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Multidimensional liquid chromatography coupled to mass spectrometry for the analysis of complex mixtures of proteins.

机译:多维液相色谱与质谱联用,用于分析蛋白质的复杂混合物。

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摘要

Proteomics---which is the analysis of the full complement of proteins produced by an organism---plays a crucial part in a variety of fields of research, including basic biological studies, pharmaceutical development, and clinical diagnostics. Separations are a key element of proteomic analyses. The traditional means of separating protein mixtures is two-dimensional gel electrophoresis, which offers very high resolution. Over the past several decades, alternative methods for protein separations based on liquid chromatography have been developed. These methods have advantages over gel-based analyses, including reduced bias against certain classes of proteins, straightforward automation, and easier coupling to mass spectrometry. However, in order to effectively manage the complexity of a proteome, the separation technique must be able to resolve a very large number of components. Multidimensional liquid chromatography (MDLC) is well-suited to this task. Chapter 1 of this dissertation introduces the theoretical framework behind MDLC. Previous work involving protein separations using comprehensive two-dimensional liquid chromatography (LC x LC), which is a form of MDLC, is also discussed.; Chapters 2 and 3 of the dissertation focus on the development of methods for intact protein separations using liquid chromatography. Several separation modes were evaluated, including size exclusion, ion exchange, and reversed phase. Two-dimensional separations of E. coli proteins were performed which use anion exchange in the first dimension and ultra-high pressure reversed-phase LC in the second dimension. Although high peak capacities were demonstrated, the technique was limited in that proteins could not be identified solely based on the intact protein molecular weight data which was obtained.; The research presented in Chapters 4 and 5 use the same intact-protein LC x LC separations, but also incorporates enzymatic digestion of proteins followed by LC-MS analysis of the resulting peptides. The resulting technique is a hybrid of "top-down" and "bottom-up" proteomics methods. It allows proteins to be identified on the basis of tandem mass spectra of peptides, but retains the information gained from intact protein MS. In Chapter 6, this technique was applied to study differential protein expression in yeast cultures grown under different conditions.
机译:蛋白质组学是对生物体产生的全部蛋白质进行分析的蛋白质组学,它在包括基础生物学研究,药物开发和临床诊断在内的许多研究领域中发挥着至关重要的作用。分离是蛋白质组学分析的关键要素。分离蛋白质混合物的传统方法是二维凝胶电泳,它具有很高的分辨率。在过去的几十年中,已经开发了基于液相色谱的蛋白质分离的替代方法。与基于凝胶的分析相比,这些方法具有优势,包括减少了对某些类型蛋白质的偏倚,简单的自动化方法以及更易于与质谱联用的方法。但是,为了有效地管理蛋白质组的复杂性,分离技术必须能够解析大量的组分。多维液相色谱(MDLC)非常适合此任务。本文的第一章介绍了MDLC背后的理论框架。还讨论了以前的涉及使用二维二维液相色谱(LCLC)的蛋白质进行全面分离的工作。论文的第2章和第3章重点研究了使用液相色谱法分离完整蛋白质的方法。评价了几种分离模式,包括尺寸排阻,离子交换和反相。进行了大肠杆菌蛋白质的二维分离,在第一维中使用阴离子交换,在第二维中使用超高压反相液相色谱。尽管显示出高的峰容量,但是该技术的局限性在于不能仅根据获得的完整蛋白质分子量数据鉴定蛋白质。第4章和第5章中介绍的研究使用相同的完整蛋白质LC x LC分离,但也包括蛋白质的酶消化,然后对所得肽进行LC-MS分析。最终的技术是“自上而下”和“自下而上”蛋白质组学方法的混合。它允许根据肽的串联质谱鉴定蛋白质,但保留了从完整蛋白质MS获得的信息。在第六章中,该技术被用于研究在不同条件下生长的酵母培养物中差异蛋白的表达。

著录项

  • 作者

    Evans, Charles Robert.;

  • 作者单位

    The University of North Carolina at Chapel Hill.$bChemistry.;

  • 授予单位 The University of North Carolina at Chapel Hill.$bChemistry.;
  • 学科 Chemistry Analytical.
  • 学位 Ph.D.
  • 年度 2007
  • 页码 271 p.
  • 总页数 271
  • 原文格式 PDF
  • 正文语种 eng
  • 中图分类 化学;
  • 关键词

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