流式细胞术检测红细胞衰老标志物

María Alejandra Ensinck, M. L. Brajovich, S. G. Borrás, C. Cotorruelo, C. Biondi
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引用次数: 2

摘要

背景:成熟的红细胞缺乏蛋白质合成,无法恢复失活的酶、受损的细胞骨架和膜蛋白。条带3的氧化破坏可能是导致衰老细胞抗原产生的机制的一部分。这种特异性信号通过诱导自体IgG和C3的结合来清除RBCs,从而导致吞噬作用。此外,磷脂酰丝氨酸分子出现在外膜中,CD47的表达减少。方法:采用流式细胞术分析全血中不同年龄红细胞的光散射特性、自身IgG的结合、C3补体沉积、磷脂酰丝氨酸的外化和CD47的表达。基于前向散射与侧向散射参数的点图分析显示了两个不同大小和密度的RBCs种群。将RBCs与Alexa 488 IgG、APC-anti-C3、PE-annexin-V和PE-CD47进一步孵育。通过匹配样本的Student t检验或Wilcoxon检验(验证正态性假设后)对SeRBC和YRBC群体中研究的不同变量的值进行比较。结果:衰老红细胞群体中IgG和C3阳性细胞比例明显增高。SeRBCs中膜联蛋白-V阳性RBCs的比例也较大,而CD47在该人群中的表达较低。结论:这些结果表明,流式细胞术可以区分不同年龄的红细胞群体,使该工具成为研究红细胞衰老过程的有用替代选择。这些发现将有助于更好地理解红细胞衰老过程和机制。
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Erythrocyte Senescent Markers by Flow Cytometry
Background: Mature red blood cells lack protein synthesis and are unable to restore inactivated enzymes, damaged cytoskeleton and membrane proteins. An oxidation breakdown of band 3 is probably part of the mechanism leading to the generation of a senescent cell antigen. This specific signal serves for the clearance of RBCs by inducing the binding of autologous IgG and C3, leading to phagocytosis. In addition, phosphatidilserin molecules appear in the outer membrane and the CD47 expression diminishes. Methods: Erythrocytes of different ages from whole blood were studied by flow cytometry analysing light scatter proprieties, binding of autologous IgG, C3 complement deposits, externalization of phosphatidylserine and CD47 expression. Dot-plot analysis based on forward scatter versus side scatter parameters showed two RBCs populations of different sizes and density. RBCs were further incubated with Alexa 488 IgG, APC-anti-C3, PE-annexin-V and PE-CD47. The comparison of the values obtained for the different variables studied in SeRBC and YRBC populations was carried out by the Student t-test for matched samples or by the Wilcoxon test (after verification of the normality assumption). Results: The percentage of IgG and C3 positive cells was significantly higher in senescent red blood cells population. The fraction of annexin-V positive RBCs was also larger in SeRBCs while the CD47 expression was lower in this population. Conclusions: These results indicate that flow cytometry allow differenciation of erythrocytes populations of different ages, turning this tool into an useful alternative option to study erythrocyte aging process. These findings will contribute to a better understanding of the process and mechanisms involved in erythrocyte senescence process.
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