Foreword

synapter is free and open-source software. If you use it, please support the project by citing it in publications:

Nicholas James Bond, Pavel Vyacheslavovich Shliaha, Kathryn S. Lilley, and Laurent Gatto. Improving qualitative and quantitative performance for MS\(^E\)-based label free proteomics. J. Proteome Res., 2013, 12 (6), pp 2340–2353

Questions and bugs

For bugs, typos, suggestions or other questions, please file an issue in our tracking system (https://github.com/lgatto/synapter/issues) providing as much information as possible, a reproducible example and the output of sessionInfo().

If you don’t have a GitHub account or wish to reach a broader audience for general questions about proteomics analysis using R, you may want to use the Bioconductor support site: https://support.bioconductor.org/.

1 Introduction

Here we describe the new functionality implemented in synapter 2.0. Namely this vignette covers the utilisation of the new 3D grid search, the fragment matching, intensity modeling and correction of detector saturation.

2 Workflow

The synapter2 workflow is similar to the old one in synapter1. First it is necessary to use PLGS to create the csv (and xml) files. Therefore we refer the reader to the default synapter vignette, available online and with vignette("synapter", package = "synapter").

In contrast to the original workflow the final_fragment.csv file for the identification run and a Spectrum.xml file for the quantification run are needed if the fragment matching should be applied.

Subsequently the original workflow is enhanced by the new 3D grid search and the intensity modeling. Afterwards the fragment matching could be applied. MSnbase (Gatto and Lilley 2012) is used for further analysis. The new synapter adds synapter/PLGS consensus filtering and the detector saturation correction for MSnSets.

New synapter workflow. Dark green boxes show the traditional synapter1 part and the light green boxes highlight the new synapter2 functionality.

New synapter workflow. Dark green boxes show the traditional synapter1 part and the light green boxes highlight the new synapter2 functionality.

2.1 Step-by-step workflow

2.1.1 Create a Synapter object

To demonstrate a typical step-by-step workflow we use example data that are available on http://proteome.sysbiol.cam.ac.uk/lgatto/synapter/data/. There is also an synobj2 object in synapterdata which contains the same data.

The Synapter constructor uses a named list of input files. Please note that we add identfragments (final_fragment.csv) and quantspectra (Spectrum.xml) because we want to apply the fragment matching later.

## Please find the raw data at:
## http://proteome.sysbiol.cam.ac.uk/lgatto/synapter/data/
library("synapter")

inlist <- list(
  identpeptide = "fermentor_03_sample_01_HDMSE_01_IA_final_peptide.csv.gz",
  identfragments = "fermentor_03_sample_01_HDMSE_01_IA_final_fragment.csv.gz",
  quantpeptide = "fermentor_02_sample_01_HDMSE_01_IA_final_peptide.csv.gz",
  quantpep3d = "fermentor_02_sample_01_HDMSE_01_Pep3DAMRT.csv.gz",
  quantspectra = "fermentor_02_sample_01_HDMSE_01_Pep3D_Spectrum.xml.gz",
  fasta = "S.cerevisiae_Uniprot_reference_canonical_18_03_14.fasta")

synobj2 <- Synapter(inlist, master=FALSE)
synobj2
## Object of class "Synapter" 
## Class version 2.0.0 
## Package version 1.99.0 
## Data files:
##  + Identification pep file: fermentor_03_sample_01_HDMSE_01_IA_final_peptide.csv.gz 
##  + Identification Fragment file: fermentor_02_sample_01_HDMSE_01_Pep3D_Spectrum.xml.gz 
##  + Quantitation pep file: fermentor_02_sample_01_HDMSE_01_IA_final_peptide.csv.gz 
##  + Quantitation Pep3DAMRT file: fermentor_02_sample_01_HDMSE_01_Pep3DAMRT.csv.gz 
##  + Quantitation Spectrum file: fermentor_02_sample_01_HDMSE_01_Pep3D_Spectrum.xml.gz 
##  + Fasta file: S.cerevisiae_Uniprot_reference_canonical_18_03_14.fasta 
## Log:
## [1] "Instance created on Tue Apr  4 09:01:34 2017"
## [2] "Read identification peptide data [11471,16]" 
## [ 10 lines ]
## [13] "Read identification fragment data [7078]"
## [14] "Read quantitation spectra [36539]"

2.1.2 Filtering

The first steps in each synapter analysis are filtering by peptide sequence, peptide length, ppm error and false positive rate.

Here we use the default values for each method. But the accompanying plotting methods should be used to find the best threshold:

filterUniqueDbPeptides(synobj2,
                       missedCleavages=0,
                       IisL=TRUE)
filterPeptideLength(synobj2, l=7)
plotFdr(synobj2)