Literature DB >> 24741437

The beauty of being (label)-free: sample preparation methods for SWATH-MS and next-generation targeted proteomics.

Jakob Vowinckel1, Floriana Capuano1, Kate Campbell1, Michael J Deery1, Kathryn S Lilley1, Markus Ralser2.   

Abstract

The combination of qualitative analysis with label-free quantification has greatly facilitated the throughput and flexibility of novel proteomic techniques. However, such methods rely heavily on robust and reproducible sample preparation procedures. Here, we benchmark a selection of in gel, on filter, and in solution digestion workflows for their application in label-free proteomics. Each procedure was associated with differing advantages and disadvantages. The in gel methods interrogated were cost effective, but were limited in throughput and digest efficiency. Filter-aided sample preparations facilitated reasonable processing times and yielded a balanced representation of membrane proteins, but led to a high signal variation in quantification experiments. Two in solution digest protocols, however, gave optimal performance for label-free proteomics. A protocol based on the detergent RapiGest led to the highest number of detected proteins at second-best signal stability, while a protocol based on acetonitrile-digestion, RapidACN, scored best in throughput and signal stability but came second in protein identification. In addition, we compared label-free data dependent (DDA) and data independent (SWATH) acquisition on a TripleTOF 5600 instrument. While largely similar in protein detection, SWATH outperformed DDA in quantification, reducing signal variation and markedly increasing the number of precisely quantified peptides.

Entities:  

Year:  2013        PMID: 24741437      PMCID: PMC3983906          DOI: 10.12688/f1000research.2-272.v2

Source DB:  PubMed          Journal:  F1000Res        ISSN: 2046-1402


  47 in total

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Journal:  Mol Cell Proteomics       Date:  2007-05-27       Impact factor: 5.911

5.  Large-scale quantitative assessment of different in-solution protein digestion protocols reveals superior cleavage efficiency of tandem Lys-C/trypsin proteolysis over trypsin digestion.

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  28 in total

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Review 3.  Less is More: Membrane Protein Digestion Beyond Urea-Trypsin Solution for Next-level Proteomics.

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5.  Protocol for Increasing the Sensitivity of MS-Based Protein Detection in Human Chorionic Villi.

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6.  Ultra-fast proteomics with Scanning SWATH.

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Journal:  Nat Biotechnol       Date:  2021-03-25       Impact factor: 54.908

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9.  High-precision iRT prediction in the targeted analysis of data-independent acquisition and its impact on identification and quantitation.

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10.  Regulation of highly homologous major urinary proteins in house mice quantified with label-free proteomic methods.

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