Literature DB >> 21041929

Protonation states of histidine and other key residues in deoxy normal human adult hemoglobin by neutron protein crystallography.

Andrey Kovalevsky1, Toshiyuki Chatake, Naoya Shibayama, Sam Yong Park, Takuya Ishikawa, Marat Mustyakimov, S Zoe Fisher, Paul Langan, Yukio Morimoto.   

Abstract

The protonation states of the histidine residues key to the function of deoxy (T-state) human hemoglobin have been investigated using neutron protein crystallography. These residues can reversibly bind protons, thereby regulating the oxygen affinity of hemoglobin. By examining the OMIT F(o)-F(c) and 2F(o)-F(c) neutron scattering maps, the protonation states of 35 of the 38 His residues were directly determined. The remaining three residues were found to be disordered. Surprisingly, seven pairs of His residues from equivalent α or β chains, αHis20, αHis50, αHis58, αHis89, βHis63, βHis143 and βHis146, have different protonation states. The protonation of distal His residues in the α(1)β(1) heterodimer and the protonation of αHis103 in both subunits demonstrates that these residues may participate in buffering hydrogen ions and may influence the oxygen binding. The observed protonation states of His residues are compared with their ΔpK(a) between the deoxy and oxy states. Examination of inter-subunit interfaces provided evidence for interactions that are essential for the stability of the deoxy tertiary structure.

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Year:  2010        PMID: 21041929      PMCID: PMC2967419          DOI: 10.1107/S0907444910025448

Source DB:  PubMed          Journal:  Acta Crystallogr D Biol Crystallogr        ISSN: 0907-4449


  38 in total

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Review 9.  Neutron crystallography: opportunities, challenges, and limitations.

Authors:  Matthew P Blakeley; Paul Langan; Nobuo Niimura; Alberto Podjarny
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10.  Protein structures by spallation neutron crystallography.

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Journal:  J Synchrotron Radiat       Date:  2008-04-18       Impact factor: 2.616

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  1 in total

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