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Separation of two phenotypically similar cell types via a single common marker in microfluidic channels

机译:通过微流体通道中的单个共同标记物分离两种表型相似的细胞类型

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摘要

To isolate clinically and biologically relevant cell types from a heterogeneous population, fluorescent or magnetic tagging together with knowledge of surface biomarker profiles represents the state of the art. To date, it remains exceedingly difficult to separate phenotypically and physically similar cell types from a mixed population. We report a microfluidic platform engineered to separate two highly similar cell types using a single antibody by taking advantage of subtle variations in surface receptor density and cell size. This platform utilizes antibody-conjugated surfaces in microfluidic channels together with precise modulation of fluid shear stresses to accomplish selective fractionation in a continuous flow process. Antibody conjugation density variation on the adhesive surfaces is achieved by covalently immobilizing an antibody in the presence of poly(ethylene glycol). This platform is used to demonstrate separation of two CD31 positive cell types, human umbilical vein endothelial cells and human micro vascular endothelial cells.
机译:为了从异质群体中分离出临床和生物学上相关的细胞类型,荧光或磁性标记以及表面生物标志物概况的知识代表了现有技术。迄今为止,从混合群体中分离出表型和物理上相似的细胞类型仍然极其困难。我们报道了一种微流控平台,该平台经过工程设计,可以利用表面受体密度和细胞大小的细微变化来使用一种抗体来分离两种高度相似的细胞类型。该平台利用微流体通道中的抗体偶联表面以及流体剪切应力的精确调节,在连续流动过程中实现选择性分离。通过在聚乙二醇存在下共价固定抗体,可实现粘合剂表面抗体结合密度的变化。该平台用于证明两种CD31阳性细胞类型的分离,即人脐静脉内皮细胞和人微血管内皮细胞。

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