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Practicality of membrane protein simulations…

Practicality of membrane protein simulations…. Dr Phil Biggin. Dept. of Biochemistry University of Oxford phil@biop.ox.ac.uk. Membrane Proteins – Why?. Ion channels, transporters, pumps, carriers, enzymes. Atomic level experimental information scarce (relatively) expression

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Practicality of membrane protein simulations…

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  1. Practicality of membrane protein simulations… Dr Phil Biggin Dept. of Biochemistry University of Oxford phil@biop.ox.ac.uk

  2. Membrane Proteins – Why? • Ion channels, transporters, pumps, carriers, enzymes. • Atomic level experimental information scarce (relatively) • expression • crystallization • But key drug targets:- From Terstappen & Reggiani, TIPS. 2001

  3. Outline of Procedure Obtain protein coordinates Immerse in bilayer/mimetic Solvate outside of membrane (and inside any pore regions) Add counterions (for correct concentration or to satisfy electrostatic calculations) Run simulation!

  4. Protein Coordinates… • PDB :- www.rcsb.org - X-ray/NMR • Xray  missing residues etc • NMR  which structure? • Number of human membrane proteins at high • resolution= ZERO… • So have to start from homology model (eg from modeller)

  5. Protein Coordinates… Starting from X-ray… http://www.rcsb.org/ 1BL8 •  missing residues •  incomplete residues •  mutated residues •  oligomer state •  pH • disulphides  covalent linkages ions/solutes Examine header

  6. Prepare/Repair Structure Graphically by hand (eg Quanta, Insight but these cost $$$) Swissviewer is free but more limited. Fix residues Online automated versions (eg What-If server http://www.cmbi.kun.nl:1100/WIWWWI/ Will also perform various stereochemical checks) Prior knowledge Oligomeric state Macromolecular Structure Database http://www.ebi.ac.uk/msd/ • Add polar hydrogens (Quanta, Insight but usually scripted in the other packages like pdb2gmx within the gromacs suite)

  7. Prepare/Repair Structure • pKa may be important – protonation state of ionizable residues.. • Can do ad-hoc. Look at structure and assign by eye/distance the protonation state of a particular residue. • Important for binding sites etc • BUT can dramatically effect stability of protein in simulation • For membrane proteins, situation is made more complex by presence of membrane… =78-90 Need different dielectric constants for each region (interface region tricky still) =2-6 =2-4

  8. Alignment/Positioning in Box • Things to consider:- • Existing experimental evidence • The aromatic “girdle” Z • Energetic positioning:- • Assign a hydrophobicity value to each residue (many scales to chose from!) • Calculate surface exposed area of each residue • Decide on width of hydrophobic zone of membrane (30Å) • Use Monte-Carlo to explore rigid-body movements across four degrees of freedom (3 rotational, 1 translational along Z, the bilayer normal • Lowest Energy position gives starting “orientation” with respect to box

  9. Choice of mimetic Full Bilayer Slowest but gain fullest information. Micelle Faster than bilayer. More and more NMR data now. Octane Slab (speed but no detail) Choice depends on what questions you want to ask. For example – is my homology model stable?

  10. Inserting into Octane YES Fit new protein onto existing protein (and delete existing protein) Is system similar to existing one? NO minimize Decide on box size and slab width* equilibrate Solvate helix with new octane box Run simulation! Add water (and ions if needed) * Make slab thickness slightly more than what you want as it will compress during equilibration.

  11. Inserting in a Micelle • Easiest way is to build micelle around protein • May also have experimental data as to the overall size estimate of the micelle. • Simply build by a script that relies on the geometry of the system • Solvate – might consider using an octahedral box for this system.

  12. Insertion into Bilayer… KcsA is a membrane protein so solvation includes bilayer, water and ions (sodium and chlorine for example). Add bilayer Add water/ions [Cytosolic proteins – immerse in box of pre-equilibrated water and delete overlapping (vdw spheres) molecules] Sounds a lot easier than it really is!…

  13. y (Å) x (Å) Protein into lipid • Problem… need to optimise interactions of lipids & protein • Method 1 – Roux & Woolf – pack lipid around a protein • Method 2 – Faraldo-Gomez & Smith - ‘grow’ a hole in a pre-formed bilayer • Method 3 – Use genbox (gromacs) and run long equilibration • Method 4 – Use VMD plugins (designed primarily with NAMD in mind) Change in Lipid Density FhuA inserted in POPC bilayer

  14. Insertion into Bilayer… Possible Protocol (to be explored in the practical session)  Obtain box of lipid. • Put protein into same box dimensions. • Use ‘genbox’ to ‘solvate’ the protein with that box of lipid. • Add water with ‘genbox’. • Delete waters in middle region of bilayer (perl script). • Add any counter ions. • Energy minimize. • Few hundred picoseconds of restrained MD. • Few nanoseconds of unrestrained MD (NPT). • Check lipid properties. • Perform production run (a few more nanoseconds).

  15. Insertion into Bilayer Things will equilibrate in a reasonably short time (a few ns)

  16. Solvation Now add water either side (and anywhere else you fancy) * Adding bulk is easy - add lots of small repeating boxes of water and delete overlapping atoms (as implemented in for example gromacs) * For smaller pockets, cavities and channels, you may need other “more accurate” methods:- * Eg. MMC (a grand-canonical monte-carlo approach) from Mihaly Mezei Voidoo/Flood (from Uppsala) Solvate (Grubmuller) NOTE: May be better/easier to solvate small cavities first prior to inserting into the membrane. Now add ions (number according to ionic strength) Method 1 – Random distribution Method 2 – based on electrostatic potential

  17. Ready to start? • First step is usually a minimization of sorts. • Strategy is ad-hoc really but work from bits you trust backwards. E.G. Sample strategy for membrane protein.  Constrain protein atoms – minimize waters/lipids  Constrain protein atoms – run MD for 200ps  Constrain C atoms – run MD for 200ps

  18. Run it! OK – now you are in position to run free MD! 3 • Run to equilibrium. • Use coordinate frames • beyond that. • 3. The more the merrier. 2 C RMSD (Å) 1 Take frames from here 1 2 3 4 Time (ns)

  19. Valid/stable simulation • Lots of parameters to check but probably single most useful one is • the area per lipid (describes molecular packing and describes degree of membrane fluidity). • very sensitive to simulation details, considered to be a reliable criterion. • Remember – it depends what your question is, undulations across large patches require different timescales compared to water-headgroup interactions for example.

  20. Parameters to consider in membrane simulations… • Periodic boundary conditions (PBCs) – what shape box? • Cubic, truncated octahedron, rhombic dodecahedron • Amount of “surrounding water” – typically more than 10Å margin • Ensemble - NPT commonest, but there are others (NVE for example) • Also constant surface tension simulations • Pressure and temperature coupling • E.g. Berendsen weak coupling versus Nosé-Hoover/Parrinello-Rahman • Electrostatics Treatment • Cut-off (artificial ordering?) • Ewald methods, Particle Mesh Ewald (enhance periodicity) • Reaction Field (ignore heterogenous nature of the membrane) • Frequency of dump • Large systems now (50,000-200,000 atoms) so files become large rapidly! • Suggested dump every 5ps with currently sizes.

  21. Insights from a recent Study A recent study systematically addressed some of the key issues in membrane simulations: “Methodological issues in lipid bilayer simulations”. Anézo et al. J. Phys. Chem B. 2003. 107. 9424-9433. • Parameters investigated:- electrostatic treatment (cutoff,PME,RF), cut-off radii, partial charge groupings, pressure coupling, timestep, size of system, force-field and amount of hydration water. (22 simulations some individually upto 150ns). • Treatment of electrostatics has most impact on area but all three schemes can give correct area per lipid. Combination of this and force-field is what is important. • Equilibration times of upto 25ns required for accurate assessment of properties such as area per lipid. Large area fluctuations occur on 10ns time scale. • Area per lipid cannot tell you whether force-field or method is OK. • But once area is correct, most others are usually OK (explains why so many different reports in the literature have bilayers with similar properties • No difference with pressure coupling (though Berendsen might be preferred in equilibration as it damps oscillations more effectively) • NO method is perfect! You make your choice!

  22. Where do I get lipids from? • Far easier to start with ready-equilibrated systems and insert protein into that • Scott Feller (wabash college) http://persweb.wabash.edu/facstaff/fellers/ POPC, DOPC, DPPC, SDPC • Helmut Heller (München) http://www.lrz-muenchen.de/~heller/membrane/membrane.html POPC in different phases. • Mikko Karttunen (Helsinki) http://www.lce.hut.fi/research/polymer/downloads.shtml DMTAP,DMPC,DPPC • Peter Tieleman (Calgary) http://moose.bio.ucalgary.ca/Downloads/ DPC micelles, POPC, DMPC, DPPC PLPC bilayers (topologies here as well). • And coming soon… BioSimGrid ‘lite’ http://www.biosimgrid.org/ Various bilayers all with complete topology and meta-data. More information about this site in Friday’s lecture.

  23. What if I have strange topology? Bonds and topology • If have similar existing topologies – can ‘adapt’ those. • Can work out manually (can be tiresome and boring!) • Can use PRODRG (Daan van Aalten) • If using gromacs someone might have already done it and uploaded it! Charges • Use similar atoms from similar ligands • Calculate from ab-initio (usual to use partial charges that best reproduce the molecular electrostatic potential (MEP) Vdw Parameters • Use similar atom types if possible. • Optimize to reproduce a range of themodynamic properties (eg density)

  24. Some references… D.M Hirst “A computational approach to chemistry” Blackwell scientific publications 1990. A.R. Leach “Molecular Modelling Principles and Applications” Longman Second ed. 2002. Gromacs manual @ http://www.gromacs.org “Methodological issues in lipid bilayer simulations”. Anézo et al. J. Phys. Chem B. 2003. 107. 9424-9433. J.M. Haile “Molecular Dynamics Simulation” Wiley 1997 Angwe Chemie 29 992 (1990)

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