研究目的
To develop a flow cytometry-based assay for high-throughput detection and quantification of neutrophil extracellular traps (NETs) in mixed cell populations, addressing the limitations of current fluorescence microscopy methods.
研究成果
The developed flow cytometry assay is a sensitive, specific, and reproducible method for detecting and quantifying NETosis in mixed cell populations, offering advantages over traditional microscopy methods. It has potential applications in studying diseases associated with NETosis, such as SLE.
研究不足
The assay may underestimate the late phases of NETosis due to gating strategies and requires careful handling to avoid loss of fragile NET structures. Background readings for untreated samples ranged from 7% to 20%, possibly due to PFA fixation effects.
1:Experimental Design and Method Selection:
The study utilized a flow cytometry-based assay with fluorescent-labeled antibodies against cell markers on PMNs and nucleic acid stains to measure NETosis in whole blood and purified PMNs.
2:Sample Selection and Data Sources:
Blood samples from SLE patients and healthy donors, and bone marrow cells from murine models were used.
3:List of Experimental Equipment and Materials:
Equipment included BD FACSCanto II flow cytometer, Zeiss LSM800 confocal microscope, and reagents such as SYTOX Orange, DAPI, and PMA.
4:Experimental Procedures and Operational Workflow:
PMNs were stimulated with PMA, fixed with PFA, and stained with antibodies and DNA dyes before flow cytometry analysis.
5:Data Analysis Methods:
Data were analyzed using FlowJo and Prism software, with statistical significance assessed using Student’s t-test, ANOVA, and Pearson’s correlation coefficient.
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