通过细胞 MRI 对神经母细胞瘤内源性迁移进行连续监测。
Serial monitoring of endogenous neuroblast migration by cellular MRI.
机构信息
Department of Diagnostic Radiology, Yale University School of Medicine, New Haven, CT, USA.
出版信息
Neuroimage. 2011 Aug 1;57(3):817-24. doi: 10.1016/j.neuroimage.2011.04.063. Epub 2011 May 6.
Abstract
Endogenous neural progenitor cell migration in vivo can be monitored using MRI-based cell tracking. The current protocol is that micron sized iron oxide particles (MPIOs) are injected into the lateral ventricle proximal to the neural stem cell niche in the brain. MPIOs are endocytosed and incorporated into the neural progenitor cell population, making them visible by gradient echo MRI. Here this new method is extended to serially quantify cell migration. Initially, in vivo cell labeling methodologies were optimized, as high susceptibility effects from the MPIOs generate substantial signal loss around the injection site, masking early migratory events. Then, using improved labeling conditions, a longitudinal study was conducted over two weeks to quantify the migration of labeled progenitor cells toward the olfactory bulb (OB). By 3 days following injection, we calculated 0.26% of the volume of the OB containing labeled cells. By 8days, this volume nearly doubled to 0.49% and plateaued. These MRI results are in accordance with our data on iron quantification from the OB and with those from purely immunohistochemical studies.
摘要
可以使用基于 MRI 的细胞示踪技术来监测内源性神经祖细胞在体内的迁移。目前的方案是将微米大小的氧化铁颗粒(MPIO)注射到靠近大脑神经干细胞龛的侧脑室中。MPIO 被内吞并整合到神经祖细胞群体中,使它们在梯度回波 MRI 中可见。在这里,该新方法被扩展为连续定量细胞迁移。最初,优化了体内细胞标记方法,因为 MPIO 的高磁化率效应会在注射部位周围产生大量信号损失,从而掩盖早期的迁移事件。然后,使用改进的标记条件,进行了为期两周的纵向研究,以定量标记祖细胞向嗅球(OB)的迁移。在注射后 3 天,我们计算出含有标记细胞的 OB 体积的 0.26%。到第 8 天,这个体积几乎翻了一番,达到 0.49%,并趋于稳定。这些 MRI 结果与我们从 OB 中获得的铁定量数据以及纯免疫组织化学研究的数据一致。
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