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首页> 外文期刊>Nucleic acids research >Identification of DNA-binding proteins that recognize a Conserved Type I repeat sequence in the replication origin region of Tetrahymena rDNA
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Identification of DNA-binding proteins that recognize a Conserved Type I repeat sequence in the replication origin region of Tetrahymena rDNA

机译:识别四膜虫rDNA复制起点区域中保守的I型重复序列的DNA结合蛋白的鉴定

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摘要

An origin of DNA replication has been mapped within the 5' non-transcribed spacer region of the amplified macronuclear rRNA genes (rDNA) of Tetrahymena thermophila. Mutations in 33 nt conserved AT-rich Type I repeat sequences located in the origin region cause defects in the replication and/or maintenance of amplified rDNA in vivo. Fe(ll)EDTA cleavage footprinting of restriction fragments containing the Type I repeat showed that most of the conserved nucleotides were protected by proteins in extracts of Tetrahymena cells. Two classes of proteins that bound the Type I repeat were identified and characterized using synthetic oligonucleotides in electrophoretic mobility shift assays. One of these, ds-TIBF, bound preferentially to duplex DNA and exhibited only moderate specificity for Type I repeat sequences. In contrast, a single-stranded DNA-binding protein, ssATIBF, specifically recognized the A-rich strand of the Type I repeat sequence. Deletion of the 5′ or 3′ borders of the conserved sequence significantly reduced binding of ssA-TIBF. The binding properties of ssATIBF, coupled with genetic evidence that Type I sequences function as c/s-acting rDNA replication control elements in vivo, suggest a possible role for ssA-TIBF in rDNA replication in Tetrahymena.
机译:DNA复制的起点已映射到嗜热四膜虫的扩增大核rRNA基因(rDNA)的5'非转录间隔区中。位于起始区的33nt保守的富含AT的I型重复序列的突变会导致体内扩增和rDNA复制和/或维持的缺陷。 Fe(II)EDTA切割含有I型重复序列的限制性片段的足迹表明,四膜虫细胞提取物中的大多数保守核苷酸均受到蛋白质的保护。在电泳迁移率迁移分析中使用合成的寡核苷酸鉴定并鉴定了结合I型重复序列的两类蛋白质。其中之一是ds-TIBF,它优先与双链DNA结合,并且对I型重复序列仅表现出中等的特异性。相反,单链DNA结合蛋白ssATIBF特别识别I型重复序列的富A链。保守序列的5'或3'边界的删除显着降低了ssA-TIBF的结合。 ssATIBF的结合特性,加上I型序列在体内起c / s作用的rDNA复制控制元件的遗传证据,提示ssA-TIBF在四膜虫的rDNA复制中可能发挥作用。

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