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Three residues at the interface of factor XI (FXI) monomers augment covalent dimerization of FXI
Authors:M ZUCKER  A ZIVELIN  M LANDAU†  N ROSENBERG  U SELIGSOHN
Institution:The Amalia Biron Research Institute of Thrombosis and Haemostasis, Chaim Sheba Medical Centre, Tel-Hashomer and Sackler Faculty of Medicine;;and Department of Biochemistry, George S. Wise Faculty of Life Sciences, Tel-Aviv University, Tel Aviv, Israel
Abstract:Summary.  Background:  Human plasma factor XI is a homodimer, with each monomer comprising a catalytic domain and four homologous 'apple' domains. The monomers bind to each other through non-covalent bonds and through a disulfide bond between Cys321 residues in apple 4 domains. Objective:  To identify residues essential for dimerization in the FXI monomer interface. Methods:  Specificity-determining residues in apple 4 domains were sought by sequence alignment of FXI and prekallikrein apple domains in different species. Specific residues identified in apple 4 domains were mutagenized and expressed in baby hamster kidney (BHK) cells for evaluation of their effect on FXI dimerization, analyzed by non-reduced sodium dodecylsulfate polyacrylamide gel electrophoresis and size-exclusion chromatography. Results:  Among the 19 residues of the FXI monomer interface, Leu284, Ile290 and Tyr329 were defined as specificity-determining residues. Substitutions of these residues or pairs of residues did not affect FXI synthesis and secretion from transfected BHK cells, but did impair dimerization, despite the presence of cysteine at position 321. The double mutant 284A/290A yielded predominantly a monomer, whereas all other single or double mutants yielded monomers as well as disulfide-bonded dimers. Conclusions:  The data suggest that Leu284, Ile290 and Tyr329 in the interface of FXI monomers are essential for forming non-covalently bonded dimers that facilitate formation of a disulfide-bonded stable FXI dimer.
Keywords:factor XI  factor XI dimer  factor XI dimerization  factor XI monomer
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