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人血管生成素基因在大肠杆菌中的表达;重组人丝氨酸(-1)血管生成素的分离与鉴定

Expression of the hAng gene in Escherichia coli; isolation and characterization of human recombinant Ser-(-1) angiogenin.

作者信息

Lapidus A L, Mochul'skii A V, Podkovyrov S M, Lebedeva M I, Antipin A A, Izotova L S, Zagnit'ko O P, Komolova G S, Klesov A A, Veiko V P

机构信息

All-Union Research Institute of Genetics, Ministry of Medical Industry of the USSR, Moscow.

出版信息

Biomed Sci. 1990;1(6):597-604.

PMID:2132944
Abstract

Recombinant human angiogenin has been synthesized in Escherichia coli with the aid of a human angiogenin gene (hAng) cloned by Neznanov et al (1990) from a human complementary DNA (cDNA) library. The gene has been expressed by use of a new type of expression vector called a 'TGATG vector' (plasmid pPR-TGATG-1; Mashko et al 1990a). The highest level of accumulation of the recombinant angiogenin (6%-8% of the total cell protein) was observed in E. coli strain BL21 carrying a temperature-amplifiable version of the plasmid. The synthesized polypeptide carries an additional serine residue at its N terminus in comparison with natural angiogenin. Furthermore, the initiator methionine residue of the recombinant protein is removed with high efficiency by E. coli terminal aminopeptidase. Simple procedures for purification of the recombinant angiogenin from the insoluble fraction of cell protein, and for refolding the protein allowed the isolation of almost 5 mg recombinant angiogenin g-1 wet bacterial biomass. The recombinant Ser-(-1) angiogenin displayed the same biological properties (specific RNAase activity and the ability to induce blood vessel growth on the sclera of experimental animals) as its natural counterpart isolated from human blood.

摘要

重组人血管生成素是借助涅兹纳诺夫等人(1990年)从人互补DNA(cDNA)文库中克隆的人血管生成素基因(hAng)在大肠杆菌中合成的。该基因已通过使用一种新型表达载体——“TGATG载体”(质粒pPR-TGATG-1;马什科等人,1990年a)进行表达。在携带该质粒温度可扩增版本的大肠杆菌BL21菌株中,观察到重组血管生成素的积累水平最高(占细胞总蛋白的6%-8%)。与天然血管生成素相比,合成的多肽在其N端带有一个额外的丝氨酸残基。此外,重组蛋白的起始甲硫氨酸残基被大肠杆菌末端氨肽酶高效去除。从细胞蛋白不溶性部分纯化重组血管生成素以及使蛋白复性的简单程序,使得从每克湿细菌生物质中能够分离出近5毫克的重组血管生成素。重组的Ser-(-1)血管生成素与其从人血液中分离出的天然对应物具有相同的生物学特性(特异性核糖核酸酶活性以及在实验动物巩膜上诱导血管生长的能力)。

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