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硫酸鱼精蛋白-氧化铁复合物对间充质干细胞的生物学效应及其基于弛豫测量法的细胞MRI标记优化

Biological effects of iron oxide-protamine sulfate complex on mesenchymal stem cells and its relaxometry based labeling optimization for cellular MRI.

作者信息

Mishra Sushanta Kumar, Khushu Subash, Gangenahalli Gurudutta

机构信息

NMR Research Centre, Institute of Nuclear Medicine and Allied Sciences (INMAS), DRDO, Delhi-54, India; Division of Stem Cell and Gene Therapy Research, Institute of Nuclear Medicine and Allied Sciences (INMAS), DRDO, Delhi-54, India.

NMR Research Centre, Institute of Nuclear Medicine and Allied Sciences (INMAS), DRDO, Delhi-54, India.

出版信息

Exp Cell Res. 2017 Feb 1;351(1):59-67. doi: 10.1016/j.yexcr.2016.12.025. Epub 2016 Dec 28.

DOI:10.1016/j.yexcr.2016.12.025
PMID:28040490
Abstract

Mesenchymal stem cells (MSCs) are frequently used as a therapeutic, but reliable imaging technique to longitudinally evaluate the engraftment of transplanted cells is inadequate. For magnetic resonance imaging (MRI), it is essential to understand the technical competence of in vitro stem cells labeling with iron oxide with regard to its relaxation behavior and significance of its biological expressions. The purpose of the study was to optimize the effective labeling of MSCs with high transverse relaxivity iron oxide contrast agent with protamine sulfate and also evaluate the biological effects (phenotype and function) of labeled MSCs. Our results demonstrated that 50:3µg/ml of Fe-Pro complex containing 10% serum at an incubation time of 6h were ideal for effective in vitro labeling. Relaxometry study demonstrated that almost an 8-fold increase in relaxation rate (R) was observed in labeled MSCs by comparing with unlabeled. Marginal alteration in Oct4 and CD146 genes, and phenotypic CD45 expressions were detected after labeling. T2-weighted images and histological analysis confirmed the homing of transplanted cells to the site of injury. The relaxometry based optimized labeling method of MSCs could be extrapolated for cellular MRI and may be useful in stem cell tracking in various pre-clinical and clinical studies.

摘要

间充质干细胞(MSCs)常被用作一种治疗手段,但用于纵向评估移植细胞植入情况的可靠成像技术尚不完善。对于磁共振成像(MRI)而言,了解用氧化铁对体外干细胞进行标记的技术能力,及其弛豫行为和生物学表达的意义至关重要。本研究的目的是用硫酸鱼精蛋白优化高横向弛豫率氧化铁造影剂对MSCs的有效标记,并评估标记后MSCs的生物学效应(表型和功能)。我们的结果表明,在含10%血清的条件下,6小时孵育时间、50:3µg/ml的铁-鱼精蛋白复合物对于有效的体外标记是理想的。弛豫测量研究表明,与未标记的MSCs相比,标记后的MSCs弛豫率(R)几乎增加了8倍。标记后检测到Oct4和CD146基因以及表型CD45表达有轻微改变。T2加权图像和组织学分析证实了移植细胞归巢至损伤部位。基于弛豫测量的MSCs优化标记方法可外推用于细胞MRI,可能对各种临床前和临床研究中的干细胞追踪有用。

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