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吸水链霉菌中雷帕霉素生物合成基因簇的组织:模块化聚酮合酶中酶结构域的分析

Organization of the biosynthetic gene cluster for rapamycin in Streptomyces hygroscopicus: analysis of the enzymatic domains in the modular polyketide synthase.

作者信息

Aparicio J F, Molnár I, Schwecke T, König A, Haydock S F, Khaw L E, Staunton J, Leadlay P F

机构信息

Cambridge Centre for Molecular Recognition, Department of Biochemistry, University of Cambridge, UK.

出版信息

Gene. 1996 Feb 22;169(1):9-16. doi: 10.1016/0378-1119(95)00800-4.

DOI:10.1016/0378-1119(95)00800-4
PMID:8635756
Abstract

The three giant multifunctional polypeptides of the rapamycin (Rp)-producing polyketide synthase (RAPS1, RAPS2 and RAPS3) have recently been shown to contain 14 separate sets, or modules, of enzyme activities, each module catalysing a specific round of polyketide chain extension. Detailed sequence comparison between these protein modules has allowed further characterisation of aa that may be important in catalysis or specificity. The acyl-carrier protein (ACP), beta-ketoacyl-ACP synthase (KS) and acyltransferase (AT) domains (the core domains) have an extremely high degree of mutual sequence homology. The KS domains in particular are almost perfect repeats over their entire length. Module 14 shows the least homology and is unique in possessing only core domains. The enoyl reductase (ER), beta-ketoacyl-ACP reductase (KR) and dehydratase (DH) domains are present even in certain modules where they are not apparently required. Four DH domains can be recognised as inactive by characteristic deletions in active site sequences, but for two others, and for KR and ER in module 3, the sequence is not distinguishable from that of active counterparts in other modules. The N terminus of RAPS1 contains a novel coenzyme A ligase (CL) domain that activates and attaches the shikimate-derived starter unit, and an ER activity that may modify the starter unit after attachment. The sequence comparison has revealed the surprisingly high sequence similarity between inter-domain 'linker' regions, and also a potential amphipathic helix at the N terminus of each multienzyme subunit which may promote dimerisation into active species.

摘要

最近研究表明,产生雷帕霉素(Rp)的聚酮合酶的三种巨大多功能多肽(RAPS1、RAPS2和RAPS3)含有14个独立的酶活性组,即模块,每个模块催化一轮特定的聚酮链延伸。这些蛋白质模块之间的详细序列比较使得能够进一步鉴定在催化或特异性方面可能重要的氨基酸。酰基载体蛋白(ACP)、β-酮酰基-ACP合酶(KS)和酰基转移酶(AT)结构域(核心结构域)具有极高的相互序列同源性。特别是KS结构域在其整个长度上几乎是完美的重复。模块14显示出最低的同源性,并且独特之处在于仅拥有核心结构域。烯酰还原酶(ER)、β-酮酰基-ACP还原酶(KR)和脱水酶(DH)结构域甚至存在于某些显然不需要它们的模块中。通过活性位点序列中的特征性缺失可以识别出四个DH结构域无活性,但对于另外两个结构域以及模块3中的KR和ER,其序列与其他模块中有活性的对应序列无法区分。RAPS1的N末端包含一个新型辅酶A连接酶(CL)结构域,该结构域激活并连接莽草酸衍生的起始单元,以及一种可能在连接后修饰起始单元的ER活性。序列比较揭示了结构域间“连接子”区域之间惊人的高序列相似性,并且在每个多酶亚基的N末端还存在一个潜在的两亲性螺旋,这可能促进二聚化形成活性物种。

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