| Abstract: | Differential intensity of fluorescence corresponding to the banding patterns found in single metaphases can be obtained with isolated Chinese hamster chromosomes using the fluorochrome Hoechst 33258. Removal of histones from the chromosomes with 0.2 N HCl causes an approx. 50% increase in overall size, but does not abolish the gross metaphase morphology of the chromosomes or the ability to give their characteristic fluorescent banding patterns. In an attempt to study further the factors maintaining the characteristic metaphase structure, we have treated acid-extracted isolated chromosomes with DNase I, which was found to solubilize over 99% of the DNA content, while leaving stable ‘core’ structures which retain the basic features of metaphase chromosomes such as centromeric regions and defined chromatids. The cores appear to consist mainly of non-histone protein: they are destroyed by proteolytic action and unaffected by ribonuclease A. The structural implications of these findings are discussed. |
