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Digging deep for GOLD: How buriedness may be used to
discriminate between actives and inactives in docking
Noel M. O’Boyle, Suzanne R. Brewerton and Robin Taylor
Cambridge Crystallographic Data Centre, Cambridge, UK. E-mail: oboyle@ccdc.cam.ac.uk; Web: http://www.ccdc.cam.ac.uk


Introduction
When protein-ligand docking software is used for virtual screening, the goal is to identify true
ligands (actives) in a dataset consisting mainly of non-binders (inactives). Actives tend to bind deep
in the binding site. This suggests that scaling the score assigned to particular interactions based on
the burial depth may allow better discrimination between actives and inactives. This should lead to
                                                                                                                                          Figure 1 – The goal is to make it
improved results (increased enrichments) in virtual screens. We describe the incorporation of burial                                      easy to pick out active molecules
                                                                                                                                               from a large database.
depth scaling (BDS) into the ChemScore scoring function in the docking software, GOLD.




Experimental Method
A burial depth scaling function, f(ρ), (Figure 2) was introduced into the ChemScore scoring
function that scaled individual hydrogen bonds based on the depth at which they occurred. A
constant scaling, Slipo, was introduced for lipophilic interactions (burial depth scaling for lipophilic
interactions was not found to perform better). The optimal parameter values were determined
using positive and negative data generated using the Astex Diverse Set [1], 85 high-quality
protein-ligand complexes. The positive data were correctly docked poses of the known ligands (or
in 6 cases, the locally-optimised crystal structure). For each active, negative data were generated
by docking 99 inactives which were selected to be topologically distinct from the active yet                                    Figure 2 - Burial depth scaling function f(ρ)
physicochemically similar.
By varying the parameters ρ1, ρ2, fmax, and Slipo, a brute-force optimisation procedure was used to optimise the mean rank of the score of
each active with respect to its 99 inactives. The final results were tested with a test set of new inactives.



Results
The optimisation procedure improved the
mean rank of the active molecules from
18.6 to 12.5 (top rank is 1), with only a
few actives decreasing in rank (Figures
3, 4). The overall effect was to reward
hydrogen bonds deep in the active site,
and    to   reduce   the   contribution   of
lipophilic interactions. For the test set,
                                               Figure 3 – Histogram showing the effect of BDS on           Figure 4 - Protein-ligand complexes (i) 1p62 and (ii) 1hnn. Surface
the ranks improved from 18.8 to 12.6.
                                                            the ranks of the actives.                            coloured by burial depth (red is deep, blue is shallow).




Conclusions                                                                                        Future Work
Incorporating burial depth into the ChemScore scoring function in GOLD                             Can burial depth scaling also be used during the
leads to improved enrichments across a wide range of pharmaceutically                              docking process itself, rather than simply in rescoring
relevant proteins. Negative data may successfully be used to identify and                          docked poses? Preliminary work shows that the clash
address deficiencies in empirical scoring functions (see also [2]).                                term needs to be retrained to avoid rewarding deep
                                                                                                   hydrogen bonds at the expense of good poses.
Burial depth scaling is available as an option in GOLD 4.0.

 1    Hartshorn, M. J.; Verdonk, M. L.; Chessari, G.; Brewerton, S. C.; Mooij, W. T. M.; Mortenson, P. N.; Murray, C. W. J. Med. Chem.
      2007, 50, 726-741.
 2    Pham, T. A.; Jain, A. N. J. Med. Chem. 2006, 49, 5856-5868.

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Digging deep for GOLD: How buriedness may be used to discriminate between actives and inactives in docking

  • 1. Digging deep for GOLD: How buriedness may be used to discriminate between actives and inactives in docking Noel M. O’Boyle, Suzanne R. Brewerton and Robin Taylor Cambridge Crystallographic Data Centre, Cambridge, UK. E-mail: oboyle@ccdc.cam.ac.uk; Web: http://www.ccdc.cam.ac.uk Introduction When protein-ligand docking software is used for virtual screening, the goal is to identify true ligands (actives) in a dataset consisting mainly of non-binders (inactives). Actives tend to bind deep in the binding site. This suggests that scaling the score assigned to particular interactions based on the burial depth may allow better discrimination between actives and inactives. This should lead to Figure 1 – The goal is to make it improved results (increased enrichments) in virtual screens. We describe the incorporation of burial easy to pick out active molecules from a large database. depth scaling (BDS) into the ChemScore scoring function in the docking software, GOLD. Experimental Method A burial depth scaling function, f(ρ), (Figure 2) was introduced into the ChemScore scoring function that scaled individual hydrogen bonds based on the depth at which they occurred. A constant scaling, Slipo, was introduced for lipophilic interactions (burial depth scaling for lipophilic interactions was not found to perform better). The optimal parameter values were determined using positive and negative data generated using the Astex Diverse Set [1], 85 high-quality protein-ligand complexes. The positive data were correctly docked poses of the known ligands (or in 6 cases, the locally-optimised crystal structure). For each active, negative data were generated by docking 99 inactives which were selected to be topologically distinct from the active yet Figure 2 - Burial depth scaling function f(ρ) physicochemically similar. By varying the parameters ρ1, ρ2, fmax, and Slipo, a brute-force optimisation procedure was used to optimise the mean rank of the score of each active with respect to its 99 inactives. The final results were tested with a test set of new inactives. Results The optimisation procedure improved the mean rank of the active molecules from 18.6 to 12.5 (top rank is 1), with only a few actives decreasing in rank (Figures 3, 4). The overall effect was to reward hydrogen bonds deep in the active site, and to reduce the contribution of lipophilic interactions. For the test set, Figure 3 – Histogram showing the effect of BDS on Figure 4 - Protein-ligand complexes (i) 1p62 and (ii) 1hnn. Surface the ranks improved from 18.8 to 12.6. the ranks of the actives. coloured by burial depth (red is deep, blue is shallow). Conclusions Future Work Incorporating burial depth into the ChemScore scoring function in GOLD Can burial depth scaling also be used during the leads to improved enrichments across a wide range of pharmaceutically docking process itself, rather than simply in rescoring relevant proteins. Negative data may successfully be used to identify and docked poses? Preliminary work shows that the clash address deficiencies in empirical scoring functions (see also [2]). term needs to be retrained to avoid rewarding deep hydrogen bonds at the expense of good poses. Burial depth scaling is available as an option in GOLD 4.0. 1 Hartshorn, M. J.; Verdonk, M. L.; Chessari, G.; Brewerton, S. C.; Mooij, W. T. M.; Mortenson, P. N.; Murray, C. W. J. Med. Chem. 2007, 50, 726-741. 2 Pham, T. A.; Jain, A. N. J. Med. Chem. 2006, 49, 5856-5868.