电子显微镜对含核酸结构的优先染色。

H E HUXLEY, G ZUBAY
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引用次数: 372

摘要

将提取的核组蛋白取向纤维作为试验材料,对含有高比例核酸的结构进行满意的固定、包埋和染色方法的研究。固定在pH值为6的缓冲四氧化锇溶液中,其中含有10(-2)M Ca(++),并包埋在alalite中,可以切割纤维的部分,其中的取向得到很好的保存。这些可以在2%醋酸铀酰水中强烈染色,并显示出相当精细的结构。整个胸腺组织核的某些区域也可以用同样的方法染色,并且与相邻切片的Feulgen法染色的区域相同。此外,发现纯化的DNA从2%的水溶液中几乎吸收了其自身干重的醋酸铀酰。在极短的固定时间内(0℃下5分钟左右),整个组织的染色效果最强。用醋酸铀酰染色后,用氢氧化铅进一步染色,整个组织的染色效果尤其明显。虽然单独使用氢氧化铅和醋酸铀酰的染色模式在固定时间较长的组织中是相似的((1/2小时至2小时,在0℃或20℃下),但在短暂固定的材料中,含有dna的区域相对来说没有被氢氧化铅单独染色,而含有rna的结构通常有明显的染色。还描述了用类似技术对某些病毒染色的观察结果。
本文章由计算机程序翻译,如有差异,请以英文原文为准。
Preferential staining of nucleic acid-containing structures for electron microscopy.

Oriented fibres of extracted nucleohistone were employed as test material in a study of satisfactory fixation, embedding, and staining methods for structures containing a high proportion of nucleic acid. Fixation in buffered osmium tetroxide solution at pH 6, containing 10(-2)M Ca(++), and embedding in Araldite enabled sections of the fibres to be cut in which the orientation was well preserved. These could be strongly stained in 2 per cent aqueous uranyl acetate, and showed considerable fine structure. Certain regions in the nuclei of whole thymus tissue could also be strongly stained by the same procedure, and were identical with the regions stained by the Feulgen procedure in adjacent sections. Moreover, purified DNA was found to take up almost its own dry weight of uranyl acetate from 2 per cent aqueous solution. Strongest staining of whole tissue was obtained with very short fixation times-5 minutes or so at 0 degrees C. Particularly intense staining was obtained when such tissue stained in uranyl acetate was further stained with lead hydroxide. Although the patterns of staining by lead hydroxide alone and by uranyl acetate were similar in tissues fixed for longer times ((1/2) hour to 2 hours, at 0 degrees C or 20 degrees C), in briefly fixed material the DNA-containing regions appeared relatively unstained by lead hydroxide alone, whilst often there was appreciable staining of RNA-containing structures. Observations on the staining of some viruses by similar techniques are also described.

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