YEAST VECTORS FOR THE CONTROLLED EXPRESSION OF HETEROLOGOUS PROTEINS IN DIFFERENT GENETIC BACKGROUNDS

被引：1644

作者：

MUMBERG, D ^{[1
]}

MULLER, R ^{[1
]}

FUNK, M ^{[1
]}

机构：

[1] UNIV MARBURG,INST MOLEK BIOL & TUMORFORSCH,D-35037 MARBURG,GERMANY

来源：

GENE | 1995年 / 156卷 / 01期

关键词：

SACCHAROMYCES CEREVISIAE; PLASMID; MULTICOPY VECTOR; POLYLINKER; PROMOTER; HETEROLOGOUS EXPRESSION; CDNA CLONING;

D O I：

10.1016/0378-1119(95)00037-7

中图分类号：

Q3 [遗传学];

学科分类号：

071007 ; 090102 ;

摘要：

An expression system for Saccharomyces cerevisiae (Sc) has been developed which, depending on the chosen vector, allows the constitutive expression of proteins at different levels over a range of three orders of magnitude and in different genetic backgrounds. The expression system is comprised of cassettes composed of a weak CYC1 promoter, the ADH promoter or the stronger TEF and GPD promoters, flanked by a cloning array and the CYC1 terminator. The multiple cloning array based on pBIISK (Stratagene) provides six to nine unique restriction sites, which facilitates the cloning of genes and allows for the directed cloning of cDNAs by the widely used ZAP system (Stratagene). Expression cassettes were placed into both the centromeric and 2 mu plasmids of the pRS series [Sikorski and Hieter, Genetics 122 (1989) 19-27; Christianson et al., Gene 110 (1992) 119-122] containing HIS3, TRP1, LEU2 or URA3 markers. The 32 expression vectors created by this strategy provide a powerful tool for the convenient cloning and the controlled expression of genes or cDNAs in nearly every genetic background of the currently used Sc strains.

引用

页码：119 / 122

页数：4

共 18 条

[1]

Ausubel FM., 2006, ENZYMATIC MANIPULATI

[2] CHARACTERIZATION OF A REGULATORY REGION UPSTREAM OF THE ADR2 LOCUS OF S-CEREVISIAE [J].

BEIER, DR ;

YOUNG, ET .

NATURE, 1982, 300 (5894) :724-728

[3] EXPRESSION OF HETEROLOGOUS GENES IN SACCHAROMYCES-CEREVISIAE FROM VECTORS UTILIZING THE GLYCERALDEHYDE-3-PHOSPHATE DEHYDROGENASE GENE PROMOTER [J].

BITTER, GA ;

EGAN, KM .

GENE, 1984, 32 (03) :263-274

[4] MULTIFUNCTIONAL YEAST HIGH-COPY-NUMBER SHUTTLE VECTORS [J].

CHRISTIANSON, TW ;

SIKORSKI, RS ;

DANTE, M ;

SHERO, JH ;

HIETER, P .

GENE, 1992, 110 (01) :119-122

[5]

DENIS CL, 1983, J BIOL CHEM, V258, P1165

[6] A NOVEL GENETIC SYSTEM TO DETECT PROTEIN PROTEIN INTERACTIONS [J].

FIELDS, S ;

SONG, OK .

NATURE, 1989, 340 (6230) :245-246

[7] DISTINCTLY REGULATED TANDEM UPSTREAM ACTIVATION SITES MEDIATE CATABOLITE REPRESSION OF THE CYC1 GENE OF S-CEREVISIAE [J].

GUARENTE, L ;

LALONDE, B ;

GIFFORD, P ;

ALANI, E .

CELL, 1984, 36 (02) :503-511

[8] CDI1, A HUMAN G1-PHASE AND S-PHASE PROTEIN PHOSPHATASE THAT ASSOCIATES WITH CDK2 [J].

GYURIS, J ;

GOLEMIS, E ;

CHERTKOV, H ;

BRENT, R .

CELL, 1993, 75 (04) :791-803

[9]

HARPER JW, 1993, CELL, V75, P805

[10] EXPRESSION OF A HUMAN-GENE FOR INTERFERON IN YEAST [J].

HITZEMAN, RA ;

HAGIE, FE ;

LEVINE, HL ;

GOEDDEL, DV ;

AMMERER, G ;

HALL, BD .

NATURE, 1981, 293 (5835) :717-722

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