Jan;63(1):303-10. doi: 10.1128/JVI.63.1.303-310.1989.

DOI:10.1128/JVI.63.1.303-310.1989
PMID:2521185
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC247685/
Abstract

Rat embryo cells were infected with adenovirus type 5 mutants that code for only one of the two early E1A proteins, mutants with defects in one of the two conserved regions common to the two proteins, or mutants with defects in the 46-amino-acid region unique to the 289-amino-acid E1A protein. Cells were scored for altered cell cycle progression, disruption of actin stress fibers, and activation of E2A expression. Mutants lacking either E1A protein were able to cause all of these effects; but mutants lacking a 243-amino-acid protein had less effect, and mutants lacking a 289-amino-acid protein much less effect, than wild-type virus. A mutation in any of the three conserved regions caused a defect in each E1A effect. To investigate the reported function of conserved domain 2 in mitosis, we monitored by fluorescence-activated cell sorter the reduction in Hoechst 33342 fluorescence that occurs when cells divide after undergoing a round of DNA replication in 5-bromodeoxyuridine. A smaller percentage of adenovirus-infected cells than mock-infected cells divided within a given period after completing a round of DNA replication. Viruses with mutations in conserved domain 2 were defective for initiation of cellular DNA replication, as were all other E1A mutants we have examined, but had no specific defect in cell division compared with wild-type virus. Thus, although there may be some specialization of function between the two E1A proteins and between their conserved domains, it was not apparent in the aspects of E1A function and the mutants that we examined.

摘要

用5型腺病毒突变体感染大鼠胚胎细胞,这些突变体仅编码两种早期E1A蛋白中的一种、在两种蛋白共有的两个保守区域之一有缺陷的突变体,或在289个氨基酸的E1A蛋白特有的46个氨基酸区域有缺陷的突变体。对细胞进行评分,以评估细胞周期进程的改变、肌动蛋白应力纤维的破坏以及E2A表达的激活。缺乏任何一种E1A蛋白的突变体都能够引起所有这些效应;但是与野生型病毒相比,缺乏243个氨基酸蛋白的突变体效应较小,而缺乏289个氨基酸蛋白的突变体效应更小。三个保守区域中任何一个的突变都会导致每种E1A效应出现缺陷。为了研究保守结构域2在有丝分裂中报道的功能,我们通过荧光激活细胞分选仪监测了在5-溴脱氧尿苷中进行一轮DNA复制后细胞分裂时Hoechst 33342荧光的降低。在完成一轮DNA复制后的给定时间段内,腺病毒感染的细胞比 mock感染的细胞分裂的百分比更小。与我们检测的所有其他E1A突变体一样,保守结构域2发生突变的病毒在细胞DNA复制起始方面存在缺陷,但与野生型病毒相比,在细胞分裂方面没有特定缺陷。因此,尽管两种E1A蛋白及其保守结构域之间可能存在一些功能特化,但在我们检测的E1A功能和突变体方面并不明显。

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