Screening in vivo for RNA-binding peptides from combinatorial libraries.

K Harada, S Horiya, H Zehavi, A D Frankel
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引用次数: 3

Abstract

We have modified a previously developed genetic assay system for RNA-polypeptide interactions in a attempt to more readily identify RNA-binding peptides. The first modification involved the design of a "complex" library that would contain a variety of RNA-binding polypeptides. The second modification involved the use of neomycin phosphotransferase (NPT II) as the reporter gene, therefore allowing "selection" of RNA-binding peptides by kanamycin resistance. The improved screening system should allow the identification of peptides that bind to a variety of RNA structures.

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从组合文库中筛选rna结合肽。
我们已经修改了先前开发的rna -多肽相互作用的遗传分析系统,试图更容易地识别rna结合肽。第一次修改涉及设计一个“复杂”文库,其中包含各种rna结合多肽。第二种修饰涉及使用新霉素磷酸转移酶(NPT II)作为报告基因,因此允许通过卡那霉素抗性“选择”rna结合肽。改进的筛选系统应该允许鉴定结合各种RNA结构的肽。
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