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MRI Tracking of Iron Oxide Labelled Canine Mesenchymal Stem Cells in Artificial Stifle Defects

机译:人工窒息缺损中氧化铁标记的犬间充质干细胞的 MRI 追踪

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摘要

Objectives The aim of this study was to describe ultrasmall superparamagnetic iron oxides labelling of canine adipose-derived mesenchymal stem cells (AdMSCs) and the detection and semiquantitative evaluation of the labelled cells after implantation in artificial canine stifle defects using magnetic resonance imaging. Methods Magnetic resonance imaging examinations of 10 paired (n = 20) cadaveric stifle joints were evaluated after creation of chondral defects and embedding of ultrasmall superparamagnetic iron oxides labelled canine mesenchymal stem cells. To prove the feasibility of the labelling for in vivo usage, Prussian blue staining, cell vitality tests and intralesional administration of labelled cells were conducted. Magnetic resonance imaging of ex vivo defects filled with different cell concentrations was obtained to depict the cell content semiquantitatively via signal intensity measurements (region of interest). Results Prussian blue staining showed that the labelling was effective. According to the vitality tests, it had no significant short-term influence on cell viability and proliferation rate. For the evaluation of the defect T2* sequences were feasible and stifle defects were visible allowing measurements of the signal intensity in all cases. Increasing the cell concentration within the chondral defects resulted in an inversely proportional, significant reduction of signal intensity according to the region of interest. Clinical Significance Ultrasmall superparamagnetic iron oxides labelling was effective. The detection of the AdMSCs in a complex anatomical structure like the surface of the femoral condyle was possible and the T2* signal intensity of the implant region was significantly correlated with the concentration of the AdMSCs.
机译:目的 描述超小型超顺磁性氧化铁对犬脂肪来源的间充质干细胞(AdMSCs)的标记,以及利用磁共振成像对植入人工犬窒息缺损后标记细胞的检测和半定量评估。方法 对10例成对(n=20)的尸体窒息关节进行磁共振成像检查,评估软骨缺损的产生和超小的超顺磁性氧化铁标记的犬间充质干细胞的包埋。为了证明标记在体内使用的可行性,进行了普鲁士蓝染色、细胞活力测试和标记细胞的病灶内给药。获得填充不同细胞浓度的离体缺陷的磁共振成像,以通过信号强度测量(感兴趣区域)半定量地描述细胞含量。结果 普鲁士蓝染色表明标记有效。根据活力测试,它对细胞活力和增殖率没有显著的短期影响。对于缺陷的评估,T2*序列是可行的,并且窒息缺陷是可见的,可以在所有情况下测量信号强度。增加软骨缺损内的细胞浓度导致信号强度与感兴趣区域成反比,显着降低。临床意义 超小型超顺磁性氧化铁标记有效。在股骨髁表面等复杂的解剖结构中检测AdMSCs是可能的,并且植入区域的T2*信号强度与AdMSCs的浓度显着相关。

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