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一种热休克蛋白70(Hsp70)对多药耐药基因表达的负转录调控。

Negative transcriptional regulation of multidrug resistance gene expression by an Hsp70 protein.

作者信息

Shahi Puja, Gulshan Kailash, Moye-Rowley W Scott

机构信息

Department of Molecular Physiology and Biophysics, University of Iowa, Iowa City, Iowa 52242.

Department of Molecular Physiology and Biophysics, University of Iowa, Iowa City, Iowa 52242.

出版信息

J Biol Chem. 2007 Sep 14;282(37):26822-26831. doi: 10.1074/jbc.M704772200. Epub 2007 Jul 18.

DOI:10.1074/jbc.M704772200
PMID:17636264
Abstract

One of the most common origins of multidrug resistance occurs via the overproduction of ATP-binding cassette (ABC) transporter proteins. These ABC transporters then act as broad specificity drug pumps and efflux a wide range of toxic agents out of the cell. The yeast Saccharomyces cerevisiae exhibits multiple or pleiotropic drug resistance (Pdr) often through the over-production of a plasma membrane-localized ABC transporter protein called Pdr5p. Expression of the PDR5 gene is controlled by two zinc cluster-containing transcription factors called Pdr1p and Pdr3p. Cells that lack their mitochondrial genome (rho(0) cells) strongly induce PDR5 transcription in a Pdr3p-dependent fashion. To identify proteins associated with Pdr3p that might act to regulate this factor, a tandem affinity purification (TAP) moiety was fused to Pdr3p, and this recombinant protein was purified from yeast cells. The cytosolic Hsp70 chaperone Ssa1p co-purified with TAP-Pdr3p. Overexpression of Ssa1p repressed expression of PDR5 but had no effect on expression of other genes involved in the Pdr phenotype. This Ssa1p-mediated repression required the presence of Pdr3p and did not influence Pdr1p-dependent gene expression. Loss of the nucleotide exchange factor Fes1p mimicked Ssa1p-mediated repression of PDR5. Co-immunoprecipitation experiments indicated that Ssa1p was associated with Pdr3p but not Pdr1p in yeast cells. Finally, rho(0) cells had less Ssa1p bound to Pdr3p than rho(+) cells, consistent with Ssa1p-mediated repression of Pdr3p activity serving as a key regulatory step in control of multidrug resistance in yeast.

摘要

多药耐药性最常见的起源之一是通过ATP结合盒(ABC)转运蛋白的过量产生。这些ABC转运蛋白随后充当广泛特异性的药物泵,将多种有毒物质排出细胞。酿酒酵母通常通过过量产生一种名为Pdr5p的质膜定位ABC转运蛋白,表现出多重或多效性耐药(Pdr)。PDR5基因的表达由两个含锌簇的转录因子Pdr1p和Pdr3p控制。缺乏线粒体基因组的细胞(ρ(0)细胞)以Pdr3p依赖的方式强烈诱导PDR5转录。为了鉴定与Pdr3p相关的可能调节该因子的蛋白质,将串联亲和纯化(TAP)部分与Pdr3p融合,并从酵母细胞中纯化该重组蛋白。胞质Hsp70伴侣蛋白Ssa1p与TAP-Pdr3p共纯化。Ssa1p的过表达抑制了PDR5的表达,但对参与Pdr表型的其他基因的表达没有影响。这种Ssa1p介导的抑制需要Pdr3p的存在,并且不影响Pdr1p依赖的基因表达。核苷酸交换因子Fes1p的缺失模拟了Ssa1p介导的对PDR5的抑制。免疫共沉淀实验表明,在酵母细胞中Ssa1p与Pdr3p相关,但与Pdr1p不相关。最后,ρ(0)细胞中与Pdr3p结合的Ssa1p比ρ(+)细胞少,这与Ssa1p介导的对Pdr3p活性的抑制作为酵母多药耐药性控制中的关键调节步骤一致。

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