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Directed evolution of Thermotoga neapolitana xylose isomerase: high activity on glucose at low temperature and low pH

机译:嗜热栖热菌木糖异构酶的定向进化:在低温和低pH下对葡萄糖具有高活性

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The Thermotoga neapolitana xylose isomerase (TNXI) is extremely thermostable and optimally active at 95degreesC. Its derivative, TNXI Val185Thr (V185T), is the most active type II xylose isomerase reported, with a catalytic efficiency of 25.1 s(-1) mM(-1) toward glucose at 80degreesC (pH 7.0). To further optimize TNXI's potential industrial utility, two rounds of random mutagenesis and low temperature/low pH activity screening were performed using the TNXI V185T-encoding gene as the template. Two highly active mutants were obtained, 3A2 (V185T/L282P) and 1F1 (V185T/L282P/F186S). 1F1 was more active than 3A2, which in turn was more active than TNXI V185T at all temperatures and pH values tested. 3A2 and 1F1's high activities at low temperatures were due to significantly lower activation energies (57 and 44 kJ/mol, respectively) than that of TNXI and V185T (87 kJ/mol). Mutation L282P introduced a kink in helix alpha(7) of 3A2's (alpha/beta)(8) barrel. Surprisingly, this mutation kinetically destabilized 3A2 only at pH 5.5. 1F1 displayed kinetic stability slightly above that of TNXI V185T. In 1F1, mutation F186S creates a cavity that disrupts a four-residue network of aromatic interactions. How the conformation of the neighboring residues is affected by this cavity and how these conformational changes increase 1F1's stability still remain unclear. [References: 31]
机译:Thermotoga neapolitana木糖异构酶(TNXI)具有极高的热稳定性,并在95°C时具有最佳活性。它的衍生物TNXI Val185Thr(V185T)是报道的活性最强的II型木糖异构酶,在80°C(pH 7.0)下对葡萄糖的催化效率为25.1 s(-1)mM(-1)。为了进一步优化TNXI的潜在工业实用性,使用TNXI V185T编码基因作为模板进行了两轮随机诱变和低温/低pH活性筛选。获得了两个高活性突变体:3A2(V185T / L282P)和1F1(V185T / L282P / F186S)。 1F1比3A2更具活性,而3A2在所有温度和pH值下均比TNXI V185T更具活性。 3A2和1F1在低温下的高活性是由于活化能(分别为57和44 kJ / mol)比TNXI和V185T(87 kJ / mol)低得多。突变L282P在3A2(alpha / beta)(8)枪管的螺旋alpha(7)中引入了扭结。令人惊讶地,该突变仅在pH 5.5下使3A2动力学不稳定。 1F1的动力学稳定性略高于TNXI V185T。在1F1中,突变F186S产生了一个空腔,该空腔破坏了四个残基的芳族相互作用网络。仍然不清楚该腔如何影响相邻残基的构象以及这些构象变化如何增加1F1的稳定性。 [参考:31]

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