Structure and possible mechanism of the CcbJ methyltransferase fromStreptomyces caelestis

甲基转移酶 立体化学 活动站点 甲基化 对接(动物) 链霉菌 突变体 同色链霉菌 生物合成 化学 部分 生物化学 DNA 生物 细菌 基因 遗传学 医学 护理部
作者
Jacob Bauer,Gabriela Ondrovičová,Lucie Najmanová,Vladimír Pevala,Zdeněk Kameník,Július Košťan,Jiřı́ Janata,Eva Kutějová
出处
期刊:Acta Crystallographica Section D-biological Crystallography [Wiley]
卷期号:70 (4): 943-957 被引量:12
标识
DOI:10.1107/s139900471303397x
摘要

The S -adenosyl-L-methionine (SAM)-dependent methyltransferase CcbJ from Streptomyces caelestis catalyzes one of the final steps in the biosynthesis of the antibiotic celesticetin, methylation of the N atom of its proline moiety, which greatly enhances the activity of the antibiotic. Since several celesticetin variants exist, this enzyme may be able to act on a variety of substrates. The structures of CcbJ determined by MAD phasing at 3.0 Å resolution, its native form at 2.7 Å resolution and its complex with S -adenosyl-L-homocysteine (SAH) at 2.9 Å resolution are reported here. Based on these structures, three point mutants, Y9F, Y17F and F117G, were prepared in order to study its behaviour as well as docking simulations of both CcbJ–SAM–substrate and CcbJ–SAH–product complexes. The structures show that CcbJ is a class I SAM-dependent methyltransferase with a wide active site, thereby suggesting that it may accommodate a number of different substrates. The mutation results show that the Y9F and F117G mutants are almost non-functional, while the Y17F mutant has almost half of the wild-type activity. In combination with the docking studies, these results suggest that Tyr9 and Phe117 are likely to help to position the substrate for the methyl-transfer reaction and that Tyr9 may also facilitate the reaction by removing an H + ion. Tyr17, on the other hand, seems to operate by helping to stabilize the SAM cofactor.

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