Electron microscopic specimen preparation from low concentration of cell suspension using cytospin technique.

Y Sasaki, Y Norose, A Adachi, S Sato
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Abstract

Electron microscopic examinations are sometimes limited due to the small number of cells available for analysis. The purpose of this study was to determine the limit of cell concentration for a successful transmission electron microscopic preparation. Various concentrations of monocyte cell suspension were fixed in glutaraldehyde and osmium tetroxide according to the standard methods. Cell preparations were made on silane-coated glass slides in a cytospin centrifuge. The attached cells to the glass slides were dehydrated, and embedded in epoxy resin by routine electron microscopic technique. By this method, cell suspensions containing as low as 2x10(3) cells could show approximately 5 to 10 cells in each hole of the 150-mesh grids which was designated as the lowest limit for the successful preparation with detectable cells for evaluation. The fine structure of cells was clearly evident and the preparations were uniformly free from artifacts, similar or superior to those of cell pellet preparations. This method is useful whenever dealing with the samples containing a low number of cells, particularly those of clinical samples.

用细胞自旋技术制备低浓度细胞悬浮液的电镜标本。
由于可用于分析的细胞数量少,电子显微镜检查有时受到限制。本研究的目的是确定成功的透射电子显微镜制备的细胞浓度极限。将不同浓度的单核细胞悬浮液按标准方法固定在戊二醛和四氧化二锇中。在细胞自旋离心机中,在硅烷涂覆的玻片上制备细胞。将附着于玻片上的细胞脱水,用常规电镜技术包埋在环氧树脂中。通过这种方法,含有低至2 × 10(3)个细胞的细胞悬液可以在150网格的每个孔中显示大约5到10个细胞,这被指定为成功制备可检测细胞的最低限度。细胞的精细结构清晰明显,制备的制剂均匀无伪影,类似或优于细胞颗粒制剂。这种方法适用于处理细胞数量较少的样品,特别是临床样品。
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