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Evolution of highly active enzymes by homology-independent recombination

机译:通过同源性无关的重组进化出高活性酶

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摘要

The theta-class GST enzymes hGSTT1-1 (human GSTθ-1-1) and rGSTT2-2 (rat GSTθ-2-2) share 54.3% amino acid identity and exhibit different substrate specificities. Homology-independent techniques [incremental truncation for the creation of hybrid enzymes (ITCHY) and SCRATCHY] and low-homology techniques (recombination-dependent exponential amplification PCR) were used to create libraries of chimeric enzymes containing crossovers (C/Os) at positions not accessible by DNA family shuffling. High-throughput flow cytometric screening using the fluorogenic rGSTT2-2-specific substrate 7-amino-4-chloromethyl coumarin led to the isolation of active variants with either one or two C/Os. One of these enzymes, SCR23 (83% identity to hGSTT1-1), was encoded by a gene that exchanged helices 4 and 5 of hGSTT1-1 with the corresponding sequence from rGSTT2-2. Compared with either parent, this variant was found to have an improved k_(cat) with the selection substrate and also exhibited activity for the conjugation of glutathione to ethacrynic acid, a compound that is not recognized by either parental enzyme. These results highlight the power of combinatorial homology-independent and low-homology recombination methods for the generation of unique, highly active enzymes and also suggest a possible means of enzyme "humanization."
机译:θ类GST酶hGSTT1-1(人GSTθ-1-1)和rGSTT2-2(大鼠GSTθ-2-2)具有54.3%的氨基酸同一性,并具有不同的底物特异性。同源性独立技术[用于创建杂合酶(ITCHY)和SCRATCHY的增量截短法]和低同源性技术(重组依赖型指数扩增PCR)用于创建在不存在交叉点(C / O)的嵌合酶文库DNA家庭改组可访问。使用荧光rGSTT2-2特异性底物7-氨基-4-氯甲基香豆素的高通量流式细胞术筛选可分离具有一个或两个C / O的活性变异体。这些酶之一SCR23(与hGSTT1-1的同源性为83%)由一个基因编码,该基因将hGSTT1-1的4和5螺旋与rGSTT2-2的相应序列交换。与任一亲本相比,发现该变体与选择底物具有改善的k_(cat),并且还表现出谷胱甘肽与乙炔酸缀合的活性,这是一种亲本酶均不能识别的化合物。这些结果突出了组合同源非依赖性和低同源重组方法产生独特的高活性酶的能力,并且还提出了酶“人源化”的可能手段。

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