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Cryo-electron microscopy of vitrified SV40 minichromosomes: the liquid drop model.

机译:玻璃化SV40微型染色体的低温电子显微镜:液滴模型。

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摘要

The structure of SV40 minichromosomes has been studied by cryo-electron microscopy of vitrified thin layers of solution. In high-salt buffer (130 mM NaCl), freshly prepared minichromosomes are condensed into globules 30 nm or more in diameter. On the micrograph, they appear to be formed by the close packing of 10 nm granules which give rise to a 10 nm reflection in the optical diffractogram. The globules can adopt many different conformations. At high concentration, they fuse into a homogeneous 'sea' of closely packed 10 nm granules. In low-salt buffer (less than 10 mM NaCl), the globules open, first into 10 nm filaments, and then into nucleosome-strings. The 'liquid drop' model is proposed to explain the condensed structure of the minichromosome in high-salt buffer: nucleosomes stack specifically on top of one another, thus forming the 10 nm filaments. 10 nm filaments in turn, tend to aggregate laterally. Optimizing both these interactions results in the condensation of 10 nm filaments or portions thereof into a structure similar to that of a liquid. Some implications of this model for the structure of cellular chromatin are discussed.
机译:SV40微型染色体的结构已通过玻璃化溶液薄层的低温电子显微镜进行了研究。在高盐缓冲液(130 mM NaCl)中,将新鲜制备的微型染色体浓缩成直径30 nm或更大的小球。在显微照片上,它们似乎是由10 nm颗粒的紧密堆积形成的,这些颗粒在光学衍射图中引起10 nm的反射。小球可以采用许多不同的构象。在高浓度下,它们融合成紧密堆积的10 nm颗粒的均匀“海洋”。在低盐缓冲液(小于10 mM NaCl)中,小球先开口成10 nm细丝,然后成核小体串。提出了“液滴”模型来解释微盐在高盐缓冲液中的浓缩结构:核小体特别地彼此堆叠,从而形成10 nm长丝。 10 nm的细丝又会在横向上聚集。优化这两个相互作用会导致10 nm的细丝或其部分凝结成类似于液体的结构。讨论了该模型对细胞染色质结构的一些影响。

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