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重酶解肌球蛋白修饰的肌动蛋白丝:一种用于旋转阴影法保存肌动蛋白丝的简单方法。

Heavy-meromyosin-decorated actin filaments: a simple method to preserve actin filaments for rotary shadowing.

作者信息

Mabuchi K

机构信息

Department of Muscle Research, Boston Biomedical Research Institute, Massachusetts 02114.

出版信息

J Struct Biol. 1991 Aug;107(1):22-8. doi: 10.1016/1047-8477(91)90027-t.

Abstract

It has become accepted that deep-freeze-drying at or below -90 degrees C is necessary to preserve the structure of supramolecular assemblies such as actin filaments (AFs) for metal shadowing. This has kept the metal shadowing technique from widespread use in the study of proteins complexed with AFs because of the limited availability of the apparatus for deep-freeze-drying. I report here that adsorption to freshly cleaved mica, treatment with buffered uranyl acetate in glycerol solution, rinsing, and removal of liquid eliminate the need of freeze-drying to preserve the structure of AFs. This technique, in combination with metal shadowing, was applied to the study of AFs decorated with heavy meromyosin (HMM). It was observed that (1) when HMM molecules are associated with single AFs in the majority of cases only one head of each HMM molecule makes contact at the point furthest from the neck region; (2) binding of HMM causes bundling of AFs, probably by the two heads of each molecule binding different filaments; and (3) the binding of HMM to the bundled AFs appears to be more stable than that to a single AF. This method of specimen preparation requires no freeze-drying and is therefore easily applicable to other large protein complexes.

摘要

人们已经公认,在-90摄氏度或更低温度下进行深度冷冻干燥对于保存超分子组装体(如肌动蛋白丝(AFs))的结构以进行金属投影是必要的。由于深度冷冻干燥设备的可用性有限,这使得金属投影技术在与AFs复合的蛋白质研究中未能广泛应用。我在此报告,吸附到新劈开的云母上,在甘油溶液中用醋酸铀酰缓冲液处理,冲洗并去除液体,无需冷冻干燥即可保存AFs的结构。该技术与金属投影相结合,应用于对用重酶解肌球蛋白(HMM)修饰的AFs的研究。观察到:(1)在大多数情况下,当HMM分子与单个AFs结合时,每个HMM分子只有一个头部在离颈部区域最远的点接触;(2)HMM的结合导致AFs成束,可能是因为每个分子的两个头部结合不同的丝;(3)HMM与成束的AFs的结合似乎比与单个AFs的结合更稳定。这种样品制备方法不需要冷冻干燥,因此很容易应用于其他大型蛋白质复合物。

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