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Monitoring Dendritic Cell Migration using 19F / 1H Magnetic Resonance Imaging

机译:使用19F / 1H磁共振成像监测树突状细胞迁移

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摘要

Continuous advancements in noninvasive imaging modalities such as magnetic resonance imaging (MRI) have greatly improved our ability to study physiological or pathological processes in living organisms. MRI is also proving to be a valuable tool for capturing transplanted cells in vivo. Initial cell labeling strategies for MRI made use of contrast agents that influence the MR relaxation times (T1, T2, T2*) and lead to an enhancement (T1) or depletion (T2*) of signal where labeled cells are present. T2* enhancement agents such as ultrasmall iron oxide agents (USPIO) have been employed to study cell migration and some have also been approved by the FDA for clinical application. A drawback of T2* agents is the difficulty to distinguish the signal extinction created by the labeled cells from other artifacts such as blood clots, micro bleeds or air bubbles. In this article, we describe an emerging technique for tracking cells in vivo that is based on labeling the cells with fluorine (19F)-rich particles. These particles are prepared by emulsifying perfluorocarbon (PFC) compounds and then used to label cells, which subsequently can be imaged by 19F MRI. Important advantages of PFCs for cell tracking in vivo include (i) the absence of carbon-bound 19F in vivo, which then yields background-free images and complete cell selectivityand(ii) the possibility to quantify the cell signal by 19F MR spectroscopy.
机译:磁共振成像(MRI)等非侵入性成像方式的不断发展极大地提高了我们研究活生物体的生理或病理过程的能力。 MRI也被证明是在体内捕获移植细胞的有价值的工具。 MRI的初始细胞标记策略使用的造影剂会影响MR弛豫时间(T1,T2,T2 *),并在存在标记细胞的情况下导致信号增强(T1)或耗竭(T2 *)。 T2 *增强剂(例如超小氧化铁剂(USPIO))已被用于研究细胞迁移,其中一些也已获得FDA批准用于临床。 T2 *试剂的缺点是难以将标记细胞产生的信号灭绝与其他伪影(例如血栓,微出血或气泡)区分开。在本文中,我们描述了一种新的跟踪体内细胞的技术,该技术基于富含氟( 19 F)颗粒的细胞标记。这些粒子是通过乳化全氟化碳(PFC)化合物制备的,然后用于标记细胞,随后可以通过 19 F MRI进行成像。 PFC在体内进行细胞追踪的重要优势包括:(i)体内不存在与碳结合的 19 F,这会产生无背景图像和完整的细胞选择性,以及(ii)量化PFC的可能性。 19 F MR光谱法检测细胞信号

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