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Redistribution of microtubules and Golgi apparatus in herpes simplex virus-infected cells and their role in viral exocytosis.

机译:在单纯疱疹病毒感染的细胞中微管和高尔基体的重新分布及其在病毒胞吐中的作用。

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摘要

Earlier studies have shown that the Golgi apparatus was fragmented and dispersed in herpes simplex virus 1-infected Vero and HEp-2 cells but not in human 143TK- cells, that the fragmentation and dispersal required viral functions expressed concurrently with or after the onset of DNA synthesis (G. Campadelli-Fiume, R. Brandimarti, C. Di Lazzaro, P. L. Ward, B. Roizman, and M. R. Torrisi, Proc. Natl. Acad. Sci. USA 90:2798-2802, 1993), and that in 143TK- cells, but not Vero or HEp-2 cells, infected with viral mutants lacking the UL20 gene virions were glycosylated and transported to extracellular space (J. D. Baines, P. L. Ward, G. Campadelli-Fiume, and B. Roizman, J. Virol. 65:6414-6424, 1991; E. Avitabile, P. L. Ward, C. Di Lazzaro, M. R. Torrisi, B. Roizman, and G. Campadelli-Fiume, J. Virol. 68:7397-7405, 1994). Experiments designed to elucidate the role of the microtubules and of intact or fragmented Golgi apparatus in the exocytosis of virions showed the following. (i) In all cell lines tested (Vero, 143TK-, BHK, and Hep-2) microtubules underwent fragmentation particularly evident at the cell periphery and then reorganized into bundles which circumvent the nucleus. This event was not affected by inhibitors of viral DNA synthesis. We conclude that redistribution of microtubules may be required but is not sufficient for the fragmentation and dispersal of the Golgi apparatus. (ii) In all infected cell lines tested, nocodazole caused fragmentation and dispersal of the Golgi and a far more extensive depolymerization of the microtubules than was seen in untreated, infected Vero or HEp-2 cells. Taxol precluded the depolymerization of the microtubules and fragmentation of the Golgi in both infected cell lines. Neither nocodazole nor taxol affected the exocytosis of infectious virus from Vero, HEp-2, or 143TK- cells infected with wild-type virus. We conclude that the effects of nocodazole or of taxol are dominant over the effects of viral infection in the cell lines tested and that viral exocytosis is independent of the organization of microtubules or of the integrity of the Golgi apparatus. Lastly, the data suggest that herpes simplex viruses have evolved an exocytic pathway for which the UL20 protein is a component required in some cells but not others and in which this protein does not merely compensate for the fragmentation and dispersal of the Golgi apparatus.
机译:较早的研究表明,高尔基体破碎并分散在单纯疱疹病毒1感染的Vero和HEp-2细胞中,而不是在人143TK细胞中,这种破碎和分散需要病毒功能与DNA发作同时或之后表达。合成(G.Campadelli-Fiume,R.Brandimarti,C.Di Lazzaro,PL Ward,B.Roizman和MR Torrisi,Proc.Natl.Acad.Sci.USA 90:2798-2802,1993),以及143TK -将感染缺乏UL20基因病毒体的病毒突变体的细胞而不是Vero或HEp-2细胞进行糖基化并将其转运到细胞外空间(JD Baines,PL Ward,G.Campadelli-Fiume和B.Roizman,J.Virol。参见,例如,J.Vis.65:6414-6424,1991; E.Avitabile,PL Ward,C.Di Lazzaro,MR Torrisi,B.Roizman,和G.Campadelli-Fiume,J.Virol.68:7397-7405,1994)。旨在阐明微管以及完整或破碎的高尔基体在病毒粒子胞吐中的作用的实验显示如下。 (i)在所有测试的细胞系(Vero,143TK-,BHK和Hep-2)中,微管都在细胞外围特别明显地破碎,然后重组为绕核的束。该事件不受病毒DNA合成抑制剂的影响。我们得出结论,可能需要重新分配微管,但不足以使高尔基体碎裂和分散。 (ii)在所有测试的感染细胞系中,诺考达唑引起高尔基体的碎裂和分散,并且微管的解聚作用比未处理的,感染的Vero或HEp-2细胞更为广泛。紫杉醇排除了两种感染细胞系中微管的解聚和高尔基体的断裂。诺考达唑和紫杉醇均未影响感染了野生型病毒的Vero,HEp-2或143TK细胞感染性病毒的胞吐作用。我们得出的结论是,在测试的细胞系中,诺考达唑或紫杉醇的作用优于病毒感染的作用,并且病毒的胞吐作用与微管的组织或高尔基体的完整性无关。最后,数据表明单纯疱疹病毒已经进化出一种胞外途径,其中某些细胞需要UL20蛋白,而其他细胞则不需要,而且该蛋白不仅补偿了高尔基体的分裂和分散。

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