Practical tips for construction of custom Peptide libraries and affinity selection by using commercially available phage display cloning systems.

IF 1.3 Q4 BIOCHEMISTRY & MOLECULAR BIOLOGY Journal of Nucleic Acids Pub Date : 2012-01-01 Epub Date: 2012-09-09 DOI:10.1155/2012/295719
Keisuke Fukunaga, Masumi Taki
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引用次数: 38

Abstract

Phage display technology is undoubtedly a powerful tool for affinity selection of target-specific peptide. Commercially available premade phage libraries allow us to take screening in the easiest way. On the other hand, construction of a custom phage library seems to be inaccessible, because several practical tips are absent in instructions. This paper focuses on what should be born in mind for beginners using commercially available cloning kits (Ph.D. with type 3 vector and T7Select systems for M13 and T7 phage, respectively). In the M13 system, Pro or a basic amino acid (especially, Arg) should be avoided at the N-terminus of peptide fused to gp3. In both systems, peptides containing odd number(s) of Cys should be designed with caution. Also, DNA sequencing of a constructed library before biopanning is highly recommended for finding unexpected bias.

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实用提示构建自定义肽库和亲和选择使用市上可用的噬菌体展示克隆系统。
噬菌体展示技术无疑是靶向肽亲和选择的有力工具。市售的预制噬菌体库使我们能够以最简单的方式进行筛选。另一方面,自定义噬菌体库的构建似乎是不可访问的,因为在说明中缺少一些实用技巧。本文重点介绍了初学者使用市售克隆试剂盒(博士学位,分别使用M13和T7噬菌体的3型载体和T7选择系统)时应注意的事项。在M13体系中,与gp3融合的肽的n端应避免出现Pro或碱性氨基酸(特别是Arg)。在这两种系统中,含有奇数Cys的肽应该谨慎设计。此外,强烈建议在生物筛选之前对构建的文库进行DNA测序,以发现意想不到的偏差。
本文章由计算机程序翻译,如有差异,请以英文原文为准。
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来源期刊
Journal of Nucleic Acids
Journal of Nucleic Acids BIOCHEMISTRY & MOLECULAR BIOLOGY-
CiteScore
3.10
自引率
21.70%
发文量
5
审稿时长
12 weeks
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