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Measurement of Instantaneous Velocity Vectors of Organelle Transport: Mitochondrial Transport and Bioenergetics in Hippocampal Neurons

机译:细胞器运输的瞬时速度矢量的测量:线粒体运输和海马神经元中的生物能。

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摘要

Impaired transport of mitochondria, in dendrites and axons of neurons, and bioenergetic deficit are increasingly recognized to be of pathological importance in neurodegenerative diseases. To study the relationship between transport and bioenergetics, we have developed what to our knowledge is a novel technique to quantify organelle velocity in cultured cells. The aim was to combine measurement of motion and bioenergetic parameters while minimizing photodynamic oxidative artifacts evoked by fluorescence excitation. Velocity determination from sequential fluorescence images is not trivial, and here we describe an application of “optical flow”, the flow of gray values in grayscale images, to this problem. Based on the principles of photon shot noise occurring in low light level fluorescence microscopy, we describe and validate here an optical flow-based, robust method to measure velocity vectors for organelles expressing fluorescent proteins. This method features instantaneous velocity determination from a pair of images by detecting motion of edges, with no assumptions about the separation or shapes of the objects in the image. Optical flow was used in combination with single mitochondrion assay of mitochondrial thiol redox status by mitochondrially targeted redox-sensitive green fluorescent protein and measurement of mitochondrial membrane potential by tetramethylrhodamine methyl ester. Mitochondrial populations of resting cultured hippocampal neurons were analyzed. It was found that mitochondria with more oxidized thiol redox status have lower membrane potentials and are smaller in size. These mitochondria are more motile than the average; however, mitochondrial motility is only slightly dependent on the observed bioenergetic parameters and is correlated the best to the size of the mitochondria.
机译:人们越来越认识到,在神经元的树突和轴突中线粒体的运输受损以及生物能缺陷在神经退行性疾病中具有重要的病理学意义。为了研究运输与生物能学之间的关系,我们已经开发出一种据我们所知的量化培养细胞中细胞器速度的新技术。目的是将运动和生物能参数的测量结合起来,同时将荧光激发引起的光动力氧化伪影降至最低。从顺序荧光图像确定速度并非易事,这里我们描述了“光流”(灰度图像中灰度值的流)对这个问题的应用。基于低光水平荧光显微镜中发生的光子散粒噪声的原理,我们在此描述和验证一种基于光流的鲁棒方法,用于测量表达荧光蛋白的细胞器的速度向量。该方法的特征是通过检测边缘的运动从一对图像中即时确定速度,而无需假设图像中对象的分离或形状。光流与线粒体靶向氧化还原敏感的绿色荧光蛋白的线粒体硫醇氧化还原状态的单线粒体检测结合,并通过四甲基若丹明甲酯测量线粒体膜电位。分析了静息培养的海马神经元的线粒体种群。发现具有更高氧化硫醇氧化还原状态的线粒体具有较低的膜电位并且尺寸较小。这些线粒体比平均线粒体更有活力。然而,线粒体的运动性仅略微取决于所观察到的生物能参数,并且与线粒体的大小最相关。

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