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用于测定支链淀粉酶活性的比色和荧光底物。

Colourimetric and fluorometric substrates for measurement of pullulanase activity.

作者信息

McCleary Barry V, Mangan David, McKie Vincent, Cornaggia Claudio, Ivory Ruth, Rooney Edward

机构信息

Megazyme International Ireland, Bray Business Park, Southern Cross Road, Bray, County Wicklow, Ireland.

Megazyme International Ireland, Bray Business Park, Southern Cross Road, Bray, County Wicklow, Ireland.

出版信息

Carbohydr Res. 2014 Jul 1;393:60-9. doi: 10.1016/j.carres.2014.04.014. Epub 2014 Apr 28.

DOI:10.1016/j.carres.2014.04.014
PMID:24938640
Abstract

Specific and highly sensitive colourimetric and fluorometric substrate mixtures have been prepared for the measurement of pullulanase and limit-dextrinase activity and assays employing these substrates have been developed. These mixtures comprise thermostable α- and β-glucosidases and either 4,6-O-benzylidene-2-chloro-4-nitrophenyl-β-maltotriosyl (1-6) α-maltotrioside (BzCNPG3G3, 1) as a colourimetric substrate or 4,6-O-benzylidene-4-methylumbelliferyl-β-maltotriosyl (1-6) α-maltotrioside (BzMUG3G3, 2) as a fluorometric substrate. Hydrolysis of substrates 1 and 2 by exo-acting enzymes such as amyloglucosidase, β-amylase and α-glucosidase is prevented by the presence of the 4,6-O-benzylidene group on the non-reducing end D-glucosyl residue. The substrates are not hydrolysed by any α-amylases studied, (including those from Aspergillus niger and porcine pancreas) and are resistant to hydrolysis by Pseudomonas sp. isoamylase. On hydrolysis by pullulanase, the 2-chloro-4-nitrophenyl-β-maltotrioside (3) or 4-methylumbelliferyl-β-maltotrioside (4) liberated is immediately hydrolysed to D-glucose and 2-chloro-4-nitrophenol or 4-methylumbelliferone. The reaction is terminated by the addition of a weak alkaline solution leading to the formation of phenolate ions in solution whose concentration can be determined using either spectrophotometric or fluorometric analysis. The assay procedure is simple to use, specific, accurate, robust and readily adapted to automation.

摘要

已制备出用于测定支链淀粉酶和极限糊精酶活性的特异性高灵敏度比色和荧光底物混合物,并开发了使用这些底物的测定方法。这些混合物包含热稳定的α-和β-葡萄糖苷酶,以及作为比色底物的4,6-O-亚苄基-2-氯-4-硝基苯基-β-麦芽三糖基(1-6)α-麦芽三糖(BzCNPG3G3,1)或作为荧光底物的4,6-O-亚苄基-4-甲基伞形酮基-β-麦芽三糖基(1-6)α-麦芽三糖(BzMUG3G3,2)。非还原端D-葡萄糖基残基上的4,6-O-亚苄基基团可防止外切酶如淀粉葡糖苷酶、β-淀粉酶和α-葡萄糖苷酶对底物1和2的水解。所研究的任何α-淀粉酶(包括来自黑曲霉和猪胰腺的α-淀粉酶)都不会水解这些底物,并且它们对假单胞菌属异淀粉酶的水解具有抗性。支链淀粉酶水解后,释放出的2-氯-4-硝基苯基-β-麦芽三糖苷(3)或4-甲基伞形酮基-β-麦芽三糖苷(4)会立即水解为D-葡萄糖和2-氯-4-硝基苯酚或4-甲基伞形酮。通过加入弱碱性溶液终止反应,导致溶液中形成酚盐离子,其浓度可使用分光光度法或荧光分析法测定。该测定方法使用简单、特异性强、准确、稳健且易于实现自动化。

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