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首页> 外文期刊>Journal of Virology >Encephalomyocarditis virus 3C protease: efficient cell-free expression from clones which link viral 5' noncoding sequences to the P3 region.
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Encephalomyocarditis virus 3C protease: efficient cell-free expression from clones which link viral 5' noncoding sequences to the P3 region.

机译:脑肌瘤炎病毒3C蛋白酶:从将病毒5'非编码序列链接到P3区域的克隆的无高的细胞表达。

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All picornaviral peptides are derived by progressive posttranslational cleavage of a giant precursor polyprotein. Translation of encephalomyocarditis virus (EMC) RNA in rabbit reticulocyte extracts produces active viral peptides, including protease 3C, which is responsible for many cleavage reactions within the processing cascade. DNA plasmids containing 5' noncoding sequences of EMC linked to other portions of the viral genome were constructed and transcribed into RNA. Like virion RNA, the clone-derived transcripts directed efficient protein translation in vitro. The 5'-linked constructions may represent examples of a general method for cell-free expression of any cloned gene segment. One construction produced a self-cleaving P3 region precursor, which contained active 3C protease. A genetically engineered insertion within the 3C sequences eliminated endogenous self-cleavage activity without altering the ability of the P3 peptide to serve as substrate in bimolecular reactions with added 3C. Another plasmid encoding the L-VP0 portion of the capsid region was used to demonstrate that scission between the leader peptide (L) and capsid protein VP0 can be catalyzed by 3C. The enzyme responsible for this step was previously unidentified. A rapid purification scheme for isolation of 3C from EMC-infected HeLa cells is also presented.
机译:所有皮诺拉夫肽肽都是通过对巨型前体多蛋白的逐步发生裂解来源的。腹腔内的翻译兔网状细胞提取物中的脑膜炎炎病毒(EMC)RNA产生活性病毒肽,包括蛋白酶3c,其负责加工级联内的许多切割反应。含有与病毒基因组的其他部分连接的EMC的5'非编码序列的DNA质粒被构建并转录成RNA。像病毒肝RNA,克隆衍生的转录物在体外有效蛋白翻译。 5'-连接的结构可以表示任何克隆基因链段的无细胞表达的一般方法的实例。一种结构产生了一种自切割的P3区前体,其含有活性3C蛋白酶。在3C序列内的遗传工程插入消除了内源性自切割活性,而不改变P3肽用作添加3C的分散反应中的基材的能力。编码衣壳区域的L-VP0部分的另一个质粒用于证明,前导肽(L)和衣壳蛋白VP0之间的裂殖可以通过3C催化。原始的酶原因是未识别的。还提出了一种从EMC感染的HeLa细胞中分离3C的快速纯化方案。

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