PRODUCTION OF RECOMBINANT BOVINE ENTEROKINASE CATALYTIC SUBUNIT IN ESCHERICHIA-COLI USING THE NOVEL SECRETORY FUSION PARTNER DSBA

被引：112

作者：

COLLINSRACIE, LA ^{[1
]}

MCCOLGAN, JM ^{[1
]}

GRANT, KL ^{[1
]}

DIBLASIOSMITH, EA ^{[1
]}

MCCOY, JM ^{[1
]}

LAVALLIE, ER ^{[1
]}

机构：

[1] GENET INST INC,CAMBRIDGE,MA 02140

来源：

BIO-TECHNOLOGY | 1995年 / 13卷 / 09期

关键词：

D O I：

10.1038/nbt0995-982

中图分类号：

Q81 [生物工程学（生物技术）]; Q93 [微生物学];

学科分类号：

071005 ; 0836 ; 090102 ; 100705 ;

摘要：

Enterokinase (EK) is a heterodimeric serine protease which plays a key role in initiating the proteolytic digestion cascade in the mammalian duodenum. The enzyme acts by converting trypsinogen to trypsin via a highly specific cleavage following the pentapeptide recognition sequence (Asp)(4)-Lys. This stringent site specificity gives EK great potential as a fusion protein cleavage reagent. Recently, a cDNA encoding the catalytic (light) chain of bovine enterokinase (EK(L)) was identified, characterized, and transiently expressed in mammalian COS cells. We report here the production of EK(L) in Escherichia coli by a novel secretory expression system that utilizes E. coli DsbA protein as an N-terminal fusion partner. The EK(L) cDNA was fused in-frame to the 3'-end of the coding sequence for DsbA, with the two domains of the fusion protein separated by a linker sequence encoding an enterokinase recognition site. Active, processed recombinant EK(L) (rEK(L)) was generated from this fusion protein via an autocatalytic cleavage reaction. The enzymatic properties of the bacterially produced rEK(L) were indistinguishable from the previously described COS-derived enzyme. Both forms of rEK(L) were capable of cleaving peptides, polypeptides and trypsinogen with the same specificity exhibited by the native heterodimeric enzyme purified from bovine duodena. Interestingly, rEK(L) activated trypsinogen poorly relative to the native heterodimeric enzyme, but was superior in its ability to cleave artificial fusion proteins containing the (Asp)(4)-Lys recognition sequence.

引用

页码：982 / 987

页数：6

共 34 条

[1] IDENTIFICATION OF A PROTEIN REQUIRED FOR DISULFIDE BOND FORMATION INVIVO
BARDWELL, JCA
MCGOVERN, K
BECKWITH, J
[J]. CELL, 1991, 67 (03) : 581 - 589
[2] BRICTEUXGREGOIR.S, 1972, COMP BIOCH PHYSL B, V42, P23
[3] THROMBIN SPECIFICITY - REQUIREMENT FOR APOLAR AMINO-ACIDS ADJACENT TO THE THROMBIN CLEAVAGE SITE OF POLYPEPTIDE SUBSTRATE
CHANG, JY
[J]. EUROPEAN JOURNAL OF BIOCHEMISTRY, 1985, 151 (02): : 217 - 224
[4] AN INVESTIGATION INTO THE MINIMUM REQUIREMENTS FOR PEPTIDE HYDROLYSIS BY MUTATION OF THE CATALYTIC TRIAD OF TRYPSIN
COREY, DR
CRAIK, CS
[J]. JOURNAL OF THE AMERICAN CHEMICAL SOCIETY, 1992, 114 (05) : 1784 - 1790
[5] MUTATIONS THAT ALLOW DISULFIDE BOND FORMATION IN THE CYTOPLASM OF ESCHERICHIA-COLI
DERMAN, AI
PRINZ, WA
BELIN, D
BECKWITH, J
[J]. SCIENCE, 1993, 262 (5140) : 1744 - 1747
[6] HIGH-EFFICIENCY TRANSFORMATION OF ESCHERICHIA-COLI BY HIGH-VOLTAGE ELECTROPORATION
DOWER, WJ
MILLER, JF
RAGSDALE, CW
[J]. NUCLEIC ACIDS RESEARCH, 1988, 16 (13) : 6127 - 6145
[7] DUPLAY P, 1984, J BIOL CHEM, V259, P606
[8] EXPRESSION OF ATRIAL NATRIURETIC FACTOR AS A CLEAVABLE FUSION PROTEIN WITH CHLORAMPHENICOL ACETYLTRANSFERASE IN ESCHERICHIA-COLI
DYKES, CW
BOOKLESS, AB
COOMBER, BA
NOBLE, SA
HUMBER, DC
HOBDEN, AN
[J]. EUROPEAN JOURNAL OF BIOCHEMISTRY, 1988, 174 (02): : 411 - 416
[9] FEHLHAMMER H, 1977, J MOL BIOL, V11, P415
[10] AN EVALUATION OF DIFFERENT ENZYMATIC CLEAVAGE METHODS FOR RECOMBINANT FUSION PROTEINS, APPLIED ON DES(1-3)INSULIN-LIKE GROWTH FACTOR-I
FORSBERG, G
BAASTRUP, B
RONDAHL, H
HOLMGREN, E
POHL, G
HARTMANIS, M
LAKE, M
[J]. JOURNAL OF PROTEIN CHEMISTRY, 1992, 11 (02): : 201 - 211

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