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肝细胞的福尔根-萘酚黄S细胞光度测定法。甲醛诱导的收缩对细胞核萘酚黄S结合的影响。

Feulgen-Naphthol Yellow S cytophotometry of liver cells. The effect of formaldehyde induced shrinkage on nuclear Naphthol Yellow S binding.

作者信息

Gaub J

出版信息

Histochemistry. 1976 Nov 12;49(4):293-301. doi: 10.1007/BF00496132.

Abstract
  1. In isolated liver cells, fixed in 4 per cent formaldehyde (NFS) for Feulgen-Naphthol Yellow S (F-NYS) staining of DNA and protein, nuclear shrinkage increases the nuclear concentration of solids to 46 per cent (w/v) before the start of the NYS staining. 2. When a fixative mixture of methanol:acetic acid:formalin (85:5:10 by volume; MAF) is used, the concentration of nuclear solids during NYS staining remain at a physiological level of 19 per cent. 3. By exposing liver cells to NFS for 10 to 120 seconds before fixation in MAF, increasing nuclear shrinkage can be induced with increasing pretreatment in NFS. Nuclear NYS binding decreases in parallel with the decreasing nuclear volume in cells thus treated. As the shrinkage induced reduction in NYS binding may vary with the net charge of nuclear non-histone proteins, MAF fixation must be preferred for quantitative determinations of nuclear non-histone protein in F-NYS stained, isolated cells. 4. Fixation in MAF offers the same advantages as NFS fixation as regards the small loss of proteins during the Feulgen staining procedure and the excellent reproducibility of the F-NYS staining. Storage of MAF fixed cells in the fixative for a few days does not alter their F-NYS staining properties. 5. In MAF fixed, F-NYS stained cells there is no NYS binding to histone basic amino acid residues.
摘要
  1. 在分离的肝细胞中,用4%甲醛(NFS)固定以进行DNA和蛋白质的福尔根-萘酚黄S(F-NYS)染色,在NYS染色开始前,核收缩使核内固体物质浓度增加到46%(w/v)。2. 当使用甲醇:乙酸:福尔马林(体积比85:5:10;MAF)的固定剂混合物时,NYS染色期间核内固体物质浓度保持在19%的生理水平。3. 在MAF固定前将肝细胞暴露于NFS中10至120秒,随着在NFS中预处理时间增加,可诱导核收缩增加。如此处理的细胞中,核NYS结合与核体积减小平行下降。由于收缩诱导的NYS结合减少可能因核非组蛋白的净电荷而异,对于F-NYS染色的分离细胞中核非组蛋白的定量测定,MAF固定必须是首选。4. 在福尔根染色过程中蛋白质损失小以及F-NYS染色具有出色的可重复性方面,MAF固定与NFS固定具有相同的优势。将MAF固定的细胞在固定剂中储存几天不会改变其F-NYS染色特性。5. 在MAF固定、F-NYS染色的细胞中,NYS不与组蛋白碱性氨基酸残基结合。

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