Temporal regulation of the Dictyostelium glycogen phosphorylase 2 gene

被引:5
|
作者
Rutherford, CL
Selmin, O
PetersWeigel, S
机构
[1] Biology Department, Molec. and Cellular Biology Section, Virginia Polytech. Inst. and S., Blacksburg
来源
BIOCHIMICA ET BIOPHYSICA ACTA-GENE STRUCTURE AND EXPRESSION | 1997年 / 1351卷 / 1-2期
关键词
Dictyostelium; glycogen phosphorylase; transcription factor; development;
D O I
10.1016/S0167-4781(96)00182-0
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
The product of the glycogen phosphorylase-2 gene in Dictyostelium functions to provide the glucose units that an used to construct the structural components of the terminal stage of development. In this report, we link a 1233 bp upstream gp2 fragment to a luciferase reporter gene in order to study the sequences that are involved in the temporal expression of the gene. Various deletions of the promoter-luciferase fusion were then transformed into Dictyostelium cells. All deletion constructs, from -1216 to -486 nucleotides from the translational start codon, showed the same temporal pattern of expression as the authentic gp2 gene, as well as similar luciferase activities. Removal of an additional 37 nucleotides resulted in nearly 100-fold decrease in activity, yet retained the normal temporal expression of luciferase. Analysis of DNA binding proteins with the gel shift assay revealed a stage-dependent pattern of proteins that bound to the gp2 promoter. A similar pattern of temporal expression of the binding proteins was observed with either the full-length probe or with oligonucleotide probes that contained sequences that were identified as putative regulator sites. Likewise, the full-length and oligonucleotide probes demonstrated identical binding patterns during several steps of purification of the DNA binding proteins. SDS-PAGE and Southwestern blot analysis of a DNA affinity purified fraction, identified a 23 kDa peptide as the binding protein.
引用
收藏
页码:111 / 125
页数:15
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