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核小体和多聚核小体的偏振光散射——原位和体外研究

Polarized light scattering of nucleosomes and polynucleosomes--in situ and in vitro studies.

作者信息

Diaspro A, Bertolotto M, Vergani L, Nicolini C

机构信息

Institute of Biophysics, School of Medicine, University of Genoa, Ponente, Italy.

出版信息

IEEE Trans Biomed Eng. 1991 Jul;38(7):670-8. doi: 10.1109/10.83568.

Abstract

Nucleosomes, chromatin and nuclei, extracted from rat hepatocytes, are studied by a new "in house" experimental configuration which measures circular intensity differential scattering (CIDS) and other elements of the polarized light scattering matrix. The Mueller matrix elements, S14 and S34, that are related to the geometric parameters of the superhelical arrangement of polynucleosomes point to the existence of a quaternary structure at low ionic strength for chromatin prepared by the cold-water method, which is lost by shearing, and is not found in the soluble chromatin prepared through the nuclease method. Only salt addition to a final concentration of 5 mM MgCl2, 150 mM NaCl and 10 mM Tris HCl (pH 7) yields a sizeable (S14 + S34) signal in the latter chromatin, which is however still different from the corresponding signal of native nuclei and of "cold-water" chromatin. Comfortingly, the (S14 + S34) signal from isolated nucleosomes is consistently very low (nearly zero) as predicted by multiple dipole simulation within the framework of classical electrodynamics. Results are discussed in terms of the topological constraints present in the native long chromatin fiber, which are lost after limited nuclease digestion and after shearing.

摘要

从大鼠肝细胞中提取的核小体、染色质和细胞核,通过一种新的“内部”实验配置进行研究,该配置可测量圆强度差散射(CIDS)和偏振光散射矩阵的其他元素。与多核小体超螺旋排列的几何参数相关的穆勒矩阵元素S14和S34表明,通过冷水法制备的染色质在低离子强度下存在四级结构,这种结构会因剪切而丧失,并且在通过核酸酶法制备的可溶性染色质中未发现。只有添加最终浓度为5 mM MgCl2、150 mM NaCl和10 mM Tris HCl(pH 7)的盐,才能在后者的染色质中产生可观的(S14 + S34)信号,然而该信号仍与天然细胞核和“冷水”染色质的相应信号不同。令人欣慰的是,正如经典电动力学框架内的多偶极模拟所预测的那样,分离出的核小体的(S14 + S34)信号始终非常低(几乎为零)。根据天然长染色质纤维中存在的拓扑约束对结果进行了讨论,这些约束在有限的核酸酶消化和剪切后会丧失。

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