PURIFICATION, CLONING, AND PRIMARY STRUCTURE OF AN ENANTIOMER-SELECTIVE AMIDASE FROM BREVIBACTERIUM SP STRAIN-R312 - STRUCTURAL EVIDENCE FOR GENETIC COUPLING WITH NITRILE HYDRATASE

被引：146

作者：

MAYAUX, JF ^{[1
]}

CERBELAUD, E ^{[1
]}

SOUBRIER, F ^{[1
]}

FAUCHER, D ^{[1
]}

PETRE, D ^{[1
]}

机构：

[1] RHONE POULENC RECH, CATALYSE ENZYMAT LAB, F-69192 ST FONS, FRANCE

来源：

JOURNAL OF BACTERIOLOGY | 1990年 / 172卷 / 12期

关键词：

D O I：

10.1128/jb.172.12.6764-6773.1990

中图分类号：

Q93 [微生物学];

学科分类号：

071005 ; 100705 ;

摘要：

An enantiomer-selective amidase active on several 2-aryl and 2-aryloxy propionamides was identified and purified from Brevibacterium sp. strain R312. Oligonucleotide probes were designed from limited peptide sequence information and were used to clone the corresponding gene, named amdA. Highly significant homologies were found at the amino acid level between the deduced sequence of the enantiomer-selective amidase and the sequences of known amidases such as indoleacetamide hydrolases from Pseudomonas syringae and Agrobacterium tumefaciens and acetamidase from Aspergillus nidulans. Moreover, amdA is found in the same orientation and only 73 bp upstream from the gene coding for nitrile hydratase, strongly suggesting that both genes are part of the same operon. Our results also showed that Rhodococcus sp. strain N-774 and Brevibacterium sp. strain R312 are probably identical, or at least very similar, microorganisms. The characterized amidase is an apparent homodimer of M(r) 2 x 54,671 which exhibited under our conditions a specific activity of about 13 to 17 μmol of 2-(4-hydroxyphenoxy)propionic R acid formed per min per mg of enzyme from the racemic amide. Large amounts of an active recombinant enzyme could be produced in Escherichia coli at 30°C under the control of an E. coli promoter and ribosome-binding site.

引用

页码：6764 / 6773

页数：10

共 31 条

[1]

ARNAUD A, 1976, CR ACAD SCI D NAT, V283, P571

[2] A NEW ENZYME NITRILE HYDRATASE WHICH DEGRADES ACETONITRILE IN COMBINATION WITH AMIDASE [J].

ASANO, Y ;

TANI, Y ;

YAMADA, H .

AGRICULTURAL AND BIOLOGICAL CHEMISTRY, 1980, 44 (09) :2251-2252

[3] CONTINUOUS IMMOBILIZED CELL REACTOR FOR AMIDE HYDROLYSIS [J].

BERNET, N ;

THIERY, A ;

MAESTRACCI, M ;

ARNAUD, A ;

RIOS, GM ;

GALZY, P .

JOURNAL OF INDUSTRIAL MICROBIOLOGY, 1987, 2 (03) :129-136

[4] THE RELATIONSHIP BETWEEN BASE COMPOSITION AND CODON USAGE IN BACTERIAL GENES AND ITS USE FOR THE SIMPLE AND RELIABLE IDENTIFICATION OF PROTEIN-CODING SEQUENCES [J].

BIBB, MJ ;

FINDLAY, PR ;

JOHNSON, MW .

GENE, 1984, 30 (1-3) :157-166

[5] CHEMICAL ASYMMETRIC-SYNTHESIS [J].

BROWN, JM ;

DAVIES, SG .

NATURE, 1989, 342 (6250) :631-636

[6]

BUI K, 1984, J GEN MICROBIOL, V130, P89

[7] THE NUCLEOTIDE-SEQUENCE OF THE AMDS GENE OF ASPERGILLUS-NIDULANS AND THE MOLECULAR CHARACTERIZATION OF 5' MUTATIONS [J].

CORRICK, CM ;

TWOMEY, AP ;

HYNES, MJ .

GENE, 1987, 53 (01) :63-71

[8] CHEMICAL SYNTHESIS OF A GENE CODING FOR HUMAN ANGIOGENIN, ITS EXPRESSION IN ESCHERICHIA-COLI AND CONVERSION OF THE PRODUCT INTO ITS ACTIVE FORM [J].

DENEFLE, P ;

KOVARIK, S ;

GUITTON, JD ;

CARTWRIGHT, T ;

MAYAUX, JF .

GENE, 1987, 56 (01) :61-70

[9] MOLECULAR-CLONING AND NUCLEOTIDE-SEQUENCE OF THE CORYNEBACTERIUM-GLUTAMICUM-PHEA GENE [J].

FOLLETTIE, MT ;

SINSKEY, AJ .

JOURNAL OF BACTERIOLOGY, 1986, 167 (02) :695-702

[10] GENERATION OF DNA PROBES FOR PEPTIDES WITH HIGHLY DEGENERATE CODONS USING MIXED PRIMER PCR [J].

GIRGIS, SI ;

ALEVIZAKI, M ;

DENNY, P ;

FERRIER, GJM ;

LEGON, S .

NUCLEIC ACIDS RESEARCH, 1988, 16 (21) :10371-10371

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