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基于液滴微流控的脂质体介导的单细胞转染

Lipoplex-Mediated Single-Cell Transfection via Droplet Microfluidics.

机构信息

Department of Biomedical Engineering, University of California, Irvine, Irvine, CA, 92697, USA.

Department of Biochemistry, The Chinese University of Hong Kong, Hong Kong SAR, China.

出版信息

Small. 2018 Oct;14(40):e1802055. doi: 10.1002/smll.201802055. Epub 2018 Sep 10.

DOI:10.1002/smll.201802055
PMID:30199137
Abstract

While lipoplex (cationic lipid-nucleic acid complex)-mediated intracellular delivery is widely adopted in mammalian cell transfection, its transfection efficiency for suspension cells, e.g., lymphatic and hematopoietic cells, is reported at only ≈5% or even lower. Here, efficient and consistent lipoplex-mediated transfection is demonstrated for hard-to-transfect suspension cells via a single-cell, droplet-microfluidics approach. In these microdroplets, monodisperse lipoplexes for effective gene delivery are generated via chaotic mixing induced by the serpentine microchannel and co-confined with single cells. Moreover, the cell membrane permeability increases due to the shear stress exerted on the single cells when they pass through the droplet pinch-off junction. The transfection efficiency, examined by the delivery of the pcDNA3-EGFP plasmid, improves from ≈5% to ≈50% for all three tested suspension cell lines, i.e., K562, THP-1, Jurkat, and with significantly reduced cell-to-cell variation, compared to the bulk method. Efficient targeted knockout of the TP53BP1 gene for K562 cells via the CRISPR (clustered regularly interspaced short palindromic repeats)-CAS9 (CRISPR-associated nuclease 9) mechanism is also achieved using this platform. Lipoplex-mediated single-cell transfection via droplet microfluidics is expected to have broad applications in gene therapy and regenerative medicine by providing high transfection efficiency and low cell-to-cell variation for hard-to-transfect suspension cells.

摘要

尽管脂质体(阳离子脂质-核酸复合物)介导的细胞内递呈被广泛应用于哺乳动物细胞转染,但它对悬浮细胞(如淋巴和造血细胞)的转染效率仅约为 5%,甚至更低。在这里,通过单细胞液滴微流控方法,展示了高效且一致的脂质体介导的悬浮细胞转染。在这些微滴中,通过蛇形微通道诱导的混沌混合生成用于有效基因传递的单分散脂质体,并与单个细胞共限制。此外,当单个细胞通过液滴的挤压连接点时,它们会受到剪切力的作用,从而增加细胞膜的通透性。通过 pcDNA3-EGFP 质粒的传递来检测转染效率,对于所有三种测试的悬浮细胞系(即 K562、THP-1 和 Jurkat),从约 5%提高到约 50%,与批量方法相比,细胞间的变异性显著降低。还使用该平台实现了针对 K562 细胞的 TP53BP1 基因的高效靶向敲除,该基因通过 CRISPR(成簇规律间隔短回文重复)-CAS9(CRISPR 相关核酸酶 9)机制。通过液滴微流控进行的脂质体介导的单细胞转染有望通过为难以转染的悬浮细胞提供高效的转染效率和低的细胞间变异性,在基因治疗和再生医学中得到广泛应用。

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