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A High-Throughput Screening System Based on Droplet Microfluidics for Glucose Oxidase Gene Libraries

机译:基于液滴微流控技术的葡萄糖氧化酶基因文库高通量筛选系统

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摘要

Glucose oxidase (GOx) is an important industrial enzyme that can be optimized for specific applications by mutagenesis and activity-based screening. To increase the efficiency of this approach, we have developed a new ultrahigh-throughput screening platform based on a microfluidic lab-on-chip device that allows the sorting of GOx mutants from a saturation mutagenesis library expressed on the surface of yeast cells. GOx activity was measured by monitoring the fluorescence of water microdroplets dispersed in perfluorinated oil. The signal was generated via a series of coupled enzyme reactions leading to the formation of fluorescein. Using this new method, we were able to enrich the yeast cell population by more than 35-fold for GOx mutants with higher than wild-type activity after two rounds of sorting, almost double the efficiency of our previously described flow cytometry platform. We identified and characterized novel GOx mutants, the most promising of which (M6) contained a combination of six point mutations that increased the catalytic constant k by 2.1-fold compared to wild-type GOx and by 1.4-fold compared to a parental GOx variant. The new microfluidic platform for GOx was therefore more sensitive than flow cytometry and supports comprehensive screens of gene libraries containing multiple mutations per gene.
机译:葡萄糖氧化酶(GOx)是一种重要的工业酶,可通过诱变和基于活性的筛选针对特定应用进行优化。为了提高这种方法的效率,我们基于微流控实验室芯片设备开发了一种新的超高通量筛选平台,该平台可以从酵母细胞表面表达的饱和诱变文库中筛选出GOx突变体。通过监测分散在全氟化油中的水微滴的荧光来测量GOx活性。信号是通过一系列导致荧光素形成的偶联酶反应产生的。使用这种新方法,经过两轮分选,我们能够使具有高于野生型活性的GOx突变体的酵母细胞群富集35倍以上,几乎是我们先前描述的流式细胞仪平台效率的两倍。我们鉴定并鉴定了新颖的GOx突变体,其中最有前途的(M6)包含六个点突变的组合,与野生型GOx相比,其催化常数k增加了2.1倍,与亲本GOx变体相比增加了1.4倍。因此,新的GOx微流控平台比流式细胞仪更灵敏,并支持全面筛选包含每个基因多个突变的基因库。

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