multiplexed protein quantification using the isobaric tmt … · 2017. 9. 12. · step 12 –...
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Rosa Viner HUPO 2015
Multiplexed protein quantification using the isobaric TMT method: Improving reproducibility and protein coverage with PD 2.1
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TMT quantification in PD 2.0 and previous
• Using reporter ion intensity values from MS/MS of MS3 spectrum
• Calculate ratios for each PSM based on intensity values • Calculate peptide group and protein ratios using median and
variability of PSM ratios • “Normalization” of protein ratios using median ratio of “Top N”
proteins
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Changes to TMT quantification in PD 2.1
1) S/N thresholds 2) Protein abundances from summed peptide S/N 3) Scaled abundances 4) New UI for ratio calculation 5) Correction factors for TMT 10-plex 6) Option to include razor peptides for protein quantification
Note that almost of all these changes are also applied to isotope-labeled quantification (e.g. SILAC)
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Collaboration with Harvard Medical School for TMT quantification
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Gygi Method for TMT quantification – Step 1
1. Extract S/N values for each reporter ion in the MS/MS data 29May3013_DJB_mouse_tmt8_BR1_unfrac_165min_dda15_1 #8401 RT: 34.83 AV: 1 NL: 1.49E5T: FTMS + c NSI d Full ms2 [email protected] [115.00-1000.00]
126.0 126.5 127.0 127.5 128.0 128.5 129.0 129.5 130.0 130.5 131.0m/z
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Inte
nsity
128.1343N=2338.33
127.1310N=2329.52
131.1381N=2364.68
126.1276N=2320.72
129.1377N=2347.13
130.1412N=2355.93
127.6893N=2334.42
126.5369N=2324.31
m/z Intensity Noise S/N 126.1276 63932.3 2320.72 27.5 127.1248 19174.9 2329.47 8.2 127.131 110637.3 2329.52 47.5
128.1065 8073.1 2338.08 3.5 128.1343 148797.8 2338.33 63.6 129.1314 41537.8 2347.07 17.7 129.1377 49185.8 2347.13 21.0 130.1346 5600.5 2355.87 2.4 130.1412 31675.4 2355.93 13.4 131.1381 100762.8 2364.68 42.6
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Why S/N?
• S/N is proportional to the number of ions in any Orbitrap detector, while intensity measurements will differ across instruments
• The measurement error is related to the number of detected ions
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S/N thresholds for different resolutions
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Gygi Method for TMT quantification – step 2
2. Filter peptides with precursor isolation interference
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Gygi Method for TMT quantification – step 3
3. Sum S/N values for peptides to summed protein S/N
S/N too low
S/N too low
Too much precursor interference
Sum totals
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Gygi Method for TMT quantification – step 4
4. Normalization based on total protein S/N
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Gygi Method for TMT quantification – Step 4
4. Normalization using a single selected protein
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Gygi Method for TMT quantification – Step 5
5. Scale total intensity across channels to 100%
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Summed S/N values displayed in PD 2.1
Summed protein S/N
Peptide group S/N
PSM S/N values
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Pros/Cons of the summed S/N approach
Pros: • Higher abundance peptides are weighted more strongly • Outliers due to low abundance peptides are eliminated • Summed S/N values are easily profiled • Summed S/N values are tolerant of missing values
• Ratios will produce 0 or infinite values for reporter ions with 0 intensity
• Very straightforward Cons: • No measure of variability of individual peptide measurements
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PD 2.1 TMT quantification
• Slight modifications to the Gygi approach • Use “Average S/N” threshold across all channels
• More easily applied to reporter ion quantification methods with different numbers of quantification channels
• User enters a single S/N value • Normalize on total peptide signal rather than protein signal
• Summed peptide group abundances across each sample • More like a TIC normalization
• Scale each channel to an average of 100% rather than a total of 100% • Easier to see which channels are changing • Easier to choose heat map colors
• Ratios are still calculated • User has a choice to inspect the summed S/N values, the scaled abundances,
or the ratios for any given peptide or protein
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Protein and peptide quantifier node in Consensus workflow (new parameters in PD 2.1)
Average S/N per channel
New normalization options
Correction factors
Option to display log2 ratios
Razor peptides
Scaling
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Previous versions of PD – use intensity thresholds
• User can set an intensity threshold for acceptance of a reporter ion in a given PSM for use in peptide group and protein quantification
PD 1.4 PD 2.0
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PD 2.1 S/N calculation
• PD 2.1 asks for an Average S/N value across all measured report ions for a given method
• If the average S/N value is above the user set value, the PSM is included in the peptide and protein quantification:
Average = 8.75 (< 10)
Average = 10.1 (> 10)
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Normalization in PD 2.1
New normalization options: 1) Total Peptide Amount 2) Specific Protein Amount 3) None
If specific protein amount is chosen, the user can choose an indexed FASTA files with the list of proteins to use for normalization.
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Scaling in PD 2.1
• Averaged scaled abundance equals 100 regardless of number of channels
• Scaled abundance values are displayed for peptide groups and proteins
• Samples or channels with higher abundance will be colored red while samples or channels with lower abundance are colored blue:
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Sorting scaled abundance columns in PD 2.1
• Select column name and click up or down triangle to sort:
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New custom ratio calculation in PD 2.1
Sample group selection
Manual ratios
Bulk ratio calculation
Selected ratios for display in report
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Custom ratios in PD 2.1 – example 2
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What about statistics?
• Ratio variabilities no longer available for a single experiment • However, when analyzing replicates, standard errors are
calculated for ratios • How do I know when I have replicate data?
• Value in final result will be the average of the four datasets
• Standard errors will
be calculated for each peptide and protein across replicates
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Results from biological replicate search
• Replicates grouped into ratios + standard errors
Blue bars = average scaled abundance
Error bars = standard error of all replicates
Grey bars = individual dataset abundances
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TMT 10-plex correction factor certificate
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New user interface for adding correction factors
Correction factors are not required for high resolution TMT 6-plex or iodo-TMT
experiments
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Example Dataset – Gygi group MCP paper on diauxic shift in yeast • TMT 10-plex experiment on an Orbitrap Fusion using the
TMT MS3 method • Monitored yeast protein abundances while monitoring
glucose depletion • 10 time points (5, 7, 9, 11, 13, 15, 17, 25, 29, 33 hr), 3
replicates, each with 12 fractions
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Yeast datasets are available for download from PRIDE
Replicate 1
Replicate 2
Replicate 3
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Step 1 – Create new quantitative method using correction factors from TMT CofA
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• Type in percentages exactly as shown in certificate (numbers between 0 and 100):
• Save as new method.
Step 1 (cont.) -
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Step 2 - Create New Study
Choose quan method that was just created
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Step 3 – Set up study factors
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Step 4 – Import data files
• Choose “Add Fractions” to combine all data files from a multidimensional separation into a single logical file:
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Step 5 – Assign Quan Method to each sample
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Step 6 - Assign study factors to reporter ions
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Step 7 – Create New Analysis
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Step 8 – Choose processing workflow
Make sure to select yeast FASTA database and add appropriate PTM’s (e.g. TMT 6 plex, carbamidomethylation)
Reporter ion quantification set to MS3 by default in this method Default processing workflow
for TMT SPS MS3 method
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Step 9 – Choose consensus workflow
Workflows with “Quan” in title include Peptide and Protein Quantifier node
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Step 10 – Modify Peptide and Protein Quantifier
* * *
*
Starred settings are recommended
* *
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Step 11- Drag files into analysis
Select all three files above and then left click, hold, and drag to input files box in analysis
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Step 12 – Grouping and Quantification tab
1) Choose study factor
2) Select 5 hr as denominator(or any other factor of interest)
3) Click “Add Ratios”
Note that all abundance values calculated for each study factor will be the average of the 3 replicates
Click “Run!”
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Search results - >4700 proteins, >88000 unique peptides
Heat shock protein increases in abundance with decreasing glucose
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Search results - >4700 proteins, >88000 unique peptides
DNA-directed RNA polymerase I decreases in abundance with decreasing glucose
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Extra credit – Profiling of scaled intensities in ProteinCenter 1) Export the proteins page to Excel 2) Rename the column with accession numbers as “KEY” 3) Rename the grouped abundance columns to AQR1, AQR2,
AQR3, etc.
4) Save as .csv
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Profiling in ProteinCenter
• Import .csv into ProteinCenter • Click on the dataset and navigate to Profiling tab • Move all “AQR#” values to “Selected” • Choose an appropriate group count (10-15 works) • Click “Profile”
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Profiling results
Click to see list of proteins
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Cluster 1 – Proteins listed in order of decreasing emPAI
Cytoplasmic ribosomal proteins are highly overrepresented in this cluster. On average, ribosomal proteins are decreasing in abundance as the number of cells increase in time.
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Cluster 4 – proteins that increase in abundance after glucose depletion
Proteins from TCA Cycle are overrepresented
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Cluster 5 – proteins that match glucose concentration
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Cluster 11 – pattern not identified in Gygi paper
Many mitochondrial ribosomal proteins
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Conclusions
• With scaled abundances, ratio calculations become less important • Immune to “0” values in the denominator • Can export for profiling
• New user interfaces are much easier to use than in previous releases • Ratio calculation page much improved over 2.0 • Correction factors easy to add
• Best quantitative results from any PD release so far!