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首页> 外文期刊>Applied Microbiology and Biotechnology >A first continuous 4-aminoantipyrine (4-AAP)-based screening system for directed esterase evolution
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A first continuous 4-aminoantipyrine (4-AAP)-based screening system for directed esterase evolution

机译:第一个基于连续4-氨基安替比林(4-AAP)的定向酯酶进化筛选系统

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摘要

Esterases hydrolyze ester bonds with an often high stereoselectivity as well as regioselectivity and are therefore industrially employed in the synthesis of pharmaceuticals, in food processing, and in laundry detergents. Continuous screening systems based on p-nitrophenyl- (e.g., p-nitrophenyl acetate) or umbelliferyl-esters are commonly used in directed esterase evolution campaigns. Ongoing challenges in directed esterase evolution are screening formats which offer a broad substrate spectrum, especially for complex aromatic substrates. In this report, a novel continuous high throughput screening system for indirect monitoring of esterolytic activity was developed and validated by detection of phenols employing phenyl benzoate as substrate and p-nitrobenzyl esterase (pNBEBL from Bacillus licheniformis) as catalyst. The released phenol directly reacts with 4-aminoantipyrine yielding the red compound 1,5-dimethyl-4-(4-oxo-cyclohexa-2,5-dienylidenamino)-2-phenyl-1,2-dihydro-pyrazol-3-one. In this continuous B. licheniformis esterase activity detection system (cBLE-4AAP), the product formation is followed through an increase in absorbance at 509 nm. The cBLE-4AAP screening system was optimized in 96-well microtiter plate format in respect to standard deviation (5 %), linear detection range (15 to 250 mu M), lower detection limit (15 mu M), and pH (7.4 to 10.4). The cBLE-4AAP screening system was validated by screening a random epPCR pNBEBL mutagenesis library (2000 clones) for improved esterase activity at elevated temperatures. Finally, the variant T3 (Ser378Pro) was identified which nearly retains its specific activity at room temperature (WT 1036 U/mg and T3 929 U/mg) and shows compared to WT a 4.7-fold improved residual activity after thermal treatment (30 min incubation at 69.4 A degrees C; WT 170 U/mg to T3 804 U/mg).
机译:酯酶通常以高的立体选择性和区域选择性水解酯键,因此在工业上用于药物合成,食品加工和洗衣洗涤剂中。基于对硝基苯基-(例如,对硝基苯基乙酸酯)或伞形酯的连续筛选系统通常用于定向酯酶进化活动中。直接酯酶进化中的持续挑战是筛选形式,其提供了广泛的底物谱,尤其是对于复杂的芳香族底物。在本报告中,开发了一种新颖的连续高通量筛选系统,用于间接监测酯水解活性,并通过检测苯酚苯酚为底物,对硝基苄基酯酶(地衣芽孢杆菌的pNBEBL)为催化剂的酚进行了验证。释放的苯酚与4-氨基安替比林直接反应,生成红色化合物1,5-二甲基-4-(4-氧代-环己-2,5-二烯基亚氨基)-2-苯基-1,2-二氢吡唑-3- 。在这种连续的地衣芽孢杆菌酯酶活性检测系统(cBLE-4AAP)中,通过增加509 nm处的吸光度来跟踪产物的形成。 cBLE-4AAP筛选系统针对标准偏差(5%),线性检测范围(15至250μM),较低检测限(15μM)和pH(7.4至10.4)。通过筛选随机epPCR pNBEBL诱变文库(2000个克隆)来验证cBLE-4AAP筛选系统在高温下酯酶活性的提高。最后,鉴定出变体T3(Ser378Pro)在室温下几乎保持其比活性(WT 1036 U / mg和T3 929 U / mg),并且与WT相比,热处理(30分钟)后残留活性提高了4.7倍。在69.4 A摄氏度下孵育; WT 170 U / mg至T3 804 U / mg)。

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