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作 者:焦丽华[1] 刘文芳[1] 景明 肖玲[1] 赵菁蓉
出 处:《中国输血杂志》1997年第1期8-10,共3页Chinese Journal of Blood Transfusion
摘 要:以低温乙醇法从人血浆中分离的组分I(Cohn’s组分I)为原料,采用有机溶剂/表面活性剂(S/D)法进行病毒灭活处理,并用乙醇沉淀法去除S/D。实验结果证明:用S/D处理的Cohn’s组分I经8%的乙醇2次沉淀后,其Tween80残留量<20μg/ml,TNBP残留量<10μg/ml。用醋酸纤维薄膜电泳法测定,纤维蛋白原纯度为92.75%,可凝固蛋白含量为95.52%,相对回收率为87.46%(n=3);S/D处理前后纤维蛋白原的凝固活力分别为8.06±0.08和8.94±0.70。SDS-PAGE、IE电泳和分子筛凝胶层析(FPLC)显示无变性的纤维蛋白原存在,提示:乙醇低温条件下沉淀去除S/D,不仅能保持纤维蛋白原的生物活性和天然结构基本不变,且可使制品进一步纯化。The inactivation of virus in Cohns fraction Ⅰ separated from human plasma using cold ethanol method was performed by solvent/detergent(S/D) treatment,and the S/D residual in that fraction was removed by ethanol precipitation.The experimental result showed that Tween 80 residual and TNBP residual in Cohns fraction Ⅰ treated by S/D were <20μg/ml and <10μg/ml,respectively after 8% ethanol precipitation in twice.It was confirmed by cellulose acetate electrophoresis that the purity of fibrinogen was 92.75%,the clottable protein concentration was 95.52% and the relative recovery rate was 87.46%( n =3) and that the clottability of fibrinogen was 8.06±0.08 and 8.94±0.70,respectively before and after S/D treatment.The results of SDS PAGE,immunoelectrophoresis and FPLC demonstrated that there was no denatured fibrinogen,indicating that ethanol precipitation at low temperature for removal of S/D residual in Cohns fraction Ⅰ may not only keep the biological activity and structure of fibrinogen unchanged basically,but also make the product further purified
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