The effect of postprandial in vivo and experimental in vitro hyperlipidemia on human peripheral blood monocytes

Q4 Pharmacology, Toxicology and Pharmaceutics
I. Mănescu, Mariuca Manescu, Elena Cristina Preda, D. Manu, M. Dobreanu
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引用次数: 0

Abstract

Abstract Objective: In this study, we aimed to investigate the effect of transient postprandial in vivo and prolonged experimental in vitro hyperlipidemia on human peripheral blood monocytes. Methods: Peripheral blood was collected from seven healthy subjects after an overnight fast and three hours after a standardized high-fat meal. Both fasting and postprandial samples were stained for surface markers CD14/CD11b and intracellular lipids using BODIPY493/503. Postprandial samples only were used for isolation of peripheral blood mononuclear cells that were further incubated overnight with postprandial hyperlipidemic autologous plasma, then stained as described above. All samples were analyzed on a FACSAria III flow cytometer. Results: Flow cytometric analysis revealed two monocyte populations (CD14+): CD14low and CD14high. In fasting, these populations show similar morphology (FSC/SSC), but different expressions of CD14, CD11b, and BODIPY493/503. At three hours postprandially, a moment of maximum hyperlipidemia, neither population suffered significant changes. After the 24-hour incubation, cell activation was observed in both populations: similar fold change increase in SSC, increase in FSC for CD14high cells only, similar foldchange increase in CD14, slightly higher foldchange increase in CD11b for CD14low monocytes, and significantly higher foldchange increase in lipid content for CD14high monocytes. CD14high monocytes appear to undergo a more intense activation than CD14low monocytes. Conclusions: We conclude that all monocytes react after prolonged in vitro exposure to plasma lipids, each subset having its own activation pattern. All monocyte types may play a role in inflammation and the development of plaques. Monocyte assays are a valuable tool for the investigation of atherosclerosis at the cellular level.
餐后体内及实验外高脂血症对人外周血单核细胞的影响
摘要目的:本研究旨在探讨体内短暂性餐后高脂血症和体外长时间实验性高脂血症对人外周血单核细胞的影响。方法:采集7名健康受试者空腹过夜和标准高脂餐后3小时的外周血。使用BODIPY493/503对空腹和餐后样品进行表面标记物CD14/CD11b和细胞内脂质染色。餐后样本仅用于分离外周血单个核细胞,这些细胞与餐后高脂血症自体血浆进一步孵育过夜,然后按上述方法染色。所有样本在FACSAria III型流式细胞仪上进行分析。结果:流式细胞术分析显示两个单核细胞群(CD14+): CD14低和CD14高。在禁食时,这些人群表现出相似的形态(FSC/SSC),但CD14、CD11b和BODIPY493/503的表达不同。在餐后3小时,也就是高脂血症最严重的时刻,两种人群都没有明显的变化。24小时孵育后,在两组细胞中均观察到细胞活化:SSC有相似的折叠变化增加,仅CD14高细胞有FSC增加,CD14有相似的折叠变化增加,CD14低单核细胞CD11b的折叠变化增加略高,CD14高单核细胞的脂质含量有明显更高的折叠变化增加。cd14高的单核细胞似乎比cd14低的单核细胞经历更强烈的激活。结论:我们得出结论,所有单核细胞在长时间体外暴露于血浆脂质后都有反应,每个亚群都有自己的激活模式。所有单核细胞类型都可能在炎症和斑块的形成中发挥作用。单核细胞检测是在细胞水平上研究动脉粥样硬化的一种有价值的工具。
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来源期刊
Acta Marisiensis - Seria Medica
Acta Marisiensis - Seria Medica Pharmacology, Toxicology and Pharmaceutics-Pharmacology, Toxicology and Pharmaceutics (all)
CiteScore
0.40
自引率
0.00%
发文量
0
审稿时长
24 weeks
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