DNA连接酶
分子生物学
寡核苷酸
DNA
嘌呤霉素
信使核糖核酸
限制性酶
生物
尼克翻译
基因组文库
DNA聚合酶
遗传学
蛋白质生物合成
基因
基序列
作者
T. Kondo,Minori Eguchi,N. Tsuzuki,Naoya Murata,Tomoshige Fujino,Gosuke Hayashi,Hiroshi Murakami
出处
期刊:Bio-protocol
[Bio-Protocol]
日期:2021-01-01
卷期号:11 (16): e4125-e4125
被引量:2
标识
DOI:10.21769/bioprotoc.4125
摘要
Recently, we developed transcription/translation coupled with the association of puromycin linker (TRAP) display as a quick in vitro selection method to obtain antibody-like proteins. For the in vitro selection, it is important to prepare mRNA libraries among which the diversity is high. Here, we describe a method for the preparation of monobody mRNA libraries with greater than 1013 theoretical diversity. First, we synthesized two long single-stranded DNAs that corresponded to fragments of monobody DNA, with random codons in the BC and FG loops. These oligonucleotides were ligated by T4 DNA ligase with the support of guide oligonucleotides containing 3' ends that were protected by a modification. After amplifying the product DNAs by PCR, one end of each DNA fragment was digested with the type II restriction enzyme BsaI, and the resulting DNA fragments were ligated using T4 DNA ligase. After amplification of the DNA product, mRNAs were synthesized by T7 RNA polymerase. This method is simple and could be used for the preparation of mRNA libraries for various antibody-like proteins. Graphic abstract: Construction of a highly diverse mRNA library.
科研通智能强力驱动
Strongly Powered by AbleSci AI