Shrake A, Fisher M T, McFarland P J, Ginsburg A
Section on Protein Chemistry, National Heart, Lung, and Blood Institute, Bethesda, Maryland 20892.
Biochemistry. 1989 Jul 25;28(15):6281-94. doi: 10.1021/bi00441a021.
Glutamine synthetase (GS), Mr 622,000, from Escherichia coli contains 12 active sites formed at heterologous interfaces between subunits [Almassy, R. J., Janson, C. A., Hamlin, R., Xuong, N.-H., & Eisenberg, D. (1986) Nature (London) 323, 304-309]. Temperature-induced changes in UV spectra from 3 to 68 degrees C were reversible with the Mn2+- or Mg2+-enzyme at pH 7.0 (50 degrees C) in 100 mM KCl. No dissociation or aggregation of dodecamer occurred at high temperatures. The thermal transition involves the exposure of approximately 0.7 of the 2 Trp residues/subunit (by UV difference spectroscopy) and 2 of the 17 Tyr residues/subunit (change in exposure from 4.7 to 6.7 Tyr/subunit by second-derivative spectral analysis). Monitoring changes in Trp and Tyr exposure independently gives data that conform to a two-state model for partial unfolding with Tm values (where delta G unfolding = 0) differing by 2-3 degrees C at each level of [Mn2+] studied and with average delta HvH values of 80 and 94 kcal/mol, respectively. These observations suggest that two regions of the oligomeric structure unfold separately as independent transitions (random model). However, the data can be fit equally with a sequential model in which the Trp transition occurs first upon heating. By fitting with either model, Tm values increase from approximately 47 to approximately 54 degrees C with increasing free [Mn2+] from 3.6 to 49 microM but decrease from approximately 54 to approximately 43 degrees C by further increasing free [Mn2+] from 0.05 to 10 mM; such behavior indicates that the high-temperature form of the enzyme binds Mn2+ more weakly but has more binding sites than the native enzyme. The high-temperature Mn-enzyme form is somewhat less unfolded than is the catalytically inactive apoenzyme, which undergoes no further Trp or Tyr exposure on heating and therefore is assumed to be the high-temperature form of divalent cation-free GS. Adding substrates [ADP, L-Met-(SR)-sulfoximine, Gln, Gln + NH2OH, or Gln + ADP] to Mn.GS increased Tm to varying extents by preferential binding to the folded form. Indeed, the transition-state analogue complex GS.(Mn2.ADP.L-Met-(S)-sulfoximine phosphate)12 was stable in the folded form to at least 72 degrees C. Moreover, an Arrhenius plot for gamma-glutamyl transfer activity was linear from 4 to 72 degrees C with Ea = 18.3 kcal/mol.(ABSTRACT TRUNCATED AT 400 WORDS)
来自大肠杆菌的谷氨酰胺合成酶(GS),分子量为622,000,含有12个活性位点,这些活性位点形成于亚基之间的异源界面处[阿尔马西,R. J.,詹森,C. A.,哈姆林,R.,徐昂,N.-H.,& 艾森伯格,D.(1986年)《自然》(伦敦)323,304 - 309]。在100 mM KCl、pH 7.0(50℃)条件下,温度从3℃升至68℃引起的紫外光谱变化,对于Mn²⁺ - 或Mg²⁺ - 酶是可逆的。在高温下十二聚体未发生解离或聚集。热转变涉及每个亚基中约0.7个色氨酸残基(通过紫外差示光谱法)和17个酪氨酸残基中的2个(通过二阶导数光谱分析,每个亚基的暴露变化从4.7个酪氨酸变为6.7个酪氨酸)的暴露。分别监测色氨酸和酪氨酸暴露的变化,得到的数据符合部分展开的两态模型,在所研究的每个[Mn²⁺]水平下,熔点(Tm)值(其中ΔG展开 = 0)相差2 - 3℃,平均ΔHvH值分别为80和94千卡/摩尔。这些观察结果表明,寡聚结构的两个区域作为独立的转变分别展开(随机模型)。然而,数据也可以用顺序模型同样很好地拟合,其中加热时色氨酸转变首先发生。通过用任何一种模型拟合,随着游离[Mn²⁺]从3.6微摩尔增加到49微摩尔,Tm值从约47℃增加到约54℃,但随着游离[Mn²⁺]从0.05毫摩尔进一步增加到10毫摩尔,Tm值从约54℃降低到约43℃;这种行为表明,酶的高温形式与Mn²⁺结合较弱,但比天然酶具有更多的结合位点。高温Mn - 酶形式的展开程度比催化无活性的脱辅基酶略小,脱辅基酶加热时色氨酸或酪氨酸不再进一步暴露,因此被认为是无二价阳离子的GS的高温形式。向Mn.GS中添加底物[ADP、L - 甲硫氨酸 - (SR) - 亚砜亚胺基、谷氨酰胺、谷氨酰胺 + NH₂OH或谷氨酰胺 + ADP],通过优先结合折叠形式,在不同程度上提高了Tm。实际上,过渡态类似物复合物GS.(Mn₂.ADP.L - 甲硫氨酸 -(S) - 亚砜亚胺基磷酸)₁₂在折叠形式下至少稳定到72℃。此外,γ - 谷氨酰转移活性的阿伦尼乌斯图在4℃至72℃之间呈线性,活化能(Ea) = 18.3千卡/摩尔。(摘要截断于400字)
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