首页> 美国卫生研究院文献>The EMBO Journal >Interactions of purified transcription factors: binding of yeast MAT alpha 1 and PRTF to cell type-specific upstream activating sequences.
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Interactions of purified transcription factors: binding of yeast MAT alpha 1 and PRTF to cell type-specific upstream activating sequences.

机译:纯化的转录因子的相互作用:酵母MATα1和PRTF与细胞类型特异性上游激活序列的结合。

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摘要

Pheromone receptor transcription factor (PRTF) and MAT alpha 1 are protein transcription factors that are involved in the regulation of the alpha-specific genes in Saccharomyces cerevisiae. We have expressed MAT alpha 1 as a fusion protein in Escherichia coli and purified it from inclusion bodies in milligram quantities. The MAT alpha 1 protein was obtained after specific cleavage of the fusion protein. Quantitative band shift electrophoresis was used to determine the equilibrium dissociation constants that describe the multicomponent binding equilibrium between the PRTF and MAT alpha 1 proteins, and alpha-specific STE3 upstream activating sequence (UAS) DNA. The dissociation constant for the complex of PRTF and the a-specific UAS of STE2 was also measured and found to be 5.9 X 10(-11) M, only three times less than that for the PRTF-STE3 UAS complex. Analyses of these complexes by DNase I footprinting demonstrate that the PRTF binding site is confined to the palindromic P-box sequence in the case of the STE3 UAS, but extends symmetrically from this central region to cover 28 bp for the STE2 UAS. When MAT alpha 1 is bound to the PRTF-STE3 complex, the region of DNA protected is enlarged to that seen for the PRTF-STE2 complex. Our results using these two purified factors in vitro suggest that PRTF has nearly the same affinity for a- and alpha-specific UAS elements and that transcriptional activation requires a particular conformational state for the PRTF-DNA complex which occurs in the PRTF-STE2 and MAT alpha 1-PRTF-STE3 complexes, but not in the PRTF-STE3 complex.
机译:信息素受体转录因子(PRTF)和MAT alpha 1是参与酿酒酵母中alpha特异性基因调控的蛋白质转录因子。我们已经将MATα1表达为大肠杆菌中的融合蛋白,并以毫克量从包涵体中纯化了它。在特异性切割融合蛋白后获得MATα1蛋白。定量带移电泳用于确定平衡解离常数,该常数描述了PRTF和MAT alpha 1蛋白与α特异性STE3上游激活序列(UAS)DNA之间的多组分结合平衡。还测量了PRTF和STE2的a特异性UAS的复合物的解离常数,为5.9 X 10(-11)M,仅比PRTF-STE3 UAS的复合物的解离常数小三倍。通过DNase I足迹对这些复合物的分析表明,在STE3 UAS的情况下,PRTF结合位点局限于回文P-box序列,但从该中心区域对称延伸,覆盖STE2 UAS的28 bp。当MAT alpha 1与PRTF-STE3复合物结合时,受保护的DNA区域会扩大到PRTF-STE2复合物所见的区域。我们在体外使用这两种纯化因子的结果表明PRTF对a和α特异性UAS元素具有几乎相同的亲和力,并且转录激活需要PRTF-STE2和MAT中出现的PRTF-DNA复合物具有特定的构象状态alpha 1-PRTF-STE3复合体,但不在PRTF-STE3复合体中。

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