IMPROVED EXPRESSION CLONING USING REPORTER GENES AND EPSTEIN-BARR-VIRUS ORI-CONTAINING VECTORS

被引：13

作者：

SHEN, ES ^{[1
]}

COOKE, GM ^{[1
]}

HORLICK, RA ^{[1
]}

机构：

[1] DUPONT MERCK PHARMACEUT CO,EXPTL STN,WILMINGTON,DE 19880

来源：

GENE | 1995年 / 156卷 / 02期

关键词：

ANGIOTENSIN II; CYTOMEGALOVIRUS; EBV; EBNA1; T-ANTIGEN; TSA201;

D O I：

10.1016/0378-1119(95)00038-8

中图分类号：

Q3 [遗传学];

学科分类号：

071007 ; 090102 ;

摘要：

Levels of expression of two reporter genes cloned into SV40 or Epstein-Barr virus (EBV) ori-containing plasmids were measured following transient transfection of cell lines constitutively expressing T-antigen or EBV nuclear antigen 1 (EBNA1). The TSA201 and COS7 cell lines stably produce T-antigen and support replication of the SV40 ori-containing constructs while the 293EBNA cell line produces EBNA1 and supports replication of EBV osi-containing plasmids. We found that 293EBNA cells express >25-fold more beta-galactosidase (beta Gal) per mg protein than COS7 cells and 11-fold more beta Gal than TSA201 cells. We also demonstrate that 293EBNA cells are able to express 70-100-fold more angiotensin II type-1 receptor (AT1) per mg protein than COS7 or TSA201 cells. We examined the suitability of each cell line for use in expression cloning using a NaOH 'scrape' method as an improvement over emulsion autoradiography for detection, Measurable AT1 signals can be detected when reporter plasmids are diluted up to 1000-fold for COS7 and TSA201 cells, and up to 80 000-fold for 293EBNA cells. These data demonstrate that 293EBNA cells offer a significant improvement in expression cloning technology as compared to the conventionally used T-antigen-based cell lines.

引用

页码：235 / 239

页数：5

共 31 条

[1] AUSUBEL FM, 1990, CURRENT PROTOCOLS MO
[2] THE USE OF ENGINEERED E1A GENES TO TRANSACTIVATE THE HCMV-MIE PROMOTER IN PERMANENT CHO CELL-LINES
COCKETT, MI
BEBBINGTON, CR
YARRANTON, GT
[J]. NUCLEIC ACIDS RESEARCH, 1991, 19 (02) : 319 - 325
[3] EXPRESSION CLONING OF THE MURINE ERYTHROPOIETIN RECEPTOR
DANDREA, AD
LODISH, HF
WONG, GG
[J]. CELL, 1989, 57 (02) : 277 - 285
[4] DUBRIDGE RB, 1987, MOL CELL BIOL, V7, P3791
[5] EXPRESSION CLONING OF A RECEPTOR FOR MURINE GRANULOCYTE COLONY-STIMULATING FACTOR
FUKUNAGA, R
ISHIZAKAIKEDA, E
SETO, Y
NAGATA, S
[J]. CELL, 1990, 61 (02) : 341 - 350
[6] EXPRESSION CLONING OF A RECEPTOR FOR HUMAN GRANULOCYTE-MACROPHAGE COLONY-STIMULATING FACTOR
GEARING, DP
KING, JA
GOUGH, NM
NICOLA, NA
[J]. EMBO JOURNAL, 1989, 8 (12) : 3667 - 3676
[7] CLONING OF THE HUMAN AND MURINE INTERLEUKIN-7 RECEPTORS - DEMONSTRATION OF A SOLUBLE FORM AND HOMOLOGY TO A NEW RECEPTOR SUPERFAMILY
GOODWIN, RG
FRIEND, D
ZIEGLER, SF
JERZY, R
FALK, BA
GIMPEL, S
COSMAN, D
DOWER, SK
MARCH, CJ
NAMEN, AE
PARK, LS
[J]. CELL, 1990, 60 (06) : 941 - 951
[8] THE HUMAN CYTOMEGALO-VIRUS MAJOR IMMEDIATE EARLY PROMOTER CAN BE TRANS-ACTIVATED BY ADENOVIRUS EARLY PROTEINS
GORMAN, CM
GIES, D
MCCRAY, G
HUANG, M
[J]. VIROLOGY, 1989, 171 (02) : 377 - 385
[9] CHARACTERISTICS OF A HUMAN CELL LINE TRANSFORMED BY DNA FROM HUMAN ADENOVIRUS TYPE-5
GRAHAM, FL
SMILEY, J
RUSSELL, WC
NAIRN, R
[J]. JOURNAL OF GENERAL VIROLOGY, 1977, 36 (JUL) : 59 - 72
[10] LOCALIZATION OF ANGIOTENSIN-II RECEPTOR SUBTYPES IN THE RABBIT ADRENAL AND KIDNEY
HERBLIN, WF
DIAMOND, SM
TIMMERMANS, PBMWM
[J]. PEPTIDES, 1991, 12 (03) : 581 - 584

← 1 2 3 4 →