An argyrophil III method for the demonstration of micro- and oligodendroglia.

F Gallyas
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Abstract

Micro- and oligodendroglia, plasma and nucleoli of nerve cells, capillary wall and nuclei of astrocytes become visible when sections of formol fixed human brain are immersed, without any previous treatment, into a physical developer of pH 10.5. The staining is inhibited by the catalytic activity of the tissue elements involved. By means of pretreatments with 1% performic acid and 30% sodium rhodanide dissolved in 0.4% sodium hydroxide, the catalytic activity in the unwanted tissue elements is suppressed, and this results in an elective demonstration of micro- and oligodendroglia. Reducing groups of the tissue or any kind of performed nuclei play no role in this silver staining.

一种微胶质细胞和少突胶质细胞的显示方法。
将福尔摩固定的人脑切片不经任何处理,浸入pH为10.5的物理显影剂中,可以看到微胶质细胞和少突胶质细胞、神经细胞的血浆和核仁、毛细血管壁和星形胶质细胞的细胞核。染色被所涉及的组织元素的催化活性所抑制。通过1%甲酸和30% rhodanide钠溶解于0.4%氢氧化钠的预处理,抑制了对不需要的组织元素的催化活性,这导致了微胶质细胞和少突胶质细胞的选择性展示。组织的还原基团或任何类型的细胞核在银染色中不起作用。
本文章由计算机程序翻译,如有差异,请以英文原文为准。
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