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如何使两亲性分子穿过脂质双层:不同的ABC转运蛋白有不同的机制?

How to move an amphipathic molecule across a lipid bilayer: different mechanisms for different ABC transporters?

作者信息

Theodoulou Frederica L, Carrier David J, Schaedler Theresia A, Baldwin Stephen A, Baker Alison

机构信息

Biological Chemistry and Crop Protection Department, Rothamsted Research, Harpenden, AL5 2JQ, U.K.

Centre for Plant Sciences, School of Molecular and Cellular Biology, University of Leeds, Leeds LS2 9JT, U.K.

出版信息

Biochem Soc Trans. 2016 Jun 15;44(3):774-82. doi: 10.1042/BST20160040.

Abstract

Import of β-oxidation substrates into peroxisomes is mediated by ATP binding cassette (ABC) transporters belonging to subfamily D. In order to enter the β-oxidation pathway, fatty acids are activated by conversion to fatty acyl-CoA esters, a reaction which is catalysed by acyl-CoA synthetases (ACSs). Here, we present evidence for an unusual transport mechanism, in which fatty acyl-CoA substrates are accepted by ABC subclass D protein (ABCD) transporters, cleaved by the transporters during transit across the lipid bilayer to release CoA, and ultimately re-esterified in the peroxisome lumen by ACSs which interact with the transporter. We propose that this solves the biophysical problem of moving an amphipathic molecule across the peroxisomal membrane, since the intrinsic thioesterase activity of the transporter permits separate membrane translocation pathways for the hydrophobic fatty acid moiety and the polar CoA moiety. The cleavage/re-esterification mechanism also has the potential to control entry of disparate substrates into the β-oxidation pathway when coupled with distinct peroxisomal ACSs. A different solution to the movement of amphipathic molecules across a lipid bilayer is deployed by the bacterial lipid-linked oligosaccharide (LLO) flippase, PglK, in which the hydrophilic head group and the hydrophobic polyprenyl tail of the substrate are proposed to have distinct translocation pathways but are not chemically separated during transport. We discuss a speculative alternating access model for ABCD proteins based on the mammalian ABC transporter associated with antigen processing (TAP) and compare it to the novel mechanism suggested by the recent PglK crystal structures and biochemical data.

摘要

β-氧化底物进入过氧化物酶体是由属于D亚家族的ATP结合盒(ABC)转运蛋白介导的。为了进入β-氧化途径,脂肪酸通过转化为脂肪酰辅酶A酯而被激活,这一反应由酰基辅酶A合成酶(ACSs)催化。在此,我们提供了一种不同寻常的转运机制的证据,即脂肪酰辅酶A底物被ABC D亚类蛋白(ABCD)转运蛋白接受,在跨脂质双层转运过程中被转运蛋白切割以释放辅酶A,最终在过氧化物酶体腔中由与转运蛋白相互作用的ACSs重新酯化。我们认为,这解决了将两亲性分子转运过过氧化物酶体膜的生物物理问题,因为转运蛋白的内在硫酯酶活性允许疏水脂肪酸部分和极性辅酶A部分有独立的膜转运途径。当与不同的过氧化物酶体ACSs偶联时,切割/重新酯化机制也有可能控制不同底物进入β-氧化途径。细菌脂质连接寡糖(LLO)翻转酶PglK采用了一种不同的解决两亲性分子跨脂质双层转运的方法,其中底物的亲水头部基团和疏水聚异戊二烯尾部被认为有不同并的转运途径,但在转运过程中没有化学分离。我们基于与抗原加工相关的哺乳动物ABC转运蛋白(TAP)讨论了一种关于ABCD蛋白的推测性交替访问模型,并将其与最近PglK晶体结构和生化数据所提示新型机制进行比较。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/8c3e/4900756/7276a58952fe/bst0440774fig1.jpg

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