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Genes Encoding Cher-TPR Fusion Proteins Are Predominantly Found in Gene Clusters Encoding Chemosensory Pathways with Alternative Cellular Functions

机译:编码雪儿-TpR融合蛋白的基因主要是发现在基因簇编码化学感受途径与替代细胞功能

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摘要

Chemosensory pathways correspond to major signal transduction mechanisms and can be classified into the functional families flagellum-mediated taxis, type four pili-mediated taxis or pathways with alternative cellular functions (ACF). CheR methyltransferases are core enzymes in all of these families. CheR proteins fused to tetratricopeptide repeat (TPR) domains have been reported and we present an analysis of this uncharacterized family. We show that CheR-TPRs are widely distributed in GRAM-negative but almost absent from GRAM-positive bacteria. Most strains contain a single CheR-TPR and its abundance does not correlate with the number of chemoreceptors. The TPR domain fused to CheR is comparatively short and frequently composed of 2 repeats. The majority of CheR-TPR genes were found in gene clusters that harbor multidomain response regulators in which the REC domain is fused to different output domains like HK, GGDEF, EAL, HPT, AAA, PAS, GAF, additional REC, HTH, phosphatase or combinations thereof. The response regulator architectures coincide with those reported for the ACF family of pathways. Since the presence of multidomain response regulators is a distinctive feature of this pathway family, we conclude that CheR-TPR proteins form part of ACF type pathways. The diversity of response regulator output domains suggests that the ACF pathways form a superfamily which regroups many different regulatory mechanisms, in which all CheR-TPR proteins appear to participate. In the second part we characterize WspC of Pseudomonas putida, a representative example of CheR-TPR. The affinities of WspC-Pp for S-adenosylmethionine and S-adenosylhomocysteine were comparable to those of prototypal CheR, indicating that WspC-Pp activity is in analogy to prototypal CheRs controlled by product feed-back inhibition. The removal of the TPR domain did not impact significantly on the binding constants and consequently not on the product feed-back inhibition. WspC-Pp was found to be monomeric, which rules out a role of the TPR domain in self-association.
机译:化学感觉途径对应于主要的信号转导机制,可以分为鞭毛介导的滑行,四菌毛介导的滑行或具有替代细胞功能(ACF)的功能家族。 CheR甲基转移酶是所有这些家族中的核心酶。已经报道了融合到四肽重复序列(TPR)域的CheR蛋白,并且我们对该家族进行了分析。我们显示,CheR-TPRs广泛分布于GRAM阴性,但GRAM阳性细菌几乎不存在。大多数菌株仅包含一个CheR-TPR,其丰度与化学感受器的数量无关。与CheR融合的TPR结构域相对较短,通常由2个重复序列组成。大多数CheR-TPR基因位于带有多域响应调节因子的基因簇中,其中REC域融合到不同的输出域,例如HK,GGDEF,EAL,HPT,AAA,PAS,GAF,其他REC,HTH,磷酸酶或其组合。响应调节器架构与ACF通路家族报道的架构一致。由于多域响应调节剂的存在是该途径家族的独特特征,因此我们得出结论,CheR-TPR蛋白形成ACF类型途径的一部分。响应调节器输出域的多样性表明,ACF途径形成了一个超家族,该家族重新组合了许多不同的调节机制,所有CheR-TPR蛋白似乎都参与其中。在第二部分中,我们表征恶臭假单胞菌的WspC,这是CheR-TPR的代表性例子。 WspC-Pp对S-腺苷甲硫氨酸和S-腺苷同型半胱氨酸的亲和力与原型CheR的亲和力相当,表明WspC-Pp活性类似于受产品反馈抑制控制的原型CheRs。 TPR结构域的去除对结合常数没有显着影响,因此对产物的反馈抑制没有影响。 WspC-Pp被发现是单体的,这排除了TPR域在自我缔合中的作用。

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