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用于基于液滴的微流控筛选的新型糖苷酶底物。

New glycosidase substrates for droplet-based microfluidic screening.

作者信息

Najah Majdi, Mayot Estelle, Mahendra-Wijaya I Putu, Griffiths Andrew D, Ladame Sylvain, Drevelle Antoine

机构信息

Institut de Science et d'Ingénierie Supramoléculaires (ISIS), Université de Strasbourg, CNRS UMR 7006 , 8 allée Gaspard Monge, 67083 Strasbourg Cedex, France.

出版信息

Anal Chem. 2013 Oct 15;85(20):9807-14. doi: 10.1021/ac4022709. Epub 2013 Sep 30.

DOI:10.1021/ac4022709
PMID:24079367
Abstract

Droplet-based microfluidics is a powerful technique allowing ultra-high-throughput screening of large libraries of enzymes or microorganisms for the selection of the most efficient variants. Most applications in droplet microfluidic screening systems use fluorogenic substrates to measure enzymatic activities with fluorescence readout. It is important, however, that there is little or no fluorophore exchange between droplets, a condition not met with most commonly employed substrates. Here we report the synthesis of fluorogenic substrates for glycosidases based on a sulfonated 7-hydroxycoumarin scaffold. We found that the presence of the sulfonate group effectively prevents leakage of the coumarin from droplets, no exchange of the sulfonated coumarins being detected over 24 h at 30 °C. The fluorescence properties of these substrates were characterized over a wide pH range, and their specificity was studied on a panel of relevant glycosidases (cellulases and xylanases) in microtiter plates. Finally, the β-d-cellobioside-6,8-difluoro-7-hydroxycoumarin-4-methanesulfonate substrate was used to assay cellobiohydrolase activity on model bacterial strains (Escherichia coli and Bacillus subtilis) in a droplet-based microfluidic format. These new substrates can be used to assay glycosidase activities in a wide pH range (4-11) and with incubation times of up to 24 h in droplet-based microfluidic systems.

摘要

基于微滴的微流控技术是一种强大的技术,可对大量酶或微生物文库进行超高通量筛选,以选择最有效的变体。微滴微流控筛选系统中的大多数应用都使用荧光底物通过荧光读数来测量酶活性。然而,重要的是微滴之间几乎没有或没有荧光团交换,而大多数常用底物都不满足这一条件。在此,我们报告了基于磺化7-羟基香豆素支架的糖苷酶荧光底物的合成。我们发现磺酸根基团的存在有效地防止了香豆素从微滴中泄漏,在30℃下24小时内未检测到磺化香豆素的交换。在很宽的pH范围内对这些底物的荧光特性进行了表征,并在微量滴定板中对一组相关糖苷酶(纤维素酶和木聚糖酶)研究了它们的特异性。最后,β-d-纤维二糖苷-6,8-二氟-7-羟基香豆素-4-甲磺酸盐底物用于在基于微滴的微流控形式中测定模型细菌菌株(大肠杆菌和枯草芽孢杆菌)上的纤维二糖水解酶活性。这些新底物可用于在宽pH范围(4-11)内测定糖苷酶活性,并且在基于微滴的微流控系统中孵育时间长达24小时。

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