MATURATION OF HUMAN-IMMUNODEFICIENCY-VIRUS PARTICLES ASSEMBLED FROM THE GAG PRECURSOR PROTEIN REQUIRES INSITU PROCESSING BY GAG POL PROTEASE

被引：30

作者：

ROSS, EK

FUERST, TR

ORENSTEIN, JM

ONEILL, T

MARTIN, MA

VENKATESAN, S

机构：

[1] NIAID,MED MICROBIOL LAB,ROOM 36,BLDG 4,BETHESDA,MD 20892

[2] MOLEC VACCINES INC,GAITHERSBURG,MD

[3] GEORGE WASHINGTON UNIV,SCH MED,DEPT PATHOL,WASHINGTON,DC 20052

来源：

AIDS RESEARCH AND HUMAN RETROVIRUSES | 1991年 / 7卷 / 05期

关键词：

D O I：

10.1089/aid.1991.7.475

中图分类号：

R392 [医学免疫学]; Q939.91 [免疫学];

学科分类号：

100102 ;

摘要：

The vaccinia virus expression system was used to determine the role of human immunodeficiency virus type 1 (HIV-1) protease in viral morphogenesis and maturation. The unprocessed p55 gag precursor polyprotein alone was assembled to form HIV-1 particles which budded from cells. The particles were spherical and immature, containing an electron-dense shell in the particle submembrane; there was no evidence of core formation. Expression of both gag and pol proteins from a recombinant containing the complete gag-pol coding sequences resulted in intracellular processing of gag-pol proteins and the production of mature particles with electrondense cores characteristic of wild-type HIV virions. To ascertain the role of protein processing in particle maturation, the pol ORF in the gag-pol recombinant was truncated to limit expression of the pol gene to the protease domain. With this recombinant expressing p55 gag and protease, intracellular processing was observed. Some of the resultant particles were partially mature and contained processed gag protein subunits. In contrast, particle maturation was not observed when the HIV-1 protease and p55 gag were coexpressed from separate recombinants, despite evidence of intracellular gag processing. These findings suggest that HIV-1 protease must be an integral component of the full-length gag-pol precursor for optimal processing and virion maturation.

引用

页码：475 / 483

页数：9

共 34 条

[21] LOEB DD, 1989, PROTEASES RETROVIRUS, P111
[22] Mackett M., 1985, DNA CLONING PRACTICA, P191
[23] THE GAG GENE-PRODUCTS OF HUMAN IMMUNODEFICIENCY VIRUS TYPE-1 - ALIGNMENT WITHIN THE GAG OPEN READING FRAME, IDENTIFICATION OF POSTTRANSLATIONAL MODIFICATIONS, AND EVIDENCE FOR ALTERNATIVE GAG PRECURSORS
MERVIS, RJ
AHMAD, N
LILLEHOJ, EP
RAUM, MG
SALAZAR, FHR
CHAN, HW
VENKATESAN, S
[J]. JOURNAL OF VIROLOGY, 1988, 62 (11) : 3993 - 4002
[24] 3-DIMENSIONAL STRUCTURE OF ASPARTYL PROTEASE FROM HUMAN IMMUNODEFICIENCY VIRUS HIV-1
NAVIA, MA
FITZGERALD, PMD
MCKEEVER, BM
LEU, CT
HEIMBACH, JC
HERBER, WK
SIGAL, IS
DARKE, PL
SPRINGER, JP
[J]. NATURE, 1989, 337 (6208) : 615 - 620
[25] COMPLETE NUCLEOTIDE-SEQUENCE OF THE AIDS VIRUS, HTLV-III
RATNER, L
HASELTINE, W
PATARCA, R
LIVAK, KJ
STARCICH, B
JOSEPHS, SF
DORAN, ER
RAFALSKI, JA
WHITEHORN, EA
BAUMEISTER, K
IVANOFF, L
PETTEWAY, SR
PEARSON, ML
LAUTENBERGER, JA
PAPAS, TS
GHRAYEB, J
CHANG, NT
GALLO, RC
WONGSTAAL, F
[J]. NATURE, 1985, 313 (6000) : 277 - 284
[26] MYRISTYLATION SITE IN PR65GAG IS ESSENTIAL FOR VIRUS PARTICLE FORMATION BY MOLONEY MURINE LEUKEMIA-VIRUS
REIN, A
MCCLURE, MR
RICE, NR
LUFTIG, RB
SCHULTZ, AM
[J]. PROCEEDINGS OF THE NATIONAL ACADEMY OF SCIENCES OF THE UNITED STATES OF AMERICA, 1986, 83 (19) : 7246 - 7250
[27] MYRISTYLATION IS REQUIRED FOR INTRACELLULAR-TRANSPORT BUT NOT FOR ASSEMBLY OF D-TYPE RETROVIRUS CAPSIDS
RHEE, SS
HUNTER, E
[J]. JOURNAL OF VIROLOGY, 1987, 61 (04) : 1045 - 1053
[28] NUCLEOTIDE-SEQUENCE AND EXPRESSION OF AN AIDS-ASSOCIATED RETROVIRUS (ARV-2)
SANCHEZPESCADOR, R
POWER, MD
BARR, PJ
STEIMER, KS
STEMPIEN, MM
BROWNSHIMER, SL
GEE, WW
RENARD, A
RANDOLPH, A
LEVY, JA
DINA, D
LUCIW, PA
[J]. SCIENCE, 1985, 227 (4686) : 484 - 492
[29] PRODUCTION OF HUMAN-IMMUNODEFICIENCY-VIRUS (HIV)-LIKE PARTICLES FROM CELLS INFECTED WITH RECOMBINANT VACCINIA VIRUSES CARRYING THE GAG GENE OF HIV
SHIODA, T
SHIBUTA, H
[J]. VIROLOGY, 1990, 175 (01) : 139 - 148
[30] STEPHENS EB, 1988, ANNU REV MICROBIOL, V42, P489

← 1 2 3 4 →