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Molecular Mechanisms, Thermodynamics, and Dissociation Kinetics of Knob-Hole Interactions in Fibrin

动力学 离解(化学) 纤维蛋白 热力学 化学 材料科学 物理化学 物理 医学 经典力学 免疫学
作者
Olga Kononova,Rustem I. Litvinov,Artem Zhmurov,Andrey Alekseenko,Chia Ho Cheng,Silvi Agarwal,Kenneth A. Marx,John W. Weisel,Valeri Barsegov
出处
期刊:Journal of Biological Chemistry [Elsevier]
卷期号:288 (31): 22681-22692 被引量:29
标识
DOI:10.1074/jbc.m113.472365
摘要

Polymerization of fibrin, the primary structural protein of blood clots and thrombi, occurs through binding of knobs 'A' and 'B' in the central nodule of fibrin monomer to complementary holes 'a' and 'b' in the beta- and gamma-nodules, respectively, of another monomer. We characterized the A:a and B:b knob-hole interactions under varying solution conditions using Molecular Dynamics simulations of the structural models of fibrin(ogen) fragment D complexed with synthetic peptides GPRP (knob 'A' mimetic) and GHRP (knob 'B' mimetic). The strength of A:a and B:b knob-hole complexes was roughly equal, decreasing with pulling force; yet, the dissociation kinetics were sensitive to variations in acidity (pH=5-7) and temperature (T=25-37 C). There were similar structural changes in holes 'a' and 'b' during forced dissociation of the knob-hole complexes: elongation of loop I, stretching of interior region, and translocation of the moveable flap. The disruption of the knob-hole interactions was not an "all-or-none" transition, as it occurred through distinct two-step or single-step pathways with or without intermediate states. The knob-hole bonds were stronger, tighter, and more brittle at pH=7 than at pH=5. The B:b knob-hole bonds were weaker, looser, and more compliant than the A:a knob-hole bonds at pH=7, but stronger, tighter, and less compliant at pH=5. Surprisingly, the knob-hole bonds were stronger, not weaker, at elevated temperature (T=37 C) compared to T=25 C due to the helix-to-coil transition in loop I, which helps stabilize the bonds. These results provide detailed qualitative and quantitative characteristics underlying the most significant non-covalent interactions involved in fibrin polymerization.

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