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Generating addressable protein microarrays with PROfusion~(TM) covalent mRNA-protein fusion technology

机译:利用PROfusion〜(TM)共价mRNA-蛋白质融合技术生成可寻址的蛋白质微阵列

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摘要

An mRNA-protein fusion consists of a polypeptide covalently linked to its corresponding mRNA. These species, prepared individually or en masse by in vitro translation with a modified mRNA conjugate (the PROfusion~(TM) process), link phenotype to genotype and enable powerful directed evolution schemes. We have exploited the informational content of the nucleic acid component of the mRNA-protein fusion to create an addressable protein microarray that self-assembles via hybridization to surface-bound DNA capture probes. The nucleic acid component not only directs the mRNA-protein fusion to the proper coordinate of the microarray, but also positions the protein in a uniform orientation. We demonstrate the feasibility of this protein chip concept with several mRNA-protein fusions, each possessing a unique peptide epitope sequence. These addressable proteins could be visualized on the microarray both by autoradiography and highly specific monoclonal antibody binding. The anchoring of the protein to the chip surface is surprisingly robust, and the system is sensitive enough to detect-sub-attomole quantities of displayed protein without signal amplification. Such protein arrays should be useful for functional screening in massively parallel formats, as well as other applications involving immobilized peptides and proteins.
机译:mRNA-蛋白融合物由与其相应的mRNA共价连接的多肽组成。这些物种可以单独制备,也可以通过体外修饰修饰的mRNA缀合物(PROfusionTM方法)进行大规模制备,将表型与基因型联系起来,并实现了功能强大的定向进化方案。我们已经利用mRNA-蛋白质融合的核酸成分的信息含量来创建可寻址的蛋白质微阵列,该微阵列通过与表面结合的DNA捕获探针杂交而自组装。核酸成分不仅将mRNA-蛋白质融合引导到微阵列的适当坐标,而且将蛋白质定位在一致的方向上。我们证明了该蛋白芯片概念与几个mRNA-蛋白融合体的可行性,每个融合体均具有独特的肽表位序列。通过放射自显影和高度特异性的单克隆抗体结合,可以在微阵列上可视化这些可寻址蛋白质。蛋白质锚定在芯片表面的功能出奇地坚固,并且该系统足够灵敏,可以检测到亚原子量的展示蛋白质,而无需信号放大。此类蛋白质阵列应可用于大规模平行形式的功能筛选,以及涉及固定化肽和蛋白质的其他应用。

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