Optimized in vitro isolation of different subpopulation of immune cells from peripheral blood and comparative techniques for generation of monocyte-derived macrophages in small ruminants

外周血单个核细胞 生物 免疫系统 浅黄色外套 单核细胞 流式细胞术 体外 人口 分子生物学 男科 免疫学 CD14型 医学 生物化学 环境卫生
作者
Noive Arteche-Villasol,Júlio Benavides,José Espinosa,Raquel Vallejo,M. Royo,M.C. Ferreras,Valentín Pérez Pérez,Daniel Gutiérrez-Expósito
出处
期刊:Veterinary Immunology and Immunopathology [Elsevier BV]
卷期号:230: 110131-110131 被引量:11
标识
DOI:10.1016/j.vetimm.2020.110131
摘要

• Lymphoprep™ allows the simultaneous isolation of PBMCs and neutrophils. • Magnetic cell separation offers the highest purity of monocyte population. • The use of GM-CSF is highly recommended for an optimal generation of MDMs. • Purified monocytes throughout adherence method lead the highest number of MDMs. Peripheral blood from healthy sheep ( n = 3) and goats ( n = 3) were employed to establish an efficient method for simultaneous isolation of peripheral blood mononuclear cells (PBMCs) and neutrophils and to standardize protocols for monocyte purification and generation of monocyte-derived macrophages (MDMs). In both species, a significantly enriched population of PBMCs, with higher purity and number of cells determined by flow cytometry, was achieved when processing through a density gradient a mixture of buffy-coat and red blood cell layer (RBC) in comparison to the use of just the buffy-coat ( p < 0.05). Neutrophils could be subsequently isolated from the layer, located underneath PBMCs fraction with significant higher purity rates, higher than 85 % determined by flow cytometry, than those obtained with protocols without density gradients (< 60 %) ( p < 0.05). This technique would allow the isolation of both cell populations from the same sample of blood. A pure cell population of monocytes, CD14 + cells, was purified from PBMCs when using immunomagnetic columns, which allow for 17 % (nº monocytes/nº PBMCs) of yield and high percentages of expression of CD14 + (88 %), MHC-II + (91.5 %) and CD11b + (94 %) established by flow cytometry. On the other hand, the classical and non-expensive purification of monocytes from PBMCs based on the adherence capacity of the former, allowed significantly lower yield of monocytes (4.6 %), with percentages of surface markers expression that dropped to 35 %, 65 % and 55 %, respectively ( p < 0.001), suggesting the isolation of a mixed population of cells. The addition of GM-CSF to the culture, at concentration from 25 to 125 ng/mL, enhanced proportionally the number of MDMs generated compared to the absence of supplementation or the use of autologous serum from 5% to 20 %. However, purification of monocytes through the adherence method achieved higher yields of MDMs than those isolated through immunomagnetic columns in both species ( p < 0.001). Under the conditions of this study, the use of centrifugation in density gradients allow for the simultaneous purification of PBMCs and neutrophils, with high purity of both populations, from the same sample of blood. The isolation of monocytes could be subsequently achieved through two different methods, i.e. based on immunomagnetic columns or adherence. The preference between both methods would depend on the necessities of the experiment, the initial sample with high purity of monocytes or a final population of MDMs required.
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