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Measurement of thin filament lengths by distributed deconvolution analysis of fluorescence images.

机译:通过荧光图像的分布式反卷积分析来测量细丝长度。

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摘要

The lengths of the actin (thin) filaments in sarcomeres directly influence the physiological properties of striated muscle. Although electron microscopy techniques provide the highest precision and accuracy for measuring thin filament lengths, significant obstacles limit their widespread use. Here, we describe distributed deconvolution, a fluorescence-based method that determines the location of specific thin filament components such as tropomodulin (Tmod) or probes such as phallacidin (a phalloidin derivative). Using Tmod and phallacidin fluorescence, we were able to determine the thin filament lengths of isolated chicken pectoralis major myofibrils with an accuracy and precision comparable to electron microscopy. Additionally, phallacidin fluorescence intensity at the Z line provided information about the width of Z lines. Furthermore, we detected significant variations in thin filaments lengths among individual myofibrils from chicken posterior latissimus dorsai and embryonic chick cardiac myocytes, suggesting that a ruler molecule (e.g., nebulin) does not strictly determine thin filament lengths in these muscles. This versatile method is applicable to myofibrils in living cells that exhibit significant variation in sarcomere lengths, and only requires a fluorescence microscope and a CCD camera.
机译:肉瘤中肌动蛋白(细)丝的长度直接影响横纹肌的生理特性。尽管电子显微镜技术为测量细丝长度提供了最高的精度和准确度,但是明显的障碍限制了它们的广泛使用。在这里,我们描述了分布式反卷积,这是一种基于荧光的方法,用于确定特定细丝成分(例如原代调节蛋白(Tmod))或探针(如鬼笔环肽(鬼笔环肽衍生物))的位置。使用Tmod和Phallacidin荧光,我们能够确定分离的鸡胸大肌主要肌原纤维的细丝长度,其准确性和精密度可与电子显微镜媲美。另外,在Z线的鬼笔环肽荧光强度提供了关于Z线宽度的信息。此外,我们检测到了鸡背阔肌和胚胎鸡心肌细胞的单个肌原纤维中细丝长度的显着变化,这表明标尺分子(例如,星云蛋白)不能严格确定这些肌肉中的细丝长度。这种通用的方法适用于活细胞中的肌原纤维,肌纤维长度在肌节长度上有显着变化,只需要荧光显微镜和CCD照相机即可。

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