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纳升级液滴中细菌细胞密度的高通量监测:未修饰的革兰氏阳性和革兰氏阴性细菌的无标记检测。

High-Throughput Monitoring of Bacterial Cell Density in Nanoliter Droplets: Label-Free Detection of Unmodified Gram-Positive and Gram-Negative Bacteria.

机构信息

Institute of Physical Chemistry, Polish Academy of Sciences, Kasprzaka 44/52, 01-224 Warsaw, Poland.

International Centre for Translational Eye Research, Institute of Physical Chemistry, Polish Academy of Sciences, Kasprzaka 44/52, 01-224 Warsaw, Poland.

出版信息

Anal Chem. 2021 Jan 19;93(2):843-850. doi: 10.1021/acs.analchem.0c03408. Epub 2020 Dec 10.

DOI:10.1021/acs.analchem.0c03408
PMID:33301291
Abstract

Droplet microfluidics disrupted analytical biology with the introduction of digital polymerase chain reaction and single-cell sequencing. The same technology may also bring important innovation in the analysis of bacteria, including antibiotic susceptibility testing at the single-cell level. Still, despite promising demonstrations, the lack of a high-throughput label-free method of detecting bacteria in nanoliter droplets prohibits analysis of the most interesting strains and widespread use of droplet technologies in analytical microbiology. We use a sensitive and fast measurement of scattered light from nanoliter droplets to demonstrate reliable detection of the proliferation of encapsulated bacteria. We verify the sensitivity of the method by simultaneous readout of fluorescent signals from bacteria expressing fluorescent proteins and demonstrate label-free readout on unlabeled Gram-negative and Gram-positive species. Our approach requires neither genetic modification of the cells nor the addition of chemical markers of metabolism. It is compatible with a wide range of bacterial species of clinical, research, and industrial interest, opening the microfluidic droplet technologies for adaptation in these fields.

摘要

液滴微流控技术通过引入数字聚合酶链式反应和单细胞测序技术,颠覆了分析生物学领域。同样的技术也可能为细菌分析带来重要的创新,包括单细胞水平的抗生素药敏试验。然而,尽管有很有前景的演示,但是缺乏高通量的、无需标记的纳米级液滴中细菌检测方法,限制了对最有趣的菌株的分析,也限制了液滴技术在分析微生物学中的广泛应用。我们使用纳米级液滴散射光的灵敏快速测量来证明对封装细菌增殖的可靠检测。我们通过同时读取表达荧光蛋白的细菌的荧光信号来验证该方法的灵敏度,并在未标记的革兰氏阴性和革兰氏阳性菌上进行无标记的读出。我们的方法既不需要对细胞进行基因修饰,也不需要添加代谢的化学标记物。它与广泛的临床、研究和工业感兴趣的细菌种类兼容,为这些领域中微流控液滴技术的应用开辟了道路。

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