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首页> 外文期刊>Combinatorial chemistry & high throughput screening >Ultrahigh-throughput screening system for directed glucose oxidase evolution in yeast cells.
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Ultrahigh-throughput screening system for directed glucose oxidase evolution in yeast cells.

机译:用于酵母细胞中定向葡萄糖氧化酶进化的超高通量筛选系统。

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摘要

A compartmentalized tyramide labeling system (CoaTi) employing flow cytometry for sorting of yeast cells was developed as ultrahigh-throughput screening for Glucose oxidase (GOx) from Aspergillus niger. CoaTi combines in vitro compartmentalization technology with the CARD reporter system which uses fluorescein tyramide labels for detection of peroxidase activity. Physical connection between cells and fluorescein tyramide radicals was achieved by compartmentalization of yeast cells inside microdroplets of single water-in-oil emulsions. After reaction cells were recovered from single emulsions and sorted by flow cytometry, an error prone PCR mutant library of Glucose oxidase (GOx) containing 10(7) cells and ~10(5) of different GOx variants was screened. Mutagenic conditions of GOx mutant library were selected to generate <1 % of active GOx population in order to explore influence of high mutation frequency on GOx activity. GOx variant Mut12 that contains 5 mutations (N2Y, K13E, T30V, I94V, K152R) showed a 1.2 times decreased K(m) (22.0 vs 18.1 mM) and a 2.7 fold increased k(cat) (150 s(-1) vs 54.8 s(-1)) compared to wt GOx. Compared to the employed parent B11 GOx (16 mM, 80 s(-1)) it has a slightly increased K(m) and 1.8 times increased k(cat).
机译:开发了一种采用流式细胞术对酵母细胞进行分选的区隔酪胺标记系统(CoaTi),作为黑曲霉中葡萄糖氧化酶(GOx)的超高通量筛选。 CoaTi将体外分隔技术与CARD报告系统结合在一起,该系统使用荧光素酪酰胺标记来检测过氧化物酶活性。细胞和荧光素酪酰胺自由基之间的物理连接是通过将单个油包水型乳剂的微滴内的酵母细胞分隔开来实现的。从单个乳状液中回收反应细胞并通过流式细胞仪分选后,筛选出一个容易出错的葡萄糖氧化酶(GOx)PCR突变体文库,其中包含10(7)个细胞和〜10(5)个不同的GOx变体。选择GOx突变体文库的诱变条件以产生<1%的活性GOx种群,以探索高突变频率对GOx活性的影响。包含5个突变(N2Y,K13E,T30V,I94V,K152R)的GOx变异Mut12显示K(m)降低了1.2倍(22.0对18.1 mM),k(cat)升高了2.7倍(150 s(-1)对与wt GOx相比为54.8 s(-1))。与使用的父代B11 GOx(16 mM,80 s(-1))相比,它的K(m)略有增加,而k(cat)则增加了1.8倍。

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