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Sequence-independent construction of ordered combinatorial libraries with predefined crossover points

机译:具有预定义交叉点的有序组合库的与序列无关的构造

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摘要

Combinatorial libraries coding for mosaic enzymes with predefined crossover points constitute useful tools to address and model structure-function relationships and for functional optimization of enzymes based on multivariate statistics. The presented method, called sequence-independent generation of a chimera-ordered library (SIGNAL), allows easy shuffling of any predefined amino acid segment between two or more proteins. This method is particularly well adapted to the exchange of protein structural modules. The procedure could also be well suited to generate ordered combinatorial libraries independent of sequence similarities in a robotized manner. Sequence segments to be recombined are first extracted by PCR from a single-stranded template coding for an enzyme of interest using a biotin-avidin-based method. This technique allows the reduction of parental template contamination in the final library. Specific PCR primers allow amplification of two complementary mosaic DNA fragments, overlapping in the region to be exchanged. Fragments are finally reassembled using a fusion PCR. The process is illustrated via the construction of a set of mosaic CYP2B enzymes using this highly modular approach.
机译:编码具有预定交叉点的镶嵌酶的组合文库构成了有用的工具,用于处理和建模结构-功能关系,并基于多变量统计信息对酶的功能进行优化。所提出的方法称为嵌合顺序有序文库(SIGNAL)的序列非依赖性生成,可轻松改组两个或多个蛋白质之间的任何预定义氨基酸片段。该方法特别适合于蛋白质结构模块的交换。该程序也很适合以自动方式生成与序列相似性无关的有序组合文库。首先,使用基于生物素-亲和素的方法通过PCR从编码目的酶的单链模板中提取待重组的序列片段。此技术可以减少最终库中父母模板的污染。特定的PCR引物可扩增两个互补的镶嵌DNA片段,在要交换的区域重叠。最后使用融合PCR重新组装片段。通过使用这种高度模块化的方法构建一组镶嵌CYP2B酶来说明该过程。

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