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Notch 表皮生长因子样(EGF)重复序列的位点特异性 O-糖基化:糖基化效率受单个 EGF 重复序列的正确折叠和氨基酸序列的影响。

Site-specific O-glucosylation of the epidermal growth factor-like (EGF) repeats of notch: efficiency of glycosylation is affected by proper folding and amino acid sequence of individual EGF repeats.

机构信息

Department of Biochemistry and Cell Biology, Institute of Cell and Developmental Biology, Stony Brook University, Stony Brook, New York 11794, USA.

出版信息

J Biol Chem. 2012 Oct 5;287(41):33934-44. doi: 10.1074/jbc.M112.401315. Epub 2012 Aug 7.

Abstract

O-Glucosylation of epidermal growth factor-like (EGF) repeats in the extracellular domain of Notch is essential for Notch function. O-Glucose can be elongated by xylose to the trisaccharide, Xylα1-3Xylα1-3Glcβ1-O-Ser, whose synthesis is catalyzed by the consecutive action of three glycosyltransferases. A UDP-glucose:protein O-glucosyltransferase (Poglut/Rumi) transfers O-glucose to serine within the O-glucose consensus. Subsequently, either of two UDP-xylose:glucoside xylosyltransferases (Gxylt1 or Gxylt2) transfers xylose to O-glucose. Finally, a UDP-xylose:xyloside xylosyltransferase (Xxylt1) transfers xylose to Xylα1-3Glcβ1-O-EGF. Our prior site-mapping studies demonstrated that O-glucose consensus sites are modified at high but variable stoichiometries in mouse Notch1 and identified a novel glycosylation site with alanine in place of proline, suggesting a revised, broader consensus sequence (CXSX(P/A)C). Here we examined the molecular basis for this site specificity. A panel of EGF repeats from human coagulation factor 9 (FA9), mouse Notch1, and Notch2 were bacterially expressed and purified by reverse phase HPLC for use in in vitro enzyme assays. We demonstrate that proper folding of EGF repeats is essential for glycosylation by Poglut/Rumi, that alanine can substitute for proline in the context of coagulation factor 9 EGF repeat for O-glucose transfer, confirming the new consensus sequence, and that positively charged residues within the O-glucose consensus sequence reduce efficiency of glycosylation by Poglut/Rumi. Moreover, proper folding of EGF repeats is also important for the activities of Gxylt1, Gxylt2, and Xxylt1. These results indicate that protein folding and amino acid sequences of individual EGF repeats fundamentally affect both attachment and elongation of O-glucose glycans.

摘要

表皮生长因子样(EGF)重复序列在 Notch 细胞外域的 O-连接糖基化对于 Notch 功能至关重要。O-葡萄糖可以通过木糖延长为三糖,Xylα1-3Xylα1-3Glcβ1-O-Ser,其合成由三个糖基转移酶的连续作用催化。UDP-葡萄糖:蛋白 O-葡萄糖基转移酶(Poglut/Rumi)将 O-葡萄糖转移到 O-葡萄糖共识中的丝氨酸。随后,两种 UDP-木糖:糖苷木糖基转移酶(Gxylt1 或 Gxylt2)中的一种将木糖转移到 O-葡萄糖。最后,UDP-木糖:木糖苷木糖基转移酶(Xxylt1)将木糖转移到 Xylα1-3Glcβ1-O-EGF。我们之前的位点映射研究表明,在小鼠 Notch1 中,O-葡萄糖共识位点以高但可变的化学计量比修饰,并鉴定了一个带有丙氨酸取代脯氨酸的新型糖基化位点,提示了一个经过修订的、更广泛的共识序列(CXSX(P/A)C)。在这里,我们研究了这种位点特异性的分子基础。一组来自人凝血因子 9(FA9)、小鼠 Notch1 和 Notch2 的 EGF 重复序列通过反相 HPLC 表达和纯化,用于体外酶测定。我们证明 Poglut/Rumi 的糖基化需要 EGF 重复序列的正确折叠,凝血因子 9 EGF 重复序列中的丙氨酸可以替代脯氨酸进行 O-葡萄糖转移,从而确认新的共识序列,并且 O-葡萄糖共识序列中的正电荷残基降低 Poglut/Rumi 的糖基化效率。此外,EGF 重复序列的正确折叠对于 Gxylt1、Gxylt2 和 Xxylt1 的活性也很重要。这些结果表明,蛋白质折叠和单个 EGF 重复序列的氨基酸序列从根本上影响 O-葡萄糖聚糖的附着和延伸。

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