胎鼠神经干细胞超顺磁性氧化铁颗粒标记移植后MRI研究  被引量：2

作　　者：薛静[1] 高培毅[1] 李晋[2] 孙崇然[2] 黄华[2] 安沂华[2] 

机构地区：[1]首都医科大学附属北京天坛医院神经影像中心,北京100050 [2]北京市神经外科研究所神经干细胞室,100050

出　　处：《放射学实践》2006年第2期110-113,共4页Radiologic Practice

基　　金：北京市自然科学基金资助项目(7062013);北京市自然科学基金资助项目(7032009);国家自然科学基金资助项目(30370427)

摘　　要：目的:探讨超顺磁性氧化铁颗粒(SPIO)标记神经干细胞的方法,以及标记细胞正常大鼠脑内移植后MR成像的方法学研究。方法:多聚左旋赖氨酸介导的SPIO标记胎鼠神经干细胞,进行台盼兰染色和普鲁士兰染色分别检测标记细胞的存活率和标记率。选取SD大鼠15只,简单随机法分为3组:第1组于大鼠右侧尾状核移植未标记的NSCs,第2组于大鼠右侧尾状核移植标记的NSCs,第3组右侧尾状核移植游离的SPIO颗粒,移植后第1、4、8周进行MRI。8周后处死大鼠,行组织切片普鲁士兰染色。结果:体外标记的神经干细胞普鲁士兰染色发现铁颗粒聚集于细胞浆内,标记率为100%;标记细胞与未标记细胞的台盼兰染色结果无显著差异。移植后MRI,第1组注射点未见低信号影;第2组注射点T2WI及GRE序列均可见类圆形低信号影;第3组大鼠注射后1周注射点可见低信号影,4周后低信号影变淡且边缘变模糊,8周后低信号影T2WI已不明显。与T2WI序列比较,GRE序列显示标记细胞更清晰,但显示范围较扩散。脑组织切片的普鲁士兰染色显示,第1组大鼠脑组织切片未见异常蓝染细胞,第2组注射点可见蓝染细胞,第3组注射点可见稍许散在蓝色颗粒状物质。结论:多聚左旋赖氨酸介导下SPIO可用于标记神经干细胞,标记细胞移植后MRI可以无创性观察移植神经干细胞的位置及分布情况。Objective：To explore the methods of labeling neural stem cells （NSCs） with superparamagnetic iron oxide （SPIO） particles, and to monitor the labeled cells after transplantation into the rat with MR scanning. Methods：Neural stem cells,labeled with SPIO mediated by poly-L-lysine,underwent Trypan blue staining to observe cell viability of the labeled cells and Prussian blue staining to evaluate the labeling rate. Fifteen rats were divided into three groups in random： the unlabeled and labeled NSCs, and free SPIO particles were transplanted into the right caudate nucleus respectively. MR scanning was performed to monitor the transplanted cells after 1,4,8 weeks. After MR imaging, the rats were killed and un derwent Prussian blue staining of the histological section. Results.. Prussian blue staining of the cells showed numerous blue stained particles in the cytoplasm of the labeled cells. There was no significant difference between the results of Trypan blue staining in labeled and unlabeled cells. The MR imaging showed significant hypointensity in the transplanted areas after 1, 4,8 weeks in the group of transplantation of the labeled cells. No any abnormal low signal intensity was observed in the rats of transplantation of the unlabeled cells. For free SPIO particle group,hypointensity also could be observed after 4 weeks, but the T2 relaxation time was prolonged, and after 8 weeks, the low signal intensity became blurred. The Prussian blue staining of the perfused tissue showed numerous blue stained cells in the right caudate nucleus, which was the same area with the MR imaging. Conclusion： Poly L-lysine mediated SPIO can be used to label NSCs,and MR scanning is useful in tracking the location and distribution of the labeled neural stem cells after transplantation.

关 键 词：超顺磁性氧化铁 磁共振成像 干细胞 

分 类 号：R310[医药卫生—基础医学]