van Dijk Sabine J, Witt Christian C, Harris Samantha P
Department of Cellular and Molecular Medicine, University of Arizona, 1656 East Mabel Street, Tucson, AZ 85724, USA.
Department of Anaesthesiology and Operative Intensive Care, University Hospital Mannheim, Medical Faculty Mannheim, Heidelberg University, Theodor-Kutzer-Ufer 1-3, 68167 Mannheim, Germany.
J Mol Cell Cardiol. 2015 Nov;88:124-32. doi: 10.1016/j.yjmcc.2015.09.006. Epub 2015 Oct 8.
Cardiac myosin binding protein C (cMyBP-C) is an essential regulator of cross bridge cycling. Through mechanisms that are incompletely understood the N-terminal domains (NTDs) of cMyBP-C can activate contraction even in the absence of calcium and can also inhibit cross bridge kinetics in the presence of calcium. In vitro studies indicated that the proline-alanine rich (p/a) region and C1 domain are involved in these processes, although effects were greater using human proteins compared to murine proteins (Shaffer et al. J Biomed Biotechnol 2010, 2010: 789798). We hypothesized that the p/a and C1 region are critical for the timing of contraction. In this study we tested this hypothesis using a mouse model lacking the p/a and C1 region (p/a-C1(-/-) mice) to investigate the in vivo relevance of these regions on cardiac performance. Surprisingly, hearts of adult p/a-C1(-/-) mice functioned normally both on a cellular and whole organ level. Force measurements in permeabilized cardiomyocytes from adult p/a-C1(-/-) mice and wild type (Wt) littermate controls demonstrated similar rates of force redevelopment both at submaximal and maximal activation. Maximal and passive force and calcium sensitivity of force were comparable between groups as well. Echocardiograms showed normal isovolumetric contraction times, fractional shortening and ejection fraction, indicating proper systolic function in p/a-C1(-/-) mouse hearts. p/a-C1(-/-) mice showed a slight but significant reduction in isovolumetric relaxation time compared to Wt littermates, yet this difference disappeared in older mice (7-8months of age). Moreover, stroke volume was preserved in p/a-C1(-/-) mice, corroborating sufficient time for normal filling of the heart. Overall, the hearts of p/a-C1(-/-) mice showed no signs of dysfunction even after chronic stress with an adrenergic agonist. Together, these results indicate that the p/a region and the C1 domain of cMyBP-C are not critical for normal cardiac contraction in mice and that these domains have little if any impact on cross bridge kinetics in mice. These results thus contrast with in vitro studies utilizing proteins encoding the human p/a region and C1 domain. More detailed insight in how individual domains of cMyBP-C function and interact, across species and over the wide spectrum of conditions in which the heart has to function, will be essential to a better understanding of how cMyBP-C tunes cardiac contraction.
心肌肌球蛋白结合蛋白C(cMyBP-C)是横桥循环的重要调节因子。通过尚未完全了解的机制,cMyBP-C的N端结构域(NTDs)即使在没有钙的情况下也能激活收缩,并且在有钙的情况下还能抑制横桥动力学。体外研究表明,富含脯氨酸-丙氨酸的(p/a)区域和C1结构域参与了这些过程,尽管与鼠类蛋白相比,使用人类蛋白时效果更明显(Shaffer等人,《生物医学与生物技术杂志》,2010年,2010: 789798)。我们假设p/a和C1区域对收缩的时机至关重要。在本研究中,我们使用缺乏p/a和C1区域的小鼠模型(p/a-C1(-/-)小鼠)来检验这一假设,以研究这些区域对心脏功能的体内相关性。令人惊讶的是,成年p/a-C1(-/-)小鼠的心脏在细胞和整个器官水平上均功能正常。对成年p/a-C1(-/-)小鼠和野生型(Wt)同窝对照的透化心肌细胞进行的力测量表明,在次最大和最大激活时,力的重新发展速率相似。两组之间的最大力、被动力和力的钙敏感性也相当。超声心动图显示等容收缩时间、缩短分数和射血分数正常,表明p/a-C1(-/-)小鼠心脏的收缩功能正常。与Wt同窝小鼠相比,p/a-C1(-/-)小鼠的等容舒张时间略有但显著缩短,但这种差异在老年小鼠(7-8月龄)中消失。此外,p/a-C1(-/-)小鼠的 stroke volume得以保留,证实心脏有足够的时间进行正常充盈。总体而言,即使在用肾上腺素能激动剂进行慢性应激后,p/a-C1(-/-)小鼠的心脏也没有功能障碍的迹象。总之,这些结果表明,cMyBP-C的p/a区域和C1结构域对小鼠的正常心脏收缩并不关键,并且这些结构域对小鼠横桥动力学几乎没有影响。因此,这些结果与利用编码人类p/a区域和C1结构域的蛋白质进行的体外研究形成对比。更详细地了解cMyBP-C的各个结构域如何在不同物种以及心脏必须发挥功能的广泛条件下发挥作用并相互作用,对于更好地理解cMyBP-C如何调节心脏收缩至关重要。
