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通过冷冻电子显微镜和X射线晶体学确定的T = 3二十面体动物病毒中准等效性的功能意义。

Functional implications of quasi-equivalence in a T = 3 icosahedral animal virus established by cryo-electron microscopy and X-ray crystallography.

作者信息

Cheng R H, Reddy V S, Olson N H, Fisher A J, Baker T S, Johnson J E

机构信息

Department of Biological Sciences, Purdue University, West Lafayette, Indiana 47907.

出版信息

Structure. 1994 Apr 15;2(4):271-82. doi: 10.1016/s0969-2126(00)00029-0.

Abstract

BACKGROUND

Studies of simple RNA animal viruses show that cell attachment, particle destabilization and cell entry are complex processes requiring a level of capsid sophistication that is difficult to achieve with a shell containing only a single gene product. Nodaviruses [such as Flock House virus (FHV)] are an exception. We have previously determined the structure of FHV at 3 A resolution, and now combine this information with data from cryo-electron microscopy in an attempt to clarify the process by which nodaviruses infect animal cells.

RESULTS

A difference map was computed in which electron density at 22 A resolution, derived from the 3.0 A resolution X-ray model of the FHV capsid protein, was subtracted from the electron density derived from the cryo-electron microscopy reconstruction of FHV at 22 A resolution. Comparisons of this density with the X-ray model showed that quasi-equivalent regions of identical polypeptide sequences have markedly different interactions with the bulk RNA density. Previously reported biphasic kinetics of particle maturation and the requirement of subunit cleavage for particle infectivity are consistent with these results.

CONCLUSIONS

On the basis of this study we propose a model for nodavirus infection that is conceptually similar to that proposed for poliovirus but differs from it in detail. The constraints of a single protein type in the capsid lead to a noteworthy use of quasi-symmetry not only to control the binding of a 'pocket factor' but also to modulate maturation cleavage and to release a pentameric helical bundle (with genomic RNA attached) that may further interact with the cell membrane.

摘要

背景

对简单RNA动物病毒的研究表明,细胞附着、病毒颗粒不稳定和细胞进入是复杂的过程,需要衣壳具备一定的复杂性,而仅包含单一基因产物的外壳难以实现这一点。诺达病毒(如禽呼肠孤病毒)是个例外。我们之前已确定禽呼肠孤病毒在3埃分辨率下的结构,现在将该信息与低温电子显微镜数据相结合,试图阐明诺达病毒感染动物细胞的过程。

结果

计算了一个差异图,其中从禽呼肠孤病毒衣壳蛋白的3.0埃分辨率X射线模型得出的22埃分辨率电子密度,从22埃分辨率的禽呼肠孤病毒低温电子显微镜重建得出的电子密度中减去。将该密度与X射线模型进行比较表明,相同多肽序列的准等效区域与整体RNA密度的相互作用明显不同。先前报道的病毒颗粒成熟的双相动力学以及颗粒感染性对亚基切割的要求与这些结果一致。

结论

基于本研究,我们提出了一个诺达病毒感染模型,该模型在概念上与脊髓灰质炎病毒的模型相似,但在细节上有所不同。衣壳中单一蛋白质类型的限制导致了准对称性的显著应用,不仅用于控制“口袋因子”的结合,还用于调节成熟切割并释放可能与细胞膜进一步相互作用的五聚体螺旋束(附着有基因组RNA)。

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