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Influence of enhanced troponin C Ca2+-binding affinity on cooperative thin filament activation in rabbit skeletal muscle

机译:肌钙蛋白C Ca2 +结合亲和力增强对家兔骨骼肌协同细丝活化的影响

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摘要

We studied how enhanced skeletal troponin C (sTnC) Ca2+-binding affinity affects cooperative thin filament activation and contraction in single demembranated rabbit psoas fibres. Three sTnC mutants were created and incorporated into skeletal troponin (sTn) for measurement of Ca2+ dissociation, resulting in the following order of rates: wild-type (WT) sTnC–sTn > sTnCF27W–sTn > M80Q sTnC–sTn > M80Q sTnCF27W–sTn. Reconstitution of sTnC-extracted fibres increased Ca2+ sensitivity of steady-state force (pCa50) by 0.08 for M80Q sTnC, 0.15 for sTnCF27W and 0.32 for M80Q sTnCF27W with minimal loss of slope (nH, degree of cooperativity). Near-neighbour thin filament regulatory unit (RU) interactions were reduced in fibres by incorporating mixtures of WT or mutant sTnC and D28A, D64A sTnC (xxsTnC) that does not bind Ca2+ at N-terminal sites. Reconstitution with sTnC: xxsTnC mixtures to 20% of pre-exchanged maximal force reduced pCa50 by 0.35 for sTnC: xxsTnC, 0.25 for M80Q sTnC: xxsTnC, and 0.10 for M80Q sTnCF27W: xxsTnC. It is interesting that pCa50 increased by ∼0.1 for M80Q sTnC and ∼0.3 for M80Q sTnCF27W when near-neighbour RU interactions were reduced; these values are similar in magnitude to those for fibres reconstituted with 100% mutant sTnC. After reconstitution with sTnC: xxsTnC mixtures, nH decreased to a similar value for all mutant sTnCs. Altered sTnC Ca2+-binding properties (M80Q sTnCF27W) did not affect strong crossbridge inhibition by 2,3-butanedione monoxime when near-neighbour thin filament RU interactions were reduced. Together these results suggest increased sTnC Ca2+ affinity strongly influences Ca2+ sensitivity of steady-state force without affecting near-neighbour thin filament RU cooperative activation or the relative contribution of crossbridges versus Ca2+ to thin filament activation.
机译:我们研究了增强的骨骼肌肌钙蛋白C(sTnC)Ca2 +结合亲和力如何影响单个去膜兔腰大肌纤维中的协同细丝活化和收缩。创建了三个sTnC突变体,并将其整合到骨骼肌钙蛋白(sTn)中以测量Ca2 +的解离,其产生速率如下:野生型(WT)sTnC–sTn> sTnCF27W–sTn> M80Q sTnC–sTn> M80Q sTnCF27W 。重组sTnC提取的纤维可使M80Q sTnC的稳态力(pCa50)的Ca2 +敏感性增加0.08,对于sTnCF27W则为0.15,对于M80Q sTnCF27W则为0.32,同时最小的斜率损失(nH,协同度)。通过掺入野生型或突变型sTnC和D28A,D64A sTnC(xxsTnC)的混合物减少了纤维中近邻细丝调节单元(RU)的相互作用,这些混合物在N端不结合Ca2 +。用sTnC:xxsTnC混合物重构至预先交换的最大力的20%,对于sTnC:xxsTnC,pCa50降低0.35,对于M80Q sTnC:xxsTnC降低0.25,对于M80Q sTnCF27W:xxsTnC降低0.10。有趣的是,当减少近邻RU的相互作用时,pCa50对于M80Q sTnC增加约0.1,对于M80Q sTnCF27W增加约0.3。这些值的大小与用100%突变sTnC重构的纤维的大小相似。用sTnC:xxsTnC混合物重构后,所有突变sTnC的nH均降低至相似值。 sTnC Ca 2+结合性质的改变(M80Q sTnCF27W)在减少邻近细丝RU相互作用时不会影响2,3-丁二酮一肟的强横桥抑制作用。这些结果共同表明,增加的sTnC Ca2 +亲和力会强烈影响稳态力的Ca2 +敏感性,而不会影响邻近的细丝RU协同激活或横桥相对于Ca2 +对细丝激活的相对贡献。

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