CLONING AND EXPRESSION IN ESCHERICHIA-COLI OF THE STRUCTURAL GENE CODING FOR THE MONOMERIC PROTEIN OF THE S-LAYER OF THERMUS-THERMOPHILUS HB8

被引：22

作者：

FARALDO, MLM ^{[1
]}

DEPEDRO, MA ^{[1
]}

BERENGUER, J ^{[1
]}

机构：

[1] UNIV AUTONOMA MADRID,FAC CIENCIAS,CSIC,CTR BIOL MOLEC,E-28049 MADRID,SPAIN

来源：

JOURNAL OF BACTERIOLOGY | 1991年 / 173卷 / 17期

关键词：

D O I：

10.1128/jb.173.17.5346-5351.1991

中图分类号：

Q93 [微生物学];

学科分类号：

071005 ; 100705 ;

摘要：

The gene coding for the 100 kDa monomeric protein (P100) of the S layer of Thermus thermophilus HB8 has been cloned in the Escherichia coli plasmid vector pUC9. Recombinant plasmids were selected by colony screening with anti-P100 rabbit antiserum. The gene, named slpA (for surface layer protein A), was identified in a bacterial clone harboring a hybrid plasmid, pMF4, with a 5.8-kbp insert. This plasmid consistently expressed a protein specifically recognized by anti-P100) antiserum. Expression was apparently independent of P(tac), indicating that the promoter for P100 is functional in E. coli. Most E. coli strains transformed with plasmids containing the 5.8-kbp insert cloned in pMF4 expressed two proteins with apparent masses of 52 and 50 kDa, which were strongly recognized by anti-P100 antiserum in Western immunoblots. The 52-kDa fragment could be overproduced, and the sequence of the N-terminal undecapeptide, determined by microsequencing, indicated that it could correspond to the N-terminal domain of P100. Expression of slpA in lon mutants of E. coli led to accumulation of a protein indistinguishable from native P100, indicating that the complete gene was cloned and that the product of lon, protease La, was involved in proteolytic degradation of P100 synthesized in E. coli.

引用

页码：5346 / 5351

页数：6

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