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通过修饰 R 环相互作用增强薄荷基焦磷酸合酶的特异性。

Enhanced specificity of mint geranyl pyrophosphate synthase by modifying the R-loop interactions.

机构信息

Institute of Biological Chemistry, Academia Sinica, Taipei 115, Taiwan.

出版信息

J Mol Biol. 2010 Dec 17;404(5):859-73. doi: 10.1016/j.jmb.2010.10.011. Epub 2010 Oct 19.

DOI:10.1016/j.jmb.2010.10.011
PMID:20965200
Abstract

Isoprenoids, most of them synthesized by prenyltransferases (PTSs), are a class of important biologically active compounds with diverse functions. The mint geranyl pyrophosphate synthase (GPPS) is a heterotetramer composed of two LSU·SSU (large/small subunit) dimers. In addition to C(10)-GPP, the enzyme also produces geranylgeranyl pyrophosphate (C(20)-GGPP) in vitro, probably because of the conserved active-site structures between the LSU of mint GPPS and the homodimeric GGPP synthase from mustard. By contrast, the SSU lacks the conserved aspartate-rich motifs for catalysis. A major active-site cavity loop in the LSU and other trans-type PTSs is replaced by the regulatory R-loop in the SSU. Only C(10)-GPP, but not C(20)-GGPP, was produced when intersubunit interactions of the R-loop were disrupted by either deletion or multiple point mutations. The structure of the deletion mutant, determined in two different crystal forms, shows an intact (LSU·SSU)(2) heterotetramer, as previously observed in the wild-type enzyme. The active-site of LSU remains largely unaltered, except being slightly more open to the bulk solvent. The R-loop of SSU acts by regulating the product release from LSU, just as does its equivalent loop in a homodimeric PTS, which prevents the early reaction intermediates from escaping the active site of the other subunit. In this way, the product-retaining function of R-loop provides a more stringent control for chain-length determination, complementary to the well-established molecular ruler mechanism. We conclude that the R-loop may be used not only to conserve the GPPS activity but also to produce portions of C(20)-GGPP in mint.

摘要

异戊二烯,其中大部分由 prenyltransferases (PTSs) 合成,是一类具有多种功能的重要生物活性化合物。薄荷基焦磷酸香叶基转移酶 (GPPS) 是由两个 LSU·SSU(大亚基/小亚基)二聚体组成的杂四聚体。除了 C(10)-GPP 外,该酶还在体外产生香叶基二磷酸 (C(20)-GGPP),这可能是由于薄荷 GPPS 的 LSU 与来自芥菜的同源二聚体 GGPP 合酶之间保守的活性位点结构所致。相比之下,SSU 缺乏催化所需的保守天冬氨酸丰富基序。在 LSU 和其他转位型 PTS 中的主要活性位点腔环被 SSU 中的调节 R 环取代。只有当 R 环的亚基间相互作用被缺失或多点突变破坏时,才会产生 C(10)-GPP,但不会产生 C(20)-GGPP。两种不同晶体形式测定的缺失突变体结构显示完整的 (LSU·SSU)(2) 杂四聚体,如先前在野生型酶中观察到的那样。LSU 的活性位点除了略微向大体积溶剂敞开外,基本上没有改变。SSU 的 R 环通过调节 LSU 中产物的释放起作用,就像在同源二聚体 PTS 中的等效环一样,防止早期反应中间体从另一个亚基的活性位点逸出。通过这种方式,R 环的产物保留功能为链长确定提供了更严格的控制,与已建立的分子标尺机制互补。我们得出结论,R 环不仅可用于保留 GPPS 活性,还可用于在薄荷中产生部分 C(20)-GGPP。

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