学术探索
学术期刊
新闻热点
数据分析
智能评审

COMPARISON OF CONFORMATIONAL-CHANGES OF PREGNANCY ZONE PROTEIN AND HUMAN ALPHA-2-MACROGLOBULIN, A STUDY USING HYDROPHOBIC AFFINITY PARTITIONING

被引:15
作者
JENSEN, PEH
HAGGLOF, EM
ARBELAEZ, LF
STIGBRAND, T
SHANBHAG, VP
机构
[1] UMEA UNIV,DEPT BIOCHEM,S-90187 UMEA,SWEDEN
[2] UMEA UNIV,DEPT MED BIOCHEM & BIOPHYS,S-90187 UMEA,SWEDEN
来源
BIOCHIMICA ET BIOPHYSICA ACTA | 1993年 / 1164卷 / 02期
关键词
CONFORMATIONAL CHANGE; HYDROPHOBIC AFFINITY PARTITIONING; PREGNANCY ZONE PROTEIN; ALPHA-2-MACROGLOBULIN; PROTEINASE INHIBITION; (HUMAN);
D O I
10.1016/0167-4838(93)90242-J
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
Conformational changes of human alpha2-macroglobulin (alpha2M) and pregnancy zone protein (PZP), reflected in changes in surface hydrophobicity, have been studied. The results show that the conformation of alpha2M is governed by the degree of 'trapping'. Thus, cleavage in the bait region and of the thiol ester by proteinase treatment causes a two-fold increase in surface hydrophobicity of alpha2M. However, the increase is still higher (three-fold) when the thiol esters in alpha2M alone are cleaved by methylamine. Cyanylation of the thiol groups exposed upon methylamine treatment yields a derivative with the same hydrophobicity as native alpha2M. Treatment of this derivative with chymotrypsin restores the hydrophobicity to that of methylamine-treated alpha2M. Since the C-terminal 18 kDa fragment of alpha2M exhibits no hydrophobicity, the change in hydrophobicity seems not to reside in the receptor binding site. In contrast to alpha2M, modification of both native and methylamine-treated PZP with chymotrypsin gives a reduction (about 40%) in hydrophobicity. The change in hydrophobicity is insignificant on treatment with methylamine alone. Furthermore, hydrophobic interactions appear not to contribute to tetramerization of PZP. The present study indicates major differences in the conformational states of alpha2M and PZP as reflected in the hydrophobic surfaces exhibited.
引用
收藏
页码:152 / 158
页数:7
相关论文
共 33 条
[1]   INTERACTION OF ALPHA2-MACROGLOBULIN WITH PROTEINASES - CHARACTERISTICS AND SPECIFICITY OF REACTION, AND A HYPOTHESIS CONCERNING ITS MOLECULAR MECHANISM [J].
BARRETT, AJ ;
STARKEY, PM .
BIOCHEMICAL JOURNAL, 1973, 133 (04) :709-&
[2]   DIFFERENCES IN HYDROPHOBIC PROPERTIES FOR HUMAN ALPHA-2-MACROGLOBULIN AND PREGNANCY ZONE PROTEIN AS STUDIED BY AFFINITY PHASE PARTITIONING [J].
BIRKENMEIER, G ;
CARLSSONBOSTEDT, L ;
SHANBHAG, V ;
KRIEGEL, T ;
KOPPERSCHLAGER, G ;
SOTTRUPJENSEN, L ;
STIGBRAND, T .
EUROPEAN JOURNAL OF BIOCHEMISTRY, 1989, 183 (02) :239-243
[3]  
BJORK I, 1985, BIOCHEM J, V231, P451
[4]  
BJORK I, 1985, BIOCHEMISTRY-US, V24, P2653
[5]   MECHANISM OF ALPHA-2-MACROGLOBULIN PROTEINASE INTERACTIONS - STUDIES WITH TRYPSIN AND PLASMIN [J].
CHRISTENSEN, U ;
SOTTRUPJENSEN, L .
BIOCHEMISTRY, 1984, 23 (26) :6619-6626
[6]   PREGNANCY ZONE PROTEIN, A PROTEINASE-BINDING MACROGLOBULIN - INTERACTIONS WITH PROTEINASES AND METHYLAMINE [J].
CHRISTENSEN, U ;
SIMONSEN, M ;
HARRIT, N ;
SOTTRUPJENSEN, L .
BIOCHEMISTRY, 1989, 28 (24) :9324-9331
[7]   PREGNANCY ZONE PROTEIN, A PROTEINASE BINDING ALPHA-MACROGLOBULIN - STOPPED-FLOW KINETIC-STUDIES OF ITS INTERACTION WITH CHYMOTRYPSIN [J].
CHRISTENSEN, U ;
SOTTRUPJENSEN, L ;
HARRIT, N .
BIOCHIMICA ET BIOPHYSICA ACTA, 1991, 1076 (01) :91-96
[8]   INHIBITION AND PARTIAL REVERSAL OF THE METHYLAMINE-INDUCED CONVERSION OF SLOW TO FAST ELECTROPHORETIC FORMS OF HUMAN ALPHA-2-MACROGLOBULIN BY MODIFICATION OF THE THIOLS [J].
CUNNINGHAM, LW ;
CREWS, BC ;
GETTINS, P .
BIOCHEMISTRY, 1990, 29 (06) :1638-1643
[9]   PRIMARY STRUCTURE OF PREGNANCY ZONE PROTEIN - MOLECULAR-CLONING OF A FULL-LENGTH PZP CDNA CLONE BY THE POLYMERASE CHAIN-REACTION [J].
DEVRIENDT, K ;
VANDENBERGHE, H ;
CASSIMAN, JJ ;
MARYNEN, P .
BIOCHIMICA ET BIOPHYSICA ACTA, 1991, 1088 (01) :95-103
[10]   A CONSERVED REGION IN ALPHA-MACROGLOBULINS PARTICIPATES IN BINDING TO THE MAMMALIAN ALPHA-MACROGLOBULIN RECEPTOR [J].
ENGHILD, JJ ;
THOGERSEN, IB ;
ROCHE, PA ;
PIZZO, SV .
BIOCHEMISTRY, 1989, 28 (03) :1406-1412
1234