Ligand migration through the internal hydrophobic cavities in human neuroglobin

  1. Stefania Abbruzzettia,
  2. Serena Faggianob,
  3. Stefano Brunob,
  4. Francesca Spyrakisc,d,
  5. Andrea Mozzarellib,d,
  6. Sylvia Dewildee,
  7. Luc Moense and
  8. Cristiano Viappiania,1
  1. aDipartimento di Fisica, National Enterprise for nanoScience and nanoTechnology (NEST) CNR-INFM,
  2. bDipartimento di Biochimica e Biologia Molecolare, and
  3. cDipartimento di Chimica Generale ed Inorganica, Chimica Analitica, Chimica Fisica, Università degli Studi di Parma, 43100 Parma, Italy; and
  4. dNational Institute of Biostructures and Biosystems,
  5. eDepartment of Biomedical Sciences, University of Antwerp, Antwerp, Belgium

  1. Edited by William A. Eaton, National Institutes of Health, Bethesda, MD, and approved September 11, 2009 (received for review May 22, 2009)

Abstract

Neuroglobin (Ngb), a member of the globin superfamily, was found in the brain of vertebrates and is suggested to play a neuroprotective function under hypoxic conditions by scavenging nitrogen monoxide (NO) through a dioxygenase activity. In order for such a reaction to efficiently take place and to minimize the release of reactive intermediates in the cytosol, the cosubstrates O2 and NO and other unstable reaction intermediates should bind sequentially to docking sites in the protein matrix. We have characterized the accessibility of these sites by analyzing the geminate CO rebinding kinetics to the heme moiety observed upon nanosecond flash photolysis of the Ngb-CO complex encapsulated in silica gels. The geminate rebinding phase showed a remarkable complexity, revealing the presence of a system of secondary docking sites where ligands are stored for hundreds of microseconds. Most kinetics steps display little temperature dependence, demonstrating that ligands can easily migrate through the cavities, except for the slowest reaction intermediate, possibly reflecting a structural conformational change reshaping the system of cavities. This conformational change is unrelated with distal His E7 binding to the heme, as it persists for the HE7L mutant. Overall, data are consistent with the presence of a discrete system of docking sites, possibly acting as reservoirs for the putative cosubstrates and for other reactive species involved in the physiologically relevant reaction.

Footnotes

  • 1To whom correspondence should be addressed. E-mail: cristiano.viappiani{at}fis.unipr.it

  • Author contributions: S.A., S.F., S.B., A.M., S.D., L.M., and C.V. designed research; S.A., S.F., S.B., F.S., S.D., L.M., and C.V. performed research; S.A., S.F., S.B., F.S., and C.V. analyzed data; and S.A., S.B., F.S., A.M., S.D., L.M., and C.V. wrote the paper.

  • The authors declare no conflict of interest.

  • This article is a PNAS Direct Submission.

  • This article contains supporting information online at www.pnas.org/cgi/content/full/0905433106/DCSupplemental.

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  1. Published online before print October 22, 2009, doi: 10.1073/pnas.0905433106 PNAS November 10, 2009 vol. 106 no. 45 18984-18989
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