AI Article Synopsis

  • NADPH oxidase is crucial for the innate immune response, and p47 (phox) is a key regulatory component in its activation.
  • Manipulating the p47 (phox) linker region affects its ability to bind to the phosphoinositide PI(3,4)P2, impacting its conformation and binding dynamics.
  • Despite showing strong binding to PI(3,4)P2, a glycine mutant of p47 (phox) significantly reduces NADPH oxidase activity, indicating that the linker region is vital for maintaining the protein's autoinhibited state and for proper activation of the oxidase.

Article Abstract

NADPH oxidase is essential in the human innate immune response. p47 (phox), a cytosolic NADPH oxidase component, plays a regulatory role in the activation of NADPH oxidase. Our manipulation of p47 (phox) by mutation and amino acid deletion shows that the linker region between the PX and N-terminal SH3 domain plays a role in blocking the binding of the phosphoinositide 3,4-bisphosphate [PI(3,4)P2], a lipid second messenger generated upon neutrophil activation. Replacement of linker residues 151-158 with glycine alters NMR-measured spin lattice relaxation rates and sedimentation velocity compared to those of the wild-type protein, suggesting that the PX domain is released from its autoinhibited conformation. Liposome binding and surface plasmon resonance experiments confirm this result, showing that this mutant has a similar binding affinity for the isolated PX domain toward PI(3,4)P2. However, an in vitro NADPH oxidase activity assay reveals that this glycine mutant of the full-length protein greatly reduced NADPH oxidase activity upon activation even though it displayed PI(3,4)P2 binding activity comparable to that of the isolated PX domain. Our results highlight an active role of the PX-SH3 linker region in maintaining p47 (phox) in its fully autoinhibited form and demonstrate that binding of p47 (phox) to membrane phospholipids is mechanistically distinct from NADPH oxidase activation.

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Source
http://www.ncbi.nlm.nih.gov/pmc/articles/PMC2745045PMC
http://dx.doi.org/10.1021/bi8005847DOI Listing

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