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作 者:左彦珍[1] 胡亚涛[2] 李玉红[2] 许倩[3]
机构地区:[1]承德医学院药理学教研室,河北承德067000 [2]承德医学院病理学教研室,河北承德067000 [3]承德医学院基础研究所,河北承德067000
出 处:《广东医学》2015年第5期665-669,共5页Guangdong Medical Journal
基 金:2012年河北省科学技术研究与发展计划(第五批)项目(编号:H2012406010);河北省高等学校自然科学研究青年基金项目(编号:2010103)
摘 要:目的对4种建立滋养细胞的方法进行比较,以期寻求一种简便高效的人早孕滋养细胞的体外培养方法,为相关研究提供基础。方法早孕绒毛通过胰酶联合胶原酶消化分离后,分别采用直接接种、差速贴壁联合差速消化法、人外周血淋巴细胞分离液分离纯化法、完整绒毛消化联合简化的percoll密度梯度分离法4种方法纯化培养,倒置显微镜观察细胞形态,应用HE染色、免疫组化和免疫细胞化学法检测细胞纯度。结果直接接种、差速贴壁联合差速消化法、人外周血淋巴细胞分离液分离纯化法得到的细胞细胞角蛋白7(CK-7)表达阳性率不足60%;简化的percoll密度梯度分离法得到的细胞CK-7表达阳性率达90%以上。结论完整绒毛消化联合简化的percoll密度梯度分离纯化可以得到大量较高纯度的滋养细胞以供后期实验。Objective To study the methodology for purification of human first trimester trophoblast cells from placentas with different methods , thus to seek a simple method for purification of human first trimester trophoblast cells in vitro.Methods Target cells isolated from first trimester human placenta with trypsin and collagenase Ⅰ were incubated directly; purified by differential time attachment and digestion ; purified by lymphocyte separation medium ; and dissociated in trypsin /collagenase Ⅰ with purification by simplified percoll gradient centrifugation , respectively.Morphologic observa-tion was applied with inverted phase contrast microscope , with purity was assessed by HE staining and immunocytochemis -try.Results Cytokeratin -7 positive cells were more than 90% only with the last method, while cytokeratin -7 positive cells were less than 60% with the other methods.Conclusion First trimester human trophoblast cells can be obtained through whole first trimester human placenta digestion and followed by simplified percoll gradient centrifugation purification .
关 键 词:早孕滋养细胞 原代培养 胎盘 人外周血淋巴细胞分离液 percoll密度梯度 差速 细胞角蛋白-7 CYTOKERATIN -7
分 类 号:R329.24[医药卫生—人体解剖和组织胚胎学]
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