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与细胞核和质膜均发生反应的人类自身抗体在高盐条件下对组蛋白H2A、H2B、H3和H4的八聚体表现出特异性。

Human autoantibodies that react with both cell nuclei and plasma membranes display specificity for the octamer of histones H2A, H2B, H3, and H4 in high salt.

作者信息

Rekvig O P, Hannestad K

出版信息

J Exp Med. 1980 Dec 1;152(6):1720-33. doi: 10.1084/jem.152.6.1720.

Abstract

Sera of some patients with systemic lupus erythematosus and related diseases contain a polyclonal antibody population (cross-reactive antinuclear antibodies [X-ANA]) that react specifically with both core mononucleosomes and plasma membranes of viable nucleated cells. Native mononucleosomes and nucleosome cores assembled from long DNA and the inner histones were indistinguishable in terms of inhibition of binding of X-ANA to nuclei of tissue sections and to polynucleosomes on the walls of plastic tubes. In contrast, mononucleosomes selectively depleted of histones H2A and H2B did not inhibit these reactions. A method was developed for isolation of X-ANA from serum that took advantage of the dual specificity of these antibodies. Immunosedimentation in sucrose density gradients revealed that 125I-labeled Fab' fragments of highly pure X-ANA formed complexes with the inner histones H2A, H2B, H3, and H4 in 2 M NaCL, but not in 0.15 M salt. These results indicate that X-ANA recognize an epitope of the inner histone in 2 M salt, and that in 0.15 M NaCL this epitope is not formed unless the histones interact with DNA to generate a nucleosome structure. Furthermore, in light of the previous demonstration that the epitope is destroyed by trypsin, it may be localized in the N-terminal region of histone H2A or H2B.

摘要

一些系统性红斑狼疮及相关疾病患者的血清中含有一种多克隆抗体群体(交叉反应性抗核抗体[X-ANA]),该抗体群体能与核心单核小体和活有核细胞的质膜发生特异性反应。就抑制X-ANA与组织切片细胞核及塑料管壁上的多聚核小体结合而言,天然单核小体以及由长链DNA和内部组蛋白组装而成的核小体核心并无差异。相比之下,选择性去除组蛋白H2A和H2B的单核小体则无法抑制这些反应。利用这些抗体的双重特异性,开发了一种从血清中分离X-ANA的方法。蔗糖密度梯度免疫沉淀显示,高纯度X-ANA的125I标记Fab'片段在2M NaCl中能与内部组蛋白H2A、H2B、H3和H4形成复合物,但在0.15M盐溶液中则不能。这些结果表明,X-ANA在2M盐溶液中识别内部组蛋白的一个表位,而在0.15M NaCl中,除非组蛋白与DNA相互作用形成核小体结构,否则该表位不会形成。此外,鉴于之前的研究表明该表位会被胰蛋白酶破坏,它可能位于组蛋白H2A或H2B的N端区域。

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