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作 者:贺蕾[1] 杨江华[2] 姚应水[3] 王涛[2] 杨进孙[2] 苏川[1]
机构地区:[1]南京医科大学病原生物学系,江苏南京210029 [2]皖南医学院附属弋矶山医院感染性疾病科,安徽芜湖241001 [3]皖南医学院预防医学教研室,安徽芜湖241002
出 处:《皖南医学院学报》2009年第4期239-241,254,共4页Journal of Wannan Medical College
基 金:国家自然科学基金青年基金项目(30700694);安徽省自然科学基金项目(070413111)
摘 要:目的:建立免疫磁珠法,分离纯化小鼠肝脏Kupffer细胞并进行功能鉴定。方法:采用原位肝脏酶灌注、制备肝非实质细胞悬液、加入PE标记的大鼠抗小鼠F4/80一抗,然后结合山羊抗大鼠IgG Dynabeads免疫磁珠分选Kupffer细胞,流式细胞仪检测其纯度并检测其吞噬功能。结果:在经过胶原酶Ⅳ型消化、免疫磁分选,获得小鼠肝Kupffer细胞产量约为(8.05±0.34)×106/鼠肝,细胞纯度为(96.6±0.7)%,细胞活力大于90%。结论:应用免疫磁珠法能有效地分离纯化小鼠肝脏Kupffer细胞,为体外进一步研究提供了高纯度和活力的Kupffer细胞群。Objective :To establish the way of irnmunomagnetic bead separation for isolating and purifying mouse liver Kupffer cells and exploring their phagocytic function. Methods:The techniques included the processes of liver perfusion in situ, preparation of non-parenchymal cells suspension, isolation using anti-mouse F4/80 antibody and sheep anti-rat IgG Dynabeads. Finally, flow cytometry was used to detect the purity and phagocytic function. Results: By collagenase Ⅳ digestion and immunomagnetic bead separation, Kupffer cells were obtained in the amount of (8.05±0. 34) × 10^6/mouse liver. The purity was (96.6 ± 0.7 ) % and more than 90% of cells were viable. Conclusion: Mouse Kupffer cells can be isolated and purified by immunomagnetic bead separation, which makes it possible to further the study of this cell population in vitro.
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