ROLE OF LYSINE-67 IN THE ACTIVE-SITE OF CLASS-C BETA-LACTAMASE FROM CITROBACTER-FREUNDII GN346

被引:59
作者
TSUKAMOTO, K [1 ]
TACHIBANA, K [1 ]
YAMAZAKI, N [1 ]
ISHII, Y [1 ]
UJIIE, K [1 ]
NISHIDA, N [1 ]
SAWAI, T [1 ]
机构
[1] CHIBA UNIV, FAC PHARMACEUT SCI, DIV MICROBIAL CHEM, 1-33 YAYOI CHO, CHIBA 260, JAPAN
来源
EUROPEAN JOURNAL OF BIOCHEMISTRY | 1990年 / 188卷 / 01期
关键词
D O I
10.1111/j.1432-1033.1990.tb15365.x
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
Citrobacter freundii GN346 produces a class C β‐lactamase exhibiting the substrate profile of a typical cephalosporinase. The structural and promoter regions of the cephalosporinase gene, comprising 1408 nucleotides, were completely sequenced. The amino acid sequence of the mature enzyme, comprising 361 amino acids, and its molecular mass, 39878 Da, were determined. The active site was confirmed to be Ser‐64. The amino acid sequence of the enzyme differs from that of the cephalosporinase of C. freundii OS60 by nine residues. The nucleotide sequence of the promoter region suggests a possible attenuator structure. Lys‐67, one of the most conserved residues found in class A and C β‐lactamases and penicillin‐binding proteins, was converted into arginine, threonine or glutamic acid through site‐directed mutagenesis. The Glu‐67 enzyme had lost the catalytic activity and the Thr‐67 enzyme only showed a trace of activity. The Arg‐67 enzyme, which retained a significant amount of the activity, was purified. The Km values of the Arg‐67 enzyme for cephalothin, cephaloridine and benzylpenicillin are 13–19 times those of the wild‐type enzyme; the kcat values for the three substrates are 37%, 3%, and 36% those of the wild‐type enzyme, respectively. Copyright © 1990, Wiley Blackwell. All rights reserved
引用
收藏
页码:15 / 22
页数:8
相关论文
共 45 条
  • [1] NUCLEOTIDE-SEQUENCE ANALYSIS OF THE CHLORAMPHENICOL RESISTANCE TRANSPOSON TN9
    ALTON, NK
    VAPNEK, D
    [J]. NATURE, 1979, 282 (5741) : 864 - 869
  • [2] THE STRUCTURE OF BETA-LACTAMASES
    AMBLER, RP
    [J]. PHILOSOPHICAL TRANSACTIONS OF THE ROYAL SOCIETY B-BIOLOGICAL SCIENCES, 1980, 289 (1036) : 321 - 331
  • [3] BUSH K, 1987, DEV IND MICROBIOL, V27, P153
  • [4] CARTER P, 1985, OLIGONUCLEOTIDE SITE
  • [5] FLUOROGRAPHIC DETECTION OF RADIOACTIVITY IN POLYACRYLAMIDE GELS WITH THE WATER-SOLUBLE FLUOR, SODIUM-SALICYLATE
    CHAMBERLAIN, JP
    [J]. ANALYTICAL BIOCHEMISTRY, 1979, 98 (01) : 132 - 135
  • [6] OLIGONUCLEOTIDE-DIRECTED MUTAGENESIS AS A GENERAL AND POWERFUL METHOD FOR STUDIES OF PROTEIN FUNCTION
    DALBADIEMCFARLAND, G
    COHEN, LW
    RIGGS, AD
    MORIN, C
    ITAKURA, K
    RICHARDS, JH
    [J]. PROCEEDINGS OF THE NATIONAL ACADEMY OF SCIENCES OF THE UNITED STATES OF AMERICA-BIOLOGICAL SCIENCES, 1982, 79 (21): : 6409 - 6413
  • [7] HERZBERG O, 1987, SCIENCE, V236, P697
  • [8] THE ACTIVE-SITE OF THE P99 BETA-LACTAMASE FROM ENTEROBACTER-CLOACAE
    JORIS, B
    DUSART, J
    FRERE, JM
    VANBEEUMEN, J
    EMANUEL, EL
    PETURSSON, S
    GAGNON, J
    WALEY, SG
    [J]. BIOCHEMICAL JOURNAL, 1984, 223 (01) : 271 - 274
  • [9] THE ACTIVE-SITE-SERINE PENICILLIN-RECOGNIZING ENZYMES AS MEMBERS OF THE STREPTOMYCES R61 DD-PEPTIDASE FAMILY
    JORIS, B
    GHUYSEN, JM
    DIVE, G
    RENARD, A
    DIDEBERG, O
    CHARLIER, P
    FRERE, JM
    KELLY, JA
    BOYINGTON, JC
    MOEWS, PC
    KNOX, JR
    [J]. BIOCHEMICAL JOURNAL, 1988, 250 (02) : 313 - 324
  • [10] PROPERTIES OF A CLASS-C BETA-LACTAMASE FROM SERRATIA-MARCESCENS
    JORIS, B
    DEMEESTER, F
    GALLENI, M
    MASSON, S
    DUSART, J
    FRERE, JM
    VANBEEUMEN, J
    BUSH, K
    SYKES, R
    [J]. BIOCHEMICAL JOURNAL, 1986, 239 (03) : 581 - 586
12345