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A DNA-binding protein factor recognizes two binding domains within the octopine synthase enhancer element.

机译:DNA结合蛋白因子识别章鱼碱合酶增强子元件内的两个结合域。

摘要

A protein that binds to the enhancing element of the octopine synthase gene has been identified in nuclear extracts from maize cell suspension cultures. Two protein-DNA complexes are distinguishable by electrophoretic mobility in gel retardation assays. Footprint analyses of these low and high molecular weight complexes show, respectively, half and complete protection of the ocs-element DNA from cleavage by methidiumpropyl-EDTA.FE(II). Two lines of evidence indicate that the element has two recognition sites, each of which can bind identical protein units. Elements that are mutated in one or the other half and form only the low molecular weight complex interfere with the formation of both the low and high molecular weight complexes by the wild-type element. Protein isolated from a complex with only one binding site occupied can bind to the wild-type ocs-element and generate complexes with protein occupying one or both binding sites. Occupation of both sites of the ocs-element is a prerequisite for transcriptional enhancement.
机译:已经从玉米细胞悬浮培养物的核提取物中鉴定出与章鱼碱合酶基因的增强元件结合的蛋白质。在凝胶延迟测定中,电泳迁移率可区分两种蛋白质-DNA复合物。这些低分子量和高分子量复合物的足迹分析分别显示了ocs元素DNA的一半和完全保护不受甲基丙基EDTA.FE(II)的裂解的影响。有两条证据表明该元件具有两个识别位点,每个识别位点都可以结合相同的蛋白质单元。在一个或另一半中突变且仅形成低分子量复合物的元素会干扰野生型元素同时形成低分子量和高分子量复合物。从仅占据一个结合位点的复合物中分离出的蛋白质可以与野生型ocs元素结合,并生成具有占据一个或两个结合位点的蛋白质的复合物。占领ocs元素的两个位点是转录增强的先决条件。

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