Kavipurapu P R, Jones M E
J Biol Chem. 1976 Sep 25;251(18):5589-99.
Complex U, which contains the last two enzymes (orotate phosphoribosyltransferase (EC 2.4.2.10) and orotidylate decarboxylase (EC 4.1.23)) of the six enzymes for the de novo biosynthesis of UMP, has been purified 200-fold from mouse Ehrlich ascites cells. The specific activity of the orotate phosphoribosyltransferase and the orotidylate decarboxylase activities of the complex were 0.115 and 0.290 mumol of product/mg of protein/min; the recovery of the activities was high being 20 to 30%. The rate of the two activities remained similar to that of the homogenate. At the sixth step of the fractionation, one can obtain a fraction that has lost phosphoribosyltransferase activity but retains decarboxylase activity. The apparent molecular weights, as determined by density gradient centrifugation, of the native complex and the fraction containing only decarboxylase activity are identical, 55,700 +/- 4,000. Both activities of complex U are labile to very mild treatments such as dilution, dialysis, or storage at 3 degrees. Dithiothreitol and 5-phosphoribosyl-1-pyrophosphate (PP-Rib-P), but not orotic acid or MgCl2, can stabilize either or both of the enzyme activities. The degree of stabilization by three of these chemicals varies with the reagent(s) used, with the nature of the treatment, and with the concentration of Complex U. When PP-Rib-P, Mg2+ and dithiothreitol are present in the diluting buffer the activity losses were slowed and then followed by a partial recovery of the phosphoribosyltransferase activity. Maximum activities of both enzymes are observed by adding undiluted complex to a complete reaction mixture without preincubation. The complex cannot be exposed to pH values of 4 or below, or pH 9 or above. The stability studies have led to the development of conditions that permit one, for the first time, to subject the complex to electrophoresis and to recover a large percentage of both enzyme activities, rather than only decarboxylase activity as has occurred in the past. The electrophoretic studies indicate that PP-Rib-P produces a complex whose conformation and/or net charge differ significantly from that of the complex in the absence of PP-Rib-P. Kinetic characteristics of the transferase are a pH optimum between 6.5 and 7.5, apparent Km values for orotate, PP-Rib-P, and Mg2+ of 1.9 muM, 16 muM, and 2.9 mM, respectively; for the decarboxylase, a sharp pH optimum of 7.0 is observed, and a Km value for orotidine 5'-phosphate of 0.8 muM.
复合物U含有从头合成尿苷一磷酸(UMP)的六种酶中的最后两种酶(乳清酸磷酸核糖转移酶(EC 2.4.2.10)和乳清酸核苷酸脱羧酶(EC 4.1.2.3)),已从小鼠艾氏腹水细胞中纯化了200倍。该复合物中乳清酸磷酸核糖转移酶和乳清酸核苷酸脱羧酶活性的比活性分别为0.115和0.290 μmol产物/ mg蛋白质/分钟;活性回收率很高,为20%至30%。这两种活性的速率与匀浆的速率相似。在分级分离的第六步,可以获得一个失去磷酸核糖转移酶活性但保留脱羧酶活性的级分。通过密度梯度离心测定,天然复合物和仅含有脱羧酶活性的级分的表观分子量相同,为55,700±4,000。复合物U的两种活性对非常温和的处理(如稀释、透析或在3℃下储存)都不稳定。二硫苏糖醇和5-磷酸核糖-1-焦磷酸(PP-Rib-P),而不是乳清酸或MgCl2,可以稳定一种或两种酶活性。这三种化学物质的稳定程度因所用试剂、处理性质和复合物U的浓度而异。当PP-Rib-P、Mg2+和二硫苏糖醇存在于稀释缓冲液中时,活性损失减慢,随后磷酸核糖转移酶活性部分恢复。将未稀释的复合物加入到完整的反应混合物中且不进行预孵育时,可观察到两种酶的最大活性。该复合物不能暴露于pH值为4或更低,或pH值为9或更高的环境中。稳定性研究促成了这样一些条件的建立,使得人们首次能够对该复合物进行电泳,并回收大部分的两种酶活性,而不是像过去那样只回收脱羧酶活性。电泳研究表明,PP-Rib-P产生一种复合物,其构象和/或净电荷与不存在PP-Rib-P时的复合物有显著差异。转移酶的动力学特性为:最适pH在6.5至7.5之间,乳清酸、PP-Rib-P和Mg2+的表观Km值分别为1.9 μM、16 μM和2.9 mM;对于脱羧酶,观察到最适pH为7.0,5'-磷酸乳清苷的Km值为0.8 μM。
