2011
DOI: 10.1074/jbc.m111.251769
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Molecular Determinants of Phospholipid Synergy in Blood Clotting

Abstract: Many regulatory processes in biology involve reversible association of proteins with membranes. Clotting proteins bind to phosphatidylserine (PS) on cell surfaces, but a clear picture of this interaction has yet to emerge. We present a novel explanation for membrane binding by GLA domains of clotting proteins, supported by biochemical studies, solid-state NMR analyses, and molecular dynamics simulations. The model invokes a single “phospho-l-serine-specific” interaction and multiple “phosphate-specific” intera… Show more

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Cited by 100 publications
(145 citation statements)
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References 32 publications
(57 reference statements)
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“…5). In agreement, lyso-PE (which contains no sn2 fatty acid) was previously shown to not support activity of the tenase complex in PS liposomes (27). Our finding that short chain PE poorly supports coagulation whereas short chain PS supports coagulation normally, suggests that these molecules interact differentially with coagulation factors through their Gla domains.…”
Section: -4 and Si Results)supporting
confidence: 75%
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“…5). In agreement, lyso-PE (which contains no sn2 fatty acid) was previously shown to not support activity of the tenase complex in PS liposomes (27). Our finding that short chain PE poorly supports coagulation whereas short chain PS supports coagulation normally, suggests that these molecules interact differentially with coagulation factors through their Gla domains.…”
Section: -4 and Si Results)supporting
confidence: 75%
“…Each Gla domain is thought to have one specific interaction with the carboxylate on the headgroup of PS and approximately six interactions with phosphates on any PL except PC. This idea means that PS is required for coagulation to take place but PE can enhance the rate of these reactions (27). To date, the interaction between APL and coagulation factors was (C and D) Platelets were activated with 10 μM rotenone for 180 min, or with 1 μM ABT-737 for 60 min, after preincubation with inhibitors (Q-VD-OPH, caspase inhibitor, 10 μM), EGTA (1 mM), BAPTA-AM (10 μM), then surface APL analyzed as described in Materials and Methods.…”
Section: -4 and Si Results)mentioning
confidence: 99%
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“…Although good charge measurement data are available for proteins and nucleic acids (8,9), obtaining charge measurements in lipids has posed experimental difficulties. This lack of solid charge information is unfortunate because the membrane composition, including charge, is of fundamental importance for a variety of cellular and physiological functions (10).…”
Section: Introductionmentioning
confidence: 99%