Banchev T B, Srebreva L N, Zlatanova J S
Institute of Molecular Biology, Bulgarian Academy of Sciences, Sofia.
Mol Cell Biochem. 1990 Jun 25;95(2):167-75. doi: 10.1007/BF00219975.
The aim of this work was to study the accessibility of histone H1(0) and its structural domains to antibody binding in high molecular mass chromatin fragments of different conformations. Three types of specific antibody populations were used: (1) anti-H1(0) which reacted with antigenic determinants situated along the whole polypeptide chain, (2) anti-GH5 or anti-GH1(0) which recognized epitopes located in the globular region of H1(0) and (3) anti-C-tail antibodies reacting specifically with fragment 99-193 of the protein molecule. The immunoreactivity of the chromatin-bound antigen was investigated by solid-phase ELISA performed on glutaraldehyde-cross-linked chromatin and by an inhibition assay carried out with native chromatin in solution. The results of both methods were unidirectional and showed that: (1) the accessibility of H1(0) did not change with the compaction of the fiber; (2) the G-domain was not accessible to antibodies either in the relaxed or in the condensed state of the fragments, (3) the binding of the C-terminus-specific antibodies was different for isolated monosomes and for the chromatin fiber and (4) the degree of exposure of the epitopes of H1(0) in chromatin was much less than that of histone H1.
这项工作的目的是研究组蛋白H1(0)及其结构域在不同构象的高分子量染色质片段中与抗体结合的可及性。使用了三种类型的特异性抗体群体:(1) 与沿整个多肽链分布的抗原决定簇反应的抗H1(0),(2) 识别位于H1(0)球状区域的表位的抗GH5或抗GH1(0),以及 (3) 与蛋白质分子的99 - 193片段特异性反应的抗C末端抗体。通过对戊二醛交联染色质进行的固相ELISA以及对溶液中的天然染色质进行的抑制试验,研究了染色质结合抗原的免疫反应性。两种方法的结果都是单向的,并且表明:(1) H1(0)的可及性不会随纤维的压缩而改变;(2) 在片段的松弛或浓缩状态下,抗体都无法接近G结构域;(3) 分离的单核小体和染色质纤维对C末端特异性抗体的结合情况不同;(4) H1(0)在染色质中的表位暴露程度远低于组蛋白H1。