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Targeted Mass Spectrometry-Based Approach for Protein-Ligand Binding Analyses in Complex Biological Mixtures Using a Phenacyl Bromide Modification Strategy

机译:基于目标质谱的复杂生物混合物中蛋白-配体结合分析的方法,使用苯乙酰溴修饰策略

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The characterization of protein folding stability changes on the proteomic scale is useful for protein-target discovery and for the characterization of biological states. The Stability of Proteins from Rates of Oxidation (SPROX) technique is one of several mass spectrometry-based techniques recently established for the making proteome-wide measurements of protein folding and stability. A critical part of proteome-wide applications of SPROX is the identification and quantitation of methionine-containing peptides. Demonstrated here is a targeted mass spectrometry based proteomics strategy for the detection and quantitation of methionine-containing peptides in SPROX experiments. The strategy involves the use of phenacyl bromide (PAB) for the targeted detection and quantitation of methionine-containing peptides in SPROX using selective reaction monitoring (SRM) on a triple quadrupole mass spectrometer (QQQ-MS). As proof-of-principle, the known binding interaction of Cyclosporine A with cyclophilin A protein in a yeast cell lysate is successfully detected and quantified using a targeted SRM workflow. Advantages of the described workflow over other SPROX protocols include a 20-fold reduction in the amount of total protein needed for analysis and the ability to work with the endogenous proteins in a given sample (e.g., stabile isotope labeling with amino acids in cell culture is not necessary).
机译:蛋白质组学规模上蛋白质折叠稳定性变化的表征对于蛋白质靶标发现和生物学状态表征很有用。蛋白质的氧化速率稳定性(SPROX)技术是最近建立的几种基于质谱的技术之一,可用于蛋白质组范围内蛋白质折叠和稳定性的测量。 SPROX在蛋白质组学中的应用的关键部分是鉴定和定量含甲硫氨酸的肽。这里展示的是基于目标质谱的蛋白质组学策略,用于在SPROX实验中检测和定量含蛋氨酸的肽。该策略涉及在三重四极杆质谱仪(QQQ-MS)上使用选择性反应监测(SRM),将苯甲酰溴(PAB)用于SPROX中目标检测和定量甲硫氨酸的肽。作为原理证明,使用靶向SRM工作流程成功检测并定量了环孢菌素A与亲环素A蛋白在酵母细胞裂解物中的已知结合相互作用。相对于其他SPROX协议,所描述的工作流程的优势包括分析所需的总蛋白质量减少了20倍,并且能够与给定样品中的内源蛋白质一起工作(例如,在细胞培养中用氨基酸标记稳定的同位素)不必要)。

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