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Methods of Preparing Supplementing Fractions from Fresh Unheated Bovine Sera for Use In Modified Direct Complement-Fixation Tests

机译:从新鲜的未加热的牛血清制备补充级分的方法用于改良的直接补体固定试验

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摘要

Two methods of preparing partially purified, relatively stable supplementing factor from fresh bovine serum are described: gel filtration through Sephadex G-25, and anion exchange chromatography on a diethylaminoethyl (DEAE) cellulose column. In both procedures, an active, reconstituted precipitate prepared by dialysis of fresh unheated normal serum in the cold for 18 hours against phosphate buffer pH 6.2, 0.02 M, serves as the starting material.The Sephadex G-25 column is equilibrated with acetate buffer pH 5.4, 0.2 M. The most actively-supplementing material appears in the eluates in which the pH has risen to 7.5 or higher. For the DEAE cellulose chromatography a gradient system is used: initial phosphate buffer 0.03 M, pH 8.0, limiting buffer Na H2PO4, 0.3 M. The greater part of the supplementing activity is eluated between pH 5.6 and 6.0, although some of the earlier fractions are also reactive. Pooled active eluates stored in the frozen state for nine months or longer maintained their supplementing titre in modified complement-fixation tests of two bacterial antigen-bovine antibody systems.
机译:描述了两种从新鲜牛血清制备部分纯化,相对稳定的补充因子的方法:通过Sephadex G-25进行凝胶过滤,以及在二乙氨基乙基(DEAE)纤维素柱上进行阴离子交换色谱。在这两种方法中,活性的重组沉淀物都是通过将新鲜的未加热的正常血清在pH 6.2、0.02 M的磷酸盐缓冲液中于冷环境下透析18小时而制得的,将其作为起始原料。Sephadex G-25色谱柱用pH值为pH的醋酸盐缓冲液进行平衡。 5.4,0.2M。在pH值升至7.5或更高的洗脱液中,活性最强的物质出现。对于DEAE纤维素色谱法,使用梯度系统:初始磷酸盐缓冲液0.03 M,pH 8.0,极限缓冲液Na H2PO4,0.3M。补充活性的较大部分在pH 5.6和6.0之间洗脱,尽管一些较早的馏分是也反应。在两个细菌抗原-牛抗体系统的改良补体固定测试中,以冷冻状态存储9个月或更长时间的合并的活性洗脱液保持其补充效价。

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