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首页> 外文期刊>Biochemistry >Engineering of variants of the restriction endonuclease EcoRV that depend in their cleavage activity on the flexibility of sequences flanking the recognition site
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Engineering of variants of the restriction endonuclease EcoRV that depend in their cleavage activity on the flexibility of sequences flanking the recognition site

机译:限制性内切酶EcoRV变体的工程设计,其切割活性取决于识别位点两侧序列的柔性

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The present work describes mutants of the restriction enzyme EcoRV that discriminate very efficiently between oligodeoxynucleotide substrates with an EcoRV recognition sequence in different sequence context. All of these EcoRV variants harbor substitutions at position 226, where in the cocrystal structure of the specific EcoRV/DNA complex an arginine contacts the backbone of the DNA substrate upstream of the recognition sequence, and cleave an oligodeoxynucleotide with an EcoRV site in a nonflexible sequence context (the recognition site being flanked by runs of A and T) with much higher catalytic efficiency (k(cat)/K-m) than an oligodeoxynucleotide with an EcoRV site In a flexible sequence context (the recognition site being flanked by runs of AT), in contrast to the wild-type enzyme, that cleaves both substrates with the same catalytic efficiency. Steady-state and single-turnover kinetics indicate that the enhanced selectivity of the mutants is due to the catalytic step of the reaction. It is possible to enhance the discriminatory power of these EcoRV variants through the choice of appropriate reaction conditions, in particular low salt concentration and low reaction temperatures. It must be emphasized that the enhanced selectivity of these EcoRV variants toward EcoRV sites in a flexible and nonflexible sequence context, respectively, is not only seen with oligodeoxynucleotides, but also with plasmid substrates. [References: 40]
机译:本工作描述了限制性酶EcoRV的突变体,该突变体可在不同序列背景下非常有效地区分具有EcoRV识别序列的寡脱氧核苷酸底物。所有这些EcoRV变体都在226位具有替换位,在特定EcoRV / DNA复合体的共晶体结构中,精氨酸在识别序列上游与DNA底物的骨架接触,并在非柔性序列中切割带有EcoRV位点的寡脱氧核苷酸上下文(识别位点位于A和T序列的两侧)比具有EcoRV位点的寡脱氧核苷酸的催化效率(k(cat)/ Km)高得多,在灵活的序列上下文中(识别位点位于AT序列的两侧)与野生型酶相反,它以相同的催化效率裂解两种底物。稳态和单周转动力学表明突变体的选择性提高是由于反应的催化步骤。通过选择合适的反应条件,尤其是低盐浓度和低反应温度,可以增强这些EcoRV变体的区分能力。必须强调的是,不仅在寡聚脱氧核苷酸中,而且在质粒底物上,都分别看到了这些EcoRV变体在柔性和非柔性序列中对EcoRV位点的选择性增强。 [参考:40]

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