Measurement of canine Th17 cells by flow cytometry

A Knebel; A Kämpe; R Carlson; K Rohn; A Tipold

doi:10.1016/j.vetimm.2021.110366

Measurement of canine Th17 cells by flow cytometry

Vet Immunol Immunopathol. 2022 Jan:243:110366. doi: 10.1016/j.vetimm.2021.110366. Epub 2021 Dec 7.

Authors

A Knebel¹, A Kämpe², R Carlson², K Rohn³, A Tipold²

Affiliations

¹ Department of Small Animal Medicine and Surgery, University of Veterinary Medicine, Hannover, Germany. Electronic address: anna.knebel@tiho-hannover.de.
² Department of Small Animal Medicine and Surgery, University of Veterinary Medicine, Hannover, Germany.
³ Department of Biometry, Epidemiology and Information Processing, University of Veterinary Medicine Hannover, Hannover, Germany.

PMID: 34896773
DOI: 10.1016/j.vetimm.2021.110366

Abstract

Th17 cells are T helper cells which play an important role during inflammation and autoimmune disease. To investigate the role of these cells in diseases in dogs in a clinical setting, methods for fast identification had to be established. Th17 cells are a rare cell population, for their measurement stimulation is recommended. To examine more samples simultaneously and to receive a relatively high purity of cell population of CD3 + CD4+ cells, different methods on various levels of preselection of cells as well as the possibility of storing blood overnight for measuring Th17 cells by flow cytometry were investigated. Firstly, to receive a high number of mononuclear cells, two different density gradients were compared and analysed. Furthermore, the enrichment of CD3 + CD4+ cells via depletion of CD8alpha+, CD11b + and CD21+ cells by cell sorting (autoMACS Pro Separator) was tested. It was also investigated whether stimulation processes led to better interpretation of results and whether there was a significant difference in measurement of directly processed blood samples and samples that had been stored overnight. In conclusion, the use of the density gradient (Lymph24+ Spin Medium) resulted in a purer cell population through a significant decrease in polymorphonuclear cells (*p = 0.01). After cell sorting, a significant difference in cell population purity was detected. Within the target fraction (containing mainly CD3 + CD4+ cells), CD8alpha+, CD21+, CD11b + cell percentages were significantly lower (***p < 0.001, *p < 0.02, ***p < .0001, respectively), and CD3 + CD4+ cell percentage was significantly higher (***p < .0001). There was a significant difference in Th17 cell percentage between unstimulated and stimulated cell populations (***p < .0001), but no significant difference in the percentage of unstimulated Th17 cells (p = 0.29) or stimulated Th17 cells (p = 0.71) in stored blood in comparison to directly processed EDTA blood samples. Finally, a modified protocol that offers an efficient way to investigate samples that were stored overnight by means of flow cytometry was evolved to research the role of Th17 cells in dogs with different diseases or in healthy populations.

Keywords: Cell sorting; Dog; Flow cytometry; Stimulation; Th17 cells.

MeSH terms

Animals
Cell Separation / veterinary
Dogs
Flow Cytometry* / veterinary
Leukocytes
Neutrophils
Th17 Cells*