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High-throughput comparative proteome analysis using a quantitative cysteinyl-peptide enrichment technology

机译:使用定量半胱氨酸肽富集技术进行高通量比较蛋白质组分析

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A new quantitative cysteinyl-peptide enrichment technology (QCET) was developed to achieve higher efficiency, greater dynamic range, and higher throughput in quantitative proteomics that use stable-isotope labeling techniques combined with high-resolution liquid chromatography (LC)-mass spectrometry (MS). This approach involves 180 labeling of tryptic peptides, high-efficiency enrichment of cysteine-containing peptides, and confident protein identification and quantification using the accurate mass and time tag strategy. Proteome profiling of naive and in vitro-differentiated human mammary epithelial cells using QCET resulted in the identification and quantification of 603 proteins in a single LC-Fourier transform ion cyclotron resonance MS analysis. Advantages of this technology include the following: (1) a simple, highly efficient method for enriching cysteinyl-peptides; (2) a high-throughput strategy suitable for extensive proteome analysis; and (3) improved labeling efficiency for better quantitative measurements. This technology enhances both the functional analysis of biological systems and the detection of potential clinical biomarkers.
机译:开发了一种新的定量半胱氨酰肽富集技术(QCET),以实现定量蛋白质组学的更高效率,更大的动态范围和更高的通量,该蛋白质组学使用稳定同位素标记技术与高分辨率液相色谱(LC)-质谱(MS) )。该方法涉及180种胰蛋白酶肽的标记,高效富集含半胱氨酸的肽,以及使用准确的质量和时间标签策略对蛋白质进行可靠的鉴定和定量。使用QCET对天然和体外分化的人类乳腺上皮细胞进行蛋白质组分析,可在单个LC-Fourier变换离子回旋共振MS分析中鉴定和定量603种蛋白质。该技术的优点包括:(1)一种简单,高效的富集半胱氨酰肽的方法; (2)适合大量蛋白质组分析的高通量策略; (3)提高了标记效率,可以进行更好的定量测量。该技术可增强生物系统的功能分析和潜在临床生物标志物的检测。

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