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基于微孔板磁珠的双筒色谱-串联质谱技术高通量蛋白质组学分析对细菌分离株进行分析。

High-throughput proteotyping of bacterial isolates by double barrel chromatography-tandem mass spectrometry based on microplate paramagnetic beads and phylopeptidomics.

机构信息

Laboratoire Innovations technologiques pour la Détection et le Diagnostic (Li2D), Service de Pharmacologie et Immunoanalyse (SPI), CEA, INRA, F-30207 Bagnols sur Cèze, France.

Laboratoire Innovations technologiques pour la Détection et le Diagnostic (Li2D), Service de Pharmacologie et Immunoanalyse (SPI), CEA, INRA, F-30207 Bagnols sur Cèze, France.

出版信息

J Proteomics. 2020 Aug 30;226:103887. doi: 10.1016/j.jprot.2020.103887. Epub 2020 Jun 30.

Abstract

Tandem mass spectrometry-based proteotyping of microorganisms presents several advantages over whole-cell MALDI-TOF mass spectrometry: because a larger number of signals are recorded with better accuracy and precision, the approach allows for the identification of microorganisms at more resolved taxonomic levels, and can easily manage complex samples. Additionally, the use of SP3 paramagnetic beads for cell lysis and protein cleanup simplifies sample preparation for proteotyping. Based on these features, we have developed and tested a 96-well plate platform for high-throughput proteotyping of a large variety of bacteria. We evaluated the performance of the platform in terms of bacterial load and found no cross-contamination between wells. Likewise, phylopeptidomics analysis revealed no alteration in the relative quantifications of microorganisms. Finally, we applied this new format for rapid proteotyping of a large set of dental isolates using double-barrel chromatography coupled to tandem mass spectrometry, which maximizes the number of spectra per unit of time. The procedure allowed us to establish whether these isolates were pure strains or mixtures of strains and to identify the microorganisms at the most resolved taxonomic level. SIGNIFICANCE: The rapid and accurate identification of microorganisms is a clinical priority in medical diagnostics; however, specimens containing mixtures of microorganisms are difficult to analyze and the procedure is time-consuming. Tandem mass spectrometry proteotyping allows the fast identification of complex mixtures of microorganisms, known or unknown, and can also establish the biomass ratio of each component. We describe here a new workflow for preparing microbial samples in a 96-well-plate format for tandem mass spectrometry proteotyping and document its advantages and limitations. We demonstrate that this new format coupled to a highly efficient double-barrel LC-MS/MS system allows proteotyping of 96 isolates in 55 h.

摘要

基于串联质谱的微生物蛋白质组学分析比全细胞 MALDI-TOF 质谱分析具有多项优势:由于记录了更多的信号,具有更好的准确性和精密度,该方法允许在更精细的分类水平上鉴定微生物,并且可以轻松处理复杂的样本。此外,使用 SP3 顺磁珠进行细胞裂解和蛋白质净化可简化蛋白质组学分析的样品制备。基于这些特点,我们开发并测试了一种高通量 96 孔板平台,用于对各种细菌进行高通量蛋白质组学分析。我们从细菌负荷的角度评估了该平台的性能,发现孔之间没有交叉污染。同样, phylopeptidomics 分析显示微生物的相对定量没有变化。最后,我们使用双筒色谱串联质谱法对大量牙科分离物进行了快速蛋白质组学分析,这种新格式最大限度地提高了单位时间内的谱数量。该程序使我们能够确定这些分离物是纯菌株还是菌株混合物,并以最精细的分类水平鉴定微生物。意义:快速准确地鉴定微生物是医学诊断中的临床重点;然而,含有微生物混合物的标本难以分析,且过程耗时。串联质谱蛋白质组学允许快速鉴定复杂的未知或已知微生物混合物,还可以确定每个成分的生物量比例。我们在这里描述了一种新的工作流程,用于以 96 孔板格式制备微生物样品,进行串联质谱蛋白质组学分析,并记录其优点和局限性。我们证明,这种新格式与高效的双筒 LC-MS/MS 系统相结合,可在 55 小时内对 96 个分离物进行蛋白质组学分析。

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