diff --git a/parameter_files/Nglyco-HCD_fragger.params b/parameter_files/Nglyco-HCD_fragger.params index 19b660c..fd99275 100644 --- a/parameter_files/Nglyco-HCD_fragger.params +++ b/parameter_files/Nglyco-HCD_fragger.params @@ -1,16 +1,16 @@ -# MSFragger-4.0 +# MSFragger-4.1 database_name = # Path to the protein database file in FASTA format. num_threads = 11 # Number of CPU threads to use. precursor_mass_lower = -20 # Lower bound of the precursor mass window. precursor_mass_upper = 20 # Upper bound of the precursor mass window. precursor_mass_units = 1 # Precursor mass tolerance units (0 for Da, 1 for ppm). -data_type = 0 # Data type (0 for DDA, 1 for DIA, 2 for gas-phase fractionation DIA, 3 for wide-window acquisition DDA). +data_type = 0 # Data type (0 for DDA, 1 for DIA, 2 for gas-phase fractionation DIA, 3 for DDA+). precursor_true_tolerance = 20 # True precursor mass tolerance (window is +/- this value). precursor_true_units = 1 # True precursor mass tolerance units (0 for Da, 1 for ppm). fragment_mass_tolerance = 20 # Fragment mass tolerance (window is +/- this value). fragment_mass_units = 1 # Fragment mass tolerance units (0 for Da, 1 for ppm). -calibrate_mass = 2 # Perform mass calibration (0 for OFF, 1 for ON, 2 for ON and find optimal parameters). +calibrate_mass = 2 # Perform mass calibration (0 for OFF, 1 for ON, 2 for ON and find optimal parameters, 4 for ON and find the optimal fragment mass tolerance). use_all_mods_in_first_search = 0 # Use all variable modifications in first search (0 for No, 1 for Yes). decoy_prefix = rev_ # Prefix of the decoy protein entries. Used for parameter optimization only. @@ -25,7 +25,8 @@ precursor_mass_mode = corrected # One of isolated/selected/corrected. remove_precursor_peak = 1 # Remove precursor peaks from tandem mass spectra. 0 = not remove; 1 = remove the peak with precursor charge; 2 = remove the peaks with all charge states (only for DDA mode). remove_precursor_range = -1.500000,1.500000 # m/z range in removing precursor peaks. Only for DDA mode. Unit: Th. intensity_transform = 0 # Transform peaks intensities with sqrt root. 0 = not transform; 1 = transform using sqrt root. -activation_types = all # Filter to only search scans of provided activation type(s). Allowed: All, HCD, CID, ETD, ECD. +activation_types = all # Filter to only search scans of provided activation type(s), separated by /. Allowed: All, HCD, CID, ETD, ECD. +analyzer_types = all # Filter to only include scans matching the provided analyzer type(s) in search, separated by /. Only support the mzML and raw format. Allowed types: all, FTMS, ITMS. group_variable = 0 # Specify the variable used to decide the PSM group in the group FDR estimation. 0 = no group FDR; 1 = num_enzyme_termini; 2 = PE from protein header. require_precursor = 1 # If required, PSMs with no precursor peaks will be discarded. For DIA data type only. 0 = no, 1 = yes. reuse_dia_fragment_peaks = 0 # Allow the same peak matches to multiple peptides. For DIA data type only. 0 = no, 1 = yes. diff --git a/parameter_files/closed_fragger.params b/parameter_files/closed_fragger.params index 825461c..ad1f154 100644 --- a/parameter_files/closed_fragger.params +++ b/parameter_files/closed_fragger.params @@ -1,16 +1,16 @@ -# MSFragger-4.0 +# MSFragger-4.1 database_name = # Path to the protein database file in FASTA format. num_threads = 11 # Number of CPU threads to use. precursor_mass_lower = -20 # Lower bound of the precursor mass window. precursor_mass_upper = 20 # Upper bound of the precursor mass window. precursor_mass_units = 1 # Precursor mass tolerance units (0 for Da, 1 for ppm). -data_type = 0 # Data type (0 for DDA, 1 for DIA, 2 for gas-phase fractionation DIA, 3 for wide-window acquisition DDA). +data_type = 0 # Data type (0 for DDA, 1 for DIA, 2 for gas-phase fractionation DIA, 3 for DDA+). precursor_true_tolerance = 20 # True precursor mass tolerance (window is +/- this value). precursor_true_units = 1 # True precursor mass tolerance units (0 for Da, 1 for ppm). fragment_mass_tolerance = 20 # Fragment mass tolerance (window is +/- this value). fragment_mass_units = 1 # Fragment mass tolerance units (0 for Da, 1 for ppm). -calibrate_mass = 2 # Perform mass calibration (0 for OFF, 1 for ON, 2 for ON and find optimal parameters). +calibrate_mass = 2 # Perform mass calibration (0 for OFF, 1 for ON, 2 for ON and find optimal parameters, 4 for ON and find the optimal fragment mass tolerance). use_all_mods_in_first_search = 0 # Use all variable modifications in first search (0 for No, 1 for Yes). decoy_prefix = rev_ # Prefix of the decoy protein entries. Used for parameter optimization only. @@ -25,7 +25,8 @@ precursor_mass_mode = selected # One of isolated/selected/corrected. remove_precursor_peak = 1 # Remove precursor peaks from tandem mass spectra. 0 = not remove; 1 = remove the peak with precursor charge; 2 = remove the peaks with all charge states (only for DDA mode). remove_precursor_range = -1.500000,1.500000 # m/z range in removing precursor peaks. Only for DDA mode. Unit: Th. intensity_transform = 0 # Transform peaks intensities with sqrt root. 0 = not transform; 1 = transform using sqrt root. -activation_types = all # Filter to only search scans of provided activation type(s). Allowed: All, HCD, CID, ETD, ECD. +activation_types = all # Filter to only search scans of provided activation type(s), separated by /. Allowed: All, HCD, CID, ETD, ECD. +analyzer_types = all # Filter to only include scans matching the provided analyzer type(s) in search, separated by /. Only support the mzML and raw format. Allowed types: all, FTMS, ITMS. group_variable = 0 # Specify the variable used to decide the PSM group in the group FDR estimation. 0 = no group FDR; 1 = num_enzyme_termini; 2 = PE from protein header. require_precursor = 1 # If required, PSMs with no precursor peaks will be discarded. For DIA data type only. 0 = no, 1 = yes. reuse_dia_fragment_peaks = 0 # Allow the same peak matches to multiple peptides. For DIA data type only. 0 = no, 1 = yes. diff --git a/parameter_files/nonspecific_fragger.params b/parameter_files/nonspecific_fragger.params index 069bc13..ad64aaa 100644 --- a/parameter_files/nonspecific_fragger.params +++ b/parameter_files/nonspecific_fragger.params @@ -1,16 +1,16 @@ -# MSFragger-4.0 +# MSFragger-4.1 database_name = # Path to the protein database file in FASTA format. num_threads = 11 # Number of CPU threads to use. precursor_mass_lower = -20 # Lower bound of the precursor mass window. precursor_mass_upper = 20 # Upper bound of the precursor mass window. precursor_mass_units = 1 # Precursor mass tolerance units (0 for Da, 1 for ppm). -data_type = 0 # Data type (0 for DDA, 1 for DIA, 2 for gas-phase fractionation DIA, 3 for wide-window acquisition DDA). +data_type = 0 # Data type (0 for DDA, 1 for DIA, 2 for gas-phase fractionation DIA, 3 for DDA+). precursor_true_tolerance = 15 # True precursor mass tolerance (window is +/- this value). precursor_true_units = 1 # True precursor mass tolerance units (0 for Da, 1 for ppm). fragment_mass_tolerance = 20 # Fragment mass tolerance (window is +/- this value). fragment_mass_units = 1 # Fragment mass tolerance units (0 for Da, 1 for ppm). -calibrate_mass = 2 # Perform mass calibration (0 for OFF, 1 for ON, 2 for ON and find optimal parameters). +calibrate_mass = 2 # Perform mass calibration (0 for OFF, 1 for ON, 2 for ON and find optimal parameters, 4 for ON and find the optimal fragment mass tolerance). use_all_mods_in_first_search = 0 # Use all variable modifications in first search (0 for No, 1 for Yes). decoy_prefix = rev_ # Prefix of the decoy protein entries. Used for parameter optimization only. @@ -25,7 +25,8 @@ precursor_mass_mode = selected # One of isolated/selected/corrected. remove_precursor_peak = 1 # Remove precursor peaks from tandem mass spectra. 0 = not remove; 1 = remove the peak with precursor charge; 2 = remove the peaks with all charge states (only for DDA mode). remove_precursor_range = -1.500000,1.500000 # m/z range in removing precursor peaks. Only for DDA mode. Unit: Th. intensity_transform = 1 # Transform peaks intensities with sqrt root. 0 = not transform; 1 = transform using sqrt root. -activation_types = all # Filter to only search scans of provided activation type(s). Allowed: All, HCD, CID, ETD, ECD. +activation_types = all # Filter to only search scans of provided activation type(s), separated by /. Allowed: All, HCD, CID, ETD, ECD. +analyzer_types = all # Filter to only include scans matching the provided analyzer type(s) in search, separated by /. Only support the mzML and raw format. Allowed types: all, FTMS, ITMS. group_variable = 0 # Specify the variable used to decide the PSM group in the group FDR estimation. 0 = no group FDR; 1 = num_enzyme_termini; 2 = PE from protein header. require_precursor = 1 # If required, PSMs with no precursor peaks will be discarded. For DIA data type only. 0 = no, 1 = yes. reuse_dia_fragment_peaks = 0 # Allow the same peak matches to multiple peptides. For DIA data type only. 0 = no, 1 = yes. diff --git a/parameter_files/open_fragger.params b/parameter_files/open_fragger.params index 91ebb32..c189e89 100644 --- a/parameter_files/open_fragger.params +++ b/parameter_files/open_fragger.params @@ -1,16 +1,16 @@ -# MSFragger-4.0 +# MSFragger-4.1 database_name = # Path to the protein database file in FASTA format. num_threads = 11 # Number of CPU threads to use. precursor_mass_lower = -150 # Lower bound of the precursor mass window. precursor_mass_upper = 500 # Upper bound of the precursor mass window. precursor_mass_units = 0 # Precursor mass tolerance units (0 for Da, 1 for ppm). -data_type = 0 # Data type (0 for DDA, 1 for DIA, 2 for gas-phase fractionation DIA, 3 for wide-window acquisition DDA). +data_type = 0 # Data type (0 for DDA, 1 for DIA, 2 for gas-phase fractionation DIA, 3 for DDA+). precursor_true_tolerance = 20 # True precursor mass tolerance (window is +/- this value). precursor_true_units = 1 # True precursor mass tolerance units (0 for Da, 1 for ppm). fragment_mass_tolerance = 20 # Fragment mass tolerance (window is +/- this value). fragment_mass_units = 1 # Fragment mass tolerance units (0 for Da, 1 for ppm). -calibrate_mass = 2 # Perform mass calibration (0 for OFF, 1 for ON, 2 for ON and find optimal parameters). +calibrate_mass = 2 # Perform mass calibration (0 for OFF, 1 for ON, 2 for ON and find optimal parameters, 4 for ON and find the optimal fragment mass tolerance). use_all_mods_in_first_search = 0 # Use all variable modifications in first search (0 for No, 1 for Yes). decoy_prefix = rev_ # Prefix of the decoy protein entries. Used for parameter optimization only. @@ -25,7 +25,8 @@ precursor_mass_mode = corrected # One of isolated/selected/corrected. remove_precursor_peak = 1 # Remove precursor peaks from tandem mass spectra. 0 = not remove; 1 = remove the peak with precursor charge; 2 = remove the peaks with all charge states (only for DDA mode). remove_precursor_range = -1.500000,1.500000 # m/z range in removing precursor peaks. Only for DDA mode. Unit: Th. intensity_transform = 0 # Transform peaks intensities with sqrt root. 0 = not transform; 1 = transform using sqrt root. -activation_types = all # Filter to only search scans of provided activation type(s). Allowed: All, HCD, CID, ETD, ECD. +activation_types = all # Filter to only search scans of provided activation type(s), separated by /. Allowed: All, HCD, CID, ETD, ECD. +analyzer_types = all # Filter to only include scans matching the provided analyzer type(s) in search, separated by /. Only support the mzML and raw format. Allowed types: all, FTMS, ITMS. group_variable = 0 # Specify the variable used to decide the PSM group in the group FDR estimation. 0 = no group FDR; 1 = num_enzyme_termini; 2 = PE from protein header. require_precursor = 1 # If required, PSMs with no precursor peaks will be discarded. For DIA data type only. 0 = no, 1 = yes. reuse_dia_fragment_peaks = 0 # Allow the same peak matches to multiple peptides. For DIA data type only. 0 = no, 1 = yes.