4.5 Article

Regulator-dependent mechanisms of C3b processing by factor I allow differentiation of immune responses

Journal

NATURE STRUCTURAL & MOLECULAR BIOLOGY
Volume 24, Issue 8, Pages 643-+

Publisher

NATURE PUBLISHING GROUP
DOI: 10.1038/nsmb.3427

Keywords

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Funding

  1. Top grant by the Council for Chemical Sciences of the Netherlands Organization for Scientific Research (NWO-CW) [700.54.304]
  2. European Research Council [233229]
  3. European Community [283570]
  4. FP7/DIREKT [602699]
  5. US National Institutes of Health [AI068730, AI030040]
  6. National Science Foundation [1423304]
  7. Institute for Chemical Immunology, an NWO Gravitation project - Ministry of Education, Culture and Science of the Netherlands
  8. European Research Council (ERC) [233229] Funding Source: European Research Council (ERC)

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The complement system labels microbes and host debris for clearance. Degradation of surface-bound C3b is pivotal to direct immune responses and protect host cells. How the serine protease factor I (FI), assisted by regulators, cleaves either two or three distant peptide bonds in the CUB domain of C3b remains unclear. We present a crystal structure of C3b in complex with FI and regulator factor H (FH; domains 1-4 with 19-20). FI binds C3b-FH between FH domains 2 and 3 and a reoriented C3b C-terminal domain and docks onto the first scissile bond, while stabilizing its catalytic domain for proteolytic activity. One cleavage in C3b does not affect its overall structure, whereas two cleavages unfold CUB and dislodge the thioester-containing domain (TED), affecting binding of regulators and thereby determining the number of cleavages. These data explain how FI generates late-stage opsonins iC3b or C3dg in a context-dependent manner, to react to foreign, danger or healthy self signals.

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