中国组织工程研究与临床康复
中國組織工程研究與臨床康複
중국조직공정연구여림상강복
JOURNAL OF CLINICAL REHABILITATIVE TISSUE ENGINEERING RESEARCH
2008年
41期
8171-8174
,共4页
马忠仁%冯玉萍%李明生%冯若飞%乔自林%李琼毅%侯兰新%李倬
馬忠仁%馮玉萍%李明生%馮若飛%喬自林%李瓊毅%侯蘭新%李倬
마충인%풍옥평%리명생%풍약비%교자림%리경의%후란신%리탁
新生牛皮%胶原蛋白海绵%羔羊肾细胞%生物相容性%生物材料
新生牛皮%膠原蛋白海綿%羔羊腎細胞%生物相容性%生物材料
신생우피%효원단백해면%고양신세포%생물상용성%생물재료
背景:现已证实,人肌腱、牛肌腱、鼠尾、猪皮、新生牛跟腱制备的胶原蛋白海绵有良好的细胞相容性.目的:采用新生牛皮提取胶原蛋白、制备生物医用胶原蛋白海绵,观察其与羔羊肾成纤维细胞的相容性.设计、时间及地点:对比观察实验,于2006-05/2007-02在西北民族大学生命科学与工程学院生物工程与技术国家民委重点实验室完成.材料:出生24 h内宰杀的新生尕里巴牛犊皮,岷县黑裘皮羔羊肾原代成纤维细胞.方法:取新生牛犊皮,经脱毛、胃蛋白酶+冰醋酸联合处理、盐析、透析、冻干后制备胶原蛋白海绵.将海绵与羔羊肾F3代成纤维细胞混悬液共培养,分别设胶原海绵材料组、阴性对照组(生理盐水)、阳性对照组(橡胶塞浸提液).主要观察指标:应用倒置相差显微镜及JVC数码摄像系统观察、拍摄与记录细胞形态、生长情况.培养20,35 d,对共培养物进行AO染色,观察细胞在胶原海绵中的增殖情况.培养65 d后制石蜡切片,行苏术精一伊红染色,观察细胞在胶原海绵中的生长情况.结果:阳性对照组细胞培养24 h细胞圆缩,不贴壁,3 d后伞部死亡.胶原海绵材料组与阴性对照组细胞形态均正常,细胞贴壁生长良好.随着培养时间的延长,海绵孔隙逐渐变小,细胞数量增加,形态变小,海绵外观从柔软、混浊变得挺拔、透明.AO染色显示培养20,35 d的胶原海绵-羔羊肾成纤维细胞共培养物中有大鼍细胞存在,并且在胶原蛋白空隙中有大量细胞成团簇状生长.苏木精-伊红染色显示有大量蓝色细胞核和新生的红色胶原纤维.结论:制备的新生牛皮胶原蛋白海绵对岷县黑裘皮羔羊肾成纤维细胞有良好的相容性.
揹景:現已證實,人肌腱、牛肌腱、鼠尾、豬皮、新生牛跟腱製備的膠原蛋白海綿有良好的細胞相容性.目的:採用新生牛皮提取膠原蛋白、製備生物醫用膠原蛋白海綿,觀察其與羔羊腎成纖維細胞的相容性.設計、時間及地點:對比觀察實驗,于2006-05/2007-02在西北民族大學生命科學與工程學院生物工程與技術國傢民委重點實驗室完成.材料:齣生24 h內宰殺的新生尕裏巴牛犢皮,岷縣黑裘皮羔羊腎原代成纖維細胞.方法:取新生牛犢皮,經脫毛、胃蛋白酶+冰醋痠聯閤處理、鹽析、透析、凍榦後製備膠原蛋白海綿.將海綿與羔羊腎F3代成纖維細胞混懸液共培養,分彆設膠原海綿材料組、陰性對照組(生理鹽水)、暘性對照組(橡膠塞浸提液).主要觀察指標:應用倒置相差顯微鏡及JVC數碼攝像繫統觀察、拍攝與記錄細胞形態、生長情況.培養20,35 d,對共培養物進行AO染色,觀察細胞在膠原海綿中的增殖情況.培養65 d後製石蠟切片,行囌術精一伊紅染色,觀察細胞在膠原海綿中的生長情況.結果:暘性對照組細胞培養24 h細胞圓縮,不貼壁,3 d後傘部死亡.膠原海綿材料組與陰性對照組細胞形態均正常,細胞貼壁生長良好.隨著培養時間的延長,海綿孔隙逐漸變小,細胞數量增加,形態變小,海綿外觀從柔軟、混濁變得挺拔、透明.AO染色顯示培養20,35 d的膠原海綿-羔羊腎成纖維細胞共培養物中有大鼉細胞存在,併且在膠原蛋白空隙中有大量細胞成糰簇狀生長.囌木精-伊紅染色顯示有大量藍色細胞覈和新生的紅色膠原纖維.結論:製備的新生牛皮膠原蛋白海綿對岷縣黑裘皮羔羊腎成纖維細胞有良好的相容性.
배경:현이증실,인기건、우기건、서미、저피、신생우근건제비적효원단백해면유량호적세포상용성.목적:채용신생우피제취효원단백、제비생물의용효원단백해면,관찰기여고양신성섬유세포적상용성.설계、시간급지점:대비관찰실험,우2006-05/2007-02재서북민족대학생명과학여공정학원생물공정여기술국가민위중점실험실완성.재료:출생24 h내재살적신생소리파우독피,민현흑구피고양신원대성섬유세포.방법:취신생우독피,경탈모、위단백매+빙작산연합처리、염석、투석、동간후제비효원단백해면.장해면여고양신F3대성섬유세포혼현액공배양,분별설효원해면재료조、음성대조조(생리염수)、양성대조조(상효새침제액).주요관찰지표:응용도치상차현미경급JVC수마섭상계통관찰、박섭여기록세포형태、생장정황.배양20,35 d,대공배양물진행AO염색,관찰세포재효원해면중적증식정황.배양65 d후제석사절편,행소술정일이홍염색,관찰세포재효원해면중적생장정황.결과:양성대조조세포배양24 h세포원축,불첩벽,3 d후산부사망.효원해면재료조여음성대조조세포형태균정상,세포첩벽생장량호.수착배양시간적연장,해면공극축점변소,세포수량증가,형태변소,해면외관종유연、혼탁변득정발、투명.AO염색현시배양20,35 d적효원해면-고양신성섬유세포공배양물중유대타세포존재,병차재효원단백공극중유대량세포성단족상생장.소목정-이홍염색현시유대량람색세포핵화신생적홍색효원섬유.결론:제비적신생우피효원단백해면대민현흑구피고양신성섬유세포유량호적상용성.
BACKGROUND:It is confirmed that collagen sponge prepared from human tendon,bovine tendon,rat tail,pig skin and newborn bovine tendon have good cytocompatibility.OBJECTIVE:To extract collagen from newborn bovine skin,prepare the collagen sponge for biomedical application,and observe the biocompatibility and cytocompatibility of collagen sponge with lamb fibroblasts.DESIGN,TIME AND SETTING:Controlled study was performed in the Key Laboratory of Bioengineering of State Ethical Committee,Life Science and Engineering College,Northwest University for Nationalities from May 2006 to February 2007.MATERIALS:Newborn Galiba bovine within 24 hours and black fur lamb kidney fibroblasts were used.METHODS:Newborn bovine skin was harvested to prepare the collagen sponge with a series of procedures,including depilation,pepsin+glacial acetic acid,salting-out,dialysis and freeze drying.The obtained collagen sponge was inoculated with fibroblast suspension,which were divided into collagen sponge group,negative control group (saline) and positive control group (rubber bung leaching liquor).MAIN OUTCOME MEASURES:Inverted phase contrast microscope and JVC digital camera system were used to observe the cell morphology and growth.Acridine orange dyeing was used to observe the proliferation of cell in collagen sponge at 20 and 35 days of culture.Hematoxylin-eosin staining was used to observe the growth of cells in collagen sponge at 65 days of culture.RESULTS:The cells of positive control group were not adhesive and all died three days later.Those of collagen sponge group and negative control group were normal and adhesive.With the prolong of culture time,the sponge pore decreased gradually,sponge appearance became eminent and transparent,the cell increased in number but decreased in morphology.Acridine orange dyeing at 20 and 35 days of culture showed that a large amount of cells appeared in the co-culture of collagen sponge with lamb kidney fibroblast,and pack of cell clumps grew.Abundant blue nuclei and newborn red collagen fiber were found by hematoxylin-eosin staining.CONCLUSION:The collagen sponge from newborn bovine skin has a good biocompatibility with lamb kidney fibroblast cell of black fur,and no cytotoxicity appears.
