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在经溶血型神经节苷脂GM1衍生化的硅胶珠上对霍乱毒素进行受体特异性大规模纯化。

Receptor-specific large-scale purification of cholera toxin on silica beads derivatized with lysoGM1 ganglioside.

作者信息

Tayot J L, Holmgren J, Svennerholm L, Lindblad M, Tardy M

出版信息

Eur J Biochem. 1981 Jan;113(2):249-58. doi: 10.1111/j.1432-1033.1981.tb05060.x.

Abstract
  1. A receptor-specific affinity chromatographic method for large-scale purification of cholera toxin is described. The receptor ganglioside for cholera toxin, GM1, is hydrolysed to lysoGM1 which is then covalently coupled, via stabilized Schiff's bases, to porous silica beads (Spherosil) onto which a layer of DEAE-dextran has been adsorbed and cross-linked before coupling. Columns of these Spherosil-DEAE-dextran-lysoGM1 beads, in contrast to particles derivatized with lysoGA1, bound the cholera toxin of Vibrio cholerae culture filtrates, after which the toxin could be eluted with the aid of an acid citrate buffer (pH 2.8). 2. The toxin-binding capacity was directly proportional to the amount of lysoGM1 in the column: 2.3 mg/mu mol lysoGM1. The yield of purified toxin after acid elution and pH neutralization was essentially quantitative (83-107%). 3. The affinity-purified toxin contained less than 5% impurities, but consisted of a mixture of predominantly intact holotoxin and B subunit protomer which could readily be separated by gel filtration on Sephadex G-100. 4. Scaling up of the technique was possible: a 1 kg column enabled us to treat 1000-1 cultures of V. cholerae and thus to isolate 20 g of cholera toxin per cycle.
摘要
  1. 本文描述了一种用于大规模纯化霍乱毒素的受体特异性亲和色谱法。霍乱毒素的受体神经节苷脂GM1被水解为溶血型GM1,然后通过稳定的席夫碱共价偶联到多孔硅胶珠(Spherosil)上,在偶联之前,已在该硅胶珠上吸附并交联了一层DEAE-葡聚糖。与用溶血型GA1衍生化的颗粒相比,这些Spherosil-DEAE-葡聚糖-溶血型GM1珠柱能结合霍乱弧菌培养滤液中的霍乱毒素,之后可用酸性柠檬酸盐缓冲液(pH 2.8)洗脱毒素。2. 毒素结合能力与柱中溶血型GM1的量成正比:每微摩尔溶血型GM1为2.3毫克。经酸洗脱和pH中和后,纯化毒素的产率基本为定量(83 - 107%)。3. 亲和纯化的毒素杂质含量低于5%,但主要由完整的全毒素和B亚基原聚体的混合物组成,可通过在Sephadex G - 100上进行凝胶过滤轻易分离。4. 该技术可以扩大规模:一个1千克的柱使我们能够处理1000 - 1份霍乱弧菌培养物,从而每个循环分离出20克霍乱毒素。

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