Structural basis and functional effects of the interaction between complement inhibitor C4b-binding protein and DNA.

Okroj, Marcin; Jenkins, Huw T; Herbert, Andrew P; Barlow, Paul N; Blom, Anna M

Structural basis and functional effects of the interaction between complement inhibitor C4b-binding protein and DNA.

Mark

Okroj, Marcin ^LU ; Jenkins, Huw T ; Herbert, Andrew P ; Barlow, Paul N and Blom, Anna M (2008) In Molecular Immunology 46. p.62-69

Abstract: Human C4b-binding protein (C4BP) is a soluble, multiple-subunit inhibitor of complement that circulates in blood. Recently C4BP was shown to bind DNA, reduce DNA release from necrotic cells and limit DNA-mediated complement activation in solution. Herein we employed nuclear magnetic resonance spectroscopy to measure chemical shift perturbations and used them to restrain the computational docking of a B-form 10-base-pair DNA molecule onto the solution structure of C4BP alpha-chain complement control protein (CCP) domains 1-2 (C4BP12). Six amino acid residues located on one face of the interdomain junction - Val(38), Ser(40), Thr(43), Tyr(62), Lys(63) and Arg(64) - exhibited the largest chemical shift changes. In the model, the DNA lies in a... (More); Human C4b-binding protein (C4BP) is a soluble, multiple-subunit inhibitor of complement that circulates in blood. Recently C4BP was shown to bind DNA, reduce DNA release from necrotic cells and limit DNA-mediated complement activation in solution. Herein we employed nuclear magnetic resonance spectroscopy to measure chemical shift perturbations and used them to restrain the computational docking of a B-form 10-base-pair DNA molecule onto the solution structure of C4BP alpha-chain complement control protein (CCP) domains 1-2 (C4BP12). Six amino acid residues located on one face of the interdomain junction - Val(38), Ser(40), Thr(43), Tyr(62), Lys(63) and Arg(64) - exhibited the largest chemical shift changes. In the model, the DNA lies in a cleft formed by the interdomain interface. The double-helix is perpendicular to the long axis of C4BP12 consistent with the multiple arms of C4BP binding to adjacent sites on a longer DNA molecule. The DNA lies in a region previously shown to bind C4b and heparin and these molecules (but not C3b) inhibited the DNA-C4BP interaction. Nonetheless, crucial C4BP functions such as cofactor activity for factor I cleavage of C4b and C3b, and decay acceleration of the classical C3 convertase appeared not to be affected by the presence of DNA. Taken together these results reinforce the case for the occupation of some of the seven arms of C4BP in a multivalent interaction with DNA or surface bound glycosaminoglycans while other arms engage C4b or C3b. (Less)

Please use this url to cite or link to this publication: https://lup.lub.lu.se/record/1223040

author

Okroj, Marcin ^LU ; Jenkins, Huw T ; Herbert, Andrew P ; Barlow, Paul N and Blom, Anna M

organization

Protein Chemistry, Malmö (research group)

publishing date

2008

type

Contribution to journal

publication status

published

subject

Immunology in the medical area

in

Molecular Immunology

volume

46

pages

62 - 69

publisher

Pergamon Press Ltd.

external identifiers

wos:000260807700007
pmid:18715646
scopus:52949106501

ISSN

1872-9142

DOI

10.1016/j.molimm.2008.07.008

language

English

LU publication?

yes

id

b788cdcb-9f5a-4c51-80b8-5c6abff250f1 (old id 1223040)

alternative location

http://www.ncbi.nlm.nih.gov/pubmed/18715646?dopt=Abstract

date added to LUP

2016-04-04 09:34:54

date last changed

2022-01-29 18:32:36

@article{b788cdcb-9f5a-4c51-80b8-5c6abff250f1,
  abstract     = {{Human C4b-binding protein (C4BP) is a soluble, multiple-subunit inhibitor of complement that circulates in blood. Recently C4BP was shown to bind DNA, reduce DNA release from necrotic cells and limit DNA-mediated complement activation in solution. Herein we employed nuclear magnetic resonance spectroscopy to measure chemical shift perturbations and used them to restrain the computational docking of a B-form 10-base-pair DNA molecule onto the solution structure of C4BP alpha-chain complement control protein (CCP) domains 1-2 (C4BP12). Six amino acid residues located on one face of the interdomain junction - Val(38), Ser(40), Thr(43), Tyr(62), Lys(63) and Arg(64) - exhibited the largest chemical shift changes. In the model, the DNA lies in a cleft formed by the interdomain interface. The double-helix is perpendicular to the long axis of C4BP12 consistent with the multiple arms of C4BP binding to adjacent sites on a longer DNA molecule. The DNA lies in a region previously shown to bind C4b and heparin and these molecules (but not C3b) inhibited the DNA-C4BP interaction. Nonetheless, crucial C4BP functions such as cofactor activity for factor I cleavage of C4b and C3b, and decay acceleration of the classical C3 convertase appeared not to be affected by the presence of DNA. Taken together these results reinforce the case for the occupation of some of the seven arms of C4BP in a multivalent interaction with DNA or surface bound glycosaminoglycans while other arms engage C4b or C3b.}},
  author       = {{Okroj, Marcin and Jenkins, Huw T and Herbert, Andrew P and Barlow, Paul N and Blom, Anna M}},
  issn         = {{1872-9142}},
  language     = {{eng}},
  pages        = {{62--69}},
  publisher    = {{Pergamon Press Ltd.}},
  series       = {{Molecular Immunology}},
  title        = {{Structural basis and functional effects of the interaction between complement inhibitor C4b-binding protein and DNA.}},
  url          = {{http://dx.doi.org/10.1016/j.molimm.2008.07.008}},
  doi          = {{10.1016/j.molimm.2008.07.008}},
  volume       = {{46}},
  year         = {{2008}},
}

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Structural basis and functional effects of the interaction between complement inhibitor C4b-binding protein and DNA.