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单链抗体片段M6P-1具有一个6-磷酸甘露糖单糖特异性结合口袋,该口袋以分支特异性方式区分N-聚糖磷酸化†。

Single-chain antibody-fragment M6P-1 possesses a mannose 6-phosphate monosaccharide-specific binding pocket that distinguishes N-glycan phosphorylation in a branch-specific manner†.

作者信息

Blackler Ryan J, Evans Dylan W, Smith David F, Cummings Richard D, Brooks Cory L, Braulke Thomas, Liu Xinyu, Evans Stephen V, Müller-Loennies Sven

机构信息

Department of Biochemistry and Microbiology, University of Victoria, Victoria, BC Canada V8P 3P6.

Department of Biochemistry, National Center for Functional Glycomics, Emory University School of Medicine, Atlanta, GA 30322, USA.

出版信息

Glycobiology. 2016 Feb;26(2):181-92. doi: 10.1093/glycob/cwv093. Epub 2015 Oct 26.

DOI:10.1093/glycob/cwv093
PMID:26503547
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC4691289/
Abstract

The acquisition of mannose 6-phosphate (Man6P) on N-linked glycans of lysosomal enzymes is a structural requirement for their transport from the Golgi apparatus to lysosomes mediated by the mannose 6-phosphate receptors, 300 kDa cation-independent mannose 6-phosphate receptor (MPR300) and 46 kDa cation-dependent mannose 6-phosphate receptor (MPR46). Here we report that the single-chain variable domain (scFv) M6P-1 is a unique antibody fragment with specificity for Man6P monosaccharide that, through an array-screening approach against a number of phosphorylated N-glycans, is shown to bind mono- and diphosphorylated Man6 and Man7 glycans that contain terminal αMan6P(1 → 2)αMan(1 → 3)αMan. In contrast to MPR300, scFv M6P-1 does not bind phosphodiesters, monophosphorylated Man8 or mono- or diphosphorylated Man9 structures. Single crystal X-ray diffraction analysis to 2.7 Å resolution of Fv M6P-1 in complex with Man6P reveals that specificity and affinity is achieved via multiple hydrogen bonds to the mannose ring and two salt bridges to the phosphate moiety. In common with both MPRs, loss of binding was observed for scFv M6P-1 at pH values below the second pKa of Man6P (pKa = 6.1). The structures of Fv M6P-1 and the MPRs suggest that the change of the ionization state of Man6P is the main driving force for the loss of binding at acidic lysosomal pH (e.g. lysosome pH ∼ 4.6), which provides justification for the evolution of a lysosomal enzyme transport pathway based on Man6P recognition.

摘要

溶酶体酶的N - 连接聚糖上获得甘露糖6 - 磷酸(Man6P)是其通过甘露糖6 - 磷酸受体(300 kDa阳离子非依赖性甘露糖6 - 磷酸受体(MPR300)和46 kDa阳离子依赖性甘露糖6 - 磷酸受体(MPR46))从高尔基体转运至溶酶体的结构要求。在此我们报告,单链可变结构域(scFv)M6P - 1是一种对Man6P单糖具有特异性的独特抗体片段,通过针对多种磷酸化N - 聚糖的阵列筛选方法,显示其能结合含有末端αMan6P(1→2)αMan(1→3)αMan的单磷酸化和双磷酸化的Man6和Man7聚糖。与MPR300不同,scFv M6P - 1不结合磷酸二酯、单磷酸化的Man8或单磷酸化或双磷酸化的Man9结构。对与Man6P复合的Fv M6P - 1进行分辨率为2.7 Å的单晶X射线衍射分析表明,特异性和亲和力是通过与甘露糖环形成多个氢键以及与磷酸部分形成两个盐桥来实现的。与两种MPR一样,在pH值低于Man6P的第二个pKa(pKa = 6.1)时,观察到scFv M6P - 1的结合丧失。Fv M6P - 1和MPR的结构表明,Man6P电离状态的变化是在酸性溶酶体pH值(例如溶酶体pH ∼ 4.6)下结合丧失的主要驱动力,这为基于Man6P识别的溶酶体酶转运途径的进化提供了依据。

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