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Skeletal regulatory proteins enhance thin filament sliding speed and force by skeletal HMM.骨骼调节蛋白通过骨骼肌重链肌球蛋白增强细肌丝滑动速度和力量。
J Muscle Res Cell Motil. 2004;25(7):515-25. doi: 10.1007/s10974-004-3787-0. Epub 2005 Feb 9.
2
Contractile effects of the exchange of cardiac troponin for fast skeletal troponin in rabbit psoas single myofibrils.兔腰大肌单根肌原纤维中心脏肌钙蛋白与快肌骨骼肌肌钙蛋白交换后的收缩效应。
J Physiol. 2003 Nov 1;552(Pt 3):917-31. doi: 10.1113/jphysiol.2003.051615. Epub 2003 Aug 22.
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Structure of the core domain of human cardiac troponin in the Ca(2+)-saturated form.钙离子饱和状态下人类心肌肌钙蛋白核心结构域的结构
Nature. 2003 Jul 3;424(6944):35-41. doi: 10.1038/nature01780.
4
Thin filament activation and unloaded shortening velocity of rabbit skinned muscle fibres.兔去皮肤肌纤维的细肌丝激活与无负荷缩短速度
J Physiol. 2003 Jul 1;550(Pt 1):205-15. doi: 10.1113/jphysiol.2003.040899. Epub 2003 May 2.
5
Thin filament near-neighbour regulatory unit interactions affect rabbit skeletal muscle steady-state force-Ca(2+) relations.细肌丝近邻调节单元相互作用影响兔骨骼肌稳态力 - 钙离子关系。
J Physiol. 2002 Apr 15;540(Pt 2):485-97. doi: 10.1113/jphysiol.2001.013179.
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A small-molecule inhibitor of skeletal muscle myosin II.一种骨骼肌肌球蛋白II的小分子抑制剂。
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Influence of length on force and activation-dependent changes in troponin c structure in skinned cardiac and fast skeletal muscle.长度对心肌和快肌去膜纤维肌钙蛋白C结构中力及激活依赖性变化的影响。
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Modulation of contractile activation in skeletal muscle by a calcium-insensitive troponin C mutant.钙不敏感肌钙蛋白C突变体对骨骼肌收缩激活的调节作用。
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Ca2+ - and cross-bridge-dependent changes in N- and C-terminal structure of troponin C in rat cardiac muscle.大鼠心肌肌钙蛋白C的N端和C端结构中依赖钙离子和横桥的变化
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10
Cooperative mechanisms in the activation dependence of the rate of force development in rabbit skinned skeletal muscle fibers.兔去皮肤骨骼肌纤维中力发展速率的激活依赖性的协同机制。
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心肌肌钙蛋白C(TnC)和I位点骨骼肌TnC突变体改变了兔骨骼肌纤维中Ca2+与横桥对力量的贡献。

Cardiac troponin C (TnC) and a site I skeletal TnC mutant alter Ca2+ versus crossbridge contribution to force in rabbit skeletal fibres.

作者信息

Moreno-Gonzalez Alicia, Fredlund Jennifer, Regnier Michael

机构信息

Department of Bioengineering, University of Washington, Box 357962, Seattle, WA 98195-7962, USA.

出版信息

J Physiol. 2005 Feb 1;562(Pt 3):873-84. doi: 10.1113/jphysiol.2004.077891. Epub 2004 Dec 20.

DOI:10.1113/jphysiol.2004.077891
PMID:15611027
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC1665546/
Abstract

We studied the relative contributions of Ca(2+) binding to troponin C (TnC) and myosin binding to actin in activating thin filaments of rabbit psoas fibres. The ability of Ca(2+) to activate thin filaments was reduced by replacing native TnC with cardiac TnC (cTnC) or a site I-inactive skeletal TnC mutant (xsTnC). Acto-myosin (crossbridge) interaction was either inhibited using N-benzyl-p-toluene sulphonamide (BTS) or enhanced by lowering [ATP] from 5.0 to 0.5 mm. Reconstitution with cTnC reduced maximal force (F(max)) by approximately 1/3 and the Ca(2+) sensitivity of force (pCa(50)) by 0.17 unit (P < 0.001), while reconstitution with xsTnC reduced F(max) by approximately 2/3 and pCa(50) by 0.19 unit (P < 0.001). In both cases the apparent cooperativity of activation (n(H)) was greatly decreased. In control fibres 3 mum BTS inhibited force to 57% of F(max) while in fibres reconstituted with cTnC or xsTnC, reconstituted maximal force (rF(max)) was inhibited to 8.8% and 14.3%, respectively. Under control conditions 3 mum BTS significantly decreased the pCa(50), but this effect was considerably reduced in cTnC reconstituted fibres, and eliminated in xsTnC reconstituted fibres. In contrast, when crossbridge cycle kinetics were slowed by lowering [ATP] from 5 to 0.5 mm in xsTnC reconstituted fibres, pCa(50) and n(H) were increased towards control values. Combined, our results demonstrate that when the ability of Ca(2+) binding to activate thin filaments is compromised, the relative contribution of strong crossbridges to maintain thin filament activation is increased. Furthermore, the data suggest that at low levels of Ca(2+), the level of thin filament activation is determined primarily by the direct effects of Ca(2+) on tropomyosin mobility, while at higher levels of Ca(2+) the final level of thin filament activation is primarily determined by strong cycling crossbridges.

摘要

我们研究了钙离子与肌钙蛋白C(TnC)结合以及肌球蛋白与肌动蛋白结合在激活兔腰大肌纤维细肌丝过程中的相对作用。用心脏肌钙蛋白C(cTnC)或I位点无活性的骨骼肌肌钙蛋白C突变体(xsTnC)替代天然TnC,可降低钙离子激活细肌丝的能力。使用N - 苄基 - 对甲苯磺酰胺(BTS)抑制肌动蛋白 - 肌球蛋白(横桥)相互作用,或将[ATP]从5.0 mM降至0.5 mM可增强这种相互作用。用cTnC重构可使最大力量(F(max))降低约1/3,力量的钙离子敏感性(pCa(50))降低0.17个单位(P < 0.001),而用xsTnC重构可使F(max)降低约2/3,pCa(50)降低0.19个单位(P < 0.001)。在这两种情况下,激活的表观协同性(n(H))都大大降低。在对照纤维中,3 μM BTS将力量抑制至F(max)的57%,而在用cTnC或xsTnC重构的纤维中,重构后的最大力量(rF(max))分别被抑制至8.8%和14.3%。在对照条件下,3 μM BTS显著降低pCa(50),但在cTnC重构的纤维中这种效应明显减弱,在xsTnC重构的纤维中则消除。相反,当在xsTnC重构的纤维中将[ATP]从5 mM降至0.5 mM从而减缓横桥循环动力学时,pCa(50)和n(H)朝着对照值增加。综合来看,我们的结果表明,当钙离子结合激活细肌丝的能力受损时,强横桥维持细肌丝激活的相对作用增加。此外,数据表明,在低钙离子水平时,细肌丝激活水平主要由钙离子对原肌球蛋白移动性的直接影响决定,而在较高钙离子水平时,细肌丝激活的最终水平主要由活跃循环的强横桥决定。