使用镧系元素发光光谱研究翻译后腺苷酸化对大肠杆菌谷氨酰胺合成酶金属结合位点的影响。
Investigating the effects of posttranslational adenylylation on the metal binding sites of Escherichia coli glutamine synthetase using lanthanide luminescence spectroscopy.
作者信息
Reynaldo L P, Villafranca J J, Horrocks W D
机构信息
Pennsylvania State University, Department of Chemistry, University Park 16802, USA.
出版信息
Protein Sci. 1996 Dec;5(12):2532-44. doi: 10.1002/pro.5560051216.
Lanthanide luminescence was used to examine the effects of posttranslational adenylylation on the metal binding sites of Escherichia coli glutamine synthetase (GS). These studies revealed the presence of two lanthanide ion binding sites of GS of either adenylylation extrema. Individual emission decay lifetimes were obtained in both H2O and D2O solvent systems, allowing for the determination of the number of water molecules coordinated to each bound Eu3+. The results indicate that there are 4.3 +/- 0.5 and 4.6 +/- 0.5 water molecules coordinated to Eu3+ bound to the n1 site of unadenylylated enzyme, GS0, and fully adenylylated enzyme, GS12, respectively, and that there are 2.6 +/- 0.5 water molecules coordinated to Eu3+ at site n2 for both GS0 and GS12. Energy transfer measurements between the lanthanide donor-acceptor pair Eu3+ and Nd3+, obtained an intermetal distance measurement of 12.1 +/- 1.5 A. Distances between a Tb3+ ion at site n2 and tryptophan residues were also performed with the use of single-tryptophan mutant forms of E. coli GS. The dissociation constant for lanthanide ion binding to site n1 was observed to decrease from Kd = 0.35 +/- 0.09 microM for GS0 to Kd = 0.06 +/- 0.02 microM for GS12. The dissociation constant for lanthanide ion binding to site n2 remained unchanged as a function of adenylylation state; Kd = 3.8 +/- 0.9 microM and Kd = 2.6 +/- 0.7 microM for GS0 and GS12, respectively. Competition experiments indicate that Mn2+ affinity at site n1 decreases as a function of increasing adenylylation state, from Kd = 0.05 +/- 0.02 microM for GS0 to Kd = 0.35 +/- 0.09 microM for GS12. Mn2+ affinity at site n2 remains unchanged (Kd = 5.3 +/- 1.3 microM for GS0 and Kd = 4.0 +/- 1.0 microM for GS12). The observed divalent metal ion affinities, which are affected by the adenylylation state, agrees with other steady-state substrate experiments (Abell LM, Villafranca JJ, 1991, Biochemistry 30:1413-1418), supporting the hypothesis that adenylylation regulates GS by altering substrate and metal ion affinities.
利用镧系元素发光来研究翻译后腺苷酸化对大肠杆菌谷氨酰胺合成酶(GS)金属结合位点的影响。这些研究揭示了处于腺苷酸化极端状态的GS存在两个镧系离子结合位点。在H₂O和D₂O溶剂体系中均获得了各个发射衰减寿命,从而能够确定与每个结合的Eu³⁺配位的水分子数量。结果表明,与未腺苷酸化的酶GS0的n1位点结合的Eu³⁺配位的水分子分别为4.3±0.5个,与完全腺苷酸化的酶GS12的n1位点结合的Eu³⁺配位的水分子为4.6±0.5个,并且对于GS0和GS12,在n2位点与Eu³⁺配位的水分子均为2.6±0.5个。镧系供体-受体对Eu³⁺和Nd³⁺之间的能量转移测量得到金属间距离为12.1±1.5 Å。还利用大肠杆菌GS的单色氨酸突变体形式进行了n2位点的Tb³⁺离子与色氨酸残基之间的距离测量。观察到镧系离子与n1位点结合的解离常数从GS0的Kd = 0.35±0.09 μM降至GS12的Kd = 0.06±0.02 μM。镧系离子与n2位点结合的解离常数不随腺苷酸化状态而变化;GS0和GS12的Kd分别为3.8±0.9 μM和Kd = 2.6±0.7 μM。竞争实验表明,n1位点的Mn²⁺亲和力随着腺苷酸化状态的增加而降低,从GS0的Kd = 0.05±0.02 μM降至GS12的Kd = 0.35±0.09 μM。n2位点的Mn²⁺亲和力保持不变(GS0的Kd = 5.3±1.3 μM,GS12的Kd = 4.0±1.0 μM)。观察到的受腺苷酸化状态影响的二价金属离子亲和力与其他稳态底物实验结果一致(Abell LM,Villafranca JJ,1991,Biochemistry 30:1413 - 1418),支持了腺苷酸化通过改变底物和金属离子亲和力来调节GS的假说。
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