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含有组蛋白TH2B的核小体中组蛋白H2B的缺失以及免疫球蛋白与核小体的相互作用。

Absence of histone H2B in nucleosomes containing histone TH2B and interaction of immunoglobulin with nucleosomes.

作者信息

Chiu M L, Irvin J L

出版信息

Arch Biochem Biophys. 1986 Jan;244(1):42-9. doi: 10.1016/0003-9861(86)90092-5.

Abstract

Nucleosomes containing histone TH2B were isolated from chromatin subunits of rat testis nuclei (MNT) by incubating with anti-TH2B immunoglobulin (IgTH2B) which was covalently attached to agarose gels. Electrophoretic separation of histones of these isolated nucleosomes revealed that histone H2B was completely absent, suggesting that histone TH2B, the variant of H2B, existed in nucleosomes only as TH2B X TH2B and that TH2B X H2B was not likely to exist in chromatin. Sucrose gradient ultracentrifugation of mixtures of MNT and IgTH2B revealed that when excess amounts of immunologically active IgTH2B were present, complexes of higher sedimentation coefficients than MNT X IgTH2B were formed, but with limited amounts of active IgTH2B, only MNT X IgTH2B was formed. When purified IgTH2B was coated on polystyrene tubes and incubated with MNT, those MNT immobilized by the tube-coated IgTH2B adsorbed IgTH2B from diluted antiserum during subsequent incubation. Those results suggested the absence of steric hindrance in the binding of IgTH2B to MNT X IgTH2B. When MNT was coated on polystyrene tubes and incubated with DNase and then with dilute anti-TH2B antiserum, it was found that DNase digestion increased the binding of immunoglobulin to the tubes approximately 76%. Interaction of chromatin subunits of rat liver nuclei (MNL) with anti-TH2B antiserum was negligible, but DNase digestion of MNL coated on tubes was followed by considerable interaction with anti-TH2B antiserum. Those results indicated DNase unmasked at least part of the determinants encased by DNA. Anti-H2B immunoglobulin (IgH2B) interacted with histone H2B and TH2B to the same extent, and interacted significantly to a lesser extent with either MNT or MNL. DNase digestion of MNT and MNL increased binding of IgH2B approximately 170 and 117%, respectively.

摘要

通过与共价连接到琼脂糖凝胶上的抗TH2B免疫球蛋白(IgTH2B)孵育,从大鼠睾丸细胞核(MNT)的染色质亚基中分离出含有组蛋白TH2B的核小体。对这些分离出的核小体的组蛋白进行电泳分离,结果显示组蛋白H2B完全缺失,这表明H2B的变体组蛋白TH2B仅以TH2B×TH2B的形式存在于核小体中,而TH2B×H2B不太可能存在于染色质中。对MNT和IgTH2B混合物进行蔗糖梯度超速离心,结果显示,当存在过量的具有免疫活性的IgTH2B时,会形成沉降系数高于MNT×IgTH2B的复合物,但当活性IgTH2B的量有限时,仅形成MNT×IgTH2B。当将纯化的IgTH2B包被在聚苯乙烯管上并与MNT孵育时,那些被管包被的IgTH2B固定的MNT在随后的孵育过程中会从稀释的抗血清中吸附IgTH2B。这些结果表明,IgTH2B与MNT×IgTH2B结合时不存在空间位阻。当将MNT包被在聚苯乙烯管上,先后与DNA酶和稀释的抗TH2B抗血清孵育时,发现DNA酶消化使免疫球蛋白与管的结合增加了约76%。大鼠肝细胞核(MNL)的染色质亚基与抗TH2B抗血清的相互作用可忽略不计,但对包被在管上的MNL进行DNA酶消化后,其与抗TH2B抗血清发生了显著的相互作用。这些结果表明,DNA酶使至少部分被DNA包裹的决定簇暴露出来。抗H2B免疫球蛋白(IgH2B)与组蛋白H2B和TH2B的相互作用程度相同,与MNT或MNL的相互作用程度则明显较小。对MNT和MNL进行DNA酶消化后,IgH2B的结合分别增加了约170%和117%。

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