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用于多重质谱流式细胞术的活的人外周血单个核细胞条形码技术

Barcoding of live human peripheral blood mononuclear cells for multiplexed mass cytometry.

作者信息

Mei Henrik E, Leipold Michael D, Schulz Axel Ronald, Chester Cariad, Maecker Holden T

机构信息

Human Immune Monitoring Center, Institute for Immunity, Transplantation and Infection, Stanford University School of Medicine, Stanford, CA 94305; and

Human Immune Monitoring Center, Institute for Immunity, Transplantation and Infection, Stanford University School of Medicine, Stanford, CA 94305; and.

出版信息

J Immunol. 2015 Feb 15;194(4):2022-31. doi: 10.4049/jimmunol.1402661. Epub 2015 Jan 21.

Abstract

Mass cytometry is developing as a means of multiparametric single-cell analysis. In this study, we present an approach to barcoding separate live human PBMC samples for combined preparation and acquisition on a cytometry by time of flight instrument. Using six different anti-CD45 Ab conjugates labeled with Pd104, Pd106, Pd108, Pd110, In113, and In115, respectively, we barcoded up to 20 samples with unique combinations of exactly three different CD45 Ab tags. Cell events carrying more than or less than three different tags were excluded from analyses during Boolean data deconvolution, allowing for precise sample assignment and the electronic removal of cell aggregates. Data from barcoded samples matched data from corresponding individually stained and acquired samples, at cell event recoveries similar to individual sample analyses. The approach greatly reduced technical noise and minimizes unwanted cell doublet events in mass cytometry data, and it reduces wet work and Ab consumption. It also eliminates sample-to-sample carryover and the requirement of instrument cleaning between samples, thereby effectively reducing overall instrument runtime. Hence, CD45 barcoding facilitates accuracy of mass cytometric immunophenotyping studies, thus supporting biomarker discovery efforts, and it should be applicable to fluorescence flow cytometry as well.

摘要

质谱流式细胞术正在发展成为一种多参数单细胞分析方法。在本研究中,我们提出了一种对单独的活人类外周血单核细胞(PBMC)样本进行条形码标记的方法,以便在飞行时间质谱流式细胞仪上进行联合制备和采集。我们分别使用六种不同的用钯104、钯106、钯108、钯110、铟113和铟115标记的抗CD45抗体偶联物,用恰好三种不同的CD45抗体标签的独特组合对多达20个样本进行条形码标记。在布尔数据反卷积过程中,将携带多于或少于三种不同标签的细胞事件排除在分析之外,从而实现精确的样本分配并通过电子方式去除细胞聚集体。条形码标记样本的数据与相应的单独染色和采集样本的数据相匹配,细胞事件回收率与单个样本分析相似。该方法极大地降低了技术噪声,并最大限度地减少了质谱流式细胞术数据中不需要的细胞双联体事件,同时减少了湿实验操作和抗体消耗。它还消除了样本间的残留以及样本之间仪器清洁的要求,从而有效减少了仪器的整体运行时间。因此,CD45条形码标记有助于提高质谱流式细胞术免疫表型研究的准确性,从而支持生物标志物的发现工作,并且它也应该适用于荧光流式细胞术。

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