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Discovery of active proteins directly from combinatorial randomized protein libraries without display, purification or sequencing: identification of novel zinc finger proteins

机译:直接从组合随机蛋白质库中发现活性蛋白质,无需展示,纯化或测序:鉴定新型锌指蛋白质

摘要

We have successfully linked protein library screening directly with the identification of active proteins, without the need for individual purification, display technologies or physical linkage between the protein and its encoding sequence. By using ‘MAX’ randomization we have rapidly constructed 60 overlapping gene libraries that encode zinc finger proteins, randomized variously at the three principal DNA-contacting residues. Expression and screening of the libraries against five possible target DNA sequences generated data points covering a potential 40 000 individual interactions. Comparative analysis of the resulting data enabled direct identification of active proteins. Accuracy of this library analysis methodology was confirmed by both in vitro and in vivo analyses of identified proteins to yield novel zinc finger proteins that bind to their target sequences with high affinity, as indicated by low nanomolar apparent dissociation constants.
机译:我们已经成功地将蛋白质文库筛选与活性蛋白质的鉴定直接联系在一起,而无需单独的纯化,展示技术或蛋白质与其编码序列之间的物理联系。通过使用“ MAX”随机化,我们已经快速构建了60个重叠的基因文库,这些文库编码锌指蛋白,并在三个主要的DNA接触残基上进行了不同的随机化处理。针对五个可能的靶DNA序列进行文库的表达和筛选,产生了覆盖潜在的40 000个个体相互作用的数据点。对所得数据进行比较分析,可以直接鉴定活性蛋白。该文库分析方法的准确性已通过对鉴定出的蛋白质进行体外和体内分析而得到,以产生新型锌指蛋白,该锌指蛋白以高亲和力与靶序列结合,如低纳摩尔表观解离常数所示。

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