Sullivan N M, Pellett S, Wilkins T D
Infect Immun. 1982 Mar;35(3):1032-40. doi: 10.1128/iai.35.3.1032-1040.1982.
Toxin preparations were obtained by growing Clostridium difficile VPI strain 10463 in 2-liter brain heart infusion dialysis flasks at 37 degrees C for 3 days. The initial step of the purification scheme involved ultrafiltration through an XM-100 membrane filter. Two toxic activities, designated toxins A and B, were separated by ion-exchange chromatography on DEAE-NaCl gradients. Toxin A was purified to homogeneity by an acetic acid precipitation at pH 5.5. Other separation techniques, including CM Sepharose CL-6B, (NH4)2SO4 and acetic acid precipitations, and hydrophobic interaction chromatography, were examined in attempts to further purify toxin B. Although these methods failed to increase the specific activity of toxin B, they provided additional evidence that the two toxins are distinct molecules. The toxins are acid and heat labile and are inactivated by trypsin and chymotrypsin, but not by amylase. The molecular weight of toxin A, as estimated by gel filtration and gradient polyacrylamide electrophoresis, ranged from 440,000 to 500,000. The estimated molecular weight of toxin B was 360,000 to 470,000.
毒素制剂通过将艰难梭菌VPI 10463菌株在2升脑心浸液透析瓶中于37℃培养3天获得。纯化方案的第一步包括通过XM - 100膜过滤器进行超滤。两种毒性活性,分别命名为毒素A和毒素B,通过在DEAE - NaCl梯度上的离子交换色谱法分离。毒素A通过在pH 5.5下进行乙酸沉淀纯化至同质。还研究了其他分离技术,包括CM Sepharose CL - 6B、硫酸铵和乙酸沉淀以及疏水相互作用色谱法,试图进一步纯化毒素B。尽管这些方法未能提高毒素B的比活性,但它们提供了额外的证据表明这两种毒素是不同的分子。这些毒素对酸和热不稳定,可被胰蛋白酶和糜蛋白酶灭活,但不被淀粉酶灭活。通过凝胶过滤和梯度聚丙烯酰胺电泳估计,毒素A的分子量在440,000至500,000之间。毒素B的估计分子量为360,000至470,000。
