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病毒K28杀伤毒素基因cDNA拷贝在酵母中的克隆与表达。

Cloning and expression of a cDNA copy of the viral K28 killer toxin gene in yeast.

作者信息

Schmitt M J

机构信息

Institut für Mikrobiologie und Weinforschung, Johannes Gutenberg-Universität Mainz, Germany.

出版信息

Mol Gen Genet. 1995 Jan 20;246(2):236-46. doi: 10.1007/BF00294687.

DOI:10.1007/BF00294687
PMID:7862095
Abstract

The killer toxin K28, secreted by certain killer strains of the yeast Saccharomyces cerevisiae is genetically encoded by a 1.9 kb double-stranded RNA, M-dsRNA (M28), that is present within the cell as a cytoplasmically inherited virus-like particle (VLP). For stable maintenance and replication, M28-VLPs depend on a second dsRNA virus (LA), which has been shown to encode the major capsid protein (cap) and a capsid-polymerase fusion protein (cap-pol) that provides the toxin-coding M-satellites with their transcription and replicase functions. K28 toxin-coding M28-VLPs were isolated, purified and used in vitro for the synthesis of the single-stranded M28 transcript, which was shown to be of plus strand polarity and to bind to oligo(dT)-cellulose, indicating that M28(+)ssRNA contains an internal A-rich tract. Strand separation of the 1.9 kb M28-dsRNA and direct RNA sequencing of its 3' ends was performed in order to obtain specific DNA oligonucleotides that could be used as primers for cDNA synthesis. The nucleotide sequence of the toxin-coding M28-cDNA identified a single open reading frame (ORF) coding for a polypeptide of 345 amino acids, which contained two potential Kex2p/Kex1p processing sites and three potential sites for protein N-glycosylation. The toxin-coding cDNA was cloned and expressed in sensitive non-killer strains under the control of the yeast PGK promoter. Upon transformation, this construct conferred the complete K28 phenotype, demonstrating that both toxin and immunity determinants are contained within the cloned cDNA. In vitro translational analysis of the M28(+)ssRNA in vitro transcript identified the primary gene product of M28 as a K28 preprotoxin of 38 kDa (M-p38).

摘要

酿酒酵母某些杀伤菌株分泌的杀伤毒素K28由1.9 kb的双链RNA M-dsRNA(M28)进行基因编码,M-dsRNA在细胞内以细胞质遗传的病毒样颗粒(VLP)形式存在。为实现稳定维持和复制,M28-VLPs依赖于第二种双链RNA病毒(LA),该病毒已被证明可编码主要衣壳蛋白(cap)和衣壳-聚合酶融合蛋白(cap-pol),后者为毒素编码的M-卫星提供转录和复制酶功能。分离、纯化了编码K28毒素的M28-VLPs,并在体外用于合成单链M28转录本,结果表明该转录本具有正链极性且能与寡聚(dT)-纤维素结合,这表明M28(+)ssRNA含有一个内部富含A的区域。对1.9 kb的M28-dsRNA进行链分离并对其3'末端进行直接RNA测序,以获得可作为cDNA合成引物的特异性DNA寡核苷酸。毒素编码的M28-cDNA的核苷酸序列确定了一个单一的开放阅读框(ORF),其编码一个由345个氨基酸组成的多肽,该多肽包含两个潜在的Kex2p/Kex1p加工位点和三个潜在的蛋白质N-糖基化位点。毒素编码的cDNA在酵母PGK启动子的控制下克隆并在敏感的非杀伤菌株中表达。转化后,该构建体赋予了完整的K28表型,表明毒素和免疫决定因素均包含在克隆的cDNA中。对M28(+)ssRNA体外转录本的体外翻译分析确定M28的主要基因产物为38 kDa的K28前原毒素(M-p38)。

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