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This repository was archived by the owner on Aug 29, 2022. It is now read-only.

Notes on "typical protein:ligand setup pipeline" #7

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Notes on "typical protein:ligand setup pipeline"#7
@jchodera

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@jchodera
jchodera
opened on Feb 16, 2017

I just wanted to repost the notes on what goes into a "typical protein:ligand setup pipeline" from our meeting at MolSSI on 8 Oct 2016.

Contributors

  • John Chodera
  • Julien Michel
  • Peter Kasson
  • Oliver Beckstein

Before starting, Julien frequently does some manual inspection in a GUI:

  • missing loops
  • incomplete residues
  • cofactors: keep or discard? where to get parameters?
  • ions: keep or substitute?
  • crystal waters: keep or throw away?
  • crystal contacts, domain swapping
  • Read PDB paper to ensure that this is the protein structure that he wants to use
  • Note that assay conditions may differ from crystallographic conditions

What is our "typical" biomolecular preparation pipeline?

  • Decide which structure you want to use
  • Decide which chain to use if multiple copies
  • Reverting mutations or simulate a different construct
  • Disulfide if not in a reducing environment
  • Address PTMs
  • Julien typically uses the Maestro Protein Prep Wizard to:
    • add missing loops (up to a certain length)
    • add N/C-termini? Most people omit these
    • assign protonation states for desired pH
    • keep crystal waters; add hydrogens
    • interactively check histidine
  • Structural metal ions (e.g. Zn2+, Ca2+):
    • decide whether to retain
    • substitute with multisite models (alternatives: covalently bonded (harmonically restrained); single-site LJ)
  • Ligands and cofactors:
    • pick protonation state / tautomer
    • find or create parameters
    • covalently bound cofactors?
    • Consult Uppsala EDS to verify that ligand density justifies binding mode
    • model in rest of ligand or replace the ligand with another one (CCSD? swap from other PDB file? OpenEye)
  • Protonation states?
    • (PROPKA? 3.1 can do ligands; MCCE2?)
      Counterions and solvent
    • can do in either order
    • how big should box be? what shape? what buffer should be used? (Peter Kasson uses 20A buffer; Julien uses 12A; Oliver uses 15A)
    • for membrane proteins, at least 3-4 layers of lipids sideways; z-axis is very tricky
    • ionic strength

Challenges not yet addressed:

  • Membrane proteins
  • Proteins at surfaces/interfaces

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