Measurements of the unloaded sliding speed of and isometric force e'/> Regulation of force and unloaded sliding speed in single thin filaments: effects of regulatory proteins and calcium
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Regulation of force and unloaded sliding speed in single thin filaments: effects of regulatory proteins and calcium

机译:单细丝中力和空载滑动速度的调节:调节蛋白和钙的作用

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摘要

class="enumerated" style="list-style-type:decimal">Measurements of the unloaded sliding speed of and isometric force exerted on single thin filaments in in vitro motility assays were made to evaluate the role of regulatory proteins in the control of unloaded thin filament sliding speed and isometric force production.Regulated actin filaments were reconstituted from rabbit F-actin, native bovine cardiac tropomyosin (nTm), and either native bovine cardiac troponin (nTn), troponin containing a TnC mutant, CBMII, in which the sole regulatory site in cardiac TnC (site II) is inactivated (CBMII-Tn), or troponin containing a point mutation in TnT (I79N, where isoleucine at position 79 is replaced with asparagine) associated with familial hypertrophic cardiomyopathy (FHC).Addition of regulatory proteins to the thin filament increases both the unloaded sliding speed and the isometric force exerted by myosin heads on the thin filaments.Variation of thin filament activation by varying [Ca2+] or the fraction of CBMII/TnC bound to the thin filament at pCa 5, had little effect on the unloaded filament sliding speed until the fraction of the thin filament containing calcium bound to TnC was less than 0.15. These results suggest that [Ca2+] primarily affects the number of attached and cycling crossbridges.The presence of the FHC TnT mutant increased the thin filament sliding speed but reduced the isometric force that heavy meromyosin exerted on regulated thin filaments. These latter results, together with the increased sliding speed and isometric force seen in the presence of regulatory proteins, suggest that thin filament regulatory proteins exert significant allosteric effects on the interaction of crossbridges with the thin filament.
机译:class =“ enumerated” style =“ list-style-type:decimal”> <!-list-behavior =枚举前缀-word = mark-type = decimal max-label-size = 0-> 测量了体外运动试验中单根细丝的空载滑移速度和等距力,以评估调节蛋白在控制空载细丝滑移速度和等距力产生中的作用。 从兔F-肌动蛋白,天然牛心肌肌钙蛋白(nTm)和天然牛心肌肌钙蛋白(nTn),含有TnC突变体CBMII的肌钙蛋白中重组受调节的肌动蛋白丝,其中心脏TnC的唯一调控位点(位点II)失活(CBMII-Tn),或肌钙蛋白含有TnT点突变(I79N,其中79位的异亮氨酸被天冬酰胺取代),与家族性肥厚性心肌病(FHC)相关。 将调节蛋白添加到细丝增加了空载的滑动速度和等轴测力 通过改变[Ca 2 + ]或在pCa 5处结合到细丝上的CBMII / TnC的分数来改变细丝激活直到对TnC结合的含钙细丝的比例小于0.15,对空载丝的滑动速度几乎没有影响。这些结果表明,[Ca 2 + ]主要影响附着和循环桥的数量。 FHC TnT突变体的存在增加了细丝滑动速度,但降低了等轴测图重肌球蛋白在调节的细丝上施加的力。后一结果以及在调节蛋白存在下所观察到的增加的滑动速度和等轴测力表明,细丝调节蛋白对跨桥与细丝的相互作用具有显着的变构作用。

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