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Historical overview of research on the tobacco mosaic virus genome: genome organization infectivity and gene manipulation.

机译:烟草花叶病毒基因组研究的历史回顾:基因组组织感染性和基因操作。

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摘要

Early in the development of molecular biology, TMV RNA was widely used as a mRNA [corrected] that could be purified easily, and it contributed much to research on protein synthesis. Also, in the early stages of elucidation of the genetic code, artificially produced TMV mutants were widely used and provided the first proof that the genetic code was non-overlapping. In 1982, Goelet et al. determined the complete TMV RNA base sequence of 6395 nucleotides. The four genes (130K, 180K, 30K and coat protein) could then be mapped at precise locations in the TMV genome. Furthermore it had become clear, a little earlier, that genes located internally in the genome were expressed via subgenomic mRNAs. The initiation site for assembly of TMV particles was also determined. However, although TMV contributed so much at the beginning of the development of molecular biology, its influence was replaced by that of Escherichia coli and its phages in the next phase. As recombinant DNA technology developed in the 1980s, RNA virus research became more detached from the frontier of molecular biology. To recover from this setback, a gene-manipulation system was needed for RNA viruses. In 1986, two such systems were developed for TMV, using full-length cDNA clones, by Dawson's group and by Okada's group. Thus, reverse genetics could be used to elucidate the basic functions of all proteins encoded by the TMV genome. Identification of the function of the 30K protein was especially important because it was the first evidence that a plant virus possesses a cell-to-cell movement function. Many other plant viruses have since been found to encode comparable 'movement proteins'. TMV thus became the first plant virus for which structures and functions were known for all its genes. At the birth of molecular plant pathology, TMV became a leader again. TMV has also played pioneering roles in many other fields. TMV was the first virus for which the amino acid sequence of the coat protein was determined and first virus for which cotranslational disassembly was demonstrated both in vivo and in vitro. It was the first virus for which activation of a resistance gene in a host plant was related to the molecular specificity of a product of a viral gene. Also, in the field of plant biotechnology, TMV vectors are among the most promising. Thus, for the 100 years since Beijerinck's work, TMV research has consistently played a leading role in opening up new areas of study, not only in plant pathology, but also in virology, biochemistry, molecular biology, RNA genetics and biotechnology.
机译:在分子生物学发展的早期,TMV RNA被广泛用作一种可以很容易纯化的[校正过的] mRNA,它为蛋白质合成的研究做出了很大贡献。同样,在阐明遗传密码的早期,人工生产的TMV突变体被广泛使用,并提供了遗传密码不重叠的第一个证据。 1982年,Goelet等人。确定了6395个核苷酸的完整TMV RNA碱基序列。然后可以将四个基因(130K,180K,30K和外壳蛋白)定位在TMV基因组中的精确位置。此外,很早以前就已经知道,基因组内部的基因是通过亚基因组mRNA表达的。还确定了TMV颗粒组装的起始位点。但是,尽管TMV在分子生物学发展的初期就做出了巨大贡献,但其影响在下一阶段被大肠杆菌及其噬菌体所取代。随着1980年代重组DNA技术的发展,RNA病毒的研究变得与分子生物学的前沿越来越脱节。为了从这种挫折中恢复过来,RNA病毒需要一个基因操纵系统。 1986年,道森(Dawson)组和冈田(Okada)组使用全长cDNA克隆为TMV开发了两个这样的系统。因此,反向遗传学可用于阐明TMV基因组编码的所有蛋白质的基本功能。鉴定30K蛋白的功能尤为重要,因为这是植物病毒具有细胞间移动功能的第一个证据。此后发现许多其他植物病毒可编码类似的“运动蛋白”。因此,TMV成为第一个以其所有基因都知道其结构和功能的植物病毒。在分子植物病理学诞生之初,TMV再次成为领导者。 TMV在许多其他领域也发挥了先锋作用。 TMV是第一种确定外壳蛋白氨基酸序列的病毒,也是第一种在体内和体外均证明其共翻译反汇编的病毒。它是第一种病毒,其宿主植物中抗性基因的激活与病毒基因产物的分子特异性有关。同样,在植物生物技术领域,TMV载体是最有前途的。因此,自贝耶琳克工作100年来,TMV研究一直在开拓新的研究领域中发挥着领导作用,不仅在植物病理学领域,而且在病毒学,生物化学,分子生物学,RNA遗传学和生物技术领域。

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