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肺炎链球菌的青霉素结合蛋白2x。在大肠杆菌中的表达及可溶性酶活性衍生物的纯化。

Penicillin-binding protein 2x of Streptococcus pneumoniae. Expression in Escherichia coli and purification of a soluble enzymatically active derivative.

作者信息

Laible G, Keck W, Lurz R, Mottl H, Frère J M, Jamin M, Hakenbeck R

机构信息

Max-Planck Institut für molekulare Genetik, Berlin, Federal Republic of Germany.

出版信息

Eur J Biochem. 1992 Aug 1;207(3):943-9. doi: 10.1111/j.1432-1033.1992.tb17128.x.

Abstract

A 2.5-kb DNA fragment including the structural gene coding for the penicillin-binding protein 2x (PBP 2x) of Streptococcus pneumoniae has been cloned into the vector pJDC9 and expressed in Escherichia coli. Mapping of RNA polymerase binding sites by electron microscopy indicated that the pbpX promoter is well recognized by the E. coli enzyme. However, high-level expression occurred mainly under the control of the lac promoter upstream of the pJDC9 multiple cloning site. After induction with isopropyl beta-d-thiogalactopyranoside, PBP 2x was expressed as one of the major cellular proteins. PBP 2x produced in E. coli corresponded to the pneumococcal PBP 2x in terms of electrophoretic mobility, fractionation with the cytoplasmic membrane, and penicillin-binding capacity. Deletion of 30 hydrophobic N-terminal amino acid residues at positions 19-48 resulted in high-level expression of a cytoplasmic, soluble PBP 2x derivative (PBP 2x*) which still retained full beta-lactam-binding activity. A two-step procedure involving dye affinity chromatography was established for obtaining large amounts of highly purified enzymatically active PBP 2x*.

摘要

一个包含肺炎链球菌青霉素结合蛋白2x(PBP 2x)编码结构基因的2.5kb DNA片段已被克隆到载体pJDC9中,并在大肠杆菌中表达。通过电子显微镜对RNA聚合酶结合位点进行定位表明,pbpX启动子能被大肠杆菌酶很好地识别。然而,高水平表达主要发生在pJDC9多克隆位点上游的lac启动子控制下。用异丙基β-D-硫代半乳糖苷诱导后,PBP 2x作为主要细胞蛋白之一被表达。在大肠杆菌中产生的PBP 2x在电泳迁移率、与细胞质膜的分级分离以及青霉素结合能力方面与肺炎球菌PBP 2x相对应。删除第19 - 48位的30个疏水N端氨基酸残基导致细胞质可溶性PBP 2x衍生物(PBP 2x*)的高水平表达,该衍生物仍保留完全的β-内酰胺结合活性。建立了一种涉及染料亲和层析的两步法,用于获得大量高度纯化的具有酶活性的PBP 2x*。

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