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Single step generation of protein arrays from DNA by cell-free expression and in situ immobilisation (PISA method)

机译:单步生成蛋白质 通过无细胞表达和原位固定从DNA中提取阵列 (PISA方式)

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摘要

We describe a format for production of protein arrays termed ‘protein in situ array’ (PISA). A PISA is rapidly generated in one step directly from PCR-generated DNA fragments by cell-free protein expression and in situ immobilisation at a surface. The template for expression is DNA encoding individual proteins or domains, which is produced by PCR using primers designed from information in DNA databases. Coupled transcription and translation is carried out on a surface to which the tagged protein adheres as soon as it is synthesised. Because proteins generated by cell-free synthesis are usually soluble and functional, this method can overcome problems of insolubility or degradation associated with bacterial expression of recombinant proteins. Moreover, the use of PCR-generated DNA enables rapid production of proteins or domains based on genome information alone and will be particularly useful where cloned material is not available. Here we show that human single-chain antibody fragments (three domain, VH/K form) and an enzyme (luciferase) can be functionally arrayed by the PISA method.
机译:我们描述了一种用于生产蛋白质阵列的格式,称为“蛋白质原位阵列”(PISA)。通过无细胞蛋白表达并原位固定在表面上,可直接从PCR生成的DNA片段快速一步生成PISA。用于表达的模板是编码单个蛋白质或结构域的DNA,该DNA是使用DNA数据库信息设计的引物通过PCR产生的。标记的蛋白质一合成,就会在附着的表面上进行转录和翻译的耦合。由于通过无细胞合成产生的蛋白质通常是可溶的且具有功能,因此该方法可以克服与重组蛋白质的细菌表达有关的不溶性或降解问题。而且,使用PCR生成的DNA可以仅基于基因组信息就可以快速生产蛋白质或结构域,在无法获得克隆材料的情况下将特别有用。在这里,我们显示了人单链抗体片段(三个域,VH / K形式)和一种酶(荧光素酶)可以通过PISA方法进行功能排列。

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