首页> 美国卫生研究院文献>Acta Crystallographica Section F: Structural Biology and Crystallization Communications >Expression purification crystallization and preliminary X-ray analysis of CttA a putative cellulose-binding protein from Ruminococcus flavefaciens
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Expression purification crystallization and preliminary X-ray analysis of CttA a putative cellulose-binding protein from Ruminococcus flavefaciens

机译:CttA的表达纯化结晶和初步X射线分析CttA是黄褐球菌的推定纤维素结合蛋白

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摘要

A number of anaerobic microorganisms produce multi-modular, multi-enzyme complexes termed cellulosomes. These extracellular macromolecular nano­machines are designed for the efficient degradation of plant cell-wall carbohydrates to smaller sugars that are subsequently used as a source of carbon and energy. Cellulolytic strains from the rumens of mammals, such as Ruminococcus flavefaciens, have been shown to have one of the most complex cellulosomal systems known. Cellulosome assembly requires the binding of dockerin modules located in cellulosomal enzymes to cohesin modules located in a macromolecular scaffolding protein. Over 220 genes encoding dockerin-containing proteins have been identified in the R. flavefaciens genome. The dockerin-containing enzymes can be incorporated into the primary scaffoldin (ScaA), which in turn can bind to adaptor scaffoldins (ScaB or ScaC) and subsequently to anchoring scaffoldin (ScaE), thereby attaching the whole complex to the cell surface. However, unlike other cellulosomes such as that from Clostridium thermocellum, the Ruminococcus species lack a specific carbohydrate-binding module (CBM) on ScaA which recruits the entire complex onto the surface of the substrate. Instead, a cellulose-binding protein, CttA, comprising two putative tandem novel carbohydrate-binding modules and a C-terminal X-dockerin module, which can bind to the cohesin of ScaE, may mediate the attachment of bacterial cells to cellulose. Here, the expression, purification and crystallization of the carbohydrate-binding modular part of the CttA from R. flavefaciens are described. X-ray data have been collected to resolutions of 3.23 and to 1.61 Å in space groups P3121 or P3221 and P21, respectively. The structure was phased using bound iodide from the crystallization buffer by SAD experiments.
机译:许多厌氧微生物产生称为纤维素体的多模块,多酶复合物。这些细胞外大分子纳米机器被设计用于将植物细胞壁碳水化合物有效降解为较小的糖,随后将其用作碳和能量的来源。来自哺乳动物瘤胃的纤维素分解菌株,例如黄褐球菌(Ruminococcus flavefaciens),已被证明具有已知最复杂的纤维素系统之一。纤维素组装需要将位于纤维素酶中的dockerin模块与位于大分子支架蛋白中的cohesin模块结合。在黄曲霉基因组中已鉴定出220多个编码包含dockerin的蛋白质的基因。可以将包含dockerin的酶掺入一级支架蛋白(ScaA)中,然后依次与衔接子支架蛋白(ScaB或ScaC)结合并随后锚定支架蛋白(ScaE),从而将整个复合物附着到细胞表面。但是,与其他纤维素酶(如来自热纤梭菌的纤维素酶)不同,鲁米诺球菌菌种在ScaA上缺少特定的碳水化合物结合模块(CBM),该模块将整个复合物募集到基质表面上。取而代之的是,包含两个推定的新型糖结合模块和一个C端X-dockerin模块的纤维素结合蛋白CttA,可以结合ScaE的粘着蛋白,可以介导细菌细胞与纤维素的附着。在此,描述了黄曲霉中CttA的碳水化合物结合模块部分的表达,纯化和结晶。在空间群P3121或P3221和P21中,分别收集到的X射线数据的分辨率为3.23和1.61Å。通过SAD实验,使用结晶缓冲液中结合的碘化物对结构进行定相。

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