大肠杆菌UDP-N-乙酰胞壁酸:L-丙氨酸连接酶的动力学和晶体学研究。
Kinetic and crystallographic studies of Escherichia coli UDP-N-acetylmuramate:L-alanine ligase.
作者信息
Emanuele J J, Jin H, Jacobson B L, Chang C Y, Einspahr H M, Villafranca J J
机构信息
Division of Macromolecular Structure, Bristol-Myers Squibb Pharmaceutical Research Institute, Princeton, New Jersey 08543-4000, USA.
出版信息
Protein Sci. 1996 Dec;5(12):2566-74. doi: 10.1002/pro.5560051219.
Uridine diphosphate-N-acetylmuramate:L-alanine ligase (EC 6.3.2.8, UNAM:L-Ala ligase or MurC gene product) catalyzes the ATP-dependent ligation of the first amino acid to the sugar moiety of the peptidoglycan precursor. This is an essential step in cell wall biosynthesis for both gram-positive and gram-negative bacteria. Optimal assay conditions for initial velocity studies have been established. Steady-state assays were carried out to determine the effect of various parameters on enzyme activity. Factors studies included: cation specificity, ionic strength, buffer composition and pH. At 37 degrees C and pH 8.0, kcat was equal to 980 +/- 40 min-1, while K(m) values for ATP, UNAM, and L-alanine were, 130 +/- 10, 44 +/- 3, and 48 +/- 6 microM, respectively. Of the metals tested only Mn, Mg, and Co were able to support activity. Sodium chloride, potassium chloride, ammonium chloride, and ammonium sulfate had no effect on activity up to 75 mM levels. The enzyme, in appropriate buffer, was stable enough to be assayed over the pH range of 5.6 to 10.1. pH profiles of Vmax/K(m) for the three substrates and of Vmax were obtained. Crystallization experiments with the enzyme produced two crystal forms. One of these has been characterized by X-ray diffraction as monoclinic, space group C2, with cell dimensions a = 189.6, b = 92.1, c = 75.2 A, beta = 105 degrees, and two 54 kDa molecules per asymmetric unit. It was discovered that the enzyme will hydrolyze ATP in the absence of L-alanine. This L-alanine independent activity is dependent upon the concentrations of both ATP and UNAM; kcat for this activity is less than 4% of the biosynthetic activity measured in the presence of saturating levels of L-alanine. Numerous L-alanine analogs tested were shown to stimulate ATP hydrolysis. A number of these L-alanine analogs produced novel products as accessed by HPLC and mass spectral analysis. All of the L-alanine analogs tested as inhibitors were competitive versus L-alanine.
尿苷二磷酸-N-乙酰胞壁酸:L-丙氨酸连接酶(EC 6.3.2.8,UNAM:L-丙氨酸连接酶或MurC基因产物)催化第一个氨基酸与肽聚糖前体糖部分的ATP依赖性连接。这是革兰氏阳性菌和革兰氏阴性菌细胞壁生物合成中的一个关键步骤。已确定了初始速度研究的最佳测定条件。进行稳态测定以确定各种参数对酶活性的影响。研究的因素包括:阳离子特异性、离子强度、缓冲液组成和pH值。在37℃和pH 8.0条件下,kcat等于980±40 min-1,而ATP、UNAM和L-丙氨酸的K(m)值分别为130±10、44±3和48±6 microM。在所测试的金属中,只有锰、镁和钴能够支持活性。氯化钠、氯化钾、氯化铵和硫酸铵在高达75 mM的浓度下对活性没有影响。该酶在合适的缓冲液中足够稳定,可在pH 5.6至10.1的范围内进行测定。获得了三种底物的Vmax/K(m)和Vmax的pH曲线。用该酶进行的结晶实验产生了两种晶体形式。其中一种通过X射线衍射表征为单斜晶系,空间群C2,晶胞参数a = 189.6、b = 92.1、c = 75.2 Å,β = 105°,每个不对称单元有两个54 kDa分子。发现该酶在没有L-丙氨酸的情况下会水解ATP。这种不依赖L-丙氨酸的活性取决于ATP和UNAM的浓度;该活性的kcat小于在饱和水平的L-丙氨酸存在下测得的生物合成活性的4%。测试的许多L-丙氨酸类似物被证明能刺激ATP水解。通过HPLC和质谱分析发现,其中一些L-丙氨酸类似物产生了新的产物。作为抑制剂测试的所有L-丙氨酸类似物对L-丙氨酸均具有竞争性。
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