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铁氧化物标记间充质干细胞输注创伤性脑损伤小鼠后的归巢与跟踪:一项纵向体内 MRI 研究。

Homing and Tracking of Iron Oxide Labelled Mesenchymal Stem Cells After Infusion in Traumatic Brain Injury Mice: a Longitudinal In Vivo MRI Study.

机构信息

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

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

出版信息

Stem Cell Rev Rep. 2018 Dec;14(6):888-900. doi: 10.1007/s12015-018-9828-7.

Abstract

Stem cells transplantation has emerged as a promising alternative therapeutic due to its potency at injury site. The need to monitor and non-invasively track the infused stem cells is a significant challenge in the development of regenerative medicine. Thus, in vivo tracking to monitor infused stem cells is especially vital. In this manuscript, we have described an effective in vitro labelling method of MSCs, a serial in vivo tracking of implanted stem cells at traumatic brain injury (TBI) site through 7 T magnetic resonance imaging (MRI). Proper homing of infused MSCs was carried out at different time points using histological analysis and Prussian blue staining. Longitudinal in vivo tracking of infused MSCs were performed up to 21 days in different groups through MRI using relaxometry technique. Results demonstrated that MSCs incubated with iron oxide-poly-L-lysine complex (IO-PLL) at a ratio of 50:1.5 μg/ml and a time period of 6 h was optimised to increase labelling efficiency. T2*-weighted images and relaxation study demonstrated a significant signal loss and effective decrease in transverse relaxation time on day-3 at injury site after systemic transplantation, revealed maximum number of stem cells homing to the lesion area. MRI results further correlate with histological and Prussian blue staining in different time periods. Decrease in negative signal and increase in relaxation times were observed after day-14, may indicate damage tissue replacement with healthy tissue. MSCs tracking with synthesized negative contrast agent represent a great advantage during both in vitro and in vivo analysis. The proposed absolute bias correction based relaxometry analysis could be extrapolated for stem cell tracking and therapies in various neurodegenerative diseases.

摘要

干细胞移植因其在损伤部位的强大功效而成为一种很有前途的治疗方法。监测和非侵入性跟踪输注的干细胞是再生医学发展的一个重大挑战。因此,体内跟踪以监测输注的干细胞尤为重要。在本手稿中,我们描述了一种有效的间充质干细胞体外标记方法,通过 7T 磁共振成像(MRI)对创伤性脑损伤(TBI)部位植入的干细胞进行连续的体内跟踪。通过组织学分析和普鲁士蓝染色,在不同时间点进行适当的归巢,以观察注入的间充质干细胞。通过弛豫测量技术,使用 MRI 在不同组中对注入的间充质干细胞进行长达 21 天的纵向体内跟踪。结果表明,间充质干细胞与氧化铁-聚-L-赖氨酸复合物(IO-PLL)以 50:1.5μg/ml 的比例孵育 6 小时,可优化标记效率。T2*-加权图像和弛豫研究表明,在全身移植后第 3 天,损伤部位的信号明显丢失,横向弛豫时间有效降低,表明最大数量的干细胞归巢到病变区域。MRI 结果与不同时间点的组织学和普鲁士蓝染色进一步相关。在第 14 天之后,观察到负信号的减少和弛豫时间的增加,这可能表明损伤组织被健康组织取代。用合成的负对比剂对干细胞进行跟踪具有很大的优势,可用于体外和体内分析。所提出的基于绝对偏差校正的弛豫分析可外推用于各种神经退行性疾病的干细胞跟踪和治疗。

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