两步冷冻法对周围神经雪旺细胞生物活性的影响  被引量：7

作　　者：肖玉周[1] 姚运峰[1] 潘功平[1] 周建生[1] 胡汝麒[1] 

机构地区：[1]蚌埠医学院附属医院骨科,安徽蚌埠233004

出　　处：《中国修复重建外科杂志》2006年第8期801-804,共4页Chinese Journal of Reparative and Reconstructive Surgery

基　　金：安徽省卫生厅科研课题基金资助项目(98-162-02)~~

摘　　要：目的探讨两步冷冻法不同冷冻温度对周围神经雪旺细胞(Schwanncell,SC)生物活性的影响。方法雌性SD大鼠80只,切取双侧坐骨神经2cm,随机分为8组,每组10只20条坐骨神经。1组为新鲜对照组,不作任何处理;另7组为实验组,采用两步冷冻法分别降温至-20、-30、-40、-50、-60、-70和-80℃,保存2h后转入液氮中(-196℃)保存48h,取出后在37℃水浴箱中快速复温1min,消化收集各组SC,经Calceim-AM荧光染色,作流式细胞仪分析,求出各组细胞平均荧光强度,再经共聚焦显微镜直接观察SC荧光强度,进一步判断SC的生物活性。结果经流式细胞仪检测各组SC荧光强度为新鲜对照组242.5220±9.5684,-20℃组168.6770±10.2070,-30℃组214.9920±8.3291,-40℃组235.5260±9.2805,-50℃组222.4340±8.5155,-60℃组217.4090±9.5157,-70℃组132.3760±13.4597,-80℃组108.1320±16.0331;-40℃组荧光强度较其它实验组强,差异有统计学意义(P<0.01)。共聚焦显微镜观察各组SC生物活性,并作荧光强度分析:新鲜对照组143.7000±5.5678,-20℃组119.7000±5.1651,-30℃组121.3000±4.3474,-40℃组139.7000±5.0122,-50℃组121.0000±4.5461,-60℃组118.4000±4.9261,-70℃组81.2000±5.1164,-80℃组79.0000±5.7164;新鲜对照组SC生物活性较各实验组强,-40℃组SC生物活性较其它实验组强,差异均有统计学意义(P<0.01)。结论两步冷冻法均能较好保存SC生物活性,以-40℃组SC生物活性最好。Objective To investigate an effect of different temperature cryopreservation of the two-step freezing method on the Schwann cell biological activity in the peripheral nerve of the rat. Methods Eighty female SD rats were randomly divided into 8 groups of 10 rats each. One was the control group and 7 were the experimental groups. Two 2-cm-long sciatic nerve segments were respectively taken from both legs of each rat. In the control group, the sciatic nerve segments did not undergo the treatment of cryopreservation; however, in the 7 experimental groups, the sciatic nerve segments respectively underwent the different temperature cryopreservation of the two-step freezing method at - 20℃, - 30℃, -40℃, -50℃, - 60℃, - 70℃ and -80℃. The sciatic nerve segments were cryopreserved for 2 hours,and then placed into the liquid nigrtrogen at -196 ℃. After 48 hours of storage,the nerve segments were thawed quickly in the 37℃ water bath box for 1 minute. Then, the sciatic nerve segments each group were harvested. The cells of the sciatic nerve were incubated with Calcein-AM for 15 minutes. The average fluorescence intensity of the cells was measured by the flow cytometry. The nerve fibers were also incubated with Calcein-AM for 15 minutes. The fluorescence intensity of the cells was analyzed by the confocal fluorescence microscope. The Schwann cell biological activity intensity was measured. Results The fluorescence intensity in the -40℃ group was the strongest and the Schwann cell biological activity in this group was the best among all the groups（P〈0. 01）. The fluorescence intensity in the 8 groups measured by the flow cytometry was as follows.. 242. 522 ± 9. 568 4 in the control group, 168. 677 0±10.207 0 in the -20℃ group, 214. 992 0±8.329 1 in the -30 ℃ group, 235. 526 0±9.280 5 in the -40 ℃ group,222.434 0±8.515 5 in the -50 ℃ group,217.409 0±9.515 7 in the -60 ℃ group, 132.376 0± 13. 459 7 in the -70 ℃ group, and 108. 132 0±16. 033 1 in the -80 ℃ group. The fluorescence inten

关 键 词：冷冻保存 雪旺细胞 生物活性 

分 类 号：R318.52[医药卫生—生物医学工程]