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首页> 外文期刊>Molecular and Cellular Biology >Characterization and purification of H1TF2, a novel CCAAT-binding protein that interacts with a histone H1 subtype-specific consensus element.
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Characterization and purification of H1TF2, a novel CCAAT-binding protein that interacts with a histone H1 subtype-specific consensus element.

机译:H1TF2的表征和纯化,H1TF2是一种新型CCAAT结合蛋白,可与组蛋白H1亚型特异性共有元件相互作用。

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Definition of mechanisms regulating human histone H1 gene transcription during the cell cycle requires the isolation and biochemical characterization of protein factors which interact with specific promoter elements. Two distinct binding activities have been identified in nuclear extracts from HeLa cells and mapped within a 180-base-pair (bp) region of a cell cycle-regulated H1 gene promoter. H1TF1 bound to an H1-specific A + C-rich sequence (AC box), 100 bp upstream of the cap site; H1TF2 interacted with the H1 subtype-specific consensus element and was dependent on the presence of an intact CCAAT box for binding. H1TF2 was purified through a combination of ion-exchange and oligonucleotide affinity chromatographies. Analysis of purified fractions by sodium dodecyl sulfate-polyacrylamide gel electrophoresis and UV crosslinking showed that H1TF2 was a single polypeptide of 47 kilodaltons. This factor was distinct from previously characterized CCAAT-binding proteins in both molecular size and binding properties. Fractions containing H1TF2 activity activated transcription in vitro only if programmed with an H1 DNA template carrying an intact H1TF2-binding site.
机译:定义在细胞周期中调节人组蛋白H1基因转录的机制,要求对与特定启动子元件相互作用的蛋白质因子进行分离和生化表征。在HeLa细胞的核提取物中已鉴定出两种不同的结合活性,并在细胞周期调节的H1基因启动子的180个碱基对(bp)区域内定位。 H1TF1与一个富含H1的富含A + C的序列(AC盒)结合,位于帽位点上游100 bp; H1TF2与H1亚型特异性共有元件相互作用,并且依赖于完整的CCAAT框进行结合。 H1TF2通过离子交换和寡核苷酸亲和层析相结合纯化。通过十二烷基硫酸钠-聚丙烯酰胺凝胶电泳和UV交联分析纯化的级分显示​​,H1TF2是一个47道尔顿的单一多肽。该因子在分子大小和结合特性上不同于先前表征的CCAAT结合蛋白。仅当使用带有完整H1TF2结合位点的H1 DNA模板编程时,含有H1TF2活性的级分才能在体外激活转录。

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