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参与烟草蚀纹马铃薯Y病毒细胞间和长距离移动的衣壳蛋白决定簇。

Capsid protein determinants involved in cell-to-cell and long distance movement of tobacco etch potyvirus.

作者信息

Dolja V V, Haldeman-Cahill R, Montgomery A E, Vandenbosch K A, Carrington J C

机构信息

Department of Biology, Texas A&M University, College Station 77843.

出版信息

Virology. 1995 Feb 1;206(2):1007-16. doi: 10.1006/viro.1995.1023.

Abstract

The tobacco etch potyvirus (TEV) capsid protein (CP) is necessary for cell-to-cell and long distance transport of the virus in plants. In this study, the transport phenotypes of TEV mutants containing CPs with a substitution of the highly conserved Ser122 (termed S122W) within the core domain, or with a deletion of sequences encoding 17 amino acid residues comprising most of the variable C-terminal domain (delta C), were analyzed. The S122W and delta C mutant genomes were amplified to levels comparable to parental virus in protoplasts. The S122W mutant was encapsidation-defective, although in transgenic plants expressing wild-type CP a small number of virions were observed after prolonged incubation. Cells infected by the delta C mutant produced virions, indicating that the C-terminal domain is not necessary for encapsidation. The mutants exhibited unique defects in cell-to-cell and long distance movement in plants. The S122W mutant was confined to single, primarily inoculated epidermal cells in nontransgenic plants, but the cell-to-cell movement defect was rescued efficiently by transgenic CP. Long distance movement of this mutant was also rescued in transgenic plants, but accumulation in systemically infected tissue was low compared to parental virus. The delta C mutant exhibited a slow cell-to-cell movement phenotype in inoculated leaves and a complete inability to move systemically in nontransgenic plants. Transgenic CP was able to rescue partially the slow cell-to-cell movement defect of the delta C mutant, but not the long distance transport defect. Taken together with previous results, these data suggest that the core domain of TEV CP provides a function essential during cell-to-cell movement and that the variable N- and C-terminal regions exposed on the virion surface are necessary for long distance transport. In addition, trans-inhibition models are presented to account for the widely differing transgenic complementation efficiencies of the various movement-defective mutants.

摘要

烟草蚀纹马铃薯Y病毒(TEV)的衣壳蛋白(CP)对于该病毒在植物体内的细胞间和长距离运输是必需的。在本研究中,分析了TEV突变体的运输表型,这些突变体的CP在核心结构域中有高度保守的Ser122被替换(称为S122W),或者缺失了编码包含大部分可变C末端结构域的17个氨基酸残基的序列(ΔC)。在原生质体中,S122W和ΔC突变体基因组被扩增到与亲本病毒相当的水平。S122W突变体存在衣壳化缺陷,尽管在表达野生型CP的转基因植物中,长时间孵育后观察到少量病毒粒子。被ΔC突变体感染的细胞产生了病毒粒子,这表明C末端结构域对于衣壳化不是必需的。这些突变体在植物的细胞间和长距离移动中表现出独特的缺陷。S122W突变体在非转基因植物中局限于单个主要接种的表皮细胞,但转基因CP有效地挽救了其细胞间移动缺陷。该突变体在转基因植物中的长距离移动也得到了挽救,但与亲本病毒相比,在系统感染组织中的积累较低。ΔC突变体在接种叶片中表现出缓慢的细胞间移动表型,并且在非转基因植物中完全不能进行系统移动。转基因CP能够部分挽救ΔC突变体缓慢的细胞间移动缺陷,但不能挽救长距离运输缺陷。结合先前的结果,这些数据表明TEV CP的核心结构域在细胞间移动过程中提供了一种必需的功能,并且病毒粒子表面暴露的可变N末端和C末端区域对于长距离运输是必需的。此外,还提出了反式抑制模型来解释各种移动缺陷突变体广泛不同的转基因互补效率。

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