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Oct蛋白对小鼠乳腺肿瘤病毒启动子基础转录的刺激作用。

Stimulation of basal transcription from the mouse mammary tumor virus promoter by Oct proteins.

作者信息

Kim M H, Peterson D O

机构信息

Department of Biochemistry and Biophysics, Texas A&M University, College Station 77843-2128, USA.

出版信息

J Virol. 1995 Aug;69(8):4717-26. doi: 10.1128/JVI.69.8.4717-4726.1995.

Abstract

The steroid hormone-inducible promoter of mouse mammary tumor virus (MMTV) contains three overlapping sequences related to the consensus octamer motif ATGCAAAT. Basal promoter activity in the absence of hormone induction from a template in which all three octamer elements were mutated was decreased by two-to threefold in in vitro transcription assays. Oct-1 protein purified from HeLa cell nuclear extracts, as well as recombinant Oct-1 expressed in bacteria, recognized MMTV octamer-related sequences, as shown by DNase I footprinting. Furthermore, rabbit polyclonal antiserum directed against recombinant Oct-1 completely inhibited the formation of specific complexes between MMTV octamer-related sequences and proteins present in nuclear extracts of HeLa cells, indicating that Oct-1 is the major protein in HeLa nuclear extracts that recognizes octamer-related sequences in the MMTV promoter. In addition, depletion of Oct-1 from the nuclear extract by using Oct-1-specific antiserum or a sequence-specific DNA affinity resin decreased in vitro transcription from the wild-type MMTV promoter to a level identical to that obtained from a promoter in which all three octamer-related sequences were mutated. Addition of purified HeLa Oct-1 or recombinant Oct-1 to the depleted extract selectively increased transcription from the wild-type relative to the mutated promoter, demonstrating that Oct-1 transcription factor stimulates basal transcription from the MMTV promoter. A similar effect was observed when purified recombinant Oct-2 was added to the Oct-1-depleted extract, suggesting that Oct-2 may play an important role in MMTV transcription in B cells.

摘要

小鼠乳腺肿瘤病毒(MMTV)的类固醇激素诱导型启动子包含三个与共有八聚体基序ATGCAAAT相关的重叠序列。在体外转录试验中,来自所有三个八聚体元件均发生突变的模板的无激素诱导下的基础启动子活性降低了两到三倍。从HeLa细胞核提取物中纯化的Oct-1蛋白,以及在细菌中表达的重组Oct-1,都能识别MMTV八聚体相关序列,这通过DNA酶I足迹分析得以证明。此外,针对重组Oct-1的兔多克隆抗血清完全抑制了MMTV八聚体相关序列与HeLa细胞核提取物中存在的蛋白质之间特异性复合物的形成,表明Oct-1是HeLa细胞核提取物中识别MMTV启动子中八聚体相关序列的主要蛋白质。此外,通过使用Oct-1特异性抗血清或序列特异性DNA亲和树脂从核提取物中去除Oct-1,可使野生型MMTV启动子的体外转录降低至与所有三个八聚体相关序列均发生突变的启动子相同的水平。向耗尽的提取物中添加纯化的HeLa Oct-1或重组Oct-1,相对于突变启动子,可选择性地增加野生型的转录,表明Oct-1转录因子刺激MMTV启动子的基础转录。当将纯化的重组Oct-2添加到Oct-1耗尽的提取物中时,观察到类似的效果,这表明Oct-2可能在B细胞的MMTV转录中起重要作用。

相似文献

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