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Literature DB >> 20541506

Metal ion roles and the movement of hydrogen during reaction catalyzed by D-xylose isomerase: a joint x-ray and neutron diffraction study.

Andrey Y Kovalevsky¹, Leif Hanson, S Zoe Fisher, Marat Mustyakimov, Sax A Mason, V Trevor Forsyth, Matthew P Blakeley, David A Keen, Trixie Wagner, H L Carrell, Amy K Katz, Jenny P Glusker, Paul Langan.

Abstract

Conversion of aldo to keto sugars by the metalloenzyme D-xylose isomerase (XI) is a multistep reaction that involves hydrogen transfer. We have determined the structure of this enzyme by neutron diffraction in order to locate H atoms (or their isotope D). Two studies are presented, one of XI containing cadmium and cyclic D-glucose (before sugar ring opening has occurred), and the other containing nickel and linear D-glucose (after ring opening has occurred but before isomerization). Previously we reported the neutron structures of ligand-free enzyme and enzyme with bound product. The data show that His54 is doubly protonated on the ring N in all four structures. Lys289 is neutral before ring opening and gains a proton after this; the catalytic metal-bound water is deprotonated to hydroxyl during isomerization and O5 is deprotonated. These results lead to new suggestions as to how changes might take place over the course of the reaction.

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Year: 2010 PMID： 20541506 PMCID： PMC2887347 DOI： 10.1016/j.str.2010.03.011

Source DB: PubMed Journal: Structure ISSN： 0969-2126 Impact factor: 5.006

36 in total

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40 in total

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4. Using neutron protein crystallography to understand enzyme mechanisms.

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7. Time-of-flight neutron diffraction study of bovine γ-chymotrypsin at the Protein Crystallography Station.

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8. High-resolution neutron crystallographic studies of the hydration of the coenzyme cob(II)alamin.

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9. Refinement of macromolecular structures against neutron data with SHELXL2013.

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10. Long-Range Electrostatics-Induced Two-Proton Transfer Captured by Neutron Crystallography in an Enzyme Catalytic Site.

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