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大孔介孔硅纳米粒子促进 rno-miRNA-26a-5p 的高效转染和骨向分化的长期稳定性。

Efficient transfection and long-term stability of rno-miRNA-26a-5p for osteogenic differentiation by large pore sized mesoporous silica nanoparticles.

机构信息

School of Dentistry, The University of Queensland, Herston QLD 4006, Australia.

Taiyuan University of Technology, Taiyuan, 030024, China.

出版信息

J Mater Chem B. 2021 Mar 11;9(9):2275-2284. doi: 10.1039/d0tb02756a.

DOI:10.1039/d0tb02756a
PMID:33606863
Abstract

MicroRNA (miRNA) based therapy for bone repair has shown promising results for regulating stem cell proliferation and differentiation, an efficient and stable vector for delivery of microRNA delivery is needed. The present study explored the stability and functionality of lyophilized mesoporous silica nanoparticles with core-cone structure and coated with polyethylenimine (MSN-CC-PEI) as a system for delivering Rattus norvegicus (rno)-miRNA-26a-5p into rat marrow mesenchymal cells (rBMSCs) to promote their osteogenic differentiation. We assessed the cellular uptake and transfection efficiency of nanoparticles loaded with labelled miRNA using confocal laser scanning microscopy and flow cytometry, and the cell viability using the MTT assay. The expression levels of osteogenic genes after one and two weeks were analysed by quantitative reverse transcription-polymerase chain reaction (qRT-PCR). Extracellular matrix deposition and mineralization at 3 weeks were evaluated using Picro Sirius red and Alizarin red staining. We also assessed the performance of the delivery system after long term storage, by freeze drying rno-miRNA-26a-5p@MSN-CC-PEI with 5% trehalose and keeping them at -30 °C for 3 and 6 months. Osteogenic differentiation, matrix deposition, and mineralization were all significantly increased by rno-miRNA-26a-5p. In addition, this enhancement was not significantly altered by lyophilization and storage. Overall, these findings support the concept of MSN-CC-PEI as a delivery system for gene therapy. The complex of rno-miRNA-26a-5p@MSN-CC-PEI could efficiently transfect rBMSCs and enhance their osteogenic differentiation. In addition, the lyophilized complexes remain functional after 6 months of storage.

摘要

基于 microRNA (miRNA) 的骨修复疗法在调节干细胞增殖和分化方面显示出良好的效果,因此需要一种高效且稳定的 miRNA 递送载体。本研究探索了冻干具有核-锥结构的介孔硅纳米粒子(MSN-CC-PEI)作为一种递送大鼠 miRNA-26a-5p 进入大鼠骨髓间充质细胞(rBMSCs)的系统的稳定性和功能,以促进其成骨分化。我们使用共聚焦激光扫描显微镜和流式细胞术评估了负载标记 miRNA 的纳米粒子的细胞摄取和转染效率,并使用 MTT 法评估了细胞活力。通过定量逆转录-聚合酶链反应(qRT-PCR)分析 1 周和 2 周后成骨基因的表达水平。通过 Picrosirius 红和茜素红染色评估 3 周时细胞外基质的沉积和矿化。我们还通过冷冻干燥 rno-miRNA-26a-5p@MSN-CC-PEI 与 5%海藻糖并将其在-30°C 下保存 3 个月和 6 个月,评估了递送系统的长期储存性能。rno-miRNA-26a-5p 显著促进了成骨分化、基质沉积和矿化。此外,冻干和储存并没有显著改变这种增强作用。总的来说,这些发现支持 MSN-CC-PEI 作为基因治疗递送系统的概念。rno-miRNA-26a-5p@MSN-CC-PEI 复合物可以有效地转染 rBMSCs 并增强其成骨分化。此外,冻干复合物在储存 6 个月后仍保持功能。

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