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微流控芯片电泳在高通量核酸荧光片段分析检测中的应用。

Application of microfluidic chip electrophoresis for high-throughput nucleic acid fluorescence fragment analysis assays.

作者信息

Sun Yali, Lu Zhi-Xiang, Miller Michael, Perroud Thomas, Tong Yanhong

机构信息

PerkinElmer Health Sciences Division, Waltham, MA 02451, USA.

出版信息

NAR Genom Bioinform. 2023 Jan 31;5(1):lqad011. doi: 10.1093/nargab/lqad011. eCollection 2023 Mar.

Abstract

Nucleic acid fragment analysis via separation and detection are routine operations in molecular biology. However, analysis of small single-stranded nucleic acid fragments (<100nt) is challenging and mainly limited to labor-intensive polyacrylamide gel electrophoresis or high-cost capillary electrophoresis methods. Here we report an alternative method, a microfluidic chip electrophoresis system that provides a size resolution of 5nt and a detection time of one minute per sample of fluorescence-labeled DNA/RNA fragments. The feasibility of this system was evaluated by quantifying CRISPR-Cas9 cleavage efficiency and the detection resolution was evaluated by analyzing ssDNA/RNA adenylation and phosphorylation. We employed this system to study the RNA capping efficiency and double-stranded DNA unwinding efficiency in isothermal amplification as two examples for assay design and evaluation. The microfluidic chip electrophoresis system provides a rapid, sensitive, and high-throughput fluorescence fragment analysis (FFA), and can be applied for enzyme characterization, reaction optimization, and product quality control in various molecular biology processes.

摘要

通过分离和检测进行核酸片段分析是分子生物学中的常规操作。然而,分析小的单链核酸片段(<100nt)具有挑战性,主要限于劳动密集型的聚丙烯酰胺凝胶电泳或高成本的毛细管电泳方法。在此,我们报告一种替代方法,即一种微流控芯片电泳系统,其对荧光标记的DNA/RNA片段的尺寸分辨率为5nt,每个样品的检测时间为一分钟。通过量化CRISPR-Cas9切割效率评估该系统的可行性,通过分析单链DNA/RNA腺苷化和磷酸化评估检测分辨率。我们以等温扩增中的RNA加帽效率和双链DNA解旋效率研究为例,采用该系统进行检测设计和评估。该微流控芯片电泳系统提供了一种快速、灵敏且高通量的荧光片段分析(FFA),可应用于各种分子生物学过程中的酶表征、反应优化和产品质量控制。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/41e6/9887644/b80cb7cf24c7/lqad011fig1.jpg

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