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泛醌。醌环及其类异戊二烯侧链的生物合成。细胞内定位。

Ubiquinone. Biosynthesis of quinone ring and its isoprenoid side chain. Intracellular localization.

作者信息

Szkopińska A

机构信息

Department of Lipid Biochemistry, Institute of Biochemistry and Biophysics, Polish Academy of Sciences, Warszawa.

出版信息

Acta Biochim Pol. 2000;47(2):469-80.

PMID:11051212
Abstract

Ubiquinone, known as coenzyme Q, was shown to be the part of the metabolic pathways by Crane et al. in 1957. Its function as a component of the mitochondrial respiratory chain is well established. However, ubiquinone has recently attracted increasing attention with regard to its function, in the reduced form, as an antioxidant. In ubiquinone synthesis the para-hydroxybenzoate ring (which is the derivative of tyrosine or phenylalanine) is condensed with a hydrophobic polyisoprenoid side chain, whose length varies from 6 to 10 isoprene units depending on the organism. para-Hydroxybenzoate (PHB) polyprenyltransferase that catalyzes the condensation of PHB with polyprenyl diphosphate has a broad substrate specificity. Most of the genes encoding (all-E)-prenyltransferases which synthesize polyisoprenoid chains, have been cloned. Their structure is either homo- or heterodimeric. Genes that encode prenyltransferases catalysing the transfer of the isoprenoid chain to para-hydroxybenzoate were also cloned in bacteria and yeast. To form ubiquinone, prenylated PHB undergoes several modifications such as hydroxylations, O-methylations, methylations and decarboxylation. In eukaryotes ubiquinones were found in the inner mitochondrial membrane and in other membranes such as the endoplasmic reticulum, Golgi vesicles, lysosomes and peroxisomes. Still, the subcellular site of their biosynthesis remains unclear. Considering the diversity of functions of ubiquinones, and their multistep biosynthesis, identification of factors regulating their cellular level remains an elusive task.

摘要

泛醌,即辅酶Q,于1957年被克兰等人证明是代谢途径的一部分。其作为线粒体呼吸链组成部分的功能已得到充分证实。然而,泛醌作为抗氧化剂的还原形式的功能最近受到了越来越多的关注。在泛醌合成过程中,对羟基苯甲酸环(酪氨酸或苯丙氨酸的衍生物)与一条疏水的聚异戊二烯侧链缩合,其长度根据生物体的不同从6到10个异戊二烯单元不等。催化对羟基苯甲酸与聚异戊二烯二磷酸缩合的对羟基苯甲酸(PHB)聚异戊二烯基转移酶具有广泛的底物特异性。大多数编码合成聚异戊二烯链的(全-E)异戊二烯基转移酶的基因已被克隆。它们的结构是同二聚体或异二聚体。编码催化异戊二烯链转移到对羟基苯甲酸的异戊二烯基转移酶的基因也已在细菌和酵母中克隆。为了形成泛醌,异戊二烯基化的PHB会经历多种修饰,如羟基化、O-甲基化、甲基化和脱羧反应。在真核生物中,泛醌存在于线粒体内膜以及其他膜结构中,如内质网、高尔基体小泡、溶酶体和过氧化物酶体。然而,其生物合成的亚细胞位点仍不清楚。考虑到泛醌功能的多样性及其多步骤生物合成过程,鉴定调节其细胞水平的因素仍然是一项艰巨的任务。

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