Excitation-Contraction Coupling in Normal and Dystrophic Mammalian Muscle

正常和营养不良哺乳动物肌肉的兴奋-收缩耦合

• 批准号: 8019077
• 负责人: Julio L Vergara
• 金额: $ 32.2万
• 依托单位: UNIVERSITY OF CALIFORNIA LOS ANGELES
• 依托单位国家: 美国
• 财政年份: 2003
• 资助国家: 美国
• 起止时间: 2003-04-01 至 2014-01-31
• 项目状态: 已结题
• 来源: https://reporter.nih.gov/project-details/8019077
• 关键词: Action Potentials; Adult; Affect; Animal Model; Animals; Attenuated; Benign; Buffers; Calsequestrin; Cells; Characteristics; Complex; Coupling; Data; Development; Duchenne muscular dystrophy; Dystroglycan; Dystrophin; Egtazic Acid; Electric Stimulation; Electroporation; Energy Transfer; Fiber; Fluorescence Microscopy; Fostering; Foundations; Glycoproteins; Goals; Health; Hereditary Disease; Human; Impairment; Investigation; Knock-out; Laser Scanning Microscopy; Life; Link; Measurement; Membrane; Modeling; Molecular; Mus; Muscle; Muscle Fibers; Muscle Weakness; Muscular Dystrophies; Mutation; Myopathy; Optical Methods; Optics; Other Genetics; Pathology; Patients; Phenotype; Photons; Physiologic pulse; Physiological; Positioning Attribute; Process; Proteins; Relative (related person); Role; RyR1; SERCA1; Sarcoglycans; Sarcolemma; Sarcoplasmic Reticulum; Signal Transduction; Skeletal Muscle; Structure; Surface; System; Techniques; Testing; Therapeutic; Transgenic Animals; Transgenic Organisms; Tubular formation; Utrophin; gene therapy; human SSPN protein; in vivo; mdx mouse; mini-dystrophin; nanoscale; novel; overexpression; protein complex; research study; response; tool; two-photon; voltage clamp

DESCRIPTION (provided by applicant): The overall goal of this proposal is to obtain an in-depth understanding of the mechanistic links between alterations of the dystrophin glycoprotein complex (DGC) and impairment of the excitation-contraction coupling (ECC) process in mammalian skeletal muscle. This functional characterization will be achieved in muscle fibers from various animal models of human muscular dystrophies. We have found that Ca2+ release evoked by action potentials (APs) (or voltage-clamp pulses) in muscle fibers from two of such models, the adult mdx mouse and the phenotypic sarcospan (SSPN) overexpressing mouse (SSPN-Tg), is significantly smaller than in wild type fibers. We hypothesize that disruption of the DGC undermines the structural and functional support for the transverse tubular system (TTS) and the sarcoplasmic reticulum (SR), thus attenuating the ECC process. We will first investigate the mechanisms responsible for the impairment of Ca2+ release in mdx mice (Aim 1), the most prevalently used animal model for Duchenne Muscular Dystrophy (DMD), which lacks dystrophin in the DGC. However, since the phenotypic alterations in mdx mice are relatively benign, possibly due to utrophin substitution in the DGC, experiments will be also carried out in double knockout mdx/utrophin (mdx/utr-/-) mice that display a phenotype more comparable to that in DMD patients (Aim 2). To further characterize the link between the DGC integrity and a fully functional ECC, we will take advantage of our ability to express DGC proteins by in vivo electroporation and use transgenic animal models with other genetic conditions altering the DGC (e.g. SSPN-Tg, and Utr-TET). The last goal of the proposal is to investigate, using 2-photon laser scanning microscopy (TPLSM) the subcellular distribution of representative DGC protein components in order to assess if they are associated exclusively with the sarcolemma or if they have a more ubiquitous distribution in association with the Z-line and the TTS. This characterization will help us understand the function of the DGC in terms of ECC and sarcolemmal integrity (Aim 3). These investigations will be carried out by using electrophysiological and state-of-the-art optical methods, such as F"ster resonance energy transfer (FRET) and total internal reflection fluorescence microscopy (TIRFM), to also assess the nanoscale localization of DGC and ECC proteins with respect to the internal and external leaflets of the surface and TTS membranes. PUBLIC HEALTH RELEVANCE: In Duchenne Muscular Dystrophy (DMD) the muscles lack the protein dystrophin, an integral component of a dystrophin-glycoprotein complex (DGC). We have discovered that the absence of dystrophin in the muscle fibers of the mdx mouse, a widely used animal model of DMD, impairs their ability to release Ca2+ from the sarcoplasmic reticulum in response to electrical stimulation, thus explaining the muscle weakness observed in the DGC pathology. We now propose to investigate the mechanisms that link DGC alterations with a deficient Ca2+ release. The results will significantly broaden our understanding of muscle disease mechanisms and will potentially provide therapeutic molecular tools which are deemed necessary for further advances in gene therapy.

描述（由申请人提供）：本提案的总体目标是深入了解哺乳动物骨骼肌中肌营养不良蛋白糖蛋白复合物（DGC）改变与兴奋-收缩偶联（ECC）过程受损之间的机制联系。该功能表征将在来自人肌营养不良症的各种动物模型的肌纤维中实现。我们已经发现，由动作电位（AP）（或电压钳脉冲）在两个这样的模型，成年mdx小鼠和表型sarcospan（SSPN）过表达小鼠（SSPN-Tg）的肌纤维中诱发的Ca 2+释放，是显着小于野生型纤维。我们假设DGC的破坏破坏了横管系统（TTS）和肌浆网（SR）的结构和功能支持，从而减弱ECC过程。我们将首先研究mdx小鼠（目的1）中Ca 2+释放受损的机制，mdx小鼠是杜氏肌营养不良症（DMD）最常用的动物模型，DGC中缺乏肌营养不良蛋白。然而，由于mdx小鼠中的表型改变相对良性，可能是由于DGC中的utrophin取代，因此还将在显示出与DMD患者更相似的表型的双敲除mdx/utrophin（mdx/utr-/-）小鼠中进行实验（目的2）。为了进一步表征DGC完整性和全功能ECC之间的联系，我们将利用我们通过体内电穿孔表达DGC蛋白的能力，并使用具有改变DGC的其他遗传条件（例如SSPN-Tg和Utr-TET）的转基因动物模型。该提案的最后一个目标是使用双光子激光扫描显微镜（TPLSM）研究代表性DGC蛋白组分的亚细胞分布，以评估它们是否仅与肌膜相关，或者它们是否具有与Z线和TTS相关的更普遍的分布。这种表征将帮助我们理解DGC在ECC和肌膜完整性方面的功能（目的3）。这些研究将通过使用电生理学和最先进的光学方法进行，例如F“ster共振能量转移（FRET）和全内反射荧光显微镜（TIRFM），以评估DGC和ECC蛋白相对于表面和TTS膜的内部和外部小叶的纳米级定位。 公共卫生相关性：在杜氏肌营养不良症（DMD）中，肌肉缺乏肌营养不良蛋白，肌营养不良蛋白-糖蛋白复合物（DGC）的组成部分。我们已经发现，mdx小鼠（一种广泛使用的DMD动物模型）的肌纤维中肌营养不良蛋白的缺乏损害了它们响应于电刺激从肌浆网释放Ca 2+的能力，从而解释了在DGC病理学中观察到的肌无力。我们现在建议研究DGC改变与Ca 2+释放不足的机制。这些结果将大大拓宽我们对肌肉疾病机制的理解，并可能为基因治疗的进一步发展提供必要的治疗分子工具。