Literature DB >> 30460388

Benchtop-compatible sample processing workflow for proteome profiling of < 100 mammalian cells.

Kerui Xu1, Yiran Liang2, Paul D Piehowski3, Maowei Dou1, Kaitlynn C Schwarz1, Rui Zhao1, Ryan L Sontag3, Ronald J Moore3, Ying Zhu4, Ryan T Kelly5,6.   

Abstract

Extending proteomics to smaller samples can enable the mapping of protein expression across tissues with high spatial resolution and can reveal sub-group heterogeneity. However, despite the continually improving sensitivity of LC-MS instrumentation, in-depth profiling of samples containing low-nanogram amounts of protein has remained challenging due to analyte losses incurred during preparation and analysis. To address this, we recently developed nanodroplet processing in one pot for trace samples (nanoPOTS), a robotic/microfluidic platform that generates ready-to-analyze peptides from cellular material in ~200 nL droplets with greatly reduced sample losses. In combination with ultrasensitive LC-MS, nanoPOTS has enabled >3000 proteins to be confidently identified from as few as 10 cultured human cells and ~700 proteins from single cells. However, the nanoPOTS platform requires a highly skilled operator and a costly in-house-built robotic nanopipetting instrument. In this work, we sought to evaluate the extent to which the benefits of nanodroplet processing could be preserved when upscaling reagent dispensing volumes by a factor of 10 to those addressable by commercial micropipette. We characterized the resulting platform, termed microdroplet processing in one pot for trace samples (μPOTS), for the analysis of as few as ~25 cultured HeLa cells (4 ng total protein) or 50 μm square mouse liver tissue thin sections and found that ~1800 and ~1200 unique proteins were respectively identified with high reproducibility. The reduced equipment requirements should facilitate broad dissemination of nanoproteomics workflows by obviating the need for a capital-intensive custom liquid handling system.

Entities:  

Keywords:  Microfluidics; Proteomics; Small sample; Thin tissue sections

Mesh:

Year:  2018        PMID: 30460388      PMCID: PMC6527493          DOI: 10.1007/s00216-018-1493-9

Source DB:  PubMed          Journal:  Anal Bioanal Chem        ISSN: 1618-2642            Impact factor:   4.142


  38 in total

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5.  Universal sample preparation method for proteome analysis.

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9.  Comprehensive and quantitative proteome profiling of the mouse liver and plasma.

Authors:  Keane K Y Lai; Deepak Kolippakkam; Laura Beretta
Journal:  Hepatology       Date:  2008-03       Impact factor: 17.425

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3.  Miniaturized Filter-Aided Sample Preparation (MICRO-FASP) Method for High Throughput, Ultrasensitive Proteomics Sample Preparation Reveals Proteome Asymmetry in Xenopus laevis Embryos.

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5.  Simple and Efficient Microsolid-Phase Extraction Tip-Based Sample Preparation Workflow to Enable Sensitive Proteomic Profiling of Limited Samples (200 to 10,000 Cells).

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6.  Fully Automated Sample Processing and Analysis Workflow for Low-Input Proteome Profiling.

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8.  Automated mass spectrometry imaging of over 2000 proteins from tissue sections at 100-μm spatial resolution.

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10.  Facile One-Pot Nanoproteomics for Label-Free Proteome Profiling of 50-1000 Mammalian Cells.

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Journal:  J Proteome Res       Date:  2021-08-05       Impact factor: 4.466

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