A 2ND HEPATITIS-C VIRUS-ENCODED PROTEINASE

被引:346
作者
GRAKOUI, A
MCCOURT, DW
WYCHOWSKI, C
FEINSTONE, SM
RICE, CM
机构
[1] WASHINGTON UNIV, SCH MED, DEPT MOLEC MICROBIOL, 660 S EUCLID AVE, ST LOUIS, MO 63110 USA
[2] WASHINGTON UNIV, SCH MED, HOWARD HUGHES MED INST, ST LOUIS, MO 63110 USA
[3] US FDA, CTR EVALUAT & BIOL RES, DIV VIROL, BETHESDA, MD 20014 USA
来源
PROCEEDINGS OF THE NATIONAL ACADEMY OF SCIENCES OF THE UNITED STATES OF AMERICA | 1993年 / 90卷 / 22期
关键词
POLYPROTEIN PROCESSING; FLAVIVIRUS; ANTIVIRAL;
D O I
10.1073/pnas.90.22.10583
中图分类号
O [数理科学和化学]; P [天文学、地球科学]; Q [生物科学]; N [自然科学总论];
学科分类号
07 ; 0710 ; 09 ;
摘要
Host and viral proteinases are believed to be required for the production of at least nine hepatitis C virus (HCV)-specific polyprotein cleavage products. Although several cleavages appear to be catalyzed by host signal peptidase or the HCV NS3 serine proteinase, the enzyme responsible for cleavage at the 2/3 site has not been identified. In this report, we have defined the 2/3 cleavage site and obtained evidence which suggests that this cleavage is mediated by a second HCV-encoded proteinase, located between aa 827 and 1207. This region encompasses the C-terminal portion of the 23-kDa NS2 protein, the 2/3 cleavage site, and the serine proteinase domain of NS3. Efficient processing at the 2/3 site was observed in mammalian cells, Escherichia coli, and in plant or animal cell-free translation systems in the absence of microsomal membranes. Cleavage at the 2/3 site was abolished by alanine substitutions for NS2 residues His-952 or Cys-993 but was unaffected by several other substitution mutations, including those that inactivate NS3 serine proteinase function. Mutations abolishing cleavage at the 2/3 site did not block cleavage at other sites in the HCV polyprotein. Cotransfection experiments indicate that the 2/3 site can be cleaved in trans, which should facilitate purification and further characterization of this enzyme.
引用
收藏
页码:10583 / 10587
页数:5
相关论文
共 29 条
[1]   DENGUE-2 VIRUS NS2B AND NS3 FORM A STABLE COMPLEX THAT CAN CLEAVE NS3 WITHIN THE HELICASE DOMAIN [J].
ARIAS, CF ;
PREUGSCHAT, F ;
STRAUSS, JH .
VIROLOGY, 1993, 193 (02) :888-899
[2]   AT LEAST 5 RELATED, BUT DISTINCT, HEPATITIS-C VIRAL GENOTYPES EXIST [J].
CHA, TA ;
BEALL, E ;
IRVINE, B ;
KOLBERG, J ;
CHIEN, D ;
KUO, G ;
URDEA, MS .
PROCEEDINGS OF THE NATIONAL ACADEMY OF SCIENCES OF THE UNITED STATES OF AMERICA, 1992, 89 (15) :7144-7148
[3]   PROCESSING OF THE YELLOW-FEVER VIRUS NONSTRUCTURAL POLYPROTEIN - A CATALYTICALLY ACTIVE NS3-PROTEINASE DOMAIN AND NS2B ARE REQUIRED FOR CLEAVAGES AT DIBASIC SITES [J].
CHAMBERS, TJ ;
GRAKOUI, A ;
RICE, CM .
JOURNAL OF VIROLOGY, 1991, 65 (11) :6042-6050
[4]   EVIDENCE THAT THE N-TERMINAL DOMAIN OF NONSTRUCTURAL PROTEIN NS3 FROM YELLOW-FEVER VIRUS IS A SERINE PROTEASE RESPONSIBLE FOR SITE-SPECIFIC CLEAVAGES IN THE VIRAL POLYPROTEIN [J].
CHAMBERS, TJ ;
WEIR, RC ;
GRAKOUI, A ;
MCCOURT, DW ;
BAZAN, JF ;
FLETTERICK, RJ ;
RICE, CM .
PROCEEDINGS OF THE NATIONAL ACADEMY OF SCIENCES OF THE UNITED STATES OF AMERICA, 1990, 87 (22) :8898-8902
[5]   YELLOW-FEVER VIRUS PROTEIN-NS2A, PROTEIN-NS2B, AND PROTEIN-NS4B - IDENTIFICATION AND PARTIAL N-TERMINAL AMINO-ACID SEQUENCE-ANALYSIS [J].
CHAMBERS, TJ ;
MCCOURT, DW ;
RICE, CM .
VIROLOGY, 1989, 169 (01) :100-109
[6]   MOLECULAR-GENETICS OF PESTIVIRUSES [J].
COLLETT, MS .
COMPARATIVE IMMUNOLOGY MICROBIOLOGY AND INFECTIOUS DISEASES, 1992, 15 (03) :145-154
[7]   BOTH NONSTRUCTURAL PROTEINS NS2B AND NS3 ARE REQUIRED FOR THE PROTEOLYTIC PROCESSING OF DENGUE VIRUS NONSTRUCTURAL PROTEINS [J].
FALGOUT, B ;
PETHEL, M ;
ZHANG, YM ;
LAI, CJ .
JOURNAL OF VIROLOGY, 1991, 65 (05) :2467-2475
[8]   COMPUTER-ASSISTED PREDICTIONS OF SIGNAL PEPTIDASE PROCESSING SITES [J].
FOLZ, RJ ;
GORDON, JI .
BIOCHEMICAL AND BIOPHYSICAL RESEARCH COMMUNICATIONS, 1987, 146 (02) :870-877
[9]  
FRANCKI RIB, 1991, ARCH VIROL S, V2, P223
[10]   2 RELATED SUPERFAMILIES OF PUTATIVE HELICASES INVOLVED IN REPLICATION, RECOMBINATION, REPAIR AND EXPRESSION OF DNA AND RNA GENOMES [J].
GORBALENYA, AE ;
KOONIN, EV ;
DONCHENKO, AP ;
BLINOV, VM .
NUCLEIC ACIDS RESEARCH, 1989, 17 (12) :4713-4730
123