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冷冻保护对p21 ras结构和活性的影响:对电子自旋回波包络调制光谱学的启示

The effects of cryoprotection on the structure and activity of p21 ras: implications for electron spin-echo envelope modulation spectroscopy.

作者信息

Halkides C J, Farrar C T, Singel D J

机构信息

Department of Chemistry, University of North Carolina at Wilmington, Wilmington, North Carolina, 28403-3297, USA.

出版信息

J Magn Reson. 1998 Sep;134(1):142-53. doi: 10.1006/jmre.1998.1520.

Abstract

Electron spin-echo envelope modulation (ESEEM) spectroscopy is widely used to investigate the active sites of biological molecules in frozen solutions. Various cryoprotection techniques, particularly the addition of co-solvents, are commonly employed in the preparation of such samples. In conjunction with ESEEM studies of Mn(II) guanosine nucleotide complexes of p21 ras, we have investigated the effects of cryoprotection on the spectroscopy, the structure, and the activity of this protein. Echo decay times, which typically govern ESEEM spectral resolution, were found to vary linearly with the concentration of glycerol or methyl alpha-D-glucopyranoside (MG), with both additives equally effective on a per-mole basis. The effect of glycerol and MG on the ESEEM amplitudes of various protein nucleiwas studied in ras p21.Mn(II). 5'guanylylimido-diphosphate(p21.Mn(II)-GMPPNP) complexes: these additives did not alter the distances of these nuclei from the Mn(II) ion. In particular, in p21 incorporating [2H-3]Thr, the Mn(II)-[2H-3]Thr35 distance was found to be unaffected by the concentration of cryoprotectant or the rate of freezing. The proximity of the cryoprotectants to the Mn(II) ion was probed by 2H ESEEM in solutions made with d5-glycerol and d7-methyl alpha-D-glucopyranoside (d7-MG). In p21.Mn(II)GMPPNP, the large deuterium modulations from the d5-glycerol exhibit saturation behavior with increasing d5-glycerol concentration, implying that glycerol, a widely used cryoprotectant, replaces the aquo ligands of the Mn(II) ion. The interaction between the Mn(II) ion of p21 and MG, however, is less intimate: the deuterium ESEEM amplitudes are much smaller for samples prepared with d7-MG than with d5-glycerol. Several polyhydroxylic compounds were found to have essentially no effect on the ability of the guanosine 5'-triphosphate (GTP) hydrolysis activating protein, GAP334, to catalyze hydrolysis of p21. guanosine 5'-triphosphate. This observation implies that the introduction of cryoprotectant does not significantly perturb the structure of p21 and gives insight into the mechanism of the GTPase reaction.

摘要

电子自旋回波包络调制(ESEEM)光谱法被广泛用于研究冷冻溶液中生物分子的活性位点。在制备此类样品时,通常采用各种冷冻保护技术,特别是添加共溶剂。结合对p21 ras的Mn(II)鸟苷核苷酸复合物的ESEEM研究,我们研究了冷冻保护对此蛋白质的光谱、结构和活性的影响。发现通常决定ESEEM光谱分辨率的回波衰减时间与甘油或α-D-吡喃葡萄糖苷甲基酯(MG)的浓度呈线性变化,两种添加剂在每摩尔基础上同样有效。研究了甘油和MG对ras p21.Mn(II).5'-鸟苷酰亚胺二磷酸(p21.Mn(II)-GMPPNP)复合物中各种蛋白质核的ESEEM振幅的影响:这些添加剂没有改变这些核与Mn(II)离子的距离。特别是,在掺入[2H-3]苏氨酸的p21中,发现Mn(II)-[2H-3]苏氨酸35的距离不受冷冻保护剂浓度或冷冻速率的影响。通过在由d5-甘油和d7-α-D-吡喃葡萄糖苷甲基酯(d7-MG)制成的溶液中进行2H ESEEM探测冷冻保护剂与Mn(II)离子的接近程度。在p21.Mn(II)GMPPNP中,来自d5-甘油的大氘调制随着d5-甘油浓度的增加呈现饱和行为,这意味着甘油,一种广泛使用的冷冻保护剂,取代了Mn(II)离子上的水合配体。然而,p21的Mn(II)离子与MG之间的相互作用不太密切:用d7-MG制备的样品的氘ESEEM振幅比用d5-甘油制备的样品小得多。发现几种多羟基化合物对鸟苷5'-三磷酸(GTP)水解激活蛋白GAP334催化p21.鸟苷5'-三磷酸水解的能力基本上没有影响。这一观察结果表明,冷冻保护剂的引入不会显著扰乱p21的结构,并深入了解了GTPase反应的机制。

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