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马铃薯黄花叶双生病毒的突变分析

Mutational analysis of potato yellow mosaic geminivirus.

作者信息

Sung Y K, Coutts R H

机构信息

Biology Department, Imperial College of Science, Technology and Medicine, London, UK.

出版信息

J Gen Virol. 1995 Jul;76 ( Pt 7):1773-80. doi: 10.1099/0022-1317-76-7-1773.

DOI:10.1099/0022-1317-76-7-1773
PMID:9049382
Abstract

Mutations have been inserted into the virion and complementary sense ORFs encoding proteins with M(r)s in excess of 9 kDa of both DNA A and DNA B of potato yellow mosaic geminivirus (PYMV). Wild-type and mutant monomeric clones were tested for their ability to replicate, produce PYMV-specific DNA, spread and cause symptoms in Nicotiana benthamiana plants following biolistic inoculation. Dimeric clones of the DNA A mutants were also investigated by agroinoculation of leaf discs. In contrast to N. benthamiana plants agroinoculated with PYMV DNA A, in which the wild-type DNA A component was capable of limited independent replication and spread, both excised DNA A and B components were required for DNA replication and symptom development in plants inoculated by the biolistic method. Mixtures of both genomic components were also infectious for potato plants following biolistic inoculation. Mutations in ORFs AL1, AL2, BR1 and BL1 resulted in clones incapable of infecting N. benthamiana plants. However, the AL2 mutation, but not the AL1 mutation, allowed viral DNA replication in leaf discs. Mutations to both the AR1 and AL3 ORFs produced clones which were infectious in plants but showed a considerable delay in the production of attenuated symptoms as compared to wild-type infections. Mutating the AL3 ORF dramatically reduced viral DNA replication in both whole plants and leaf discs. Mutations to the AL4 ORF produced clones which were as infectious for both N. benthamiana and potato plants as the wild-type clones. Our results are compared with those from mutagenesis studies on related bipartite geminiviruses.

摘要

已将突变插入马铃薯黄花叶双生病毒(PYMV)的病毒粒子以及编码分子量超过9 kDa蛋白质的互补义开放阅读框(ORF)中,该病毒的DNA A和DNA B均有这些突变。对野生型和突变型单体克隆进行了测试,以检测它们在通过生物弹道接种后在本氏烟草植株中复制、产生PYMV特异性DNA、传播并引起症状的能力。还通过对叶盘进行农杆菌接种研究了DNA A突变体的二聚体克隆。与用PYMV DNA A进行农杆菌接种的本氏烟草植株不同(在该植株中野生型DNA A组分能够进行有限的独立复制和传播),通过生物弹道接种法接种的植株中,DNA复制和症状发展需要切除的DNA A和B组分。两种基因组组分的混合物在通过生物弹道接种后对马铃薯植株也具有感染性。ORF AL1、AL2、BR1和BL1中的突变导致克隆无法感染本氏烟草植株。然而,AL2突变而非AL1突变允许病毒DNA在叶盘中复制。AR1和AL3 ORF的突变产生了在植株中具有感染性的克隆,但与野生型感染相比,其产生减弱症状的时间有相当大的延迟。突变AL3 ORF显著降低了病毒DNA在整株植物和叶盘中的复制。AL4 ORF的突变产生了与野生型克隆对本氏烟草和马铃薯植株具有相同感染性的克隆。我们将结果与相关双分体双生病毒的诱变研究结果进行了比较。

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