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体外对人肾近端小管上皮细胞进行超声穿孔以增强细胞内miRNA生物标志物的释放

Sonoporation of Human Renal Proximal Tubular Epithelial Cells In Vitro to Enhance the Liberation of Intracellular miRNA Biomarkers.

作者信息

Teenan Oliver, Sahni Vishal, Henderson Robert B, Conway Bryan R, Moran Carmel M, Hughes Jeremy, Denby Laura

机构信息

Centre for Cardiovascular Science, University of Edinburgh, Queen's Medical Research Institute, Edinburgh, UK.

GlaxoSmithKline, Medical Research Centre, Stevenage, UK.

出版信息

Ultrasound Med Biol. 2022 Jun;48(6):1019-1032. doi: 10.1016/j.ultrasmedbio.2022.01.019. Epub 2022 Mar 17.

DOI:10.1016/j.ultrasmedbio.2022.01.019
PMID:35307235
Abstract

Ultrasound has previously been demonstrated to non-invasively cause tissue disruption. Small animal studies have demonstrated that this effect can be enhanced by contrast microbubbles and has the potential to be clinically beneficial in techniques such as targeted drug delivery or enhancing liquid biopsies when a physical biopsy may be inappropriate. Cavitating microbubbles in close proximity to cells increases membrane permeability, allowing small intracellular molecules to leak into the extracellular space. This study sought to establish whether cavitating microbubbles could liberate cell-specific miRNAs, augmenting biomarker detection for non-invasive liquid biopsies. Insonating human polarized renal proximal tubular epithelial cells (RPTECs), in the presence of SonoVue microbubbles, revealed that cellular health could be maintained while achieving the release of miRNAs, miR-21, miR-30e, miR-192 and miR-194 (respectively, 10.9-fold, 7.17-fold, 5.95-fold and 5.36-fold). To examine the mechanism of release, RPTECs expressing enhanced green fluorescent protein were generated and the protein successfully liberated. Cell polarization, cellular phenotype and cell viability after sonoporation were measured by a number of techniques. Ultrastructural studies using electron microscopy showed gap-junction disruption and pore formation on cellular surfaces. These studies revealed that cell-specific miRNAs can be non-specifically liberated from RPTECs by sonoporation without a significant decrease in cell viability.

摘要

先前已证明超声可无创地引起组织破坏。小动物研究表明,造影剂微泡可增强这种效应,并且在诸如靶向药物递送或在物理活检可能不合适时增强液体活检等技术中具有临床应用潜力。靠近细胞的空化微泡会增加膜通透性,使细胞内小分子泄漏到细胞外空间。本研究旨在确定空化微泡是否能够释放细胞特异性微小RNA(miRNA),从而增强用于非侵入性液体活检的生物标志物检测。在声诺维微泡存在的情况下,对人极化肾近端小管上皮细胞(RPTECs)进行超声照射,结果显示在实现miRNA(miR-21、miR-30e、miR-192和miR-194,分别增加10.9倍、7.17倍、5.95倍和5.36倍)释放的同时能够维持细胞健康。为了研究释放机制,构建了表达增强型绿色荧光蛋白的RPTECs,并成功释放了该蛋白。通过多种技术测量了超声穿孔后的细胞极化、细胞表型和细胞活力。使用电子显微镜进行的超微结构研究显示细胞表面的间隙连接破坏和孔隙形成。这些研究表明,超声穿孔可使RPTECs非特异性地释放细胞特异性miRNA,且细胞活力无显著下降。

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Sonoporation of Human Renal Proximal Tubular Epithelial Cells In Vitro to Enhance the Liberation of Intracellular miRNA Biomarkers.体外对人肾近端小管上皮细胞进行超声穿孔以增强细胞内miRNA生物标志物的释放
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