从HIV感染者中系统分离免疫细胞亚群用于miRNA分析的效用。

Utility of Systematic Isolation of immune cell subsets from HIV-infected individuals for miRNA profiling.

作者信息

Bargalló Manel E, Guardo Alberto C, Maleno Maria J, Miralles Laia, Egaña-Gorroño Lander, Escribà Tuixent, García Felipe, Gatell Jose M, Arnedo Mireia, Plana Montserrat

机构信息

Institut d'Investigacions Biomèdiques August Pi i Sunyer, Hospital Clínic de Barcelona, Barcelona, Spain.

Infectious Diseases Department, Hospital Clínic de Barcelona, Barcelona, Spain.

出版信息

J Immunol Methods. 2017 Mar;442:12-19. doi: 10.1016/j.jim.2016.12.005. Epub 2016 Dec 27.

DOI:10.1016/j.jim.2016.12.005

PMID:28039100

Abstract

INTRODUCTION

Peripheral blood mononuclear cells (PBMCs) are frequently used for genomic analyses, but several factors can affect the yield and integrity of nucleic acids, including the methods of cell collection and isolation. The goal of this work was to analyze the utility of systematic isolation of different immune cell subsets by immunomagnetic separation and the RNA integrity after isolated cells from samples of HIV-infected patients.

METHODS

PBMC from Healthy Controls (HC, n=15), Elite Controllers (EC, n=15), Viremic Controllers (VC, n=15), Viremic Progressors (VP, n=15) and HIV-infected patients on therapy (ART, n=15) were isolated by Ficoll-Paque density gradient centrifugation. Subsets were separated with monoclonal antibodies (CD56, CD14, CD4, and CD8) conjugated to microbeads. We evaluated the yield and purity of each subset isolated from PBMCs under resting and activated conditions; LPS, anti-CD3/CD28 and anti-CD16 were used to activate monocytes, PBMC, T cells and NK cells, respectively. The quality of extracted RNA was tested by 2100 Bioanalyzer.

RESULTS

In resting conditions, the average yield of CD14 (monocytes) was decreased (p=0.021) in HIV+ patients compared with healthy controls. CD56 (Natural Killer-NKs; p=0.03) and CD8 (Cytotoxic T lymphocytes-CTL p=0.001) cells were increased in HIV+ patients after 72h of activation. The purity assay detected significant differences in CD14 (p≤0.001) and CD8 (p=0.034) subpopulations when comparing PBMC isolated either from healthy controls or HIV+ patients. The number of activated cells in HIV+ presented differences in CD8 subset (p=0.003). Finally, similar quantities of high quality RNA were extracted from immune cells subsets obtained by our method. Specifically, we show that Bioanalyzer electrophenograms reveal optimal RIN values in HIV positive and negative patients in resting condition (EC:8;HC:6.5;VC:8.80;VP:8;HAART:7.5) and activated condition (EC:9;HC:6.7;VC:8.2;VP:7.2;HAART:8.6).

CONCLUSION

This method allowed us to obtain a sufficient quantity of different isolated immune cell subsets from HIV-infected individuals at different disease stages. Moreover, the assessed qualities of nucleic acids allow us to perform subsequent molecular studies, such as microRNA profiling.

摘要

引言

外周血单个核细胞（PBMC）常用于基因组分析，但包括细胞采集和分离方法在内的几个因素会影响核酸的产量和完整性。本研究的目的是分析通过免疫磁珠分离系统分离不同免疫细胞亚群的实用性以及从HIV感染患者样本中分离细胞后的RNA完整性。

方法

通过Ficoll-Paque密度梯度离心法从健康对照（HC，n = 15）、精英控制者（EC，n = 15）、病毒血症控制者（VC，n = 15）、病毒血症进展者（VP，n = 15）以及接受治疗的HIV感染患者（ART，n = 15）中分离PBMC。使用与微珠偶联的单克隆抗体（CD56、CD14、CD4和CD8）分离亚群。我们评估了在静息和激活条件下从PBMC中分离出的每个亚群的产量和纯度；分别使用脂多糖、抗CD3/CD28和抗CD16激活单核细胞、PBMC、T细胞和NK细胞。通过2100生物分析仪检测提取RNA的质量。

结果

在静息条件下，与健康对照相比，HIV阳性患者中CD14（单核细胞）的平均产量降低（p = 0.021）。激活72小时后，HIV阳性患者中CD56（自然杀伤细胞-NK；p = 0.03）和CD8（细胞毒性T淋巴细胞-CTL，p = 0.001）细胞增加。在比较从健康对照或HIV阳性患者中分离的PBMC时，纯度分析检测到CD14（p≤0.001）和CD8（p = 0.034）亚群存在显著差异。HIV阳性患者中激活细胞的数量在CD8亚群中存在差异（p = 0.003）。最后，通过我们的方法从免疫细胞亚群中提取了相似数量的高质量RNA。具体而言，我们表明生物分析仪电泳图显示HIV阳性和阴性患者在静息条件下（EC：8；HC：6.5；VC：8.80；VP：8；HAART：7.5）和激活条件下（EC：9；HC：6.7；VC：8.2；VP：7.2；HAART：8.6）的最佳RIN值。