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哺乳动物动粒的结构。

Structure of the mammalian kinetochore.

作者信息

Ris H, Witt P L

出版信息

Chromosoma. 1981;82(2):153-70. doi: 10.1007/BF00286101.

Abstract

The structure of the mammalian trilaminar kinetochore was investigated using stereo electron microscopy of chromosomes in hypotonic solutions which unraveled the chromosome but maintained microtubules. Mouse and Chinese hamster ovary cells were arrested in Colcemid and allowed to reform microtubules after Colcemid was removed. Recovered cells were then swelled, lysed or spread in hypotonic solutions which contained D2O to preserve microtubules. The chromosomes were observed in thin and thick sections and as whole mounts using high voltage electron microscopy. Bundles of microtubules were seen directly attached to chromatin, indicating that the kinetochore outer layer represents a differential arrangement of chromatin, continuous with the body of the chromosome. In cells fixed wihout pretreatment, the outer layer could be seen to be composed of hairpin loops of chromatin stacked together to form a solid layer. The hypotonically-induced unraveling of the outer layer was found to be reversible, and the typical 300 nm thick disk reformed when cells were returned to isotonic solutions. Short microtubules, newly nucleated after Colcemid removal, were found not to be attached to the kinetochore out layer, but were situated in the fibrous corona on the external surface of the outer layer. This was verified by observation of thick sections in stereo which made it possible to identify microtubules ends within the section. Thus, kinetochore microtubules are nucleated within the fibrous corona, and subsequently become attached to the outer layer.

摘要

利用低渗溶液中染色体的立体电子显微镜技术对哺乳动物三层动粒的结构进行了研究,该技术能解开染色体但保留微管。将小鼠和中国仓鼠卵巢细胞用秋水仙酰胺处理使其停滞,去除秋水仙酰胺后让其重新形成微管。然后将恢复的细胞在含有重水以保存微管的低渗溶液中膨胀、裂解或铺展。使用高电压电子显微镜在薄切片和厚切片中以及作为整装标本观察染色体。可见微管束直接附着于染色质,这表明动粒外层代表染色质的一种差异排列,与染色体主体连续。在未经预处理固定的细胞中,可看到外层由堆叠在一起形成固体层的染色质发夹环组成。发现外层因低渗诱导的解旋是可逆的,当细胞回到等渗溶液时,典型的300纳米厚的盘状结构会重新形成。发现秋水仙酰胺去除后新形成的短微管不附着于动粒外层,而是位于外层外表面的纤维冠中。通过立体观察厚切片得以证实,这使得能够识别切片内的微管末端。因此,动粒微管在纤维冠内形成,随后附着于外层。

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