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采用磁偶极力流分选仪通过磁泳对 CD34 细胞进行连续分离。

Sequential CD34 cell fractionation by magnetophoresis in a magnetic dipole flow sorter.

机构信息

Department of Biomedical Engineering, Lerner Research Institute, Cleveland Clinic, 9500 Euclid Avenue, Cleveland, Ohio 44195, USA.

出版信息

Analyst. 2010 Jan;135(1):62-70. doi: 10.1039/b908210g. Epub 2009 Nov 4.

Abstract

Cell separation and fractionation based on fluorescent and magnetic labeling procedures are common tools in contemporary research. These techniques rely on binding of fluorophores or magnetic particles conjugated to antibodies to target cells. Cell surface marker expression levels within cell populations vary with progression through the cell cycle. In an earlier work we showed the reproducible magnetic fractionation (single pass) of the Jurkat cell line based on the population distribution of CD45 surface marker expression. Here we present a study on magnetic fractionation of a stem and progenitor cell (SPC) population using the established acute myelogenous leukemia cell line KG-1a as a cell model. The cells express a CD34 cell surface marker associated with the hematopoietic progenitor cell activity and the progenitor cell lineage commitment. The CD34 expression level is approximately an order of magnitude lower than that of the CD45 marker, which required further improvements of the magnetic fractionation apparatus. The cells were immunomagnetically labeled using a sandwich of anti-CD34 antibody-phycoerythrin (PE) conjugate and anti-PE magnetic nanobead and fractionated into eight components using a continuous flow dipole magnetophoresis apparatus. The CD34 marker expression distribution between sorted fractions was measured by quantitative PE flow cytometry (using QuantiBRITE PE calibration beads), and it was shown to be correlated with the cell magnetophoretic mobility distribution. A flow outlet addressing scheme based on the concept of the transport lamina thickness was used to control cell distribution between the eight outlet ports. The fractional cell distributions showed good agreement with numerical simulations of the fractionation based on the cell magnetophoretic mobility distribution in the unsorted sample.

摘要

基于荧光和磁性标记程序的细胞分离和分级是当代研究中常用的工具。这些技术依赖于荧光染料或与抗体偶联的磁性颗粒与靶细胞的结合。细胞群体中的细胞表面标志物表达水平随细胞周期的进展而变化。在早期的工作中,我们展示了基于 CD45 表面标志物表达的群体分布,可重复性地对 Jurkat 细胞系进行磁性分级(单次通过)。在这里,我们使用已建立的急性髓性白血病细胞系 KG-1a 作为细胞模型,研究了干细胞和祖细胞(SPC)群体的磁性分级。这些细胞表达与造血祖细胞活性和祖细胞谱系决定相关的 CD34 细胞表面标志物。CD34 的表达水平大约低一个数量级,比 CD45 标志物低,这需要对磁性分级设备进行进一步改进。使用抗 CD34 抗体-藻红蛋白(PE)缀合物和抗-PE 磁性纳米珠的三明治对细胞进行免疫磁标记,并使用连续流偶极磁泳装置将细胞分成八个部分进行分级。通过使用 QuantiBRITE PE 校准珠的定量 PE 流式细胞术测量分选后各部分之间的 CD34 标志物表达分布,并显示与细胞磁泳动性分布相关。基于输送层厚度概念的流出口寻址方案用于控制八个出口之间的细胞分布。分数细胞分布与未分级样品中基于细胞磁泳动性分布的分级的数值模拟吻合良好。

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