MS core facility at MPI Biochemie - p4eu.org · Nagarjuna Nagaraj MPI of Biochemistry, Core...
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Nagarjuna Nagaraj MPI of Biochemistry, Core Facility Mass Spectrometry – [email protected]
03.12.2015
MS core facility at MPI Biochemie
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People and infrastructure Lissy Vicky Naga Nicole
• TOF(time of flight) – ESI-TOF – ESI-qTOF (high resolution TOF)
• Orbitrap – 2 X QExactiveHF bench-top machines
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MS core facility MPI-Biochemie
Top-down analysis
Bottom-up analysis
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Top-down vs bottom-up MS
Top-down – for low complexity samples like single protein or protein complex information at protein level, however less versatile Bottom-up- for omics based studies easy to handle, better separation strategies and lot of automation possible protein inference problem
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Tandem MS (MS/MS) experiment
• MS experiment – Make ions, detect them
• MSMS experiment
– Make ions, do “something” with the ions, detect the products • Peptide/ protein isolation • Peptide/ protein fragmentation
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Things offered in core facility • TOF platform (top-down ) – turn around time within two days
– Total protein mass ,limited proteolysis – Lipids, small molecules and oligos – Native mass spectrometry of intact protein complex
• qExactive HF (bottom-up) – turn around time within 3 weeks – Proteomics , interaction proteomics, phosphoprotoemics, limited
proteolysis – Occasional specialized applications – Cross-link mass spectrometry
• Protein/protein • Protein/RNA
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Protein analysis using gels
The weight of protein cannot be more precise than few 10s of Kda Gel does not provide high precision purity estimate
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Why MS for protein analysis
• Mass resolution and accuracy • 10,000 western blots; antibodies?? • Relative quantification more precise than dye
based methods • Sensitivity – up to low attomoles of peptides • Analysis of PTMs • Translational regulation vs transcriptional
regulation
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Benefits of mass accuracy
• Modern mass spectrometers generally have accuracy to the level of few parts per million – ppm
• Measurement of mass of 100000 Da protein with a mass precision of 10 ppm = 100000 ± 1 Da
Measured Masss at 1 ppm at 10 ppm at 1 ppm
100 kDa 10 Da 1 Da 0.1 Da 10 kDa 1 Da 0.1 Da 0.01 Da 1 kDa 0.1 Da 0.01 Da 0.001 Da
Deviation
Precise mass measurements help in analyzing modifications on the protein resulting in altered protein mass
100 ppm 10 ppm 1 ppm
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Protein ID + purity check in MS
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Liquid chromatography in LC-MS
• Additional dimension of separation prior to MS analysis
• Reversed phase chromatography is ideal to provide optimal ionization of proteins
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LC-MS output file 01
Infrastructure Service Issues Outlook
Chromatogram
Raw spectra
Deconvoluted spectra
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Top- down native MS
Denatured H.pylori urease (alpha 26.6 kDa, orange) and (beta 61.7 kDa, magenta) monomers of urease
Native H.pylori urease 1063.4 kDa
Nature Methods 5, 927 - 933 (2008)
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Native mass spectrometry
• Analysis of intact protein complexes and subunits
• Preserve the native state = no reversed phase chromatography
• Mainly offline analysis • Success depends on the nature of proteins
analyzed
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Native MS for GroEL
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(Shotgun) proteomics workflow
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(Shotgun) proteomics workflow
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(Shotgun) proteomics workflow
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Modes of quantitation
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SILAC vs label free: What to choose
SILAC • Least experimental error
possible • Can mix samples before
extensive processing • Very precise quantification of
less than 2 fold changes • Perfect for protein turnover
projects
• Increased complexity for MS • Labeling step required
Label free • For any sample no labeling
step • Easy for interaction studies • Does not increase the
complexity for MS analysis • Perfect for proteome
quantification, pull down
• Sample preparation should be reproducible
• Not as good as SILAC for < 2 fold change
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Types of projects - omics 1. Expression proteomics 2. PTM analysis at omics level 3. Interaction proteomics 4. PTM analysis for a targeted protein 5. Others – structure, ID verification, purity
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Expression proteomics
• Whole proteome comparison of different systems – Organism, strains, tissues, cells, organelle – verification of knockdowns and off-target/on-target
effects (abundant proteins)
• Very high success rate and easiest to do
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Routine analysis of yeast proteome
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Singleshot HeLa cell proteome
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PTM analysis at omics level • Quantitative changes in PTMs at a
global/large scale – Phospho on S,T,Y (using titanium beads) – Ubiquitination (glygly-motif antibody) – Smt3 (but not mammalian SUMO) – In principle for any PTM that has reliable enrichment strategy, and
detection strategy in mass spectrometer
• Should usually be coupled with quantitation at protein level
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PTM typical workflow
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Site-specific PTM mapping
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PTM analysis – concerns • Sample related
– Sub-stoichiometric - requires enrichment – At least 100 fold more starting material
• Quantitation – Many steps in enrichment step could affect
quantitative accuracy – Single quantitative evidence (Unlike protein that has
many peptides for quantitation)
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PTM analysis – specific protein • Trickier for lower abundant protein in a given sample • Ideally complete coverage is required for the analysis –
sometimes not achievable in practice
• Protein sequence, protease – critical for coverage, and identification of modification sites
• SILAC – depends on protease choice • In need of new methods
– manipulating ions in mass spectrometer – data acquisition strategies
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Interaction proteomics
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Interaction proteomics • Should be straight forward pull down and
analysis by LC-MSMS analysis
• However relatively low success rate in terms of “next step forward” for users with the help of MS results
• Many handling steps = more variation
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IP samples - variety • Magnetic bead based pull downs
• Coupling of antibodies to beads – Bead incompatibility with digestion buffers
• Ni-NTA pull down, flag IP, biotin/avidin IP
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Typical problems in IP • Running a gel for low amount of
sample dilutes the protein • Identify phospho and all other
PTMs • Lack of reproducible pull downs
– Gel as documentation helps in trouble shooting
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Affinity & SILAC - yes or no
• Sample mixing at early stage is possible • The bait/prey is the actual interest in study
– Ubiquitinome– covalent binding– early mixing possible – maximum enrichment required
– Ubiquitin interactome -non-covalent interaction with Ubiquitin – early mixing not possible – minimal enrichment enough
• SILAC for reliable quantitation – 20% change – SILAC is very precise – 20 fold change - SILAC not required
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Enrichment vs Purification
https://www.youtube.com/watch?v=SxjhYzdBEsw
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Limited proteolysis: remaining structure
N terminus C terminus N terminus C terminus
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Summary
• MS facility – top down (same day or within 2 days) and bottom-up offered (within 3 weeks)
• PTM analysis requires enrichment and higher starting material
• IP samples are trickier to handle • Whole proteome quantification is
straightforward
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Thank you for your attention