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作 者:周莉婷[1,2] 赵晶晶 吴彦卓 杨仲璠 姚文兵[1] 徐明波
机构地区:[1]中国药科大学生命科学与技术学院,南京210009 [2]北京双鹭药业股份有限公司,北京100041
出 处:《中国新药杂志》2011年第12期1136-1140,1148,共6页Chinese Journal of New Drugs
摘 要:目的:制备分枝杆菌多糖并考察其对小鼠淋巴细胞增殖的影响。方法:用苏通培养基培养分枝杆菌,菌体脱脂后,用5种方法提取,比较多糖得率,并用正交试验优化超声提取工艺,再用稀碱提取残渣,粗多糖经Sevag法除蛋白、DEAE-Sepharose Fast Flow层析柱纯化后得到分枝杆菌多糖;用MTT法检测分枝杆菌多糖对小鼠脾淋巴细胞增殖的影响。结果:超声后热水提取多糖得率最高,超声提取的优化工艺是提取时间40 min,固液比为1∶150,超声功率600 W;单因素试验优化的Sevag法除蛋白条件为体积比1∶5,萃取时间为20 min,萃取6次;提取得到的4种多糖组分在6.25~50 mg.L-1范围内均能显著促进脾淋巴细胞的增殖。结论:用本实验工艺成功制备了分枝杆菌多糖,制备物具有刺激小鼠脾淋巴细胞增殖的作用。Objective: To prepare Mycobacterium polysaccharides(MPS) and determine their effect on lymphocyte proliferation in mice.Methods: Mycobacterium was cultivated in Sauton's medium,and 5 methods were used to extract polysaccharides,and the extraction rates were compared.The ultrasonic extraction was optimized by an orthogonal design.Hot-water extraction residue was extracted in alkaline solution.Crude polysaccharides were purified by deproteinization and DEAE-sepharose Fast Flow chromatography.The effect of polysaccharides on mouse splenic lymphocytes was analyzed by MTT method.Results: The highest polysaccharide yield was obtained by ultrasonic and followed hot-water extraction;the best ultrasonic extraction condition defined by the orthogonal design was extracting 40 min with 150 times solvent and 600 W power.The best deproteiniation condition was extracting 6 times with 1/5 Sevag reagent,20 min for every time.All the obtained 4 kinds of mycobacterium polysaccharides apparently stimulated the proliferation of mouse splenic lymphocytes at concentrations of 6.25~50 mg·L-1.Conclusion: Mycobacterium polysaccharides are successfully prepared by this method and they can stimulate the proliferation of mouse splenic lymphocytes.
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