PROTEOLYTIC PROCESSING OF THE CARDIOVIRAL P2 REGION - PRIMARY 2A/2B CLEAVAGE IN CLONE-DERIVED PRECURSORS

被引：61

作者：

PALMENBERG, AC ^{[1
]}

PARKS, GD ^{[1
]}

HALL, DJ ^{[1
]}

INGRAHAM, RH ^{[1
]}

SENG, TW ^{[1
]}

PALLAI, PV ^{[1
]}

机构：

[1] UNIV WISCONSIN,DEPT ANIM HLTH & BIOMED SCI,MADISON,WI 53706

来源：

VIROLOGY | 1992年 / 190卷 / 02期

关键词：

D O I：

10.1016/0042-6822(92)90913-A

中图分类号：

Q93 [微生物学];

学科分类号：

071005 ; 100705 ;

摘要：

The primary 2A/2B cleavage within cardiovirus polyprotein was examined by construction of cDNA plasmids which linked fragments from the P2 region of encephalomyocarditis virus (EMCV) and Mengovirus genomes to the EMCV 5′ nontranslated region. When RNA transcripts from these clones were tested in reticulocyte extracts, the synthesized proteins were cotranslationally processed at the 2A/2B site. No viral segments outside of the P2 region were required for this activity. Engineered deletions which removed the amino-terminal two-thirds of protein 2A or the carboxyl half of protein 213 had no effect on this scission, nor did insertions into a Ser-Ala-Phe sequence (SAF) within 213, which is conserved in most cardio- and aphthoviruses. In contrast, mutations which disrupted a conserved Asn-Pro-Gly-Pro (NPGP) sequence abolished primary scission. Precursors thus inactivated were unable to serve as substrate when simultaneously expressed with active (wild-type) 2AB sequences. Microsequencing placed the EMCV primary cleavage site between the Gly/Pro pair within the NPGP sequence. It was also determined that endogenous viral protease 3C is the previously unidentified agent responsible for cardiovirus 1 D/2A scission, a cleavage that is part of the primary processing reaction in poliovirus. © 1992.

引用

页码：754 / 762

页数：9

共 22 条

[1] A SODIUM DODECYL-SULFATE POLYACRYLAMIDE-GEL ELECTROPHORESIS SYSTEM THAT SEPARATES PEPTIDES AND PROTEINS IN THE MOLECULAR-WEIGHT RANGE OF 2500 TO 90,000 [J].

ANDERSON, BL ;

BERRY, RW ;

TELSER, A .

ANALYTICAL BIOCHEMISTRY, 1983, 132 (02) :365-375

[2] MENGO-VIRUS MATURATION IS ACCOMPANIED BY C-TERMINAL MODIFICATION OF CAPSID PROTEIN-VP1 [J].

BOEGE, U ;

SCRABA, DG .

VIROLOGY, 1989, 168 (02) :409-412

[3] CLONING AND SYNTHESIS OF INFECTIOUS CARDIOVIRUS RNAS CONTAINING SHORT, DISCRETE POLY(C) TRACTS [J].

DUKE, GM ;

PALMENBERG, AC .

JOURNAL OF VIROLOGY, 1989, 63 (04) :1822-1826

[4] PROTEOLYTIC PROCESSING OF POLIOVIRUS POLYPEPTIDES - ANTIBODIES TO POLYPEPTIDE P3-7C INHIBIT CLEAVAGE AT GLUTAMINE-GLYCINE PAIRS [J].

HANECAK, R ;

SEMLER, BL ;

ANDERSON, CW ;

WIMMER, E .

PROCEEDINGS OF THE NATIONAL ACADEMY OF SCIENCES OF THE UNITED STATES OF AMERICA-BIOLOGICAL SCIENCES, 1982, 79 (13) :3973-3977

[5] A DETAILED KINETIC-ANALYSIS OF THE INVITRO SYNTHESIS AND PROCESSING OF ENCEPHALOMYOCARDITIS VIRUS PRODUCTS [J].

JACKSON, RJ .

VIROLOGY, 1986, 149 (01) :114-127

[6]

NICKLIN MJH, 1986, BIOTECHNOLOGY, V4, P36

[7] PICORNAVIRAL PROCESSING - SOME NEW IDEAS [J].

PALMENBERG, AC .

JOURNAL OF CELLULAR BIOCHEMISTRY, 1987, 33 (03) :191-198

[8] PROTEOLYTIC PROCESSING OF PICORNAVIRAL POLYPROTEIN [J].

PALMENBERG, AC .

ANNUAL REVIEW OF MICROBIOLOGY, 1990, 44 :603-623

[9] PROTEASE REQUIRED FOR PROCESSING PICORNAVIRAL COAT PROTEIN RESIDES IN THE VIRAL REPLICASE GENE [J].

PALMENBERG, AC ;

PALLANSCH, MA ;

RUECKERT, RR .

JOURNAL OF VIROLOGY, 1979, 32 (03) :770-778

[10] SITE-SPECIFIC MUTATIONS AT A PICORNAVIRUS VP3/VP1 CLEAVAGE SITE DISRUPT INVITRO PROCESSING AND ASSEMBLY OF CAPSID PRECURSORS [J].

PARKS, GD ;

PALMENBERG, AC .

JOURNAL OF VIROLOGY, 1987, 61 (12) :3680-3687

← 1 2 3 →