TY - JOUR T1 - A simple approach for accurate peptide quantification in MS-based proteomics JF - bioRxiv DO - 10.1101/703397 SP - 703397 AU - Teresa Mendes Maia AU - An Staes AU - Kim Plasman AU - Jarne Pauwels AU - Katie Boucher AU - Andrea Argentini AU - Lennart Martens AU - Tony Montoye AU - Kris Gevaert AU - Francis Impens Y1 - 2019/01/01 UR - http://biorxiv.org/content/early/2019/07/16/703397.abstract N2 - Despite its growing popularity and use, bottom-up proteomics remains a complex analytical methodology. Its general workflow consists of three main steps: sample preparation, liquid chromatography coupled to tandem mass spectrometry (LC-MS/MS) and computational data analysis. Quality assessment of the different steps and components of this workflow is instrumental to identify technical flaws and to avoid loss of precious measurement time and sample material. However, assessment of the extent of sample losses along the sample preparation protocol, in particular after proteolytic digestion, is not yet routinely implemented because of the lack of an accurate and straightforward method to quantify peptides. Here, we report on the use of a microfluidic UV/visible spectrophotometer to quantify MS-ready peptides directly in MS loading solvent, consuming only 2 μl of sample. We determined the optimal peptide amount for LC-MS/MS analysis on a Q Exactive HF mass spectrometer using a dilution series of a commercial K562 cell digest. Careful evaluation of selected LC and MS parameters allowed us to define 3 μg as an optimal peptide amount to be injected on this particular LC-MS/MS system. Finally, using tryptic digests from human HEK293T cells, we showed that injecting equal peptide amounts, rather than approximated ones, results into less variable LC-MS/MS and protein quantification data. The obtained quality improvement together with easy implementation of the approach makes it possible to routinely quantify MS-ready peptides as a next step in daily proteomics quality control. ER -