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Scalable and automated CRISPR-based strain engineering using droplet microfluidics

机译:使用液滴微流控技术进行可扩展和自动化的基于CRISPR的应变工程

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We present a droplet-based microfluidic system that enables CRISPR-based gene editing and high-throughput screening on a chip. The microfluidic device contains a 10 x 10 element array, and each element contains sets of electrodes for two electric field-actuated operations: electrowetting for merging droplets to mix reagents and electroporation for transformation. This device can perform up to 100 genetic modification reactions in parallel, providing a scalable platform for generating the large number of engineered strains required for the combinatorial optimization of genetic pathways and predictable bioengineering. We demonstrate the system's capabilities through the CRISPR-based engineering of two test cases: (1) disruption of the function of the enzyme galactokinase (galK) in E. coli and (2) targeted engineering of the glutamine synthetase gene (glnA) and the blue-pigment synthetase gene (bpsA) to improve indigoidine production in E. coli.
机译:我们提出了一种基于液滴的微流控系统,该系统可在芯片上实现基于CRISPR的基因编辑和高通量筛选。微流控装置包含一个 10 x 10 元件阵列,每个元件包含用于两种电场驱动操作的电极组:用于合并液滴以混合试剂的电润湿和用于转化的电穿孔。该设备可以并行执行多达 100 个基因修饰反应,为生成遗传途径组合优化和可预测生物工程所需的大量工程菌株提供了一个可扩展的平台。我们通过两个测试用例的基于CRISPR的工程展示了该系统的能力:(1)破坏大肠杆菌中半乳糖激酶(galK)的功能,以及(2)谷氨酰胺合成酶基因(glnA)和蓝色素合成酶基因(bpsA)的靶向工程,以改善大肠杆菌中靛蓝的产生。

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