SITE-DIRECTED MUTAGENESIS OF BETA-LACTAMASE-I - SINGLE AND DOUBLE MUTANTS OF GLU-166 AND LYS-73

被引:131
作者
GIBSON, RM
CHRISTENSEN, H
WALEY, SG
机构
[1] UNIV OXFORD, SIR WILLIAM DUNN SCH PATHOL, OXFORD OX1 3RE, ENGLAND
[2] OXFORD CTR MOLEC SCI, OXFORD 0X1 3QY, ENGLAND
来源
BIOCHEMICAL JOURNAL | 1990年 / 272卷 / 03期
关键词
D O I
10.1042/bj2720613
中图分类号
Q5 [生物化学]; Q7 [分子生物学];
学科分类号
071010 ; 081704 ;
摘要
Two single mutants and the corresponding double mutant of beta-lactamase I from Bacillus cereus 569/H were constructed and their kinetics investigated. The mutants have Lys-73 replaced by arginine (K73R), or Glu-166 replaced by aspartic acid (E166D), or both (K73R + E166D). All four rate constants in the acyl-enzyme mechanism were determined for the E166D mutant by the methods described by Christensen, Martin & Waley [(1990) Biochem. J. 266, 853-861]. Both the rate constants for acylation and deacylation for the hydrolysis of benzylpenicillin were decreased about 2000-fold in this mutant. In the K73R mutant, and in the double mutant, the rate constants for acylation were decreased about 100-fold and 10000-fold respectively. All three mutants also had lowered values for the rate constants for the formation and dissociation of the non-covalent enzyme-substrate complex. The specificities of the mutants did not differ greatly from those of wild-type beta-lactamase, but the hydrolysis of cephalosporin C by the K73R mutant gave 'burst' kinetics.
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页码:613 / 619
页数:7
相关论文
共 59 条
[11]  
CHRISTENSEN H, 1990, BIOCHEM J, V268, P808
[12]  
CHRISTENSEN H, 1990, BIOCHEM J, V266, P853
[13]   ACQUISITION OF SUBSTRATE-SPECIFIC PARAMETERS DURING CATALYTIC REACTION OF PENICILLINASE [J].
CITRI, N ;
SAMUNI, A ;
ZYK, N .
PROCEEDINGS OF THE NATIONAL ACADEMY OF SCIENCES OF THE UNITED STATES OF AMERICA, 1976, 73 (04) :1048-1052
[14]   AMINO-ACID SEQUENCE OF RABBIT MUSCLE TRIOSE PHOSPHATE ISOMERASE [J].
CORRAN, PH ;
WALEY, SG .
FEBS LETTERS, 1973, 30 (01) :97-99
[15]   BETA-LACTAMASES - MOLECULAR STUDIES [J].
COULSON, A .
BIOTECHNOLOGY & GENETIC ENGINEERING REVIEWS, 1985, 3 :219-253
[16]   BEHAVIOUR OF SOME DERIVATIVES OF 7-AMINOCEPHALOSPORANIC ACID AND 6-AMINOPENICILLANIC ACID AS SUBSTRATES, INHIBITORS AND INDUCERS OF PENICILLINASES [J].
CROMPTON, B ;
JAGO, M ;
ABRAHAM, EP ;
NEWTON, GGF ;
CRAWFORD, K .
BIOCHEMICAL JOURNAL, 1962, 83 (01) :52-&
[17]   FREE-ENERGY COMPONENT ANALYSIS - A STUDY OF THE GLUTAMIC ACID-165-] ASPARTIC ACID-165 MUTATION IN TRIOSEPHOSPHATE ISOMERASE [J].
DAGGETT, V ;
BROWN, F ;
KOLLMAN, P .
JOURNAL OF THE AMERICAN CHEMICAL SOCIETY, 1989, 111 (21) :8247-8256
[18]   OLIGONUCLEOTIDE-DIRECTED MUTAGENESIS AS A GENERAL AND POWERFUL METHOD FOR STUDIES OF PROTEIN FUNCTION [J].
DALBADIEMCFARLAND, G ;
COHEN, LW ;
RIGGS, AD ;
MORIN, C ;
ITAKURA, K ;
RICHARDS, JH .
PROCEEDINGS OF THE NATIONAL ACADEMY OF SCIENCES OF THE UNITED STATES OF AMERICA-BIOLOGICAL SCIENCES, 1982, 79 (21) :6409-6413
[19]   SEPARATION, PURIFICATION AND PROPERTIES OF BETA-LACTAMASE I AND BETA-LACTAMASE II FROM BACILLUS-CEREUS 569-H-9 [J].
DAVIES, RB ;
ABRAHAM, EP ;
MELLING, J .
BIOCHEMICAL JOURNAL, 1974, 143 (01) :115-127
[20]   ACTIVE-SITE LABELING OF TRIOSE PHOSPHATE ISOMERASE - REACTION OF BROMOHYDROXYACETONE PHOSPHATE WITH A UNIQUE GLUTAMIC-ACID RESIDUE AND MIGRATION OF LABEL TO TYROSINE [J].
DELAMARE, S ;
KNOWLES, JR ;
COULSON, AFW ;
PRIDDLE, JD ;
OFFORD, RE .
BIOCHEMICAL JOURNAL, 1972, 129 (02) :321-&
123456