Mass Cytometry: Protocol for Daily Tuning and Running Cell Samples on a CyTOF Mass Cytometer

The Journal of Immunology

Schulz

et al. 2015

Self Cite

149

194

Mass cytometry is developing as a means of multiparametric single cell analysis. Here, we present an approach to barcoding separate live human PBMC samples for combined preparation and acquisition on a CyTOF® instrument. Using six different anti-CD45 antibody (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 reduces wet work and antibody 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 should be applicable to fluorescence flow cytometry as well.

Section: Methodsmentioning

confidence: 99%

Section: Introductionmentioning

confidence: 99%

Barcoding of Live Human Peripheral Blood Mononuclear Cells for Multiplexed Mass Cytometry

Mei

The Journal of Immunology

Schulz

et al. 2015

Self Cite

149

194

“…Stringent barcoding schemes and carefully monitoring and optimizing the concentration of the injected cell sample can eliminate the majority of doublets and help alleviate this problem (28). Variations in machine performance can also be addressed by standardized daily tuning procedures and metal-loaded beads for normalization of mass cytometry data (29,30). Currently, no computational tool exists for quantifying the quality of data and identifying potentially problematic samples.…”

Section: Developmental Trajectory Detection: Wanderlustmentioning

confidence: 99%

Algorithmic Tools for Mining High-Dimensional Cytometry Data

Chester

The Journal of Immunology

2015

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The advent of mass cytometry has lead to an unprecedented increase in the number of analytes measured in individual cells, thereby increasing the complexity and information content of cytometric data. While this technology is ideally suited to detailed examination of the immune system, the applicability of the different methods for analyzing such complex data are less clear. Conventional data analysis by ‘manual’ gating of cells in biaxial dotplots is often subjective, time consuming, and neglectful of much of the information contained in a highly dimensional cytometric dataset. Algorithmic data mining has the promise to eliminate these concerns and several such tools have been recently applied to mass cytometry data. Herein, we review computational data mining tools that have been used to analyze mass cytometry data, outline their differences, and comment on their strengths and limitations. This review will help immunologists identify suitable algorithmic tools for their particular projects.

“…[14]. The length of the run will be dependent upon the volume of your sample: dilution with MilliQ water to ~1 million cells/mL is recommended for minimizing doublets as well as maximizing sample throughput ( see Note 10).…”

Section: Ics Staining Protocolmentioning

confidence: 99%

Multiparameter Phenotyping of Human PBMCs Using Mass Cytometry

Newell

Methods in Molecular Biology

2015

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The standard for single-cell analysis of phenotype and function in recent decades has been fluorescence flow cytometry. Mass cytometry is a newer technology that uses heavy metal ions, rather than fluorochromes, as labels for probes such as antibodies. The binding of these ion-labeled probes to cells is quantitated by mass spectrometry. This greatly increases the number of phenotypic and functional markers that can be probed simultaneously. Here, we review topics that must be considered when adapting existing flow cytometry panels to mass cytometry analysis. We present a protocol and representative panels for surface phenotyping and intracellular cytokine staining (ICS) assays.