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在体长期磁共振成像追踪移植于大鼠缺血肢体的内皮祖细胞及其血管生成潜能。

Long-term in vivo magnetic resonance imaging tracking of endothelial progenitor cells transplanted in rat ischemic limbs and their angiogenic potential.

机构信息

Department of Biomedical Engineering, National Cerebral and Cardiovascular Center Research Institute, Suita, Osaka, Japan.

出版信息

Tissue Eng Part A. 2011 Aug;17(15-16):2079-89. doi: 10.1089/ten.TEA.2010.0482. Epub 2011 May 25.

DOI:10.1089/ten.TEA.2010.0482
PMID:21466415
Abstract

Stem cell therapy has been used to repair ischemic tissues in the limbs, in myocardial infarctions, and in the brain. To understand the mechanisms of healing, a contrast agent capable of inducing sufficient magnetic resonance (MR) contrast would be useful in providing fundamental information about the cell migration and incorporation into the ischemic tissue. A magnetic resonance imaging contrast agent composed of dextran and gadolinium chelate was synthesized. Hydroxyl groups of dextran were activated with 1,1'-carbonylbis-1H-imidazole and reacted with propanediamine to obtain aminated dextran. This modified polymer was then reacted with mono-N-succinimidyl 1,4,7,10-tetraazacyclododecane-1,4,7,10-tetraacetate, then with fluorescein isothiocyanate, and finally reacted with gadolinium chloride solution (Dex-DOTA-Gd3(+)). Endothelial progenitor cells (EPCs) were selected as a stem cell model for magnetic resonance imaging tracking. Cells were isolated from the bone marrow harvested from the femurs and tibias of rats. Dex-DOTA-Gd3(+) was then introduced into the EPCs by electroporation. The intracellular stability and cytotoxicity of Dex-DOTA-Gd3(+) were evaluated in vitro. Dex-DOTA-Gd3(+)-labeled EPCs were transplanted into a rat model of ischemic limb, and MR images were acquired. Dex-DOTA-Gd3(+) was found to efficiently label EPCs over a long duration without significant cytotoxicity. This provides an MR signal sufficient for tracking the EPCs intramuscularly injected into the limb.

摘要

干细胞疗法已被用于修复四肢的缺血组织、心肌梗死和大脑中的缺血组织。为了了解愈合机制,一种能够诱导足够磁共振(MR)对比的造影剂将有助于提供关于细胞迁移和整合到缺血组织的基本信息。合成了一种由葡聚糖和钆螯合物组成的磁共振成像造影剂。葡聚糖的羟基用 1,1'-羰基二咪唑活化,并与丙二胺反应,得到氨基化葡聚糖。然后将改性聚合物与单-N-琥珀酰亚胺 1,4,7,10-四氮杂环十二烷-1,4,7,10-四乙酸反应,然后与异硫氰酸荧光素反应,最后与氯化钆溶液(Dex-DOTA-Gd3(+))反应。内皮祖细胞(EPCs)被选为磁共振成像跟踪的干细胞模型。从大鼠股骨和胫骨采集的骨髓中分离出细胞。然后通过电穿孔将 Dex-DOTA-Gd3(+)引入 EPCs。在体外评估了 Dex-DOTA-Gd3(+)的细胞内稳定性和细胞毒性。将 Dex-DOTA-Gd3(+)-标记的 EPCs 移植到缺血肢体的大鼠模型中,并获取 MR 图像。结果发现,Dex-DOTA-Gd3(+)能够高效标记 EPCs 长达很长一段时间,且没有明显的细胞毒性。这为跟踪肌肉内注射到肢体的 EPCs 提供了足够的 MR 信号。

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