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通过Nomarski干涉显微镜和扫描电子显微镜对姐妹染色单体差异染色进行的拓扑学检查。

Topographic examination of sister chromatid differential staining by Nomarski interference microscopy and scanning electron microscopy.

作者信息

Takayama S, Utsumi K R, Sasaki Y

出版信息

Chromosoma. 1981;82(1):113-9. doi: 10.1007/BF00285754.

Abstract

BrdU-substituted Chinese hamster chromosomes were treated with a hog Na2HPO4 solution and stained with Giemsa to produce sister chromatid differential staining (SCD). The process of SCD was examined with the Nomarski differential interference microscope and the scanning electron microscope. After the Na2HPO4 treatment alone, unifilarly BrdU-substituted (TB) chromatids appeared somewhat more severely collapsed than the bifilarly substituted (BB) chromatids. Subsequent Giemsa staining, however, brought about pronounced piling up of the Giemsa dye on the TB-chromatids but not on the BB-ones, causing highly distinct differential Giemsa staining as well as a marked differentiation in surface topography between the sister chromatids. Removal of the Giemsa dye from the differentially Giemsa stained chromosomes resulted in a disappearance of such a pronounced topographic differentiation.

摘要

用猪的Na2HPO4溶液处理经BrdU替代的中国仓鼠染色体,并用吉姆萨染色以产生姐妹染色单体差异染色(SCD)。用Nomarski微分干涉显微镜和扫描电子显微镜检查SCD过程。单独用Na2HPO4处理后,单链BrdU替代(TB)的染色单体似乎比双链替代(BB)的染色单体塌陷得更严重。然而,随后的吉姆萨染色导致吉姆萨染料在TB染色单体上大量堆积,而在BB染色单体上则没有,从而产生高度明显的吉姆萨差异染色以及姐妹染色单体之间表面形貌的显著差异。从吉姆萨差异染色的染色体上去除吉姆萨染料会导致这种明显的形貌差异消失。

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