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Usage of a Localised Microflow Device to Show that Mitochondrial Networks Are Not Extensive in Skeletal Muscle Fibres

机译:使用本地化的微流设备显示骨骼肌纤维中的线粒体网络并不广泛

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摘要

In cells, such as neurones and immune cells, mitochondria can form dynamic and extensive networks that change over the minute timescale. In contrast, mitochondria in adult mammalian skeletal muscle fibres show little motility over several hours. Here, we use a novel three channelled microflow device, the multifunctional pipette, to test whether mitochondria in mouse skeletal muscle connect to each other. The central channel in the pipette delivers compounds to a restricted region of the sarcolemma, typically 30 µm in diameter. Two channels on either side of the central channel use suction to create a hydrodynamically confined flow zone and remove compounds completely from the bulk solution to internal waste compartments. Compounds were delivered locally to the end or side of single adult mouse skeletal muscle fibres to test whether changes in mitochondrial membrane potential were transmitted to more distant located mitochondria. Mitochondrial membrane potential was monitored with tetramethylrhodamine ethyl ester (TMRE). Cytosolic free [Ca2+] was monitored with fluo-3. A pulse of carbonyl cyanide 4-(trifluoromethoxy) phenylhydrazone (FCCP, 100 µM) applied to a small area of the muscle fibre (30 µm in diameter) produced a rapid decrease in the mitochondrial TMRE signal (indicative of depolarization) to 38% of its initial value. After washout of FCCP, the TMRE signal partially recovered. At distances greater than 50 µm away from the site of FCCP application, the mitochondrial TMRE signal was unchanged. Similar results were observed when two sites along the fibre were pulsed sequentially with FCCP. After a pulse of FCCP, cytosolic [Ca2+] was unchanged and fibres contracted in response to electrical stimulation. In conclusion, our results indicate that extensive networks of interconnected mitochondria do not exist in skeletal muscle. Furthermore, the limited and reversible effects of targeted FCCP application with the multifunctional pipette highlight its advantages over bulk application of compounds to isolated cells.
机译:在神经元和免疫细胞等细胞中,线粒体可以形成动态且广泛的网络,这些网络会在几分钟内变化。相比之下,成年哺乳动物骨骼肌纤维中的线粒体在几个小时内几乎没有运动。在这里,我们使用一种新型的三通道微流装置多功能移液管,测试小鼠骨骼肌中的线粒体是否相互连接。移液器中的中央通道将化合物输送到肉瘤的狭窄区域,直径通常为30 µm。中央通道两侧的两个通道利用吸力形成流体力学上受约束的流动区域,并将化合物从大体积溶液中完全清除到内部废物室。将化合物局部递送至单只成年小鼠骨骼肌纤维的末端或侧面,以测试线粒体膜电位的变化是否传递至更远的线粒体。用四甲基罗丹明乙酯(TMRE)监测线粒体膜电位。用fluo-3监测无胞质的[Ca 2 + ]。在肌肉纤维的小面积(直径为30 µm)上施加羰基氰化物4-(三氟甲氧基)苯基)(FCCP,100 µM)脉冲可使线粒体TMRE信号(指示去极化)迅速降低至38%。它的初始值。清除FCCP后,TMRE信号部分恢复。在距FCCP应用部位大于50 µm的距离处,线粒体TMRE信号保持不变。当沿光纤的两个位置依次用FCCP脉冲时,观察到相似的结果。 FCCP脉冲后,胞质[Ca 2 + ]保持不变,并且纤维在电刺激下收缩。总之,我们的结果表明骨骼肌中不存在相互连接的线粒体的广泛网络。此外,多功能移液管靶向FCCP应用的局限性和可逆性突出了其相对于将化合物批量应用到分离细胞的优势。

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