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染色体显带机制。VII. 亚甲蓝与DNA和染色质的相互作用。

Mechanisms of chromosome banding. VII. Interaction of methylene blue with DNA and chromatin.

作者信息

Comings D E, Avelino E

出版信息

Chromosoma. 1975 Aug 11;51(4):365-79. doi: 10.1007/BF00326323.

Abstract

The binding of methylene blue to DNA and chromatin treated in various ways was examined by equilibrium dialysis. The maximum r value (moles of bound dye/mole of nucleotide) was 1.0 for DNA, 0.6 for unfixed chromatin, and 0.83 for chromatin fixed in methanol-acetic acid. When fixed chromatin was treated with saline-citrate at 60 degrees C for 3 hours, as used for G-banding chromosomes, the r value decreased from 0.83 to 0.55. When unfixed chromatin was treated as for R-banding the r values also dropped. Equilibrium dialysis indicated there was no disproportionate increase of dye binding as the concentration of DNA increased. -- These results, and others, suggest that some of the Giemsa negative regions of G- and R-banded chromosomes are due to the denaturation of non-histone proteins so that they more effectively cover the DNA and prevent side binding of the thiazin dyes.

摘要

通过平衡透析法检测了亚甲蓝与经不同方式处理的DNA和染色质的结合情况。DNA的最大r值(结合染料的摩尔数/核苷酸的摩尔数)为1.0,未固定染色质的为0.6,甲醇-乙酸固定的染色质的为0.83。当如用于G显带染色体那样,将固定染色质在60℃用柠檬酸盐缓冲液处理3小时时,r值从0.83降至0.55。当未固定染色质按R显带处理时,r值也下降。平衡透析表明,随着DNA浓度增加,染料结合没有不成比例的增加。——这些结果以及其他结果表明,G带和R带染色体的一些吉姆萨阴性区域是由于非组蛋白的变性,从而使其更有效地覆盖DNA并阻止噻嗪染料的侧链结合。

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