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Bacterial polysaccharide lyase family 33: Specificity from an evolutionarily conserved binding tunnel

聚糖 糖苷键 劈开 裂解酶 底物特异性 生物化学 糖生物学 多糖 生物 多细胞生物 化学 基因 糖蛋白
作者
Mélanie Loiodice,Élodie Drula,Zak McIver,S.V. Antonyuk,Arnaud Baslé,Marcelo A. Lima,Edwin A. Yates,Dominic P. Byrne,Jamie Coughlan,Andrew Leech,Shahram Mesdaghi,Daniel J. Rigden,Sophie Drouillard,William Helbert,Bernard Henrissat,Nicolas Terrapon,Gareth S. A. Wright,Marie Couturier,Alan Cartmell
出处
期刊:Proceedings of the National Academy of Sciences of the United States of America [National Academy of Sciences]
卷期号:122 (7)
标识
DOI:10.1073/pnas.2421623122
摘要

Acidic glycans are essential for the biology of multicellular eukaryotes. To utilize them, microbial life including symbionts and pathogens has evolved polysaccharide lyases (PL) that cleave their 1,4 glycosidic linkages via a β-elimination mechanism. PL family 33 (PL33) enzymes have the unusual ability to target a diverse range of glycosaminoglycans (GAGs), as well as the bacterial polymer, gellan gum. In order to gain more detailed insight into PL33 activities we recombinantly expressed 10 PL33 members derived from all major environments and further elucidated the detailed biochemical and biophysical properties of five, showing that their substrate specificity is conferred by variations in tunnel length and topography. The key amino acids involved in catalysis and substrate interactions were identified, and employing a combination of complementary biochemical, structural, and modeling approaches, we show that the tunnel topography is induced by substrate binding to the glycan. Structural and bioinformatic analyses revealed that these features are conserved across several lyase families as well as in mammalian GAG epimerases.
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