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体内水稻东格鲁杆状病毒基因产物的检测

Detection of rice tungro bacilliform virus gene products in vivo.

作者信息

Hay J, Grieco F, Druka A, Pinner M, Lee S C, Hull R

机构信息

Department of Virology, John Innes Centre, Norwich Research Park, Colney, United Kingdom.

出版信息

Virology. 1994 Dec;205(2):430-7. doi: 10.1006/viro.1994.1663.

DOI:10.1006/viro.1994.1663
PMID:7526539
Abstract

To study the products of the open reading frames (ORFs) of rice tungro bacilliform virus in rice plants the sequences containing ORFs I (encoding a 24-kDa protein, P24) and IV (P46) and the protease and polymerase (reverse transcriptase+RNaseH) domains of ORF III were cloned into a pGEX expression vector. The proteins, which were C-terminal fusions to glutathione S-transferase, were expressed in Escherichia coli and antisera were raised against them which, together with an antiserum against virus particles, was used to probe blots of proteins from infected and uninoculated plants and from virus preparations. The P24 antiserum detected virus-specific proteins of 74, 60, and 52 kDa, which are much bigger than expected. These proteins were found in virus preparations and immunogold labeling suggested that they might be internal in the particles. Virus-specific proteins of 33, 37, 62, and > 150 kDa were revealed by antiserum to virus particles. The antiserum to the protease revealed proteins of 13.5, 37, and 68 kDa both in extracts from infected plants and in purified virus preparations. This antiserum decorated intact virus particles as did the particle antiserum. The polymerase domain antiserum reacted with products of 56, 65, and 68 kDa in extracts from infected plants but not in virus particles. The antiserum to the ORF IV product did not detect any bands in either infected plant extracts or virus preparations. The significance of these products is discussed.

摘要

为了研究水稻东格鲁杆状病毒开放阅读框(ORF)在水稻植株中的产物,将包含ORF I(编码24 kDa蛋白,P24)和IV(P46)以及ORF III的蛋白酶和聚合酶(逆转录酶+核糖核酸酶H)结构域的序列克隆到pGEX表达载体中。这些与谷胱甘肽S-转移酶C端融合的蛋白在大肠杆菌中表达,并制备了针对它们的抗血清,该抗血清与针对病毒粒子的抗血清一起用于检测来自感染和未接种植株以及病毒制剂的蛋白质印迹。P24抗血清检测到74、60和52 kDa的病毒特异性蛋白,它们比预期的要大得多。这些蛋白存在于病毒制剂中,免疫金标记表明它们可能在病毒粒子内部。病毒粒子抗血清揭示了33、37、62和>150 kDa的病毒特异性蛋白。蛋白酶抗血清在感染植株提取物和纯化病毒制剂中均检测到13.5、37和68 kDa的蛋白。该抗血清与完整病毒粒子结合,就像粒子抗血清一样。聚合酶结构域抗血清与感染植株提取物中的56、65和68 kDa产物反应,但不与病毒粒子反应。ORF IV产物的抗血清在感染植株提取物或病毒制剂中均未检测到任何条带。文中讨论了这些产物的意义。

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