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Selective Encapsulation of Single Cells and Subcellular Organelles into Picoliter- and Femtoliter-Volume Droplets

机译:将单细胞和亚细胞器选择性封装成皮升和飞升体积的液滴

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This paper describes a method, which combines optical trapping and microfluidic-based droplet generation, for selectively and controllably encapsulating a single target cell or subcellular structure, such as a mitochondrion, into a picoliter- or femtoliter-volume aqueous droplet that is surrounded by an immiscible phase. Once the selected cell or organelle is encased within the droplet, it is stably confined in the droplet and cannot be removed. We demonstrate in droplet the rapid laser photolysis of the single cell, which essentially "freezes" the state that the cell was in at the moment of photolysis and confines the lysate within the small volume of the droplet. Using fluorescein di-β-D-galactopyranoside, which is a fluorogenic substrate for the intracellular enzyme β-galactosidase, we also assayed the activity of this enzyme from a single cell following the laser-induced lysis of the cell. This ability to entrap individual selected cells or subcellular organelles should open new possibilities for carrying out single-cell studies and single-organelle measurements.
机译:本文介绍了一种方法,该方法结合了光捕获和基于微流体的液滴生成,用于选择性和可控地将单个靶细胞或亚细胞结构(例如线粒体)封装到皮升级或飞升级体积的水滴中,该水滴被不相溶的阶段。一旦选定的细胞或细胞器被包裹在液滴中,它将被稳定地限制在液滴中并且不能被去除。我们在液滴中演示了单个细胞的快速激光光解作用,该过程基本上“冻结”了光解时细胞所处的状态,并将裂解物限制在小滴液滴中。使用荧光素二-β-D-吡喃半乳糖苷(它是细胞内酶β-半乳糖苷酶的荧光底物),我们还从激光诱导的细胞裂解物中检测了单个细胞中该酶的活性。捕获单个选定细胞或亚细胞器的能力应为开展单细胞研究和单细胞器测量开辟新的可能性。

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