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通过用放射性乙酸酐进行乙酰化反应在体外对蛋白质和病毒进行放射性标记。

Radiolabeling of proteins and viruses in vitro by acetylation with radioactive acetic anhydride.

作者信息

Montelaro R C, Rueckert R R

出版信息

J Biol Chem. 1975 Feb 25;250(4):1413-21.

PMID:163253
Abstract

We describe a convenient, rapid, and reproducible method for labeling proteins in vitro by acetylation with [3H] or [14-C]acetic anhydride dissolved in small amounts of anhydrous dioxane. The reaction is carried out at neutral pH and does not require the use of detergents, water-immiscible organic solvents, oxidizing, or reducing agents. Thus undesirable solvent-induced alterations in protein structure and biological activity are minimized. A method for calculating the specific activity of the protein and the efficiency of acetylation at known concentrations of protein and acetic anhydride is presented. Radioacetylated proteins were shown to be suitable for use as molecular weight calibration standards and as protein markers in polyacrylamide gel electrophoresis, gel filtration, and enzyme studies. Acetic anhydride was used to label intact oncornaviruses, which consist of a complex ribonucleo-protein core within a lipid envelope. Some of the viral lipid and all of the viral proteins, including the internal ones, were labeled without detectable alterations in viral morphology or buoyant density. This result suggests that acetic anhydride, evidently by virtue of its small size and neutral charge, penetrates freely throughout the viral membrane and core structures. The reactivity of RNA with acetic anhydride was less than 1% that of protein under similar reaction conditions.

摘要

我们描述了一种简便、快速且可重复的方法,用于在体外通过用溶解于少量无水二氧六环中的[³H]或[¹⁴C]乙酸酐进行乙酰化来标记蛋白质。该反应在中性pH下进行,不需要使用去污剂、与水不混溶的有机溶剂、氧化剂或还原剂。因此,溶剂引起的蛋白质结构和生物活性的不良改变被最小化。本文还介绍了一种在已知蛋白质和乙酸酐浓度下计算蛋白质比活性和乙酰化效率的方法。放射性乙酰化蛋白质被证明适用于作为聚丙烯酰胺凝胶电泳、凝胶过滤和酶研究中的分子量校准标准物和蛋白质标记物。乙酸酐被用于标记完整的肿瘤病毒,这种病毒由脂质包膜内的复杂核糖核蛋白核心组成。一些病毒脂质和所有病毒蛋白质,包括内部的蛋白质,都被标记了,而病毒形态或浮力密度没有可检测到的改变。这一结果表明,乙酸酐显然由于其体积小和电荷中性,能够自由穿透整个病毒膜和核心结构。在类似反应条件下,RNA与乙酸酐的反应活性不到蛋白质的1%。

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