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镁离子的生物结构化学:酵母苯丙氨酸转运核糖核酸(tRNA(Phe))上弱结合位点的表征。对构象变化和活性的影响。

Biostructural chemistry of magnesium ion: characterization of the weak binding sites on tRNA(Phe)(yeast). Implications for conformational change and activity.

作者信息

Reid S S, Cowan J A

机构信息

Evans Laboratory of Chemistry, Ohio State University, Columbus 43210.

出版信息

Biochemistry. 1990 Jun 26;29(25):6025-32. doi: 10.1021/bi00477a021.

Abstract

The thermodynamics and kinetics of magnesium binding to tRNA(Phe)(yeast) have been studied directly by 25Mg NMR. In 0.17 M Na+(aq), tRNA(Phe) exists in its native conformation and the number of strong binding sites (Ka greater than or equal to 10(4)) was estimated to be 3-4 by titration experiments, in agreement with X-ray structural data for crystalline tRNA(Phe) (Jack et al., 1977). The set of weakly bound ions were in slow exchange and 25Mg NMR resonances were in the near-extreme-narrowing limit. The line shapes of the exchange-broadened magnesium resonance were indistinguishable from Lorentzian form. The number of weak magnesium binding sites was determined to be 50 +/- 8 in the native conformation and a total line-shape analysis of the exchange-broadened 25 Mg2+ NMR resonance gave an association constant Ka of (2.2 +/- 0.2) X 10(2) M-1, a quadrupolar coupling constant (chi B) of 0.84 MHz, an activation free energy (delta G*) of 12.8 +/- 0.2 kcal mol-1, and an off-rate (koff) of (2.5 +/- 0.4) X 10(3) s-1. In the absence of background Na+(aq), up to 12 +/- 2 magnesium ions bind cooperatively, and 73 +/- 10 additional weak binding sites were determined. The binding parameters in the nonnative conformation were Ka = (2.5 +/- 0.2) X 10(2) M-1, chi B = 0.64 MHz, delta G* = 13.1 +/- 0.2 kcal mol-1, and koff = (1.6 +/- 0.4) X 10(3) s-1. In comparison to Mg2+ binding to proteins (chi B typically ca. 1.1-1.6 MHz) the lower chi B values suggest a higher degree of symmetry for the ligand environment of Mg2+ bound to tRNA. A small number of specific weakly bound Mg2+ appear to be important for the change from a nonnative to a native conformation. Implications for interactions with the ribosome are discussed.

摘要

通过25Mg核磁共振直接研究了镁与酵母苯丙氨酸转运核糖核酸(tRNA(Phe))结合的热力学和动力学。在0.17 M Na+(aq)中,tRNA(Phe)以其天然构象存在,通过滴定实验估计强结合位点(Ka大于或等于10(4))的数量为3 - 4,这与结晶tRNA(Phe)的X射线结构数据一致(杰克等人,1977年)。弱结合离子组处于缓慢交换状态,25Mg核磁共振共振处于近极端变窄极限。交换加宽的镁共振的线形与洛伦兹形式无法区分。在天然构象中,弱镁结合位点的数量确定为50±8,对交换加宽的25Mg2+核磁共振共振进行的全线形分析得出缔合常数Ka为(2.2±0.2)×10(2) M-1,四极耦合常数(χB)为0.84 MHz,活化自由能(ΔG*)为12.8±0.2 kcal mol-1,解离速率(koff)为(2.5±0.4)×10(3) s-1。在没有背景Na+(aq)的情况下,多达12±2个镁离子协同结合,并确定了另外73±10个弱结合位点。非天然构象中的结合参数为Ka = (2.5±0.2)×10(2) M-1,χB = 0.64 MHz,ΔG* = 13.1±0.2 kcal mol-1,koff = (1.6±0.4)×10(3) s-1。与镁与蛋白质的结合(χB通常约为1.1 - 1.6 MHz)相比,较低的χB值表明与tRNA结合的Mg2+的配体环境具有更高的对称性。少量特定的弱结合Mg2+似乎对从非天然构象转变为天然构象很重要。讨论了与核糖体相互作用的意义。

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