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利用简并引物介导的聚合酶链反应对长线形病毒基因组进行筛选。

Screening of the closterovirus genome by degenerate primer-mediated polymerase chain reaction.

作者信息

Karasev A V, Nikolaeva O V, Koonin E V, Gumpf D J, Garnsey S M

机构信息

Department of Plant Pathology, University of California, Riverside 92521-0122.

出版信息

J Gen Virol. 1994 Jun;75 ( Pt 6):1415-22. doi: 10.1099/0022-1317-75-6-1415.

DOI:10.1099/0022-1317-75-6-1415
PMID:8207405
Abstract

The genome of beet yellows virus (BYV), the type representative of the closterovirus group, encodes a homologue of the cellular heat-shock protein (HSP) 70 family. A pair of degenerate primers targeted to motifs A and E, which are highly conserved in HSP70s, was synthesized. Genomes of several definite and possible members of the closterovirus group were screened for the presence of the HSP70 gene with PCR using these degenerate primers. BYV, citrus tristeza virus (CTV), beet yellow stunt virus (BYSV) and carnation necrotic fleck virus templates produced 1 kb amplification products, which were shown by sequencing to represent fragments of the respective HSP70 genes. Further screening was performed with an additional degenerate primer targeted to the motif IV of the putative viral polymerase. This degenerate primer and specific primers complementary to the 5' region of the HSP70 genes of the respective viruses were used to estimate the distance between polymerase motif IV and the start point of the HSP70 gene for BYV (approximately 1.1 kb), CTV and BYSV (around 2.0 kb) by PCR. The amplified genome regions of CTV (3026 nucleotides) and BYSV (2837 nucleotides) were cloned and sequenced. CTV and BYSV were found to encode the gene for an additional 30K (BYSV) or 33K (CTV) protein between the polymerase and the small hydrophobic protein genes, which was absent in BYV. These two 30K proteins displayed very weak similarity to each other, unlike the highly conserved polymerases, hydrophobic proteins and HSP70s of BYV, CTV and BYSV. Degenerate primer-mediated PCR proved to be an efficient tool for rapid screening and subsequent cloning of the viral genomes.

摘要

甜菜黄化病毒(BYV)是长线形病毒属的典型代表,其基因组编码一种细胞热休克蛋白(HSP)70家族的同源物。合成了一对针对基序A和E的简并引物,这两个基序在HSP70中高度保守。使用这些简并引物,通过PCR对长线形病毒属的几个确定成员和可能成员的基因组进行筛选,以检测HSP70基因的存在。BYV、柑橘衰退病毒(CTV)、甜菜黄矮病毒(BYSV)和香石竹坏死斑点病毒模板产生了1 kb的扩增产物,测序结果表明这些产物代表各自HSP70基因的片段。使用另一个针对假定病毒聚合酶基序IV的简并引物进行进一步筛选。该简并引物和与各病毒HSP70基因5'区域互补的特异性引物用于通过PCR估计BYV(约1.1 kb)、CTV和BYSV(约2.0 kb)聚合酶基序IV与HSP70基因起始点之间的距离。CTV(3026个核苷酸)和BYSV(2837个核苷酸)的扩增基因组区域被克隆并测序。发现CTV和BYSV在聚合酶和小疏水蛋白基因之间编码一个额外的30K(BYSV)或

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