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对从十二烷基硫酸钠-聚丙烯酰胺凝胶中回收放射性标记蛋白质的系统研究。

A systematic investigation into the recovery of radioactively labeled proteins from sodium dodecyl sulfate-polyacrylamide gels.

作者信息

Zhou Shaobo, Bailey Matthew J, Dunn Michael J, Preedy Victor R, Emery Peter W

机构信息

Nutrition, Food and Health Research Centre, London, UK.

出版信息

Electrophoresis. 2004 Jan;25(1):1-7. doi: 10.1002/elps.200305699.

Abstract

We report the results of a systematic investigation designed to optimize a method for quantifying radioactivity in proteins in sodium dodecyl sulfate-polyacrylamide gels. The method involves dissolving appropriately sized pieces of gel in hydrogen peroxide and heating to 70 degrees C overnight followed by liquid scintillation counting. H(2)O(2) had no effect on the count rates of [(14)C]bovine serum albumin (BSA) when counted in a conventional liquid scintillation system, and the count rates remained stable for several days. Temperatures below 70 degrees C resulted in incomplete extraction of radioactivity from gels containing [(14)C]BSA, but there was also a significant reduction in count rates in samples incubated at 80 degrees C. At 70 degrees C recovery was not affected by the amount of sample loaded onto the gel or by the staining procedure (Coomassie Brilliant Blue or SYPRO Ruby). Recoveries were in the range of 89-94%, and the coefficient of variation for five replicate samples was 5-10%. This method offers a reliable way of measuring the amount of radioactivity in proteins that have been separated by electrophoresis. It may be useful, for example, in quantitative metabolic labeling experiments when it is necessary to know precisely how much tracer has been incorporated into a particular protein.

摘要

我们报告了一项系统性研究的结果,该研究旨在优化一种用于定量十二烷基硫酸钠-聚丙烯酰胺凝胶中蛋白质放射性的方法。该方法包括将适当大小的凝胶块溶解在过氧化氢中,并加热至70摄氏度过夜,然后进行液体闪烁计数。在传统液体闪烁计数系统中对[(14)C]牛血清白蛋白(BSA)进行计数时,H(2)O(2)对计数率没有影响,并且计数率在数天内保持稳定。低于70摄氏度的温度导致从含有[(14)C]BSA的凝胶中放射性提取不完全,但在80摄氏度孵育的样品中计数率也显著降低。在70摄氏度时,回收率不受加载到凝胶上的样品量或染色程序(考马斯亮蓝或SYPRO Ruby)的影响。回收率在89%-94%范围内,五个重复样品的变异系数为5%-10%。该方法提供了一种可靠的方式来测量通过电泳分离的蛋白质中的放射性量。例如,在需要精确知道有多少示踪剂掺入特定蛋白质的定量代谢标记实验中可能会有用。

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