Measurement of <scp>NET</scp> formation in vitro and in vivo by flow cytometry

Masuda, Sakiko; Shimizu, Shohei; Matsuo, Junji; Nishibata, Yuka; Kusunoki, Yoshihiro; Hattanda, Fumihiko; Shida, Haruki; Nakazawa, Daigo; Tomaru, Utano; Atsumi, Tatsuya; Ishizu, Akihiro

doi:10.1002/cyto.a.23169

Cited by 83 publications

(82 citation statements)

References 27 publications

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“…A side by side comparison with the assay by Gavillet et al revealed greater sensitivity in the detection of NETosis with our protocol (Fig. 3B and Supporting Information (21,25). Similar to our findings, percentage of SG + cells correlated with NET area stained using DAPI and observed on fluorescent microscopy (25).…”

Section: Discussionsupporting

confidence: 89%

“…However, the assay by Nel et al can underestimate the earlier phases of NETosis when the NETs are still PMN‐appendant. Additionally, Masuda et al utilized Sytox Green (SG), a plasma membrane‐impermeable DNA dye, to detect PMN‐appendant NET‐DNA . Similar to our findings, percentage of SG + cells correlated with NET area stained using DAPI and observed on fluorescent microscopy .…”

Section: Discussionsupporting

confidence: 87%

“…3B and Supporting Information (21,25). Similar to our findings, percentage of SG + cells correlated with NET area stained using DAPI and observed on fluorescent microscopy (25). However, SG + cells were gated solely based on FSC and SSC properties, which limit the assay to purified populations and may include debris (54).…”

Section: Discussionsupporting

confidence: 84%

“…In this report, we describe an optimized protocol utilizing a combination of SO and 4 0 ,6-diamidino-2-phenylindole (DAPI) for two-color visualization of NETs on flow cytometry (20). SO + DAPI + PMNs activated with phorbol 12-myristate 13-acetate (PMA) was dose-and time-dependent, as previously described (8,25). To verify that SO + DAPI + PMNs were not due to other forms of cell death, we determined the following findings: (1) minimal SO + DAPI + PMNs with epoptoside-induced apoptosis; (2) correlation in the percentage of SO + DAPI + PMNs with NETosis rate obtained using time-lapse live cell microscopy; and (3) colocalization of extracellular DNA and NE on flow cytometry.…”

Section: Introductionmentioning

confidence: 99%

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A Flow Cytometry‐Based Assay for High‐Throughput Detection and Quantification of Neutrophil Extracellular Traps in Mixed Cell Populations

et al. 2018

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Neutrophil extracellular traps (NETs) are web‐like structures composed of decondensed chromatin and antimicrobial proteins that are released into the extracellular space during microbial infections. This active cell death program is known as NETosis. To date, florescence microscopy is the widely accepted method for visualization and quantification of NETs. However, this method is subjective, time consuming and yields low numbers of analyzed polymorphonuclear cells (PMNs) per sample. Increasing interest has emerged on the identification of NETs using flow cytometry techniques. However, flow cytometry analysis of NETs requires particular precautions for sample preparation to obtain reproducible data. Herein, we describe a flow cytometry‐based assay for high‐throughput detection and quantification of NETosis in mixed cell populations. We used fluorescent‐labeled antibodies against cell markers on PMNs together with a combination of nucleic acid stains to measure NETosis in whole blood (WB) and purified PMNs. Using plasma membrane‐impermeable DNA‐binding dye, SYTOX Orange (SO), we found that cell‐appendant DNA of NETting PMNs were positive for SO and DAPI. The combination of optimally diluted antibody and nucleic acid dyes required no washing and yielded low background fluorescence. Significant correlations were found for NETosis from WB and purified PMNs. We then validated the assay by comparing with time‐lapse live cell fluorescence microscopy and determined very good intraassay and interassay variances. The assay was then applied to a disease associated with NETosis, systemic lupus erythematosus (SLE). We examined PMA‐induced NETosis in peripheral PMNs from SLE patients and controls and in bone marrow PMNs from multiple murine models. In summary, this assay is observer‐independent and allows for rapid assessment of a large number of PMNs per sample. Use of this assay does not require sophisticated microscopic equipment like imaging flow cytometers and may be a starting point to analyze extracellular trap formation from immune cells other than PMNs. © 2018 The Authors. Cytometry Part A published by Wiley Periodicals, Inc. on behalf of International Society for Advancement of Cytometry.

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Section: Discussionsupporting

confidence: 89%

Section: Discussionsupporting

confidence: 87%

Section: Discussionsupporting

confidence: 84%

Section: Introductionmentioning

confidence: 99%

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A Flow Cytometry‐Based Assay for High‐Throughput Detection and Quantification of Neutrophil Extracellular Traps in Mixed Cell Populations

et al. 2018

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“…Flow cytometric assays for direct quantification of cell‐bound NETs on isolated neutrophils has recently been described in a limited number of patients . The purpose of this study was to develop a method of NETs marker quantification for potential routine application using whole blood flow cytometry.…”

Section: Introductionmentioning

confidence: 99%

Quantification of NETs‐associated markers by flow cytometry and serum assays in patients with thrombosis and sepsis

Lee

Cavanaugh

Leung

et al. 2018

Int J Lab Hematology

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Nuclear cytometry and chromatin organization

2018

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The nuclear-targeting chemical probe, for the detection and quantification of DNA within cells, has been a mainstay of cytometry-from the colorimetric Feulgen stain to smart fluorescent agents with tuned functionality. The level of nuclear structure and function at which the probe aims to readout, or indeed at which a DNA-targeted drug acts, is shadowed by a wide range of detection modalities and analytical methods. These methods are invariably limited in terms of the resolution attainable versus the volume occupied by targeted chromatin structures. The scalar challenge arises from the need to understand the extent and different levels of compaction of genomic DNA and how such structures can be re-modeled, reported, or even perturbed by both probes and drugs. Nuclear cytometry can report on the complex levels of chromatin order, disorder, disassembly, and even active disruption by probes and drugs. Nuclear probes can report defining features of clinical and therapeutic interest as in NETosis and other cell death processes. New cytometric approaches continue to bridge the scalar challenges of analyzing chromatin organization. Advances in super-resolution microscopy address the resolution and depth of analysis issues in cellular systems. Typical of recent insights into chromatin organization enabled by exploiting a DNA interacting probe is ChromEM tomography (ChromEMT). ChromEMT uses the unique properties of the anthraquinone-based cytometric dye DRAQ5™ to reveal that local and global 3D chromatin structures effect differences in compaction. The focus of this review is nuclear and chromatin cytometry, with linked reference to DNA targeting probes and drugs as exemplified by the anthracenediones.

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Measurement of NET formation in vitro and in vivo by flow cytometry

Cited by 83 publications

References 27 publications

A Flow Cytometry‐Based Assay for High‐Throughput Detection and Quantification of Neutrophil Extracellular Traps in Mixed Cell Populations

A Flow Cytometry‐Based Assay for High‐Throughput Detection and Quantification of Neutrophil Extracellular Traps in Mixed Cell Populations

Quantification of NETs‐associated markers by flow cytometry and serum assays in patients with thrombosis and sepsis

Nuclear cytometry and chromatin organization

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