来自非固氮蓝藻层状席藻的谷氨酰胺合成酶的纯化及性质
Purification and properties of glutamine synthetase from the non-N2-fixing cyanobacterium Phormidium laminosum.
作者信息
Blanco F, Alańa A, Llama M J, Serra J L
机构信息
Departamento de Bioquímica y Biología Molecular, Facultad de Ciencias, Universidad del País, Bilbao, Spain.
出版信息
J Bacteriol. 1989 Feb;171(2):1158-65. doi: 10.1128/jb.171.2.1158-1165.1989.
Soluble glutamine synthetase activity (L-glutamate:ammonia ligase, ADP forming, EC 6.3.1.2) was purified to electrophoretic homogeneity from the filamentous non-N2-fixing cyanobacterium Phormidium laminosum (OH-1-p.Cl1) by using conventional purification procedures in the absence of stabilizing ligands. The pure enzyme showed a specific activity of 152 mumol of gamma-glutamylhydroxamate formed.min-1 (transferase activity), which corresponded to 4.4 mumol of Pi released.min-1 (biosynthetic activity). The relative molecular mass of the native enzyme was 602 kilodaltons and was composed of 12 identically sized subunits of 52 kilodaltons. Biosynthetic activity required the presence of Mg2+ as an essential activator, although Co2+ and Zn2+ were partially effective. The kinetics of activation by Mg2+, Co2+, and Zn2+ were sigmoidal, and concentrations required for half-maximal activity were 18 mM (h = 2.2), 6.3 mM (h = 5.6), and 6.3 mM (h = 2.45), respectively. However, transferase activity required Mn2+ (Ka = 3.5 microM), Cu2+, Co2+, or Mg2+ being less effective. The substrate affinities calculated for L-Glu, ammonium, ATP, L-Gln, and hydroxylamine were 15, 0.4, 1.9 (h = 0.75), 14, and 4.1 mM, respectively. Optimal pH and temperature were 7.2 and 55 degrees C for biosynthetic activity and 7.5 and 45 degrees C for transferase activity. The biosynthetic reaction mechanism proceeded according to an ordered three-reactant system, the binding order being ammonium, L-Glu, and ATP. The presence of Mn2+ or Mg2+ drastically affected the thermostability of transferase and biosynthetic activities. Heat inactivation of biosynthetic activity in the presence of Mn2+ obeyed first-order kinetics, with an Ea of 76.8 kcal (ca. 321 kJ) mol-1. Gly, L-Asp, L-Ala, L-Ser and, with lower efficiency, L-Lys and L-Met, L-Lys, and L-Glu inhibited only transferase activity. No cumulative inhibition was observed when mixtures of amino acids were used. Biosynthetic activity was inhibited by AMP (Ki= 7 mM), ADP (Ki= 2.3 mM), p-hydroxymercuribenzoate (Ki= 25 microM), and L-methionine-D, L-sulfoximine (Ki= 2 microM). The enzyme was not activated in vitro by chemically reduced Anabaena thioredoxin. This is the first report of glutamine synthetase activity purified from a filamentous non-N2-fixing cyanobacterium.
利用常规纯化程序,在不存在稳定配体的情况下,从丝状非固氮蓝藻层状席藻(OH - 1 - p.Cl1)中纯化出了可溶性谷氨酰胺合成酶活性(L - 谷氨酸:氨连接酶,形成ADP,EC 6.3.1.2),使其达到电泳纯。纯酶的比活性为每分钟形成152 μmol的γ - 谷氨酰异羟肟酸(转移酶活性),相当于每分钟释放4.4 μmol的无机磷酸(生物合成活性)。天然酶的相对分子质量为602千道尔顿,由12个大小相同的52千道尔顿的亚基组成。生物合成活性需要Mg²⁺作为必需激活剂,不过Co²⁺和Zn²⁺也有部分激活作用。Mg²⁺、Co²⁺和Zn²⁺的激活动力学呈S形,半最大活性所需浓度分别为18 mM(h = 2.2)、6.3 mM(h = 5.6)和6.3 mM(h = 2.45)。然而,转移酶活性需要Mn²⁺(Ka = 3.5 μM),Cu²⁺、Co²⁺或Mg²⁺的效果较差。计算得出对L - Glu、铵、ATP、L - Gln和羟胺的底物亲和力分别为15、0.4、1.9(h = 0.75)、14和4.1 mM。生物合成活性的最佳pH和温度分别为7.2和55℃,转移酶活性的最佳pH和温度分别为7.5和45℃。生物合成反应机制按有序三反应物系统进行,结合顺序为铵、L - Glu和ATP。Mn²⁺或Mg²⁺的存在极大地影响了转移酶和生物合成活性的热稳定性。在Mn²⁺存在下生物合成活性的热失活遵循一级动力学,活化能为76.8千卡(约321千焦)/摩尔。甘氨酸、L - 天冬氨酸、L - 丙氨酸、L - 丝氨酸,以及效率较低的L - 赖氨酸、L - 蛋氨酸、L - 赖氨酸和L - 谷氨酸仅抑制转移酶活性。当使用氨基酸混合物时未观察到累积抑制。生物合成活性受到AMP(Ki = 7 mM)、ADP(Ki = 2.3 mM)、对羟基汞苯甲酸(Ki = 25 μM)和L - 蛋氨酸 - D,L - 亚砜亚胺(Ki = 2 μM)的抑制。该酶在体外未被化学还原型鱼腥藻硫氧还蛋白激活。这是关于从丝状非固氮蓝藻中纯化谷氨酰胺合成酶活性的首次报道。
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