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https://doi.org/10.24099/vet. arhiv.1407

Isolation of heterophils from peripheral blood in hens and analysis of heterophil functions by flow cytometry - a methodological study

Erdal Matur ; Istanbul University-Cerrahpaşa, Veterinary Faculty, Department of Physiology, Istanbul, Turkey
Mert Erek ; Istanbul University-Cerrahpaşa, Graduate Education Institute, Istanbul, Turkey
Ezgi Ergen ; Istanbul University-Cerrahpaşa, Veterinary Faculty, Department of Physiology, Istanbul, Turkey
Bilge Acar Bolat ; Istanbul University, Faculty of Business Administration, Department of Quantitative Methods, Istanbul, Turkey
Mukaddes Özcan ; Istanbul University-Cerrahpaşa, Veterinary Faculty, Department of Physiology, Istanbul, Turkey


Puni tekst: engleski pdf 991 Kb

str. 469-482

preuzimanja: 276

citiraj


Sažetak

The aim of this study was to modify the flow cytometric method, which is used for analyzing neutrophils, to analyse the functions of avian heterophils. The blood samples used in the experiments were obtained from hens in slaughterhouses. Blood samples were collected from 10 hens for each trial. Within the scope of the present study, trials were carried out regarding the amount of blood, cell suspension, dihydrorodamine-123 (DHR-123), phorbol-12-myristate-13-acetate (PMA), and N-formyl-methionyl-leucyl-phenylalanine (fMLP), as well as the storage duration of blood samples and incubation time. The results showed that 0.5-3 ml of blood could be used to detect heterophil functions, and it would be ideal to conduct analyses using fresh blood samples. In addition, the results showed that blood stored at +4 °C for up to 8 hours may be also used if necessary. In order to isolate the cells, centrifugation for 30 minutes is sufficient, and it is appropriate to use a 30μL cell suspension. 2μL of DHR-123 should be used as a chemical probe to measure heterophil functions. Excessive use of DHR-123 affected the heterophil functions negatively. In addition, it was observed that using 2μL of fMLP, which is used as an oxidative burst stimulant, and 2μL of PMA as a stimulant of chemotaxic activity, were sufficient. It was concluded that incubation at 41 °C for 5 minutes after stimulating the heterophils is also sufficient. We conclude that the methods established in this study could be used to isolate heterophils and to analyze them by flow cytometry. Therefore, this study would contribute to further research and clinical studies in poultry.

Ključne riječi

avian; phagocytic activity; oxidative burst; chemotaxic activity

Hrčak ID:

283896

URI

https://hrcak.srce.hr/283896

Datum izdavanja:

26.9.2022.

Podaci na drugim jezicima: hrvatski

Posjeta: 888 *