BmFTZ-F1激活腹节基因转录的介质

Mediators of activation of fushi tarazu gene transcription by BmFTZ-F1.

作者信息

Li F Q, Ueda H, Hirose S

机构信息

Department of Genetics, Graduate University for Advanced Studies, Shizuoka-ken, Japan.

出版信息

Mol Cell Biol. 1994 May;14(5):3013-21. doi: 10.1128/mcb.14.5.3013-3021.1994.

DOI:10.1128/mcb.14.5.3013-3021.1994

PMID:8164657

原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC358669/

Abstract

Transcriptional activation by many eukaryotic sequence-specific regulators appears to be mediated through transcription factors which do not directly bind to DNA. BmFTZ-F1 is a silkworm counterpart of FTZ-F1, a sequence-specific activator of the fushi tarazu gene in Drosophila melanogaster. We report here the isolation of 18- and 22-kDa polypeptides termed MBF1 and MBF2, respectively, that form a heterodimer and mediate activation of in vitro transcription from the fushi tarazu promoter by BmFTZ-F1. Neither MBF1, MBF2, nor a combination of them binds to DNA. MBF1 interacts with BmFTZ-F1 and stabilizes the BmFTZ-F1-DNA complex. MBF1 also makes direct contact with TATA-binding protein (TBP). Both MBF1 and MBF2 are necessary to form a complex between BmFTZ-F1 and TBP. We propose a model in which MBF1 and MBF2 form a bridge between BmFTZ-F1 and TBP and mediate transactivation by stabilizing the protein-DNA interactions.

摘要

许多真核生物序列特异性调节因子的转录激活似乎是通过不直接与DNA结合的转录因子介导的。BmFTZ-F1是果蝇中fushi tarazu基因的序列特异性激活因子FTZ-F1的家蚕对应物。我们在此报告分别称为MBF1和MBF2的18 kDa和22 kDa多肽的分离，它们形成异二聚体并介导BmFTZ-F1对fushi tarazu启动子的体外转录激活。MBF1、MBF2及其组合均不与DNA结合。MBF1与BmFTZ-F1相互作用并稳定BmFTZ-F1-DNA复合物。MBF1还与TATA结合蛋白（TBP）直接接触。MBF1和MBF2都是在BmFTZ-F1和TBP之间形成复合物所必需的。我们提出了一个模型，其中MBF1和MBF2在BmFTZ-F1和TBP之间形成桥梁，并通过稳定蛋白质-DNA相互作用介导反式激活。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/2e74/358669/03844261bc1d/molcellb00005-0187-a.jpg

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BmFTZ-F1激活腹节基因转录的介质

Mediators of activation of fushi tarazu gene transcription by BmFTZ-F1.

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