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Preparation of developing Xenopus muscle for sarcomeric protein localization by high-resolution imaging

机译:通过高分辨率成像制备用于爪肌蛋白定位的非洲爪蟾发育中的肌肉

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Mutations in several sarcomeric proteins have been linked to various human myopathies. Therefore, having an in vivo developmental model available that develops quickly and efficiently is key for investigators to elucidate the critical steps, components and signaling pathways involved in building a myofibril; this is the pivotal foundation for deciphering disease mechanisms as well as the development of myopathy-related therapeutics. Although striated muscle cell culture studies have been extremely informative in providing clues to both the distribution and functions of sarcomeric proteins, myocytes in vivo develop in an irreproducible 3D environment. Xenopus laevis (frog) embryos are cost effective, compliant to protein level manipulations and develop relatively quickly (≤ a week) in a petri dish, thus providing a powerful system for de novo myofibrillogenesis studies. Although fluorophore-conjugated phalloidin labeling is the gold standard approach for investigating actin-thin filament architecture, it is well documented that phalloidin-labeling can be challenging and inconsistent within Xenopus embryos. Therefore we highlight several techniques that can be utilized to preserve both antibody and fluorophore-conjugated phalloidin labeling within Xenopus embryos for high-resolution fluorescence microscopy.
机译:几种肌节蛋白的突变与多种人类肌病有关。因此,对于研究人员阐明构建肌原纤维所涉及的关键步骤,成分和信号传导途径,关键在于拥有一个快速有效地体内发育模型。这是破译疾病机制以及开发与肌病相关的疗法的关键基础。尽管横纹肌细胞培养研究在提供有关肌节蛋白的分布和功能方面的线索方面提供了极为丰富的信息,但体内的肌细胞却在不可复制的3D环境中发育。非洲爪蟾(青蛙)胚胎具有成本效益,符合蛋白质水平操作,并且在培养皿中发育相对较快(≤一周),因此为新生肌纤维形成研究提供了强大的系统。尽管荧光团缀合的鬼笔环肽标记法是研究肌动蛋白细丝结构的金标准方法,但有充分的文献证明,鬼笔环肽标记法在非洲爪蟾胚胎中可能具有挑战性和不一致之处。因此,我们重点介绍了可用于在非洲爪蟾胚胎内保留抗体和与荧光团偶联的鬼笔环肽标记的几种技术,用于高分辨率荧光显微镜检查。

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