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使用焦碳酸二乙酯结合质谱检测进行蛋白质表面图谱分析。

Protein surface mapping using diethylpyrocarbonate with mass spectrometric detection.

作者信息

Mendoza Vanessa Leah, Vachet Richard W

机构信息

Department of Chemistry, University of Massachusetts, Amherst, Massachusetts 01003, USA.

出版信息

Anal Chem. 2008 Apr 15;80(8):2895-904. doi: 10.1021/ac701999b. Epub 2008 Mar 14.

Abstract

The reliability and information content of diethylpyrocarbonate (DEPC) as a covalent probe of protein surface structure has been improved when used appropriately with mass spectrometric detection. Using myoglobin, cytochrome c, and beta-2-microglobulin as model protein systems, we demonstrate for the first time that DEPC can modify Ser and Thr residues in addition to His and Tyr residues. This result expands the capability of DEPC as a structural probe because about 25% of the sequence of the average protein can now be covered using this covalent labeling reagent. In addition, we establish a new approach based on mass spectrometry to ensure the structural integrity of proteins during amino acid-specific covalent labeling reactions. This approach involves monitoring the extent of modification as a function of reagent concentration and allows any small-scale or local perturbations caused by the covalent label to be readily identified and avoided. Results indicate that these dose-response plots are much more reliable and generally applicable probes of possible protein structural changes than fluorescence or circular dichroism spectroscopies. These dose-response plots also provide a means of quantitatively comparing the reactivity of each modified residue. On the basis of comparisons to known X-ray crystal structures, we find that the solvent accessibility of the reactive atom in the side chain and the presence of a nearby charged residue most affect modification rates. Finally, this improved surface mapping method has been used to determine the effect of Cu(II) binding on the structure of beta-2-microglobulin. Results confirm that Cu(II) binds His31, but not any of the other three His residues, and changes the solvent accessibility of residues near His31 and near the N-terminus.

摘要

当与质谱检测适当地结合使用时,焦碳酸二乙酯(DEPC)作为蛋白质表面结构的共价探针,其可靠性和信息含量得到了提高。我们以肌红蛋白、细胞色素c和β-2-微球蛋白作为模型蛋白质系统,首次证明DEPC除了能修饰组氨酸(His)和酪氨酸(Tyr)残基外,还能修饰丝氨酸(Ser)和苏氨酸(Thr)残基。这一结果扩展了DEPC作为结构探针的能力,因为使用这种共价标记试剂现在可以覆盖平均蛋白质序列的约25%。此外,我们建立了一种基于质谱的新方法,以确保在氨基酸特异性共价标记反应过程中蛋白质的结构完整性。该方法涉及监测修饰程度作为试剂浓度的函数,并允许容易地识别和避免由共价标记引起的任何小规模或局部扰动。结果表明,这些剂量反应图比荧光或圆二色光谱法更可靠,并且通常是可能的蛋白质结构变化的更通用的探针。这些剂量反应图还提供了一种定量比较每个修饰残基反应性的方法。基于与已知X射线晶体结构的比较,我们发现侧链中反应性原子的溶剂可及性和附近带电残基的存在对修饰速率影响最大。最后,这种改进的表面测绘方法已被用于确定铜(II)结合对β-2-微球蛋白结构的影响。结果证实铜(II)结合His31,但不结合其他三个组氨酸残基中的任何一个,并改变了His31附近和N端附近残基的溶剂可及性。

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