Funakoshi A, Tsubota Y, Fujii K, Ibayashi H, Takagi Y
J Biochem. 1980 Oct;88(4):1113-8. doi: 10.1093/oxfordjournals.jbchem.a133064.
A simple purification method for pancreatic deoxyribonuclease I (DNase I) [EC 3.1.4.3] was developed by utilizing the technique of isoelectric focusing. The active protein was resolved in to at least four forms with different isoelectric points; the major components a, b, and c had isoelectric points at pH 5.2, 4.9, and 4.8, respectively, and that of the minor component d was at 4.7. The four components (a, b, c, and d) exhibited peaks similar to those observed by Salnikow et al. after phosphocellulose chromatography (A, B, C, and D). The four components were all free from RNase and protease activities and were very stable at 0-2 degrees C for at least four weeks. Further, each of the four peaks exhibited a single protein band after polyacrylamide electrophoresis. DNase I-a antibody was prepared; it was very specific for DNase I and precipitated with the other components (b, c, and d). The mode of endonucleolytic action of pancreatic DNase I-a purified from Worthington DP grade DNase I was investigated. The sedimentation patterns in neutral sucrose gradients of digest of circular duplex DNA in an early stage of hydrolysis suggested that DNase I produces single strand scissions in the initial attack in the presence of divalent metal ions.
利用等电聚焦技术开发了一种简单的胰腺脱氧核糖核酸酶I(DNase I)[EC 3.1.4.3]纯化方法。活性蛋白被分离为至少四种具有不同等电点的形式;主要成分a、b和c的等电点分别为pH 5.2、4.9和4.8,次要成分d的等电点为4.7。这四种成分(a、b、c和d)呈现出的峰与Salnikow等人在磷酸纤维素色谱后观察到的峰(A、B、C和D)相似。这四种成分均无核糖核酸酶和蛋白酶活性,在0-2℃下至少四周内非常稳定。此外,这四个峰在聚丙烯酰胺电泳后均呈现单一蛋白条带。制备了DNase I-a抗体;它对DNase I非常特异,并能与其他成分(b、c和d)沉淀。研究了从沃辛顿DP级DNase I中纯化的胰腺DNase I-a的内切核酸酶作用模式。水解早期环状双链DNA消化物在中性蔗糖梯度中的沉降模式表明,在二价金属离子存在下,DNase I在初始攻击中产生单链断裂。
