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PURIFICATION, CHARACTERIZATION, AND FIBRINOGEN CLEAVAGE SITES OF 3 FIBRINOLYTIC ENZYMES FROM THE VENOM OF CROTALUS-BASILISCUS-BASILISCUS

被引:24
作者
RETZIOS, AD [1 ]
MARKLAND, FS [1 ]
机构
[1] UNIV SO CALIF, SCH MED, DEPT BIOCHEM, 1303 N MISSION RD, CRL 106, LOS ANGELES, CA 90033 USA
来源
BIOCHEMISTRY | 1992年 / 31卷 / 19期
关键词
D O I
10.1021/bi00134a003
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
Three distinct fibrinolytic enzymes have been purified from the venom of Crotalus basiliscus basiliscus (the Mexican west coast rattlesnake). The high-performance liquid chromatography-based purification comprised the following steps: (a) hydrophobic interaction chromatography; (b) hydroxylapatite chromatography; (c) anion-exchange chromatography. Following hydrophobic interaction chromatography two fibrinolytic activity peaks were detected, Cbfib1 and Cbfib2. Cbfib2 was rendered homogeneous following hydroxylapatite chromatography. Upon hydroxylapatite chromatography Cbfib1 was shown to consist of two components, Cbfib1.1 and Cbfib1.2. Both Cbfib1.1 and Cbfib1.2 were purified to homogeneity using anion-exchange chromatography. SDS-polyacrylamide gel electrophoresis revealed that Cbfib1.1 and Cbfib1.2 had similar molecular weights (approximately 23 500), whereas Cbfib2 displayed a molecular weight of approximately 22 500. The enzymes do not appear to be glycosylated. Tryptic digests of all three enzymes, analyzed by high-performance reverse-phase chromatography, suggest that Cbfib1.1 and Cbfib1.2 are closely related and different from Cbfib2. The latter displayed more similarity with Cbfib1.2 than with Cbfib1.1. Specific fibrinolytic activity for all three enzymes was very similar, but general proteolytic activity varied substantially with Cbfib2 showing a 12-fold higher specific proteolytic activity when compared to Cbfib1.1 and Cbfib1.2. None of these enzymes exhibited hemorrhagic activity when injected (up to 100-mu-g) subcutaneously into mice. Cbfib1.1 and Cbfib1.2 action against fibrinogen was directed equally against both the A-alpha- and B-beta-chains. Against fibrin the rate of degradation of the alpha-chain was considerably higher than that of the beta-chain. Cbfib2 showed mainly alpha-fibrin(ogen)ase activity with limited activity on the beta-chain. Several fibrinogen cleavage sites on the A-alpha-chain have been identified: Cbfib1.1 and Cbfib1.2 cleave at Lys413-Leu414, Ser505-Thr506, and Tyr560-Ser561. Cbfib2 cleaves mainly at Gly254-Ser255 and Pro516-Met517.
引用
收藏
页码:4547 / 4557
页数:11
相关论文
共 32 条
[1]   FIBRINOLYTIC ENZYME(S) IN WESTERN DIAMONDBACK RATTLESNAKE (CROTALUS-ATROX) VENOM [J].
BAJWA, SS ;
MARKLAND, FS ;
RUSSELL, FE .
TOXICON, 1980, 18 (03) :285-&
[2]   RAPID ANALYSIS OF AMINO-ACIDS USING PRE-COLUMN DERIVATIZATION [J].
BIDLINGMEYER, BA ;
COHEN, SA ;
TARVIN, TL .
JOURNAL OF CHROMATOGRAPHY, 1984, 336 (01) :93-104
[3]  
CHARNEY J, 1947, J BIOL CHEM, V171, P501
[4]   IMMUNOLOGICAL PROPERTIES OF THE FIBRINOLYTIC ENZYME (FIBROLASE) FROM SOUTHERN COPPERHEAD (AGKISTRODON-CONTORTRIX-CONTORTRIX) VENOM AND ITS PURIFICATION BY IMMUNOAFFINITY CHROMATOGRAPHY [J].
CHEN, HM ;
GUAN, AL ;
MARKLAND, FS .
TOXICON, 1991, 29 (06) :683-694
[5]   STRUCTURE OF THERMOLYSIN - ELECTRON-DENSITY MAP AT 2.3 A RESOLUTION [J].
COLMAN, PM ;
MATTHEWS, BW ;
JANSONIUS, JN .
JOURNAL OF MOLECULAR BIOLOGY, 1972, 70 (03) :701-+
[6]  
DIDISHEIM P, 1956, P SOC EXP BIOL MED, V93, P10
[7]   A HIGHLY SENSITIVE PERIODIC ACID SILVER STAIN FOR 1,2-DIOL GROUPS OF GLYCOPROTEINS AND POLYSACCHARIDES IN POLYACRYLAMIDE GELS [J].
DUBRAY, G ;
BEZARD, G .
ANALYTICAL BIOCHEMISTRY, 1982, 119 (02) :325-329
[8]   PURIFICATION AND CHARACTERIZATION OF A FIBRINOLYTIC ENZYME FROM VENOM OF THE SOUTHERN COPPERHEAD SNAKE (AGKISTRODON-CONTORTRIX-CONTORTRIX) [J].
GUAN, AL ;
RETZIOS, AD ;
HENDERSON, GN ;
MARKLAND, FS .
ARCHIVES OF BIOCHEMISTRY AND BIOPHYSICS, 1991, 289 (02) :197-207
[9]   COVALENT STRUCTURE OF FIBRINOGEN [J].
HENSCHEN, A ;
LOTTSPEICH, F ;
KEHL, M ;
SOUTHAN, C .
ANNALS OF THE NEW YORK ACADEMY OF SCIENCES, 1983, 408 (JUN) :28-43
[10]  
HOLLEMAN WH, 1976, J BIOL CHEM, V251, P1663
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