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微量滴定板中脂肪酶的定量比浊法测定。

Quantitative turbidity assay for lipolytic enzymes in microtiter plates.

机构信息

Department of Biotechnology, Brandenburg University of Technology Cottbus - Senftenberg, 01968, Senftenberg, Germany.

出版信息

Anal Bioanal Chem. 2013 Oct;405(26):8539-47. doi: 10.1007/s00216-013-7283-5. Epub 2013 Aug 29.

Abstract

A clearing assay for lipolytic enzymes has been realized in 96-well microtiter plates. A thin layer containing emulsified tributyrin as turbidity-generating substrate was placed on a thicker supporting aqueous layer. Both layers were stabilized by a gel-forming agent. Enzyme addition leads to clearing of the emulsion detected with a standard microtiter plate reader as a decrease of extinction. Dependencies of the signal kinetics on the substrate and enzyme concentrations were studied. For 0.5-1% tributyrin content the reaction rate is not substrate-limited. An initial slope of the signal kinetics is proportional to the lipase activity. A detailed characterization of the assay was performed. Lipolysis of tributyrin was confirmed by glycerol detection. Various gel-forming agents were compared and diffusion conditions in these gels were analyzed. Agar and agarose were found to be the most suitable gel-forming agents, which do not affect enzyme diffusion whereas polyacrylamide gels block lipase diffusion and therefore are not suitable for the assay. The optimized assay prepared from 1% tributyrin emulsion in 2% agar gel was tested with six microbial lipases and porcine pancreatic lipase. The detection limit is 20-60 ng/well which is equivalent to 30 μU/well for T. lanuginosus lipase.

摘要

已经在 96 孔微量滴定板上实现了用于脂解酶的析取测定法。在较厚的支撑水层上放置一层含有乳化三丁酸甘油酯作为浊度生成底物的薄层。通过形成凝胶的试剂稳定两个层。添加酶会导致乳液变清,这可以通过标准微量滴定板读数器检测到,作为消光度的降低。研究了信号动力学对底物和酶浓度的依赖性。对于 0.5-1%的三丁酸甘油酯含量,反应速率不受底物限制。信号动力学的初始斜率与脂肪酶活性成正比。对测定法进行了详细的特征描述。通过检测甘油来确认三丁酸甘油酯的脂解作用。比较了各种形成凝胶的试剂,并分析了这些凝胶中的扩散条件。发现琼脂和琼脂糖是最合适的形成凝胶的试剂,它们不会影响酶的扩散,而聚丙烯酰胺凝胶会阻止脂肪酶的扩散,因此不适合用于测定法。用从 1%三丁酸甘油酯乳液在 2%琼脂凝胶中制备的优化测定法测试了六种微生物脂肪酶和猪胰腺脂肪酶。检测限为 20-60ng/孔,这相当于 T. lanuginosus 脂肪酶的 30μU/孔。

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