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利用荧光显微镜技术研究培养的分化期鸡胚骨骼肌细胞的膜动力学。

Membrane dynamics of differentiating cultured embryonic chick skeletal muscle cells by fluorescence microscopy techniques.

作者信息

Elson H F, Yguerabide J

出版信息

J Supramol Struct. 1979;12(1):47-61. doi: 10.1002/jss.400120106.

Abstract

Changes in membrane fluidity during myogenesis have been studied by fluorescence microscopy of individual cells growing in monolayer cultures of embryonic chick skeletal muscle cells. Membrane fluidity was determined by the techniques of fluorescence photobleaching recovery (FPR), with the use of a lipid-soluble carbocyanine dye, and by fluorescence depolarization (FD), with perylene used as the lipid probe. The fluidity of myoblast plasma membranes, as determined from FPR measurements in membrane areas above nuclei, increased during the period of myoblast fusion and then returned to its initial level. The membrane fluidity of fibroblasts, also found in these primary cultures, remained constant. The fluidity in specific regions along the length of the myoblast membrane was studied by FD, and it was observed that the extended arms of the myoblast have the highest fluidity on the cell and that the tips at the ends of the arms had the lowest fluidity. However, since the perylene probe used in the FD experiments appeared to label cytoplasmic components, changes in fluidity measured with this probe reflect changes in membrane fluidity as well as in cytoplasmic fluidity. The relative change in each of these compartments cannot yet be ascertained. Tips have specialized surface structures, filopodia and lamellipodia, which may be accompanied by a more immobile membrane as well as a more rigid cytoplasm. Rounded cells, which may also have a more convoluted surface structure, show a lower apparent membrane fluidity than extended cells.

摘要

通过对在胚胎鸡骨骼肌细胞单层培养物中生长的单个细胞进行荧光显微镜观察,研究了肌生成过程中膜流动性的变化。膜流动性通过荧光光漂白恢复(FPR)技术(使用脂溶性羰花青染料)和荧光去极化(FD)技术(使用苝作为脂质探针)来测定。根据细胞核上方膜区域的FPR测量结果,成肌细胞质膜的流动性在成肌细胞融合期间增加,然后恢复到初始水平。在这些原代培养物中也发现的成纤维细胞质膜的流动性保持恒定。通过FD研究了成肌细胞膜长度上特定区域的流动性,观察到成肌细胞的伸展臂在细胞上具有最高的流动性,而臂末端的尖端具有最低的流动性。然而,由于FD实验中使用的苝探针似乎标记了细胞质成分,用该探针测量的流动性变化反映了膜流动性以及细胞质流动性的变化。这些隔室中每一个的相对变化尚无法确定。尖端具有特殊的表面结构,丝状伪足和片状伪足,这可能伴随着更不流动的膜以及更刚性的细胞质。圆形细胞可能也具有更复杂的表面结构,其表观膜流动性低于伸展细胞。

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