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Efficient amplification of light and heavy chain variable regions and construction of a non-immune phage scFv library

机译:轻链和重链可变区的有效扩增和非免疫噬菌体scFv文库的构建

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Non-immune phage scFv library is one of the most attractive resources for therapeutics, diagnostics and basic research. As a matter of fact, quality of the library is limited by inefficient PCR cloning of antibody genes using degenerated primers. PCR using this type of primers is difficult to optimize conditions for efficient amplification, and therefore causes loss of antibody diversities. To overcome this problem, we described a novel two-step amplification of Vκ and VH genes with newly designed primer sets. Initially, we amplified Vκ and VH genes from their signal sequences to the joining region to keep antibody diversity as large as possible. Thereafter, highly degenerated primers were used to amplify the Vκ and VH genes from the framework region 1 to the joining region. The Vκ and VH genes from the second PCR then were linked by PCR overlapping extension to generate the scFv library. Fifteen clones from the library were randomly picked and sequenced, and the diversity of full-length scFvs was confirmed. Expression capability of clones in the library was 80% after confirmation using colony hybridization. The results demonstrated the efficiency of this strategy and the primer sets for construction of the scFv library.
机译:非免疫噬菌体scFv文库是用于治疗,诊断和基础研究的最具吸引力的资源之一。实际上,文库的质量受到使用简并引物的抗体基因PCR克隆效率低的限制。使用这种类型的引物进行的PCR难以优化有效扩增条件,因此会导致抗体多样性丧失。为了克服这个问题,我们描述了使用新设计的引物组对V κ和V H 基因进行新颖的两步扩增。最初,我们将V κ和V H 基因从它们的信号序列扩增到连接区域,以保持尽可能大的抗体多样性。此后,使用高度简并的引物从框架区1到连接区扩增V κ和V H 基因。然后通过PCR重叠延伸将第二次PCR的V κ和V H 基因连接起来,生成scFv文库。从文库中随机挑选15个克隆并测序,并确认了全长scFv的多样性。使用菌落杂交确认后,文库中克隆的表达能力为80%。结果证明了该策略和用于构建scFv文库的引物组的效率。

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