Département de Physiologie, Faculté de Médecine Pierre & Marie Curie site Pitié-Salpêtrière, UPMC, 91, Bd de l'Hôpital, 75013, Paris, France.
UPEC, Créteil, France.
Skelet Muscle. 2018 Jan 5;8(1):1. doi: 10.1186/s13395-017-0147-5.
Human induced pluripotent stem cells-derived myogenic progenitors develop functional and ultrastructural features typical of skeletal muscle when differentiated in culture. Besides disease-modeling, such a system can be used to clarify basic aspects of human skeletal muscle development. In the present study, we focus on the development of the excitation-contraction (E-C) coupling, a process that is essential both in muscle physiology and as a tool to differentiate between the skeletal and cardiac muscle. The occurrence and maturation of E-C coupling structures (Sarcoplasmic Reticulum-Transverse Tubule (SR-TT) junctions), key molecular components, and Ca signaling were examined, along with myofibrillogenesis.
Pax7-myogenic progenitors were differentiated in culture, and developmental changes were examined from a few days up to several weeks. Ion channels directly involved in the skeletal muscle E-C coupling (RyR1 and Cav1.1 voltage-gated Ca channels) were labeled using indirect immunofluorescence. Ultrastructural changes of differentiating cells were visualized by transmission electron microscopy. On the functional side, depolarization-induced intracellular Ca transients mediating E-C coupling were recorded using Fura-2 ratiometric Ca imaging, and myocyte contraction was captured by digital photomicrography.
We show that the E-C coupling machinery occurs and operates within a few days post-differentiation, as soon as the myofilaments align. However, Ca transients become effective in triggering myocyte contraction after 1 week of differentiation, when nascent myofibrils show alternate A-I bands. At later stages, myofibrils become fully organized into adult-like sarcomeres but SR-TT junctions do not reach their triadic structure and typical A-I location. This is mirrored by the absence of cross-striated distribution pattern of both RyR1 and Cav1.1 channels.
The E-C coupling machinery occurs and operates within the first week of muscle cells differentiation. However, while early development of SR-TT junctions is coordinated with that of nascent myofibrils, their respective maturation is not. Formation of typical triads requires other factors/conditions, and this should be taken into account when using in-vitro models to explore skeletal muscle diseases, especially those affecting E-C coupling.
人类诱导多能干细胞衍生的成肌祖细胞在体外分化时会发展出具有典型骨骼肌功能和超微结构的特征。除了疾病建模外,这种系统还可用于阐明人类骨骼肌发育的基本方面。在本研究中,我们专注于兴奋-收缩(E-C)偶联的发展,这是肌肉生理学中必不可少的过程,也是区分骨骼肌和心肌的工具。我们检查了 E-C 偶联结构(肌浆网-横管(SR-TT)连接)、关键分子成分和 Ca 信号的发生和成熟,以及肌原纤维的形成。
在培养中分化 Pax7 肌源性祖细胞,并检查从几天到几周的发育变化。使用间接免疫荧光标记直接参与骨骼肌 E-C 偶联的离子通道(RyR1 和 Cav1.1 电压门控 Ca 通道)。通过透射电子显微镜观察分化细胞的超微结构变化。在功能方面,使用 Fura-2 比率 Ca 成像记录引发 E-C 偶联的去极化诱导的细胞内 Ca 瞬变,并通过数字相差显微镜捕获肌细胞收缩。
我们表明,E-C 偶联机制在分化后几天内发生并运作,就在肌丝排列时。然而,Ca 瞬变在分化 1 周后才有效触发肌细胞收缩,此时新生肌原纤维显示交替的 A-I 带。在后期,肌原纤维完全组织成类似于成年的肌节,但 SR-TT 连接未达到其三联结构和典型的 A-I 位置。这反映在 RyR1 和 Cav1.1 通道的横纹分布模式缺失上。
E-C 偶联机制在肌肉细胞分化的第一周内发生并运作。然而,虽然 SR-TT 连接的早期发育与新生肌原纤维的发育相协调,但它们各自的成熟并不协调。典型三联体的形成需要其他因素/条件,在使用体外模型探索骨骼肌疾病时,特别是那些影响 E-C 偶联的疾病时,应考虑到这一点。
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