Witt Martin, Phung Ngoc Linh, Stalke Amelie, Walter Johanna-Gabriela, Stahl Frank, von Neuhoff Nils, Scheper Thomas
Institute of Technical Chemistry Leibniz University Hannover Hannover Germany.
Institute for Cellular and Molecular Pathology Hannover Medical School Hannover Germany.
Eng Life Sci. 2017 Aug 28;17(8):953-958. doi: 10.1002/elsc.201700047. eCollection 2017 Aug.
The selection of aptamers represents a promising route in the development of high affinity ligands. In these processes the formation of by-products is a common problem during the PCR-based amplification of complex oligonucleotide libraries. One approach to overcome this drawback is to separate each template oligonucleotide into an individual reaction compartment provided by a droplet. This method, termed emulsion PCR (ePCR), has already emerged to a standard method in sample preparation for 2nd generation sequencing. In this work, we compare different literature protocols that have been developed to generate stable emulsions for ePCR. We investigate different emulsification methods and evaluate the importance of the initial template concentration. We demonstrate that emulsion stability is of utmost importance for the successful inhibition of by-product formation and give an optimized protocol for generation of an emulsified PCR.
适配体的筛选是开发高亲和力配体的一条有前景的途径。在这些过程中,副产物的形成是基于PCR扩增复杂寡核苷酸文库时常见的问题。克服这一缺点的一种方法是将每个模板寡核苷酸分离到由液滴提供的单独反应隔室中。这种方法称为乳液PCR(ePCR),已成为第二代测序样品制备中的标准方法。在这项工作中,我们比较了为ePCR生成稳定乳液而开发的不同文献方案。我们研究了不同的乳化方法,并评估了初始模板浓度的重要性。我们证明乳液稳定性对于成功抑制副产物形成至关重要,并给出了生成乳化PCR的优化方案。
