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FindMod is a tool that can predict potential protein post-translational modifications (PTM) and find potential single amino acid substitutions in peptides

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Definition is a tool that can predict potential protein post-translational modifications (PTM) and find potential single amino acid substitutions in peptides.
de novo discovery of protein post-translational modifications (PTM). It examines peptide mass fingerprinting results of known proteins for the presence of 22 types of PTMs of discrete mass: acetylation, amidation, biotin, C-mannosylation, deamidation, N-acyl diglyceride cysteine (tripalmitate), FAD, farnesylation, formylation, geranyl-geranyl, gamma-carboxyglutamic acid, O-GlcNAc, hydroxylation, lipoyl, methylation, myristoylation, palmitoylation, phosphorylation, pyridoxal phosphate, pyrrolidone carboxylic acid, sulfatation.
The experimentally measured peptide masses are compared with the theoretical peptides calculated from a specified Swiss-Prot/TrEMBL entry or from a user-entered sequence, and mass differences are used to better characterise the protein of interest. If a mass difference corresponds to a known PTM not already annotated in UniProtKB/Swiss-Prot, "intelligent" rules are applied that examine the sequence of the peptide of interest and make predictions as to what amino acid in the peptide is likely to carry the modification.
Protein Sequence to be characterize Peptide Massses
1.Protein Sequence to be characterized You should specify the sequence of the protein you would like to characterize and for which you have determined a set of peptide masses.
• If the Protein sequence is known • If the Protein Sequence is not known
Enter the UniProtKB/Swiss-Prot ID code (e.g. TKN1_HUMAN) Or the protein accession number (e.g. P20366).
you can enter the sequence of your protein of interest, in single letter amino acid code, in either upper or lower case. The user is required to specify the biological source of the query protein
Note The characters O and U are not considered and will give an error message. However, the residue J will be treated as either Ile or Leu, which have the same average and monoisotopic masses. The characters B, X, or are accepted, but no masses are computed for peptides containing one or more of these characters.
2.Peptide Masses Enter the experimentally measured peptide masses generated from the unknown protein in the « Enter a list of peptide masses...»text field, and separate them by spaces, tabs or new lines.
NOTE You can copy a list of peptides from Excel or other applications and paste them directly into the text field. Avoid using peptide masses known to be from autodigestion of an enzyme (e.g. trypsin!), or other artefactual peaks (e.g. matrix peaks). Upload a .pkm, .dta or text file
Uploading Peptide Masses Upload the file directly from your computer (1) Click on the on the «Browse...»button (2) Select the file containing the relevant peptide mass data. (3) Click on the «Open» button The peptide masses will then be extracted automatically from this file
Expasy Tools Go to Expasy site: http://www.expasy.ch/tools/#proteome Select FinMod Tool
FindMod View
Findmod View
Types of Supported Formats (1) .pkm format (2) Sequest format (3) User Created Files
.pkm Format .pkm format, produced by the Voyager software of Perseptive Biosystems or the GRAMS software: OP=0Center X Peak Y Left X Right X Time X Mass Difference NameSTD.Misc Height Left Y Right Y %Height,Width,%Area,%Quan,H/A833.319 2189 833.260 833.378 0.016 0 0C0.? 0 762 762854.843 5078 854.769 854.917 0.001 0 0C0.? 0 3453 3453863.419 5108 863.064 863.775 0.001 0 0C0.? 0 3567 3567872.402 12519 872.347 872.456 0.002 0 0C0.? 0 11417 11417874.395 6730 874.331 874.460 0.002 0 0C0.? 0 3559 3559887.786 5903 887.540 888.031 0.003 0 0C0.? 0 4131 4131898.475 3329 898.416 898.534 0.006 0 0C0.? 0 1377 1377904.366 7432 904.199 904.533 0.001 0 0C0.? 0 5596 5596955.300 2598 955.229 955.371 0.011 0 0C0.? 0 1089 1089973.845 16689 973.749 973.941 0.001 0 0
1.001833.319 2189844.333 0.0854.843 5078863.419 5108872.402 12519874.395 6730887.786 5903898.475 3329899.555 0.0904.366 7432955.300 2598973.845 16689 The first line is considered as a comment and is ignored.
User Created Files Any user-created files can be uploaded if they correspond to the following rules: The first line does not contain any mass value (if it does, this mass value is ignored). Lines containing masses must start with the mass, and the first 20 characters must not contain any uppercase letters.
NOTE The upload option only works if you see a 'browse' button next to the text entry field. This should be the case for most recent web browser versions, e.g. Netscape 3.0 or higher, MS Internet Explorer 4.0 or higher.
The user can specify whether the program should detect only potential PTMs, only single amino acid substitutions or both. The user can choose whether all peptide masses or only those that have not been attributed a theoretical peptide in this process should be examined for potential PTMs resp. single amino acid substitutions.
ION MODE (MASSES AS [M] OR [M+H]+) You can enter the masses of your peptides as [M] or as [M+H]+, however you must select the appropriate button. If you select the [M+H]+ button, all peptide masses calculated from the database will have one proton (mass of 1 unit) added before matching with user-specified peptides.
MASS TOLERANCE Peptide masses can be specified in ppm (parts per million) or in Dalton.
DIGESTION AGENT (ENZYME) Specify the enzyme or chemical reagent that you used to generate your peptides (see the corresponding section in the PeptideMass instructions for the available enzymes and their cleavage rules).
MISSED CLEAVAGES In order to take into account partial cleavages, you can specify a maximum number (0, 1, 2 or 3) of missed cleavage sites to be allowed. If the maximum number of missed cleavages entered is 1, all concatenations of two adjoining peptides are also added to the list of theoretical peptides under consideration.
SORTING OF PEPTIDES IN THE RESULT TABLES Here you can choose if you would like the peptides to be sorted by their mass (from smallest to largest) or by their chronological order in the protein.
SEND THE RESULT BY E-MAIL  Tick the « Send the result by e-mail » box. In the « Your e-mail:» text field you should enter the correct e-mail address (e.g. name@unknown.ch) to where the results should be sent.  The email option is recommended, in particular for queries with a high number of peptide masses. This avoids timeouts («document contains no data») which can occur for the on-line option: the browser interrupts the connection with the program if the search is not terminated after a certain time (usually about 3 minutes).  Note that email results are sent in form of a html file, in exactly the same format as on-line, and that there is no loss of functionality compared to on-line display.
RESET AND PERFORM BUTTONS Once you have filled in the form according to your needs, press the button "Start FindMod". If you have made a mistake and would like all fields to be reset to their default values, press the Reset button.
OUTPUT FORMAT o Header o up to three tables.
HEADER The header contains information about the submitted protein:  A link to the UniProtKB/Swiss-Prot or UniProtKB/TrEMBL entry  The description line (if the protein is in UniProtKB), pI and molecular weight.
Then the input parameters are listed, followed by an active link to PeptideMass. This allows the user to perform a theoretical cleavage of the protein of interest.
TABLES The tables report the peptides whose experimental masses match unmodified or modified theoretical digest products of the protein of interest:  The first table reports matches to theoretical digest products as unmodified, modified with the annotations in UniProtKB/Swiss-Prot and chemically modified as specified in the input form.  The second table reports those user masses which differ from a theoretical database mass by a mass value corresponding to one of the considered PTMs.  The third table shows potential single AA substitutions detected by mass difference.
FINDMOD OUTPUT } unmodified peptides, modified peptides known in SWISS-PROT and chemically modified peptides
putatively modified peptides predicted by mass differences + putative AA substitutions {
-potentially modified peptides that agree with rules are listed - amino acids that potentially carry modifications are shown - peptides potentially modified only by mass difference - predictions can be tested by MS-MS peptide fragmentation
At the end of the output page the user will find a list of those entered matches which did not match in any of the above tables (if any).
FindMod

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FindMod

  • 1.
  • 2.
  • 3. Definition is a tool that can predict potential protein post-translational modifications (PTM) and find potential single amino acid substitutions in peptides.
  • 4. de novo discovery of protein post-translational modifications (PTM). It examines peptide mass fingerprinting results of known proteins for the presence of 22 types of PTMs of discrete mass: acetylation, amidation, biotin, C-mannosylation, deamidation, N-acyl diglyceride cysteine (tripalmitate), FAD, farnesylation, formylation, geranyl-geranyl, gamma-carboxyglutamic acid, O-GlcNAc, hydroxylation, lipoyl, methylation, myristoylation, palmitoylation, phosphorylation, pyridoxal phosphate, pyrrolidone carboxylic acid, sulfatation.
  • 5. The experimentally measured peptide masses are compared with the theoretical peptides calculated from a specified Swiss-Prot/TrEMBL entry or from a user-entered sequence, and mass differences are used to better characterise the protein of interest. If a mass difference corresponds to a known PTM not already annotated in UniProtKB/Swiss-Prot, "intelligent" rules are applied that examine the sequence of the peptide of interest and make predictions as to what amino acid in the peptide is likely to carry the modification.
  • 6. Protein Sequence to be characterize Peptide Massses
  • 7. 1.Protein Sequence to be characterized You should specify the sequence of the protein you would like to characterize and for which you have determined a set of peptide masses.
  • 8. • If the Protein sequence is known • If the Protein Sequence is not known
  • 9. Enter the UniProtKB/Swiss-Prot ID code (e.g. TKN1_HUMAN) Or the protein accession number (e.g. P20366).
  • 10. you can enter the sequence of your protein of interest, in single letter amino acid code, in either upper or lower case. The user is required to specify the biological source of the query protein
  • 11. Note The characters O and U are not considered and will give an error message. However, the residue J will be treated as either Ile or Leu, which have the same average and monoisotopic masses. The characters B, X, or are accepted, but no masses are computed for peptides containing one or more of these characters.
  • 12. 2.Peptide Masses Enter the experimentally measured peptide masses generated from the unknown protein in the « Enter a list of peptide masses...»text field, and separate them by spaces, tabs or new lines.
  • 13. NOTE You can copy a list of peptides from Excel or other applications and paste them directly into the text field. Avoid using peptide masses known to be from autodigestion of an enzyme (e.g. trypsin!), or other artefactual peaks (e.g. matrix peaks). Upload a .pkm, .dta or text file
  • 14. Uploading Peptide Masses Upload the file directly from your computer (1) Click on the on the «Browse...»button (2) Select the file containing the relevant peptide mass data. (3) Click on the «Open» button The peptide masses will then be extracted automatically from this file
  • 15. Expasy Tools Go to Expasy site: http://www.expasy.ch/tools/#proteome Select FinMod Tool
  • 18. Types of Supported Formats (1) .pkm format (2) Sequest format (3) User Created Files
  • 19. .pkm Format .pkm format, produced by the Voyager software of Perseptive Biosystems or the GRAMS software: OP=0Center X Peak Y Left X Right X Time X Mass Difference NameSTD.Misc Height Left Y Right Y %Height,Width,%Area,%Quan,H/A833.319 2189 833.260 833.378 0.016 0 0C0.? 0 762 762854.843 5078 854.769 854.917 0.001 0 0C0.? 0 3453 3453863.419 5108 863.064 863.775 0.001 0 0C0.? 0 3567 3567872.402 12519 872.347 872.456 0.002 0 0C0.? 0 11417 11417874.395 6730 874.331 874.460 0.002 0 0C0.? 0 3559 3559887.786 5903 887.540 888.031 0.003 0 0C0.? 0 4131 4131898.475 3329 898.416 898.534 0.006 0 0C0.? 0 1377 1377904.366 7432 904.199 904.533 0.001 0 0C0.? 0 5596 5596955.300 2598 955.229 955.371 0.011 0 0C0.? 0 1089 1089973.845 16689 973.749 973.941 0.001 0 0
  • 20. 1.001833.319 2189844.333 0.0854.843 5078863.419 5108872.402 12519874.395 6730887.786 5903898.475 3329899.555 0.0904.366 7432955.300 2598973.845 16689 The first line is considered as a comment and is ignored.
  • 21. User Created Files Any user-created files can be uploaded if they correspond to the following rules: The first line does not contain any mass value (if it does, this mass value is ignored). Lines containing masses must start with the mass, and the first 20 characters must not contain any uppercase letters.
  • 22. NOTE The upload option only works if you see a 'browse' button next to the text entry field. This should be the case for most recent web browser versions, e.g. Netscape 3.0 or higher, MS Internet Explorer 4.0 or higher.
  • 23. The user can specify whether the program should detect only potential PTMs, only single amino acid substitutions or both. The user can choose whether all peptide masses or only those that have not been attributed a theoretical peptide in this process should be examined for potential PTMs resp. single amino acid substitutions.
  • 24. ION MODE (MASSES AS [M] OR [M+H]+) You can enter the masses of your peptides as [M] or as [M+H]+, however you must select the appropriate button. If you select the [M+H]+ button, all peptide masses calculated from the database will have one proton (mass of 1 unit) added before matching with user-specified peptides.
  • 25. MASS TOLERANCE Peptide masses can be specified in ppm (parts per million) or in Dalton.
  • 26. DIGESTION AGENT (ENZYME) Specify the enzyme or chemical reagent that you used to generate your peptides (see the corresponding section in the PeptideMass instructions for the available enzymes and their cleavage rules).
  • 27. MISSED CLEAVAGES In order to take into account partial cleavages, you can specify a maximum number (0, 1, 2 or 3) of missed cleavage sites to be allowed. If the maximum number of missed cleavages entered is 1, all concatenations of two adjoining peptides are also added to the list of theoretical peptides under consideration.
  • 28. SORTING OF PEPTIDES IN THE RESULT TABLES Here you can choose if you would like the peptides to be sorted by their mass (from smallest to largest) or by their chronological order in the protein.
  • 29. SEND THE RESULT BY E-MAIL  Tick the « Send the result by e-mail » box. In the « Your e-mail:» text field you should enter the correct e-mail address (e.g. name@unknown.ch) to where the results should be sent.  The email option is recommended, in particular for queries with a high number of peptide masses. This avoids timeouts («document contains no data») which can occur for the on-line option: the browser interrupts the connection with the program if the search is not terminated after a certain time (usually about 3 minutes).  Note that email results are sent in form of a html file, in exactly the same format as on-line, and that there is no loss of functionality compared to on-line display.
  • 30. RESET AND PERFORM BUTTONS Once you have filled in the form according to your needs, press the button "Start FindMod". If you have made a mistake and would like all fields to be reset to their default values, press the Reset button.
  • 31. OUTPUT FORMAT o Header o up to three tables.
  • 32. HEADER The header contains information about the submitted protein:  A link to the UniProtKB/Swiss-Prot or UniProtKB/TrEMBL entry  The description line (if the protein is in UniProtKB), pI and molecular weight.
  • 33. Then the input parameters are listed, followed by an active link to PeptideMass. This allows the user to perform a theoretical cleavage of the protein of interest.
  • 34. TABLES The tables report the peptides whose experimental masses match unmodified or modified theoretical digest products of the protein of interest:  The first table reports matches to theoretical digest products as unmodified, modified with the annotations in UniProtKB/Swiss-Prot and chemically modified as specified in the input form.  The second table reports those user masses which differ from a theoretical database mass by a mass value corresponding to one of the considered PTMs.  The third table shows potential single AA substitutions detected by mass difference.
  • 35. FINDMOD OUTPUT } unmodified peptides, modified peptides known in SWISS-PROT and chemically modified peptides
  • 36. putatively modified peptides predicted by mass differences + putative AA substitutions {
  • 37. -potentially modified peptides that agree with rules are listed - amino acids that potentially carry modifications are shown - peptides potentially modified only by mass difference - predictions can be tested by MS-MS peptide fragmentation
  • 38. At the end of the output page the user will find a list of those entered matches which did not match in any of the above tables (if any).