用mRNA展示和基因连锁乳剂聚合酶链反应筛选fab片段。

IF 1.3 Q4 BIOCHEMISTRY & MOLECULAR BIOLOGY
Journal of Nucleic Acids Pub Date : 2012-01-01 Epub Date: 2012-09-23 DOI:10.1155/2012/371379
Takeshi Sumida, Hiroshi Yanagawa, Nobuhide Doi
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引用次数: 24

摘要

利用展示法进行体外筛选已成为工程重组抗体的有效工具。与噬菌体等基于细胞的展示方法相比,基于无细胞翻译系统的mRNA展示具有文库规模更大、选择过程更快的优点。然而,mRNA的展示仅限于选择单链多肽,如scFvs,因为它具有将新生多肽与其在核糖体上的编码mRNA连接起来的特性。本文提出了一种利用mRNA展示与乳剂PCR相结合的方法筛选异二聚体Fab片段的新方法。我们设计了一对互补的5' UTR序列,通过重叠延伸PCR将Fab重链和轻链基因连接在一起。我们证实,在一个Fab片段的重链和轻链上,两个mrna显示的多肽被关联成活性形式,并且一个特定的Fab片段基因在每轮模型亲和选择之后被基因链接乳状PCR富集超过100倍。我们进一步从随机的Fab片段库中进行了具有更高结合活性的Fab片段的定向进化。
本文章由计算机程序翻译,如有差异,请以英文原文为准。

In vitro selection of fab fragments by mRNA display and gene-linking emulsion PCR.

In vitro selection of fab fragments by mRNA display and gene-linking emulsion PCR.

In vitro selection of fab fragments by mRNA display and gene-linking emulsion PCR.

In vitro selection of fab fragments by mRNA display and gene-linking emulsion PCR.

In vitro selection by display methods has been an effective tool for engineering recombinant antibodies. mRNA display based on a cell-free translation system has the advantages of larger library sizes and quicker selection procedures compared with cell-based display methods such as phage display. However, mRNA display has been limited to select single-chain polypeptides such as scFvs due to its characteristic of linking a nascent polypeptide with its encoding mRNA on the ribosome. Here we demonstrated a new way of selecting heterodimeric Fab fragments by using mRNA display combined with emulsion PCR. We designed a pair of complementary 5' UTR sequences that can link the Fab heavy and light chain genes together by overlap-extension PCR in water-in-oil emulsions. We confirmed that two mRNA-displayed polypeptides for heavy and light chain of a model Fab fragment were associated into the active form and that a specific Fab fragment gene was enriched over 100-fold per round of a model affinity selection followed by the gene-linking emulsion PCR. We further performed directed evolution of Fab fragments with higher binding activity from a randomized Fab fragment library.

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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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