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Transcription factor IIIB generates extended DNA interactions in RNA polymerase III transcription complexes on tRNA genes.

机译:转录因子IIIB在tRNA基因的RNA聚合酶III转录复合物中产生扩展的DNA相互作用。

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摘要

Transcription complexes that assemble on tRNA genes in a crude Saccharomyces cerevisiae cell extract extend over the entire transcription unit and approximately 40 base pairs of contiguous 5'-flanking DNA. We show here that the interaction with 5'-flanking DNA is due to a protein that copurifies with transcription factor TFIIIB through several steps of purification and shares characteristic properties that are normally ascribed to TFIIIB: dependence on prior binding of TFIIIC and great stability once the TFIIIC-TFIIIB-DNA complex is formed. SUP4 gene (tRNATyr) DNA that was cut within the 5'-flanking sequence (either 31 or 28 base pairs upstream of the transcriptional start site) was no longer able to stably incorporate TFIIIB into a transcription complex. The TFIIIB-dependent 5'-flanking DNA protein interaction was predominantly not sequence specific. The extension of the transcription complex into this DNA segment does suggest two possible explanations for highly diverse effects of flanking-sequence substitutions on tRNA gene transcription: either (i) proteins that are capable of binding to these upstream DNA segments are also potentially capable of stimulating or interfering with the incorporation of TFIIIB into transcription complexes or (ii) 5'-flanking sequence influences the rate of assembly of TFIIIB into stable transcription complexes.
机译:在粗制酿酒酵母细胞提取物中的tRNA基因上组装的转录复合物延伸到整个转录单位和大约40个碱基对的连续5'侧翼DNA。我们在这里显示与5'侧翼DNA的相互作用是由于蛋白质通过几个纯化步骤与转录因子TFIIIB共纯化,并共享通常归因于TFIIIB的特征:依赖TFIIIC的先前结合以及一旦形成TFIIIC-TFIIIB-DNA复合物。在5'侧翼序列(转录起始位点上游31或28个碱基对)内切割的SUP4基因(tRNATyr)DNA不再能够稳定地将TFIIIB整合到转录复合物中。依赖TFIIIB的5'-侧翼DNA蛋白相互作用主要不是序列特异性的。转录复合物延伸到该DNA片段中确实为侧翼序列取代对tRNA基因转录的高度多样化的影响提供了两种可能的解释:(i)能够与这些上游DNA片段结合的蛋白质也潜在地能够刺激或干扰TFIIIB掺入转录复合物中,或(ii)5'侧翼序列影响TFIIIB组装成稳定转录复合物的速率。

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