Development of a 43 color panel for the characterization of conventional and unconventional T-cell subsets, B cells, NK cells, monocytes, dendritic cells, and innate lymphoid cells using spectral flow cytometry
| Author | Sahir, Fairooz |
| Author | Mateo, Jericha Miles |
| Author | Steinhoff, Martin |
| Author | Siveen, Kodappully Sivaraman |
| Available date | 2025-01-23T07:03:13Z |
| Publication Date | 2024 |
| Publication Name | Cytometry Part A |
| Resource | Scopus |
| Identifier | http://dx.doi.org/10.1002/cyto.a.24288 |
| ISSN | 15524922 |
| Abstract | Although many flow cytometers can analyze 30–50 parameters, it is still challenging to develop a 40+ color panel for the phenotyping of immune cells using fluorochrome conjugated antibodies due to limitations in the availability of spectrally unique fluorochromes that can be excited by the commonly used laser lines (UV, Violet, Blue, Green/Yellow-green, and Red). Spectral flowcytometry is capable of differentiating fluorochromes with significant overlap in the emission spectra, enabling the use of spectrally similar fluorochrome pairs such as Brilliant Blue 515 and FITC in a single panel. We have developed a 43 color panel to characterize most of the immune subsets within the peripheral immune system, including conventional T cells, unconventional T cells such as invariant natural killer T cells (iNKT), Gamma delta (γδ) T-cell subsets (TCR Vδ2, TCR Vγ9) and mucosal-associated invariant T cells (MAIT), B-cell subsets, natural killer (NK) cells, plasmacytoid dendritic cells, dendritic cell subsets, hematopoietic progenitor cells, basophils, and innate lymphoid cell (ILC) subsets (CD117, CRTH2). The panel includes surface markers to analyze activation (CD38, HLA-DR, ICOS/CD278), differentiation (CD45RA, CD27, CD28, CD57), expression of cytokine and chemokine receptors (CD25, CD127, CCR10, CCR6, CCR4, CXCR3, CXCR5, CRTH2/CD294), and co-inhibitory molecules and exhaustion (PD-1, CD223/LAG-3, TIGIT), which enables a deep characterization of PBMCs from peripheral blood. Cells were analyzed on a 5-laser Cytek Aurora and data analysis was done using FlowJo. This panel can help to make a thorough interpretation of immune system, specifically when specimen quantity is low. The panel has not been completely optimized but would rather act as a guide toward the development of a workflow for optimized multicolor immunophenotyping panel. |
| Sponsor | The authors would like to thank Medical Research Centre, Hamad Medical Corporation for the funding (IRGC-03-NI-17-071 to Kodappully Sivaraman Siveen; IRGC-04-SI-17-151 and MRC-03-19-039 to Martin Steinhoff) and Dr. Michal Kulinski and Dr. Majid Alam for their support. The publication of this article was funded by the Qatar National Library, Doha, Qatar. The authors would like to thank Medical Research Centre, Hamad Medical Corporation for the funding (IRGC\u201003\u2010NI\u201017\u2010071 to Kodappully Sivaraman Siveen; IRGC\u201004\u2010SI\u201017\u2010151 and MRC\u201003\u201019\u2010039 to Martin Steinhoff) and Dr. Michal Kulinski and Dr. Majid Alam for their support. The publication of this article was funded by the Qatar National Library, Doha, Qatar. |
| Language | en |
| Publisher | John Wiley and Sons Inc |
| Subject | dendritic cells immunophenotyping innate lymphoid cells spectral flow cytometry unconventional T cells |
| Type | Article |
| Pagination | 404-410 |
| Issue Number | 5 |
| Volume Number | 105 |
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