MOLECULAR-CLONING AND EXPRESSION OF THE BACTERIOPHAGE T707(PROTEIN KINASE) GENE

被引:15
|
作者
MICHALEWICZ, J [1 ]
NICHOLSON, AW [1 ]
机构
[1] WAYNE STATE UNIV, DEPT BIOL SCI, DETROIT, MI 48202 USA
来源
VIROLOGY | 1992年 / 186卷 / 02期
关键词
D O I
10.1016/0042-6822(92)90010-M
中图分类号
Q93 [微生物学];
学科分类号
071005 ; 100705 ;
摘要
The bacteriophage T7 0.7 gene encodes a protein which supports viral reproduction under specific suboptimal growth conditions. The 0.7 protein (gp0.7) shuts off host RNA polymerase-catalyzed transcription and also expresses a serine/threonine-specific, cAMP-independent protein kinase (PK) activity. To determine the role of the gp0.7 PK in viral reproduction, the 0.7 gene of the T7(JS78) mutant phage-whose gp0.7 expresses only the PK activity-was cloned in the plasmid expression vector pET-11 a. Cells containing the recombinant plasmid were viable, and upon IPTG induction produced a 30-kDa polypeptide, similar in size to the gp0.7-related polypeptide seen in T7(JS78)-infected cells. Extracts of cells containing this polypeptide can phosphorylate the exogenous substrate lysozyme. Expression of plasmid-encoded gp0.7(JS78) in vivo results in phosphorylation of the same proteins which are phosphorylated in T7(1S78)-infected cells; moreover, the plasmid-encoded gp0.7(JS78) is itself phosphorylated. The JS78 mutation changes GIn243 in gp0.7 to an amber codon, which explains the production of the truncated, 30-kDa gp0.7-related polypeptide, and implicates the 11-kDa C-terminal domain in host transcription shut-off. The T7(A23) 0.7 point mutant fails to express PK activity in infected cells. However, the truncated gp0.7(A23)-related polypeptide, expressed from a plasmid, exhibits PK activity in vivo and in vitro, but with an altered specificity. Thus, the A23 mutation, which changes Aspl00 to Asn, may identify a substrate recognition determinant. © 1992.
引用
收藏
页码:452 / 462
页数:11
相关论文
共 50 条
  • [21] CLONING AND EXPRESSION OF THE LTF GENE OF BACTERIOPHAGE-T5
    HELLER, KJ
    KRAUEL, V
    JOURNAL OF BACTERIOLOGY, 1986, 167 (03) : 1071 - 1073
  • [22] MOLECULAR-CLONING AND DIFFERENTIAL EXPRESSION OF THE MAIZE FERREDOXIN GENE FAMILY
    HASE, T
    KIMATA, Y
    YONEKURA, K
    MATSUMURA, T
    SAKAKIBARA, H
    PLANT PHYSIOLOGY, 1991, 96 (01) : 77 - 83
  • [23] MOLECULAR-CLONING AND CHARACTERIZATION OF A NOVEL MARSUPIAL MILK PROTEIN GENE
    COLLET, C
    JOSEPH, R
    NICHOLAS, K
    BIOCHEMICAL AND BIOPHYSICAL RESEARCH COMMUNICATIONS, 1989, 164 (03) : 1380 - 1383
  • [24] MOLECULAR-CLONING AND EXPRESSION OF MOUSE CD34 GENE
    SUDA, T
    SUDA, J
    MIURA, Y
    SUDO, T
    EXPERIMENTAL HEMATOLOGY, 1991, 19 (06) : 465 - 465
  • [25] MOLECULAR-CLONING AND ANALYSIS OF THE HUMAN TEC PROTEIN-TYROSINE KINASE
    SATO, K
    MANO, H
    ARIYAMA, T
    INAZAWA, J
    YAZAKI, Y
    HIRAI, H
    LEUKEMIA, 1994, 8 (10) : 1663 - 1672
  • [26] MOLECULAR-CLONING OF PLANT TRANSCRIPTS ENCODING PROTEIN-KINASE HOMOLOGS
    LAWTON, MA
    YAMAMOTO, RT
    HANKS, SK
    LAMB, CJ
    PROCEEDINGS OF THE NATIONAL ACADEMY OF SCIENCES OF THE UNITED STATES OF AMERICA, 1989, 86 (09) : 3140 - 3144
  • [27] MOLECULAR-CLONING AND INVITRO EXPRESSION OF THE CHLOROPLAST PHOSPHATE TRANSLOCATOR PROTEIN
    FLUGGE, UI
    FISCHER, K
    GROSS, A
    BIOLOGICAL CHEMISTRY HOPPE-SEYLER, 1989, 370 (07): : 643 - 644
  • [28] THE MOLECULAR-CLONING AND EXPRESSION OF THE HUMAN-GENE FOR HEAT-SHOCK PROTEIN-108
    POWER, RF
    HEADON, DR
    BIOCHEMICAL SOCIETY TRANSACTIONS, 1988, 16 (02) : 174 - 174
  • [29] MOLECULAR-CLONING AND EXPRESSION OF SALMONELLA-PARATYPHI A-52 KDA SPECIFIC PROTEIN GENE
    KORBSRISATE, S
    SARASOMBATH, S
    EKPO, P
    PONGSUNK, S
    ASIAN PACIFIC JOURNAL OF ALLERGY AND IMMUNOLOGY, 1994, 12 (01): : 27 - 37
  • [30] GENE-TRANSFER, EXPRESSION, AND MOLECULAR-CLONING OF THE HUMAN TRANSFERRIN RECEPTOR GENE
    KUHN, LC
    MCCLELLAND, A
    RUDDLE, FH
    CELL, 1984, 37 (01) : 95 - 103
12345