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Tag-Free Microfluidic Separation of Cells against Multiple Markers

机译:针对多个标记的细胞的无标签微流控分离

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Conventional cell separation against multiple markers generally requires the attachment of antibody tags, typically fluorescent or magnetic, to selected cell types in a heterogeneous suspension. This work describes how such separation can be accomplished in a series of microfluidic systems without the need for such tags. Two capture stages containing antibody-functionalized alginate hydrogels are utilized for the isolation of CD34+ and Flk1+ cells from untreated, whole human blood. The capture-release capability of these degradable coatings is harnessed by a mixing chamber and a simple valving system such that the suspension emerging from the first capture stage is prepared for the second capture stage for further enrichment. With this configuration, we demonstrate the isolation of CD34+/Flk1+ endothelial progenitor cells from blood enabled by the depletion of CD34+/Flk1-hematopoietic stem cells population. This ability to achieve isolation of cells against multiple markers in an untagged separation method is of particular significance in applications involving cell implantation-based therapeutics including tissue engineering and molecular analysis.
机译:针对多种标志物的常规细胞分离通常需要将抗体标签(通常是荧光的或磁性的)连接至异质悬浮液中的选定细胞类型。这项工作描述了如何在一系列微流体系统中完成分离,而无需这种标签。利用两个包含抗体功能化藻酸盐水凝胶的捕获阶段,从未经处理的全血中分离出CD34 +和Flk1 +细胞。这些可降解涂层的捕获释放能力通过混合室和简单的阀门系统加以利用,从而使从第一捕获阶段出来的悬浮液准备用于第二捕获阶段,以进一步富集。通过这种配置,我们证明了通过消耗CD34 + / Flk1-造血干细胞群体可以从血液中分离出CD34 + / Flk1 +内皮祖细胞。在无标签分离方法中针对多种标记物实现细胞分离的能力在涉及基于细胞植入的治疗方法(包括组织工程和分子分析)的应用中特别重要。

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