Issinger O G, Kiefer M C, Traut R R
Eur J Biochem. 1975 Nov 1;59(1):137-43. doi: 10.1111/j.1432-1033.1975.tb02434.x.
Two protein kinases differing in substrate specificity were used to phosphorylate the 30-S and the 50-S ribosomal subunits of Escherichia coli. The catalytic subunit from the rabbit skeletal muscle protein kinase phosphorylates proteins S1, S4, S9, S13 and S18 of the 30-S subunit and proteins L2, L4, L5, L16, L18 and L23 of the 50-S subunit with (gamma-32P)ATP as phosphoryl donor. A second protein kinase isolated from rabbit reticulocytes, formerly shown to phosphorylate preferentially acidic proteins and to use GTP as well as ATP, strongly phosphorylated protein S6, an acidic protein of the small ribosomal subunit, and to a lesser extent proteins L7 and L12 or the large subunit. Evidence is presented showing different phosphorylation patterns when either whole subunits or the extracted proteins were used as substrate for the protein kinase. Kinetic studies showed proteins S1 and S4 to become most rapidly phosphorylated. Although most proteins incorporated less than stoichiometric amounts of phosphate, it is shown that with a high excess of ATP L2 bound 1 mol phosphate/mol protein.
两种底物特异性不同的蛋白激酶被用于使大肠杆菌的30-S和50-S核糖体亚基磷酸化。来自兔骨骼肌蛋白激酶的催化亚基以(γ-32P)ATP作为磷酰基供体,使30-S亚基的蛋白S1、S4、S9、S13和S18以及50-S亚基的蛋白L2、L4、L5、L16、L18和L23磷酸化。从兔网织红细胞中分离出的第二种蛋白激酶,以前显示它优先使酸性蛋白磷酸化并且能利用GTP以及ATP,它强烈地使小核糖体亚基的酸性蛋白S6磷酸化,对大亚基的蛋白L7和L12磷酸化程度较低。有证据表明,当使用整个亚基或提取的蛋白作为蛋白激酶的底物时,磷酸化模式不同。动力学研究表明蛋白S1和S4磷酸化最快。尽管大多数蛋白结合的磷酰基量少于化学计量,但结果表明,在ATP大量过量的情况下,L2每摩尔蛋白结合1摩尔磷酰基。