THE MUTATION LYS234HIS YIELDS A CLASS-A BETA-LACTAMASE WITH A NOVEL PH-DEPENDENCE

被引:30
作者
BRANNIGAN, J
MATAGNE, A
JACOB, F
DAMBLON, C
JORIS, B
KLEIN, D
SPRATT, BG
FRERE, JM
机构
[1] STATE UNIV LIEGE, INST CHIM, CTR INGN PROT, B6, B-4000 Sart Tilman Par Liege, BELGIUM
[2] UNIV SUSSEX, SCH BIOL SCI, BRIGHTON BN1 9QG, E SUSSEX, ENGLAND
[3] STATE UNIV LIEGE, INST CHIM, ENZYMOL LAB, B-4000 Sart Tilman Par Liege, BELGIUM
来源
BIOCHEMICAL JOURNAL | 1991年 / 278卷
关键词
D O I
10.1042/bj2780673
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
The lysine-234 residue is highly conserved in beta-lactamases and in nearly all active-site-serine penicillin-recognizing enzymes. Its replacement by a histidine residue in the Streptomyces albus G class A beta-lactamase yielded an enzyme the pH-dependence of which was characterized by the appearance of a novel pK, which could be attributed to the newly introduced residue. At low pH, the k(cat.) value for benzylpenicillin was as high as 50 % of that of the wild-type enzyme, demonstrating that an efficient active site was maintained. Both k(cat.) and k(cat.)/K(m) dramatically decreased above pH 6 but the decrease in k(cat.)/K(m) could not be attributed to larger K(m) values. Thus a positive charge on the side chain of residue 234 appears to be more essential for transition-state stabilization than for initial recognition of the substrate ground state.
引用
收藏
页码:673 / 678
页数:6
相关论文
共 19 条
[1]   CHROMOGENIC DEPSIPEPTIDE SUBSTRATES FOR BETA-LACTAMASES AND PENICILLIN-SENSITIVE DD-PEPTIDASES [J].
ADAM, M ;
DAMBLON, C ;
PLAITIN, B ;
CHRISTIAENS, L ;
FRERE, JM .
BIOCHEMICAL JOURNAL, 1990, 270 (02) :525-529
[2]   A STANDARD NUMBERING SCHEME FOR THE CLASS-A BETA-LACTAMASES [J].
AMBLER, RP ;
COULSON, AFW ;
FRERE, JM ;
GHUYSEN, JM ;
JORIS, B ;
FORSMAN, M ;
LEVESQUE, RC ;
TIRABY, G ;
WALEY, SG .
BIOCHEMICAL JOURNAL, 1991, 276 :269-270
[3]   CLONING AND AMPLIFIED EXPRESSION IN STREPTOMYCES-LIVIDANS OF A GENE ENCODING EXTRACELLULAR BETA-LACTAMASE FROM STREPTOMYCES-ALBUS-G [J].
DEHOTTAY, P ;
DUSART, J ;
DUEZ, C ;
LENZINI, MV ;
MARTIAL, JA ;
FRERE, JM ;
GHUYSEN, JM ;
KIESER, T .
GENE, 1986, 42 (01) :31-36
[4]   AUTOMATED-ANALYSIS OF ENZYME INACTIVATION PHENOMENA - APPLICATION TO BETA-LACTAMASES AND DD-PEPTIDASES [J].
DEMEESTER, F ;
JORIS, B ;
RECKINGER, G ;
BELLEFROIDBOURGUIGNON, C ;
FRERE, JM ;
WALEY, SG .
BIOCHEMICAL PHARMACOLOGY, 1987, 36 (14) :2393-2403
[5]   THE ROLE OF LYSINE-234 IN BETA-LACTAMASE CATALYSIS PROBED BY SITE-DIRECTED MUTAGENESIS [J].
ELLERBY, LM ;
ESCOBAR, WA ;
FINK, AL ;
MITCHINSON, C ;
WELLS, JA .
BIOCHEMISTRY, 1990, 29 (24) :5797-5806
[6]   ENZYME-PRODUCTION BY GENETICALLY ENGINEERED STREPTOMYCES STRAINS - INFLUENCE OF CULTURE CONDITIONS [J].
ERPICUM, T ;
GRANIER, B ;
DELCOUR, M ;
LENZINI, VM ;
NGUYENDISTECHE, M ;
DUSART, J ;
FRERE, JM .
BIOTECHNOLOGY AND BIOENGINEERING, 1990, 35 (07) :719-726
[7]   COLONY HYBRIDIZATION - METHOD FOR ISOLATION OF CLONED DNAS THAT CONTAIN A SPECIFIC GENE [J].
GRUNSTEIN, M ;
HOGNESS, DS .
PROCEEDINGS OF THE NATIONAL ACADEMY OF SCIENCES OF THE UNITED STATES OF AMERICA, 1975, 72 (10) :3961-3965
[8]   BACTERIAL-RESISTANCE TO BETA-LACTAM ANTIBIOTICS - CRYSTAL-STRUCTURE OF BETA-LACTAMASE FROM STAPHYLOCOCCUS-AURENS PC1 AT 2.5-A RESOLUTION [J].
HERZBERG, O ;
MOULT, J .
SCIENCE, 1987, 236 (4802) :694-701
[9]   ENGINEERING A NOVEL BETA-LACTAMASE BY A SINGLE POINT MUTATION [J].
JACOB, F ;
JORIS, B ;
DIDEBERG, O ;
DUSART, J ;
GHUYSEN, JM ;
FRERE, JM .
PROTEIN ENGINEERING, 1990, 4 (01) :79-86
[10]   ROLE OF THE CONSERVED AMINO-ACIDS OF THE SDN LOOP (SER130, ASP131 AND ASN132) IN A CLASS-A BETA-LACTAMASE STUDIED BY SITE-DIRECTED MUTAGENESIS [J].
JACOB, F ;
JORIS, B ;
LEPAGE, S ;
DUSART, J ;
FRERE, JM .
BIOCHEMICAL JOURNAL, 1990, 271 (02) :399-406
12