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Characterization of Cellular Optoporation with Distance

机译:距离对细胞定位的表征

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We have developed and characterized cellular optoporation with visible wavelengths of light using standard uncoated glass cover slips as the absorptive media. A frequency-doubled Nd:YAG laser pulse was focused at the interface of the glass surface and aqueous buffer, creating a stress wave and transiently permeabilizing nearby cells. Following optoporation of adherent cells, three spatial zones were present which were distinguished by the viability of the cells and the loading efficiency (or number of extracellular molecules loaded). The loading efficiency also depended on the concentration of the extracellular molecules and the molecular weight of the molecules. In the zone farthest from the laser beam (>60 μm under these conditions), nearly all cells were both successfully loaded and viable. To illustrate the wider applicability of this optoporation method, cells were loaded with a substrate for protein kinase C and the cellular contents then analyzed by capillary electrophoresis. In contrast to peptides loaded by microinjection, optoporated peptide showed little proteolytic degradation, suggesting that the cells were minimally perturbed. Also demonstrating the potential for future work, cells were optoporated and loaded with a fluorophore in the enclosed channels of microfluidic devices.
机译:我们已经开发出了带有标准波长的未涂覆玻璃盖玻片作为吸收介质的具有可见光波长的细胞对映体,并对其进行了表征。将倍频的Nd:YAG激光脉冲聚焦在玻璃表面和水性缓冲液的界面上,产生应力波并瞬时渗透附近的细胞。贴壁细胞对抗后,存在三个空间区域,这些区域以细胞的活力和负载效率(或负载的细胞外分子数量)来区分。加载效率还取决于细胞外分子的浓度和分子的分子量。在距离激光束最远的区域(在这些条件下> 60μm)中,几乎所有细胞均已成功装载并具有活力。为了说明这种对位方法的广泛适用性,将蛋白激酶C的底物加载到细胞中,然后通过毛细管电泳分析细胞含量。与通过显微注射加载的肽相反,磷酸化的肽几乎没有蛋白水解降解,这表明细胞受到的干扰最小。同样证明了未来工作的潜力,细胞在微流体装置的封闭通道中被掩蔽并装载了荧光团。

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