Implementation of DiffDock, state-of-the-art method for molecular docking, by Gabriele Corso*, Hannes Stark*, Bowen Jing*, Regina Barzilay and Tommi Jaakkola. This repository contains code and instructions to run the method. Since 2024, Jacob Silterra has been leading the effort to maintain and improve the code. If you have any question, feel free to open an issue or reach out to us: gcorso@mit.edu and silterra@mit.edu.
Update February 2024: We have released DiffDock-L, a new version of DiffDock that provides a significant improvement in performance and generalization capacity (see the description of the new version in our new paper). By default the repository now runs the new model, please use GitHub commit history to run the original DiffDock model. Further we now provide instructions for Docker and to set up your own local UI interface.
You can also try out the model on Hugging Face Spaces.
Citation
If you use this code or the models in your research, please cite the following paper:
@inproceedings{corso2023diffdock,
title={DiffDock: Diffusion Steps, Twists, and Turns for Molecular Docking},
author = {Corso, Gabriele and Stärk, Hannes and Jing, Bowen and Barzilay, Regina and Jaakkola, Tommi},
booktitle={International Conference on Learning Representations (ICLR)},
year={2023}
}
If you use the latest version, DiffDock-L, please also cite the following paper:
@inproceedings{corso2024discovery,
title={Deep Confident Steps to New Pockets: Strategies for Docking Generalization},
author={Corso, Gabriele and Deng, Arthur and Polizzi, Nicholas and Barzilay, Regina and Jaakkola, Tommi},
booktitle={International Conference on Learning Representations (ICLR)},
year={2024}
}
Table of contents
You can directly try out the model without the need of installing anything through Hugging Face Spaces. Credit for the current HF interface goes to Jacob Silterra and for the previous version to Simon Duerr.
We will set up the environment using Anaconda. Clone the current repo
git clone https://github.com/gcorso/DiffDock.git
To set up an appropriate environment, navigate to the root of the repository and run the following commands:
conda env create --file environment.yml
conda activate diffdock
See conda documentation for more information.
A Dockerfile is provided for building a container:
docker build . -f Dockerfile -t diffdock
Alternatively, you can use a pre-built container to run the code. First, download the container from Docker Hub:
docker pull rbgcsail/diffdock
Check if you have a GPU available
docker run --rm --gpus all nvidia/cuda:11.7.1-devel-ubuntu22.04 nvidia-smi
Then, run the container:
docker run -it --gpus all --entrypoint /bin/bash rbgcsail/diffdock
If you don't have a GPU, run (it will be significantly slower):
docker run -it --entrypoint /bin/bash rbgcsail/diffdock
Inside the container
micromamba activate diffdock
You can now run the code as described below.
We support multiple input formats depending on whether you only want to make predictions for a single complex or for many at once.
The protein inputs need to be .pdb
files or sequences that will be folded with ESMFold. The ligand input can either be a SMILES string or a filetype that RDKit can read like .sdf
or .mol2
.
For a single complex: specify the protein with --protein_path protein.pdb
or --protein_sequence GIQSYCTPPYSVLQDPPQPVV
and the ligand with --ligand ligand.sdf
or --ligand "COc(cc1)ccc1C#N"
For many complexes: create a csv file with paths to proteins and ligand files or SMILES. It contains as columns complex_name
(name used to save predictions, can be left empty), protein_path
(path to .pdb
file, if empty uses sequence), ligand_description
(SMILE or file path) and protein_sequence
(to fold with ESMFold in case the protein_path is empty).
An example .csv is at data/protein_ligand_example.csv
and you would use it with --protein_ligand_csv protein_ligand_example.csv
.
And you are ready to run inference:
python -m inference --config default_inference_args.yaml --protein_ligand_csv data/protein_ligand_example.csv --out_dir results/user_predictions_small
When providing the .pdb
files you can run DiffDock also on CPU, however, if possible, we recommend using a GPU as the model runs significantly faster. Note that the first time you run DiffDock on a device the program will precompute and store in cache look-up tables for SO(2) and SO(3) distributions (typically takes a couple of minutes), this won't be repeated in following runs.
We provide a simple graphical user interface to run DiffDock on a single complex. To use it, run the following command:
python app/main.py
and navigate to http://localhost:7860 in your browser.
How to interpret the DiffDock output confidence score?
It can be hard to interpret and compare confidence score of different complexes or different protein conformations, however, here a rough guideline that we typically use (c is the confidence score of the top pose):- c > 0 high confidence
- -1.5 < c < 0 moderate confidence
- c < -1.5 low confidence
This is assuming the complex is similar to what DiffDock saw in the training set i.e. a not too large drug-like molecule bound to medium size protein (1 or 2 chains) in a conformation that is similar to the bound one (e.g. if it comes from an homologue crystal structure). If you are dealing with a large ligand, a large protein complex and/or an app/unbound protein conformation you should shift these intervals down.
Does DiffDock predict the binding affinity of the ligand to the protein?
No, DiffDock does not predict the binding affinity of the ligand to the protein. It predicts the 3D structure of the complex and it outputs a confidence score. This latter is a measure of the quality of the prediction, i.e. the model's confidence in its prediction of the binding structure. Several of our collaborators have seen this to have some correlation with binding affinity (intuitively if a ligand does not bind there will be no good pose), but it is not a direct measure of it.We are working on better affinity prediction models, but in the meantime we recommend combining DiffDock's prediction with other tools such as docking function (e.g. GNINA), MM/GBSA or absolute binding free energy calculations. For this we recommend to first relax the DiffDock's structure predictions with the tool/force field used for the affinity prediction.
Can I use DiffDock for protein-protein or protein-nucleic acid interactions?
While the program might not throw and error when fed with a large biomolecules as input, the model has only been designed, trained and tested for small molecule docking to proteins. Therefore, DiffDock is only likely to be able to deal with small peptides and nucleic acids as ligands, we do not recommend using DiffDock for the interactions of larger biomolecules. For other interactions we recommend looking at [DiffDock-PP](https://github.com/ketatam/DiffDock-PP) (rigid protein-protein interactions), [AlphaFold-Multimer](https://github.com/google-deepmind/alphafold) (flexible protein-protein interactions) or [RoseTTAFold2NA](https://github.com/uw-ipd/RoseTTAFold2NA) (protein-nucleic acid interactions).The files in data
contain the splits used for the various datasets. Below instructions for how to download each of the different datasets used for training and evaluation:
- PDBBind: download the processed complexes from zenodo, unzip the directory and place it into
data
such that you have the pathdata/PDBBind_processed
. - BindingMOAD: download the processed complexes from zenodo under
BindingMOAD_2020_processed.tar
, unzip the directory and place it intodata
such that you have the pathdata/BindingMOAD_2020_processed
. - DockGen: to evaluate the performance of
DiffDock-L
with this repository you should use directly the data from BindingMOAD above. For other purposes you can download exclusively the complexes of the DockGen benchmark already processed (e.g. chain cutoff) from zenodo downloading theDockGen.tar
file. - PoseBusters: download the processed complexes from zenodo.
- van der Mers: the protein structures used for the van der Mers data augmentation strategy were downloaded here.
If you are interested in replicating the results of the original DiffDock paper please checkout to the following commit:
git checkout v1.0
Otherwise download the data and place it as described in the "Dataset" section above.
To avoid having to compute ESM embeddings every time we evaluate on a dataset we first cache them and then run the evaluation script. Here the instructions for generating these for PDBBind but it also applies similarly to the other benchmarks. First run the following command to save the list of ESM embeddings:
python datasets/esm_embedding_preparation.py
Use the generated file data/pdbbind_sequences.fasta
to generate the ESM2 language model embeddings using the library https://github.com/facebookresearch/esm by installing their repository and executing the following in their repository:
python scripts/extract.py esm2_t33_650M_UR50D pdbbind_sequences.fasta embeddings_output --repr_layers 33 --include per_tok --truncation_seq_length 4096
This generates the embeddings_output
directory which you have to copy into the data
folder of our repository to have data/embeddings_output
.
Then run the command:
python datasets/esm_embeddings_to_pt.py
For PDBBind:
python -m evaluate --config default_inference_args.yaml --split_path data/splits/timesplit_test --split_path data/splits/timesplit_test --batch_size 10 --esm_embeddings_path data/esm2_embeddings.pt --data_dir data/PDBBind_processed/ --tqdm --split test --chain_cutoff 10 --dataset pdbbind
For DockGen:
python -m evaluate --config default_inference_args.yaml --dataset moad --data_dir data/BindingMOAD_2020_processed --unroll_clusters --tqdm --split test --esm_embeddings_path data/moad_esm2_embeddings.pt --min_ligand_size 2 --moad_esm_embeddings_sequences_path data/moad_sequences_to_id.fasta --chain_cutoff 10 --batch_size 10
For PoseBusters:
python -m evaluate --config default_inference_args.yaml --data_dir data/posebusters_benchmark_set --tqdm --dataset posebusters --split_path data/splits/posebusters_benchmark_set_ids.txt --esm_embeddings_path data/posebusters_ESM.pt --chain_cutoff 10 --batch_size 10 --protein_file protein --ligand_file ligands
To additionally save the .sdf files of the generated molecules, add the flag --save_visualisation
.
Note: the notebook data/apo_alignment.ipynb
contains the code used to align the ESMFold-generated apo-structures to the holo-structures.
If you use this code or the models in your research, please cite the following paper:
@inproceedings{corso2023diffdock,
title={DiffDock: Diffusion Steps, Twists, and Turns for Molecular Docking},
author = {Corso, Gabriele and Stärk, Hannes and Jing, Bowen and Barzilay, Regina and Jaakkola, Tommi},
booktitle={International Conference on Learning Representations (ICLR)},
year={2023}
}
If you use the latest version of our model, DiffDock-L, please also cite the following paper:
@inproceedings{corso2024discovery,
title={Deep Confident Steps to New Pockets: Strategies for Docking Generalization},
author={Corso, Gabriele and Deng, Arthur and Polizzi, Nicholas and Barzilay, Regina and Jaakkola, Tommi},
booktitle={International Conference on Learning Representations (ICLR)},
year={2024}
}
The code and model weights are released under MIT license. See the LICENSE file for details.
Components of the code of the spyrmsd package by Rocco Meli (also MIT license) were integrated in the repo.
We sincerely thank:
- Jacob Silterra for his help with the publishing and deployment of the code.
- Arthur Deng, Nicholas Polizzi and Ben Fry for their critical contributions to part of the code in this repository.
- Wei Lu and Rachel Wu for pointing out some issues with the code.