优化工作流程以修饰原代人血管细胞中的 microRNA 表达。

Optimized workflow to modify microRNA expression in primary human intravascular cells.

机构信息

Thrombosis Research Center (TREC), Institute of Clinical Medicine, UiT - The Arctic University of Norway, Tromsø, Norway.

Division of Internal Medicine, University Hospital of North Norway, Tromsø, Norway.

出版信息

BMC Immunol. 2023 Feb 15;24(1):5. doi: 10.1186/s12865-023-00540-9.

DOI:10.1186/s12865-023-00540-9

PMID:36792999

原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC9933393/

Abstract

BACKGROUND

A comprehensive dissection of the role of microRNAs (miRNAs) in gene regulation and subsequent cell functions requires a specific and efficient knockdown or overexpression of the miRNA of interest; these are achieved by transfecting the cell of interest with a miRNA inhibitor or a miRNA mimic, respectively. Inhibitors and mimics of miRNAs with a unique chemistry and/or structural modifications are available commercially and require different transfection conditions. Here, we aimed to investigate how various conditions affect the transfection efficacy of two miRNAs with high and low endogenous expression, miR-15a-5p and miR-20b-5p respectively, in human primary cells.

RESULTS

MiRNA inhibitors and mimics from two commonly used commercial vendors were employed, i.e., mirVana (Thermo Fisher Scientific) and locked nucleic acid (LNA) miRNA (Qiagen). We systematically examined and optimized the transfection conditions of such miRNA inhibitors and mimics to primary endothelial cells and monocytes using either a lipid-based carrier (lipofectamine) for delivery or an unassisted uptake. Transfection of LNA inhibitors with either phosphodiester (PE)- or phosphorothioate (PS)-modified nucleotide bonds, delivered using a lipid-based carrier, efficiently downregulated the expression levels of miR-15a-5p already 24 h following transfection. MirVana miR-15a-5p inhibitor displayed a less efficient inhibitory effect, which was not improved 48 h following a single transfection or two consecutive transfections. Interestingly, LNA-PS miR-15a-5p inhibitor efficiently reduced the levels of miR-15a-5p when delivered without a lipid-based carrier in both ECs and monocytes. When using a carrier, mirVana and LNA miR-15a-5p and miR-20b-5p mimics showed similar efficiency 48 h following transfection to ECs and monocytes. None of the miRNA mimics effectively induced overexpression of the respective miRNA when given to primary cells without a carrier.

CONCLUSION

LNA miRNA inhibitors efficiently downregulated the cellular expression of miRNA, such as miR-15a-5p. Furthermore, our findings suggest that LNA-PS miRNA inhibitors can be delivered in the absence of a lipid-based carrier, whereas miRNA mimics need the aid of a lipid-based carrier to achieve sufficient cellular uptake.

摘要

背景

全面解析 microRNAs（miRNAs）在基因调控及后续细胞功能中的作用，需要对目的 miRNA 进行特异性和高效的敲低或过表达；这可通过将 miRNA 抑制剂或 miRNA 模拟物转染至感兴趣的细胞来实现。具有独特化学性质和/或结构修饰的 miRNA 抑制剂和模拟物可从商业途径获得，且需要不同的转染条件。在此，我们旨在研究不同条件如何影响两种内源性表达水平高低不同的 miRNA（miR-15a-5p 和 miR-20b-5p）在人原代细胞中的转染效率。

结果

我们使用了两种常用商业供应商（Thermo Fisher Scientific 的 mirVana 和 Qiagen 的锁核酸（LNA）miRNA）的 miRNA 抑制剂和模拟物。我们系统地检查并优化了这些 miRNA 抑制剂和模拟物在原代内皮细胞和单核细胞中的转染条件，使用脂质体（lipofectamine）作为递送载体或非辅助摄取。使用脂质体递送具有磷酸二酯（PE）或硫代磷酸（PS）修饰核苷酸键的 LNA 抑制剂，可在转染后 24 小时内有效下调 miR-15a-5p 的表达水平。MirVana miR-15a-5p 抑制剂的抑制效果较差，单次转染或连续两次转染后 48 小时内未见改善。有趣的是，LNA-PS miR-15a-5p 抑制剂在无脂质体载体的情况下在 ECs 和单核细胞中有效降低 miR-15a-5p 的水平。当使用载体时，mirVana 和 LNA miR-15a-5p 和 miR-20b-5p 模拟物在转染后 48 小时对 ECs 和单核细胞的转染效率相似。在没有载体的情况下，没有一种 miRNA 模拟物能有效地诱导原代细胞中相应 miRNA 的过表达。