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首页> 外文期刊>Proteins: Structure, Function, and Genetics >Solution structure of the Pseudomonas putida protein PpPutA45 and its DNA complex.
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Solution structure of the Pseudomonas putida protein PpPutA45 and its DNA complex.

机译:恶臭假单胞菌蛋白PpPutA45及其DNA复合物的溶液结构。

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Proline utilization A (PutA) is a membrane-associated multifunctional enzyme that catalyzes the oxidation of proline to glutamate in a two-step process. In certain, gram-negative bacteria such as Pseudomonas putida, PutA also acts as an auto repressor in the cytoplasm, when an insufficient concentration of proline is available. Here, the N-terminal residues 1-45 of PutA from P. putida (PpPutA45) are shown to be responsible for DNA binding and dimerization. The solution structure of PpPutA45 was determined using NMR methods, where the protein is shown to be a symmetrical homodimer (12 kDa) consisting of two ribbon-helix-helix (RHH) structures. DNA sequence recognition by PpPutA45 was determined using DNA gel mobility shift assays and NMR chemical shift perturbations (CSPs). PpPutA45 was shown to bind a 14 base-pair DNA oligomer (5'-GCGGTTGCACCTTT-3'). A model of the PpPutA45-DNA oligomer complex was generated using Haddock 2.1. The antiparallel beta-sheet that results from PpPutA45 dimerization serves as the DNA recognition binding site by inserting into the DNA major groove. The dimeric core of four alpha-helices provides a structural scaffold for the beta-sheet from which residues Thr5, Gly7, and Lys9 make sequence-specific contacts with the DNA. The structural model implies flexibility of Lys9 which can make hydrogen bond contacts with either guanine or thymine. The high sequence and structure conservation of the PutA RHH domain suggest interdomain interactions play an important role in the evolution of the protein.
机译:脯氨酸利用A(PutA)是一种与膜相关的多功能酶,可在两步过程中催化脯氨酸氧化为谷氨酸。在某些革兰氏阴性细菌中,例如脯氨酸假单胞菌(Pseudomonas putida),PutA在脯氨酸浓度不足时也可作为细胞质中的自动阻遏物。在这里,来自恶臭假单胞菌(PpPutA45)的PutA的N-末端残基1-45显示出负责DNA结合和二聚化。 PpPutA45的溶液结构使用NMR方法确定,其中蛋白质显示为对称的同源二聚体(12 kDa),由两个带状螺旋-螺旋(RHH)结构组成。使用DNA凝胶迁移率位移测定法和NMR化学位移扰动(CSP)确定了PpPutA45对DNA序列的识别。显示PpPutA45结合14个碱基对的DNA寡聚物(5'-GCGGTTGCACCTTT-3')。使用Haddock 2.1生成PpPutA45-DNA寡聚物复合物的模型。由PpPutA45二聚化产生的反平行β-折叠通过插入DNA大槽而成为DNA识别结合位点。四个α-螺旋的二聚体核心为β-折叠提供了结构支架,残基Thr5,Gly7和Lys9与之形成了与DNA的序列特异性接触。结构模型暗示Lys9的柔韧性,可以使氢键与鸟嘌呤或胸腺嘧啶发生接触。 PutA RHH域的高序列和结构保守性表明域间相互作用在蛋白质的进化中起重要作用。

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