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人转录因子IIIA的纯化与特性分析

Purification and characterization of human transcription factor IIIA.

作者信息

Moorefield B, Roeder R G

机构信息

Laboratory of Biochemistry and Molecular Biology, Rockefeller University, New York, New York 10021.

出版信息

J Biol Chem. 1994 Aug 19;269(33):20857-65.

PMID:8063702
Abstract

The 5S gene-specific transcription factor, TFIIIA, was purified approximately 35,000-fold from HeLa cell extracts using a combination of conventional and affinity chromatographic methods. A single polypeptide of apparent molecular mass 42-kDa cofractionates with both 5S DNA binding and 5S transcription activities, and was conclusively identified as human TFIIIA by its ability to direct specific 5S gene transcription in vitro following elution and renaturation from SDS-polyacrylamide gels. The DNase I protection pattern of the purified human factor on a human 5S gene is similar to the pattern previously observed with Xenopus TFIIIA. A Xenopus 5S gene, but not a yeast 5S gene, is able to effectively compete for binding of the human factor. In addition, we report a previously undetected immunological cross-reactivity between human and Xenopus TFIIIA. hTFIIIA is recognized specifically both by polyclonal antisera raised against Xenopus laevis TFIIIA as well as by a monoclonal antibody generated against the amphibian protein. These observations indicate that human TFIIIA is structurally related to the Xenopus oocyte factor and that the previous inability to detect human TFIIIA by immunological methods is due primarily to the low abundance of this factor in HeLa cell extracts.

摘要

利用传统色谱法和亲和色谱法相结合的方法,从HeLa细胞提取物中纯化出5S基因特异性转录因子TFIIIA,纯化倍数约为35000倍。一条表观分子量为42 kDa的单一多肽与5S DNA结合活性和5S转录活性共分离,并通过其从SDS聚丙烯酰胺凝胶洗脱并复性后在体外指导特异性5S基因转录的能力,最终被确定为人类TFIIIA。纯化的人类因子对人类5S基因的DNase I保护模式与先前用非洲爪蟾TFIIIA观察到的模式相似。一个非洲爪蟾5S基因,而不是酵母5S基因,能够有效竞争人类因子的结合。此外,我们报道了人类和非洲爪蟾TFIIIA之间以前未检测到的免疫交叉反应性。hTFIIIA能被针对非洲爪蟾TFIIIA产生的多克隆抗血清以及针对该两栖类蛋白质产生的单克隆抗体特异性识别。这些观察结果表明,人类TFIIIA在结构上与非洲爪蟾卵母细胞因子相关,并且以前无法通过免疫方法检测到人类TFIIIA主要是由于该因子在HeLa细胞提取物中的丰度较低。

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