在同一个PtK2细胞中通过免疫荧光和电子显微镜观察到的单个微管。
Individual microtubules viewed by immunofluorescence and electron microscopy in the same PtK2 cell.
作者信息
Osborn M, Webster R E, Weber K
出版信息
J Cell Biol. 1978 Jun;77(3):R27-34. doi: 10.1083/jcb.77.3.r27.
Abstract
PtK2 cells were grown on gold grids and treated with Triton X-100 in a microtubule stabilizing buffer. The resulting cytoskeletons were fixed with glutaraldehyde and subjected to the indirect immunofluorescence procedure using monospecific tubulin antibodies. Grids were examined first by fluorescence microscopy, and the display of fluorescent cytoplasmic microtubules was recorded. The grids were then stained with uranyl acetate and the display of fibrous structures recorded by electron microscopy. Thus the display of cytoplasmic microtubular structures in the light microscope and the electron microscope can be compared within the same cytoskeleton. The results show a direct correspondence of the fluorescent fibers in the light microscope with uninterrupted fibers of diameter approximately 550 A in the electron microscope. This is the diameter reported for a single microtubule decorated around its circumference by two layers of antibody molecules. Thus under optimal conditions immunofluorescence microscopy can visualize individual microtubules.
摘要
PtK2细胞在金网上生长,并在微管稳定缓冲液中用Triton X-100处理。将所得的细胞骨架用戊二醛固定,并使用单特异性微管蛋白抗体进行间接免疫荧光程序。首先通过荧光显微镜检查网格,并记录荧光细胞质微管的显示情况。然后将网格用醋酸铀染色,并通过电子显微镜记录纤维结构的显示情况。因此,可以在同一细胞骨架内比较光学显微镜和电子显微镜下细胞质微管结构的显示情况。结果表明,光学显微镜下的荧光纤维与电子显微镜下直径约550埃的不间断纤维直接对应。这是单层微管周围由两层抗体分子修饰的报道直径。因此,在最佳条件下,免疫荧光显微镜可以观察到单个微管。
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