AI Article Synopsis

  • Researchers created two chimeric proteins combining parts of human protein S and prothrombin to study their functions, specifically focusing on the gamma-carboxyglutamic acid (Gla) domain.
  • Neither chimera showed activated protein C (APC) cofactor activity, indicating the importance of the protein S Gla domain for this function, but both were good at binding to phospholipids.
  • Computational analysis revealed key structural features in the Gla domain relevant for APC interaction and phospholipid binding, with specific residues identified as crucial for these functions through experiments with modified versions of protein S.

Article Abstract

We expressed 2 chimeras between human protein S (PS) and human prothrombin (FII) in which the prothrombin gamma-carboxyglutamic acid (Gla) domain replaced the PS Gla domain in native PS (Gla(FII)-PS) or in PS deleted of the thrombin-sensitive region (TSR) (Gla(FII)-DeltaTSR-PS). Neither PS/FII chimera had activated protein C (APC) cofactor activity in plasma clotting assays or purified systems, but both bound efficiently to phospholipids. This pointed to a direct involvement of the PS Gla domain in APC cofactor activity through molecular interaction with APC. Using computational methods, we identified 2 opposite faces of solvent-exposed residues on the PS Gla domain (designated faces 1 and 2) as potentially involved in this interaction. Their importance was supported by functional characterization of a PS mutant in which the face 1 and face 2 PS residues were reintroduced into Gla(FII)-PS, leading to significant APC cofactor activity, likely through restored interaction with APC. Furthermore, by characterizing PS mutants in which PS face 1 and PS face 2 were individually replaced by the corresponding prothrombin faces, we found that face 1 was necessary for efficient phospholipid binding but that face 2 residues were not strictly required for phospholipid binding and were involved in the interaction with APC.

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Source
http://dx.doi.org/10.1182/blood-2004-06-2176DOI Listing

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