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金属反应元件结合转录因子-1的DNA结合活性在体内和体外均被锌激活,而非其他过渡金属。

The DNA binding activity of metal response element-binding transcription factor-1 is activated in vivo and in vitro by zinc, but not by other transition metals.

作者信息

Bittel D, Dalton T, Samson S L, Gedamu L, Andrews G K

机构信息

Department of Biochemistry and Molecular Biology, University of Kansas Medical Center, Kansas City, Kansas 66160-7421, USA.

出版信息

J Biol Chem. 1998 Mar 20;273(12):7127-33. doi: 10.1074/jbc.273.12.7127.

Abstract

We examined the DNA binding activity of mouse and human MTF-1 in whole cell extracts from cells cultured in medium containing zinc or cadmium and from untreated cells after the in vitro addition of zinc or cadmium, as well as using recombinant MTF-1 transcribed and translated in vitro and treated with various transition metals. Incubation of human (HeLa) or mouse (Hepa) cells in medium containing cadmium (5-15 microM) did not lead to a significant increase (<2-fold) in the amount of MTF-1 DNA binding activity, whereas zinc (100 microM) led to a 6-15-fold increase within 1 h. MTF-1 binding activity was low, but detectable, in control whole cell extracts and was increased (>10-fold) after the in vitro addition of zinc (30 microM) and incubation at 37 degrees C for 15 min. In contrast, addition of cadmium (6 or 60 microM) did not activate MTF-1 binding activity. Recombinant mouse and human MTF-1 were also dependent on exogenous zinc for DNA binding activity. Cadmium did not facilitate activation of recombinant MTF-1, but instead inhibited the activation of the recombinant protein by zinc. Interestingly, glutathione (1 mM) protected recombinant MTF-1 from inactivation by cadmium, and allowed for activation by zinc. It was also noted that zinc-activated recombinant MTF-1 was protected from cadmium only when bound to DNA. These results suggest that cadmium interacts with the zinc fingers of MTF-1 and forms an inactive complex. Of the several transition metals (zinc, cadmium, nickel, silver, copper, and cobalt) examined, only zinc facilitated activation of the DNA binding activity of recombinant MTF-1. These data suggest that transition metals, other than zinc, that activate MT gene expression may do so by mechanisms independent of an increase in the DNA binding activity of MTF-1.

摘要

我们检测了小鼠和人类金属反应转录因子-1(MTF-1)的DNA结合活性,检测对象包括在含锌或镉的培养基中培养的细胞的全细胞提取物、体外添加锌或镉后未经处理的细胞的全细胞提取物,以及体外转录和翻译并用各种过渡金属处理的重组MTF-1。在含镉(5 - 15微摩尔)的培养基中培养人(HeLa)或小鼠(Hepa)细胞,MTF-1的DNA结合活性量没有显著增加(<2倍),而锌(100微摩尔)在1小时内导致其增加6 - 15倍。在对照全细胞提取物中,MTF-1的结合活性较低但可检测到,体外添加锌(30微摩尔)并在37℃孵育15分钟后,其活性增加(>10倍)。相反,添加镉(6或60微摩尔)并未激活MTF-1的结合活性。重组小鼠和人类MTF-1的DNA结合活性也依赖于外源锌。镉不会促进重组MTF-1的激活,反而会抑制锌对重组蛋白的激活。有趣的是,谷胱甘肽(1毫摩尔)可保护重组MTF-1不被镉失活,并使其能够被锌激活。还注意到,只有当锌激活的重组MTF-1与DNA结合时,才会受到镉的保护。这些结果表明,镉与MTF-1的锌指相互作用并形成无活性复合物。在所检测的几种过渡金属(锌、镉、镍、银、铜和钴)中,只有锌促进重组MTF-1的DNA结合活性的激活。这些数据表明,除锌以外的激活金属硫蛋白(MT)基因表达的过渡金属,可能通过与MTF-1的DNA结合活性增加无关的机制来实现。

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