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High-throughput optical injection of mammalian cells using a nondiffracting beam in a microfluidic platform

机译:在微流体平台上使用非衍射光束对哺乳动物细胞进行高通量光学注射

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Femtosecond photoporation is an optical, non-invasive method of injecting membrane impermeable substances contained within the surrounding medium into cells. The technique typically addresses individual cells in a static monolayer. While this gives excellent selectivity, it can be time consuming or impractical to treat larger samples. We build on previous work using a microfluidic platform, which allows for a suspension of cells to be dosed with femtosecond light as they flow through a microfluidic channel. A reusuable quartz chip is designed with an 's'-bend with facilitates the delivery of a 'non-diffracting' femtosecond Bessel beam along the centre of the channel. By implementing off-chip hydrodynamic focusing, cells are confined to the central region of the channel and pass along the Bessel beam core where they are photoporated. This new parallel approach allows for higher flow rates to be used compared to the previous, orthogonal, design whilst maintaining the necessary dwell time in the Bessel beam core. Optical injection of the cell membrane impermeable stain propidium iodide has been successful with two cell lines. These have yielded viable injection efficiencies of 31.0±9.5% Chinese hamster ovary cells (CHO-K1) and 20.4±4.2% human promyelocytic cells (HL60) with a cell throughput of up to 10 cells/second. This marks an order of magnitude increase compared to the previous microfluidic design.
机译:飞秒光穿孔是一种将周围介质中所含的不可渗透膜物质注入细胞的一种光学,非侵入性方法。该技术通常处理静态单层中的单个单元。尽管这提供了出色的选择性,但是处理较大的样品可能很耗时或不切实际。我们在以前使用微流体平台的工作的基础上,该平台允许细胞悬浮液在飞过微流体通道时分配飞秒光。可重复使用的石英芯片设计有“ s”形弯曲,有助于沿着通道的中心传输“非衍射”飞秒贝塞尔光束。通过进行芯片外流体动力聚焦,细胞被限制在通道的中心区域,并沿贝塞尔光束核心通过,在此处进行光穿孔。与以前的正交设计相比,这种新的并行方法允许使用更高的流速,同时在Bessel梁芯中保持必要的停留时间。光学注射细胞膜不可渗透的染色碘化丙锭已成功用于两种细胞系。这些已经产生了31.0±9.5%的中国仓鼠卵巢细胞(CHO-K1)和20.4±4.2%的人类早幼粒细胞(HL60)的可行注射效率,细胞吞吐速率高达10个细胞/秒。与以前的微流体设计相比,这标志着数量级的增加。

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