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一种含TBP的多蛋白复合物(TIF-IB)介导小鼠RNA聚合酶I的转录特异性。

A TBP-containing multiprotein complex (TIF-IB) mediates transcription specificity of murine RNA polymerase I.

作者信息

Eberhard D, Tora L, Egly J M, Grummt I

机构信息

Institute of Cell and Tumor Biology, German Cancer Research Center, Heidelberg.

出版信息

Nucleic Acids Res. 1993 Sep 11;21(18):4180-6. doi: 10.1093/nar/21.18.4180.

Abstract

TIF-IB is a transcription factor which interacts with the mouse ribosomal gene promoter and nucleates the formation of an initiation complex containing RNA polymerase I (Pol I). We have purified this factor to near homogeneity and demonstrate that TIF-IB is a large complex (< 200 kDa) which contains several polypeptides. One of the subunits present in this protein complex is the TATA-binding protein (TBP) as revealed by copurification of TIF-IB activity and TBP over different chromatographic steps including immunoaffinity purification. In addition to TBP, three tightly associated proteins (TAFs-I) with apparent molecular weights of 95, 68, and 48 kDa are contained in this multimeric complex. This subunit composition is similar--but not identical--to the analogous human factor SL1. Depletion of TBP from TIF-IB-containing fractions by immunoprecipitation eliminates TIF-IB activity. Neither TBP alone nor fractions containing other TBP complexes are capable of substituting for TIF-IB activity. Therefore, TIF-IB is a unique complex with Pol I-specific TAFs distinct from other TBP-containing complexes. The identification of TBP as an integral part of the murine rDNA promoter-specific transcription initiation factor extends the previously noted similarity of transcriptional initiation by the three nuclear RNA polymerases and underscores the importance of TAFs in determining promoter specificity.

摘要

TIF-IB是一种转录因子,它与小鼠核糖体基因启动子相互作用,并促使包含RNA聚合酶I(Pol I)的起始复合物形成。我们已将该因子纯化至接近均一状态,并证明TIF-IB是一种大型复合物(<200 kDa),包含几种多肽。通过在包括免疫亲和纯化在内的不同色谱步骤中对TIF-IB活性和TBP进行共纯化,发现该蛋白质复合物中存在的一个亚基是TATA结合蛋白(TBP)。除了TBP之外,这个多聚体复合物还包含三种紧密相关的蛋白质(TAFs-I),其表观分子量分别为95、68和48 kDa。这种亚基组成与类似的人类因子SL1相似但并不相同。通过免疫沉淀从含TIF-IB的组分中去除TBP会消除TIF-IB活性。单独的TBP或含有其他TBP复合物的组分都不能替代TIF-IB活性。因此,TIF-IB是一种独特的复合物,其具有与其他含TBP复合物不同的Pol I特异性TAFs。将TBP鉴定为小鼠rDNA启动子特异性转录起始因子的一个组成部分,扩展了先前指出的三种核RNA聚合酶转录起始的相似性,并强调了TAFs在确定启动子特异性中的重要性。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/92c4/310047/424147f5cdb3/nar00067-0035-a.jpg

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