THE HPV16 E5 PROTEIN - EXPRESSION, DETECTION, AND STABLE COMPLEX-FORMATION WITH TRANSMEMBRANE PROTEINS IN COS CELLS

被引:94
作者
HWANG, ES [1 ]
NOTTOLI, T [1 ]
DIMAIO, D [1 ]
机构
[1] YALE UNIV, SCH MED, DEPT GENET, NEW HAVEN, CT 06510 USA
来源
VIROLOGY | 1995年 / 211卷 / 01期
关键词
D O I
10.1006/viro.1995.1395
中图分类号
Q93 [微生物学];
学科分类号
071005 ; 100705 ;
摘要
The human papillomavirus-16 (HPV16) E5 gene is able to induce stable growth transformation and transient mitogenic stimulation in a variety of cultured cell systems. To characterize the biochemical properties of the hydrophobic HPV16 E5 transforming protein, we have constructed vectors expressing the wild-type HPV16 E5 gene and have generated antipeptide antisera. The 10-kDa E5 protein was readily detectable in transfected COS monkey cells by using these antisera either for immunoprecipitation of metabolically labeled cells or for immunoblotting. Coimmunoprecipitation analysis of cells coexpressing the viral protein and various growth factor receptors demonstrated stable complex formation between the E5 protein and the epidermal growth factor receptor, platelet-derived growth factor beta receptor, colony stimulating factor-1 receptor, and p185(neu). The E5 protein also formed a stable complex with the vesicular stomatitis virus glycoprotein. These experiments indicated that the HPV16 E5 protein was able to participate in complex formation with a variety of transmembrane proteins, a property which may contribute to the biological activities of the viral protein. In addition, the expression vectors and antibodies described here will be useful reagents in examining various aspects of HPV16 E5 expression and function. (C) 1995 Academic Press, Inc.
引用
收藏
页码:227 / 233
页数:7
相关论文
共 27 条
[1]   THE HUMAN PAPILLOMAVIRUS TYPE-16 E5 GENE COOPERATES WITH THE E7 GENE TO STIMULATE PROLIFERATION OF PRIMARY-CELLS AND INCREASES VIRAL GENE-EXPRESSION [J].
BOUVARD, V ;
MATLASHEWSKI, G ;
GU, ZM ;
STOREY, A ;
BANKS, L .
VIROLOGY, 1994, 203 (01) :73-80
[2]   LOCALIZATION OF BOVINE PAPILLOMAVIRUS TYPE-1 E5 PROTEIN TO TRANSFORMED BASAL KERATINOCYTES AND PERMISSIVE DIFFERENTIATED CELLS IN FIBROPAPILLOMA TISSUE [J].
BURNETT, S ;
JAREBORG, N ;
DIMAIO, D .
PROCEEDINGS OF THE NATIONAL ACADEMY OF SCIENCES OF THE UNITED STATES OF AMERICA, 1992, 89 (12) :5665-5669
[3]   TRANSFORMATION-SPECIFIC INTERACTION OF THE BOVINE PAPILLOMAVIRUS E5 ONCOPROTEIN WITH THE PLATELET-DERIVED GROWTH-FACTOR RECEPTOR TRANSMEMBRANE DOMAIN AND THE EPIDERMAL GROWTH-FACTOR RECEPTOR CYTOPLASMIC DOMAIN [J].
COHEN, BD ;
GOLDSTEIN, DJ ;
RUTLEDGE, L ;
VASS, WC ;
LOWY, DR ;
SCHLEGEL, R ;
SCHILLER, JT .
JOURNAL OF VIROLOGY, 1993, 67 (09) :5303-5311
[4]   THE E5 PROTEIN OF HPV-6, BUT NOT HPV-16, ASSOCIATES EFFICIENTLY WITH CELLULAR GROWTH-FACTOR RECEPTORS [J].
CONRAD, M ;
GOLDSTEIN, D ;
ANDRESSON, T ;
SCHLEGEL, R .
VIROLOGY, 1994, 200 (02) :796-800
[5]   THE HUMAN PAPILLOMAVIRUS TYPE-6 AND 16-E5 PROTEINS ARE MEMBRANE-ASSOCIATED PROTEINS WHICH ASSOCIATE WITH THE 16-KILODALTON PORE-FORMING PROTEIN [J].
CONRAD, M ;
BUBB, VJ ;
SCHLEGEL, R .
JOURNAL OF VIROLOGY, 1993, 67 (10) :6170-6178
[6]  
DIMAIO D, 1991, ADV CANCER RES, V56, P133
[7]   THE E5 TRANSFORMING PROTEINS OF THE PAPILLOMAVIRUSES [J].
DIMAIO, D ;
PETTI, L ;
HWANG, ES .
SEMINARS IN VIROLOGY, 1994, 5 (05) :369-379
[8]   THE BPV-1 E5-PROTEIN, THE 16-KDA MEMBRANE PORE-FORMING PROTEIN AND THE PDGF RECEPTOR EXIST IN A COMPLEX THAT IS DEPENDENT ON HYDROPHOBIC TRANSMEMBRANE INTERACTIONS [J].
GOLDSTEIN, DJ ;
ANDRESSON, T ;
SPARKOWSKI, JJ ;
SCHLEGEL, R .
EMBO JOURNAL, 1992, 11 (13) :4851-4859
[9]   THE BOVINE PAPILLOMAVIRUS TYPE-1 E5 TRANSFORMING PROTEIN SPECIFICALLY BINDS AND ACTIVATES THE BETA-TYPE RECEPTOR FOR THE PLATELET-DERIVED GROWTH-FACTOR BUT NOT OTHER RELATED TYROSINE KINASE-CONTAINING RECEPTORS TO INDUCE CELLULAR-TRANSFORMATION [J].
GOLDSTEIN, DJ ;
LI, WQ ;
WANG, LM ;
HEIDARAN, MA ;
AARONSON, S ;
SHINN, R ;
SCHLEGEL, R ;
PIERCE, JH .
JOURNAL OF VIROLOGY, 1994, 68 (07) :4432-4441
[10]   IDENTIFICATION OF THE E5 OPEN READING FRAME OF HUMAN PAPILLOMAVIRUS TYPE-16 [J].
HALBERT, CL ;
GALLOWAY, DA .
JOURNAL OF VIROLOGY, 1988, 62 (03) :1071-1075
123