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一种噬菌体装配蛋白的膜结构域。跨膜融合蛋白的跨膜定向蛋白水解。

The membrane domain of a bacteriophage assembly protein. Transmembrane-directed proteolysis of a membrane-spanning fusion protein.

作者信息

Guy-Caffey J K, Webster R E

机构信息

Department of Biochemistry, Duke University Medical Center, Durham, North Carolina 27710.

出版信息

J Biol Chem. 1993 Mar 15;268(8):5488-95.

PMID:8449911
Abstract

A tripartite fusion construct encoding the amino-terminal half of EcoRI endonuclease followed by amino acids 217-299 of the filamentous bacteriophage gene I protein (pI) attached to the enzymatic portion of alkaline phosphatase results in the production of two proteins. The larger protein, pIf, is the complete tripartite fusion protein while the smaller protein, pIf*, results from internal initiation of translation at pI methionine 241. Both pIf and pIf* span the Escherichia coli inner membrane via a 20-amino-acid hydrophobic stretch of pI with their amino termini in the cytoplasm and their carboxyl-terminal alkaline phosphatase domains in the periplasm. The alkaline phosphatase moiety of approximately 70% of pIf is released into the periplasm by in vivo proteolysis, but only about 10% of pIf* is cleaved. Neither DegP, OmpT, nor protease III are responsible for the cleavage in vivo, and leader peptidase is unable to cleave the fusion protein in vitro. Deletion and substitution analyses demonstrate that the degree of periplasmic cleavage depends on the sequence of the cytoplasmic domain of the fusion proteins. Possible mechanisms for this transmembrane-directed cleavage event are compared to proposed models for signal transduction.

摘要

一种三方融合构建体,编码EcoRI核酸内切酶的氨基末端一半,随后是丝状噬菌体基因I蛋白(pI)的氨基酸217 - 299,并连接到碱性磷酸酶的酶促部分,会产生两种蛋白质。较大的蛋白质pIf是完整的三方融合蛋白,而较小的蛋白质pIf则是由pI甲硫氨酸241处的内部翻译起始产生的。pIf和pIf都通过pI的20个氨基酸的疏水延伸跨越大肠杆菌内膜,它们的氨基末端在细胞质中,羧基末端的碱性磷酸酶结构域在周质中。大约70%的pIf的碱性磷酸酶部分通过体内蛋白水解释放到周质中,但只有约10%的pIf*被切割。DegP、OmpT和蛋白酶III都不负责体内的切割,并且前导肽酶在体外无法切割融合蛋白。缺失和取代分析表明,周质切割的程度取决于融合蛋白细胞质结构域的序列。将这种跨膜定向切割事件的可能机制与信号转导的提出模型进行了比较。

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