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来自酰胺水解酶超家族的错误注释脯氨酰二肽酶的功能鉴定。

Functional identification of incorrectly annotated prolidases from the amidohydrolase superfamily of enzymes.

作者信息

Xiang Dao Feng, Patskovsky Yury, Xu Chengfu, Meyer Amanda J, Sauder J Michael, Burley Stephen K, Almo Steven C, Raushel Frank M

机构信息

Department of Chemistry, Texas A&M University, P.O. Box 30012, College Station, Texas 77842-3012, USA.

出版信息

Biochemistry. 2009 May 5;48(17):3730-42. doi: 10.1021/bi900111q.

Abstract

The substrate profiles for two proteins from Caulobacter crescentus CB15 (Cc2672 and Cc3125) and one protein (Sgx9359b) derived from a DNA sequence ( gi|44368820 ) isolated from the Sargasso Sea were determined using combinatorial libraries of dipeptides and N-acyl derivatives of amino acids. These proteins are members of the amidohydrolase superfamily and are currently misannotated in NCBI as catalyzing the hydrolysis of l-Xaa-l-Pro dipeptides. Cc2672 was shown to catalyze the hydrolysis of l-Xaa-l-Arg/Lys dipeptides and the N-acetyl and N-formyl derivatives of lysine and arginine. This enzyme will also hydrolyze longer peptides that terminate in either lysine or arginine. The N-methyl phosphonate derivative of l-lysine was a potent competitive inhibitor of Cc2672 with a K(i) value of 120 nM. Cc3125 was shown to catalyze the hydrolysis of l-Xaa-l-Arg/Lys dipeptides but will not hydrolyze tripeptides or the N-formyl and N-acetyl derivatives of lysine or arginine. The substrate profile for Sgx9359b is similar to that of Cc2672 except that compounds with a C-terminal lysine are not recognized as substrates. The X-ray structure of Sgx9359b was determined to a resolution of 2.3 A. The protein folds as a (beta/alpha)(8)-barrel and self-associates to form a homooctamer. The active site is composed of a binuclear metal center similar to that found in phosphotriesterase and dihydroorotase. In one crystal form, arginine was bound adventitiously to the eight active sites within the octamer. The orientation of the arginine in the active site identified the structural determinants for recognition of the alpha-carboxylate and the positively charged side chains of arginine-containing substrates. This information was used to identify 18 other bacterial sequences that possess identical or similar substrate profiles.

摘要

利用二肽和氨基酸的N-酰基衍生物组合文库,测定了新月柄杆菌CB15的两种蛋白质(Cc2672和Cc3125)以及从马尾藻海分离的DNA序列(gi|44368820)衍生的一种蛋白质(Sgx9359b)的底物谱。这些蛋白质属于酰胺水解酶超家族,目前在NCBI中被错误注释为催化l-Xaa-l-Pro二肽的水解。研究表明,Cc2672催化l-Xaa-l-Arg/Lys二肽以及赖氨酸和精氨酸的N-乙酰和N-甲酰衍生物的水解。该酶还能水解以赖氨酸或精氨酸结尾的更长肽段。l-赖氨酸的N-甲基膦酸酯衍生物是Cc2672的有效竞争性抑制剂,K(i)值为120 nM。研究表明,Cc3125催化l-Xaa-l-Arg/Lys二肽的水解,但不能水解三肽或赖氨酸或精氨酸的N-甲酰和N-乙酰衍生物。Sgx9359b的底物谱与Cc2672相似,只是C端为赖氨酸的化合物不被识别为底物。Sgx9359b的X射线结构分辨率为2.3 Å。该蛋白质折叠成一个(beta/alpha)(8)桶状结构,并自缔合形成同源八聚体。活性位点由一个双核金属中心组成,类似于在磷酸三酯酶和二氢乳清酸酶中发现的中心。在一种晶体形式中,精氨酸偶然结合到八聚体内的八个活性位点上。精氨酸在活性位点中的取向确定了识别含精氨酸底物的α-羧酸盐和带正电荷侧链的结构决定因素。这些信息被用于识别其他18个具有相同或相似底物谱的细菌序列。

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