Selective purification of two distinct protein kinases (C-kinase and casein kinase II) from the membrane fraction of mouse brain by NED-affinity column chromatography.

S Kanno, M Mizugaki, T Maruyama, K Ohtsuki
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Abstract

By means of NED-affinity column chromatography, two distinct protein kinases have been selectively purified from the crude membrane extract of mouse brain. One (designated P-I kinase) was eluted from the column by the buffer containing 5 mM EGTA and the other (designated P-II kinase) was eluted by the buffer containing 0.6 M KCl. The activity of A-kinase was detected in the column passed through fraction. Biochemical characteristics of P-I and P-II kinases corresponded exactly to those of C-kinase and casein kinase II (CK-II), respectively. In addition, immunoprecipitate experiment using anti-CK-II antiserum against the beta-subunit of Drosophila CK-II showed that P-II kinase is identical to CK-II and the 62 kDa cellular polypeptide is associated with the kinase.

用ned亲和柱层析法从小鼠脑膜中选择性纯化两种不同的蛋白激酶(c激酶和酪蛋白激酶II)。
采用ned亲和柱层析法,从小鼠脑粗膜提取物中选择性纯化出两种不同的蛋白激酶。其中一个(指定P-I激酶)用含有5 mM EGTA的缓冲液从柱上洗脱,另一个(指定P-II激酶)用含有0.6 M KCl的缓冲液洗脱。a -激酶的活性通过柱穿过部分检测。P-I和P-II激酶的生化特性与c激酶和酪蛋白激酶II (CK-II)的生化特性完全一致。此外,用抗CK-II抗血清对果蝇CK-II β亚基进行免疫沉淀实验,发现P-II激酶与CK-II相同,62 kDa的细胞多肽与CK-II激酶相关。
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