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Nontranscribed spacer sequences promote in vitro transcription of Drosophila ribosomal DNA.

机译:非转录间隔子序列促进果蝇核糖体DNA的体外转录。

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摘要

Tandem repeats of ribosomal RNA transcription units in Drosophila melanogaster are separated by a nontranscribed spacer that is comprised in part of serial repeats of a 0.24 kb sequence. DNA sequence analysis shows that such repeats are imperfect copies of a region that includes the site of in vivo rRNA transcription initiation (ca. -240 to +30). Subclones of the rDNA spacer that are copies of the sequence extending from -34 through the initiation site support detectable in vitro transcription in a mixture involving a Drosophila cell-free extract, but accurate in vitro transcription is considerably enhanced when a nontranscribed spacer template includes a copy of the sequence extending upstream of -34. From a comparison of the sequences and transcription template-effectiveness of various rDNA subclones, we infer that a major promoter of RNA polymerase I activity lies between -150 and -30 in the rDNA nontranscribed spacer. The nontranscribed spacer copies of the initiation region are less effective templates for transcription than is the region of in vivo initiation, and there are differences between spacer repeats and the authentic sequence downstream of -240 that may account for this.
机译:果蝇中核糖体RNA转录单位的串联重复被一个非转录间隔区分开,该间隔区包含在0.24 kb序列的部分重复序列中。 DNA序列分析表明,此类重复序列是包含体内rRNA转录起始位点(约-240至+30)的区域的不完整拷贝。 rDNA间隔子的亚克隆是从-34延伸到起始位点的序列的拷贝,可支持在涉及果蝇无细胞提取物的混合物中检测到体外转录,但当非转录间隔子模板包含在-34上游延伸的序列的副本。从各种rDNA亚克隆的序列和转录模板有效性的比较,我们推断RNA聚合酶I活性的主要启动子位于rDNA非转录间隔区的-150和-30之间。起始区域的非转录间隔子拷贝比体内起始区域的转录模板效率低,间隔子重复序列与-240下游的真实序列之间存在差异,这可能是其原因。

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