GRR1 OF SACCHAROMYCES-CEREVISIAE IS REQUIRED FOR GLUCOSE REPRESSION AND ENCODES A PROTEIN WITH LEUCINE-RICH REPEATS

被引:144
作者
FLICK, JS [1 ]
JOHNSTON, M [1 ]
机构
[1] WASHINGTON UNIV, SCH MED, DEPT GENET, BOX 8232, 4566 SCOTT AVE, ST LOUIS, MO 63110 USA
来源
MOLECULAR AND CELLULAR BIOLOGY | 1991年 / 11卷 / 10期
关键词
D O I
10.1128/MCB.11.10.5101
中图分类号
Q5 [生物化学]; Q7 [分子生物学];
学科分类号
071010 ; 081704 ;
摘要
Growth of the yeast Saccharomyces cerevisiae on glucose leads to repression of transcription of many genes required for alternative carbohydrate metabolism. The GRR1 gene appears to be of central importance to the glucose repression mechanism, because mutations in GRR1 result in a pleiotropic loss of glucose repression (R. Bailey and A. Woodword, Mol. Gen. Genet. 193:507-512, 1984). We have isolated the GRR1 gene and determined that null mutants are viable and display a number of growth defects in addition to the loss of glucose repression. Surprisingly, grr1 mutations convert SUC2, normally a glucose-repressed gene, into a glucose-induced gene. GRR1 encodes a protein of 1,151 amino acids that is expressed constitutively at low levels in yeast cells. GRR1 protein contains 12 tandem repeats of a sequence similar to leucine-rich motifs found in other proteins that may mediate protein-protein interactions. Indeed, cell fractionation studies are consistent with this view, suggesting that GRR1 protein is tightly associated with a particulate protein fraction in yeast extracts. The combined genetic and molecular data are consistent with the idea that GRR1 protein is a primary response element in the glucose repression pathway and is required for the generation or interpretation of the signal that induces glucose repression.
引用
收藏
页码:5101 / 5112
页数:12
相关论文
共 71 条
[41]   NORMAL AND MUTANT HUMAN BETA-GLOBIN PRE-MESSENGER RNAS ARE FAITHFULLY AND EFFICIENTLY SPLICED INVITRO [J].
KRAINER, AR ;
MANIATIS, T ;
RUSKIN, B ;
GREEN, MR .
CELL, 1984, 36 (04) :993-1005
[42]   PRIMARY STRUCTURE OF AN EXTRACELLULAR-MATRIX PROTEOGLYCAN CORE PROTEIN DEDUCED FROM CLONED CDNA [J].
KRUSIUS, T ;
RUOSLAHTI, E .
PROCEEDINGS OF THE NATIONAL ACADEMY OF SCIENCES OF THE UNITED STATES OF AMERICA, 1986, 83 (20) :7683-7687
[43]   CLEAVAGE OF STRUCTURAL PROTEINS DURING ASSEMBLY OF HEAD OF BACTERIOPHAGE-T4 [J].
LAEMMLI, UK .
NATURE, 1970, 227 (5259) :680-+
[44]   ARTIFACTUAL IMMUNOFLUORESCENT LABELING IN YEAST, DEMONSTRATED BY AFFINITY PURIFICATION OF ANTIBODY [J].
LILLIE, SH ;
BROWN, SS .
YEAST, 1987, 3 (02) :63-70
[45]   CLONING OF THE ALPHA-CHAIN OF HUMAN-PLATELET GLYCOPROTEIN-IB - A TRANSMEMBRANE PROTEIN WITH HOMOLOGY TO LEUCINE-RICH ALPHA-2-GLYCOPROTEIN [J].
LOPEZ, JA ;
CHUNG, DW ;
FUJIKAWA, K ;
HAGEN, FS ;
PAPAYANNOPOULOU, T ;
ROTH, GJ .
PROCEEDINGS OF THE NATIONAL ACADEMY OF SCIENCES OF THE UNITED STATES OF AMERICA, 1987, 84 (16) :5615-5619
[46]   RECESSIVE MUTATIONS CONFERRING RESISTANCE TO CARBON CATABOLITE REPRESSION OF GALACTOKINASE SYNTHESIS IN SACCHAROMYCES-CEREVISIAE [J].
MATSUMOTO, K ;
YOSHIMATSU, T ;
OSHIMA, Y .
JOURNAL OF BACTERIOLOGY, 1983, 153 (03) :1405-1414
[47]   YEAST MIG1 REPRESSOR IS RELATED TO THE MAMMALIAN EARLY GROWTH-RESPONSE AND WILMS-TUMOR FINGER PROTEINS [J].
NEHLIN, JO ;
RONNE, H .
EMBO JOURNAL, 1990, 9 (09) :2891-2898
[48]  
NEIGEBORN L, 1987, GENETICS, V115, P247
[49]   ISOLATION AND CHARACTERIZATION OF THE REGULATORY HEX2 GENE NECESSARY FOR GLUCOSE REPRESSION IN YEAST [J].
NIEDERACHER, D ;
ENTIAN, KD .
MOLECULAR & GENERAL GENETICS, 1987, 206 (03) :505-509
[50]   S-POMBE GENE SDS22+ ESSENTIAL FOR A MIDMITOTIC TRANSITION ENCODES A LEUCINE-RICH REPEAT PROTEIN THAT POSITIVELY MODULATES PROTEIN PHOSPHATASE-1 [J].
OHKURA, H ;
YANAGIDA, M .
CELL, 1991, 64 (01) :149-157
12345678