Best practices for applying HDX-MS to FBLD

Among the many biophysical techniques presented at the recent Novalix meeting, hydrogen/deuterium exchange mass spectrometry (HDX-MS) was mentioned only a few times. Practical Fragments last covered it nearly four years ago in the context of a paper that described theoretical challenges and improvements to the method for assessing fragment binding modes. A new open-access Comm. Chem. paper from Tiago Bandeiras, Alessio Bortoluzzi, and collaborators at iBET-Instituto de Biologia Experimental e Tecnológica and Merck KGaA implements some of these suggestions.

 

The researchers find only two examples where HDX-MS had been applied to fragments, one of which we covered here. The new paper focuses mostly on Cyclophilin D (CypD), a mitochondrial protein implicated in several diseases. A screen we wrote about in 2020 described several fragment hits, some of which were crystallographically found to bind in three overlapping sites designated the proline pocket, the aniline pocket, and the pyrazolo pocket.  The researchers chose a binder from each pocket to study as well as two more fragments whose binding sites were not known. All five fragments are extremely weak hits, with at best 7 mM (yes, millimolar) affinity as assessed by SPR, making this a particularly challenging test case.

 

As a reminder, HDX-MS examines the exchange of deuterium from D₂O to protein backbone amides. Nearby ligands can slow this exchange, and mapping the locations and magnitude of these changes reveals where the ligand binds. Optimization experiments were initially run on a compound with a K_D of 44 mM for the aniline pocket. Three protein concentrations were tested. Since the highest (10 µM) yielded the highest number of detected peptides, it was used for subsequent experiments.

 

As suggested in the 2022 paper, compound was added both to the initial protein solution as well as to the deuterium exchange buffer. The fragment was tested at 2.5, 5, and 10 mM, and changes in deuterium uptake were found in all cases, which is remarkable given that the theoretical occupancies range from 5 to 18%. An experiment using substoichiometric concentrations of a high affinity ligand confirmed that 18% protein occupancy is sufficient to generate a reliable signal.

 

Still, given the low occupancy, the researchers used statistical methods to ensure that changes in signals were significant. Mapping those that were onto the structure of the protein confirmed that the fragment bound to the aniline pocket.

 

A second fragment was tested by HDX-MS, and the results confirmed that it binds in the pyrazolo pocket, as previously shown by crystallography. However, for a third fragment that had been shown to bind in the proline pocket, the results suggested instead that it binds in the aniline pocket. The proline pocket exhibited very low levels of deuterium exchange, but when the researchers increased the pH from 7.4 to 9 they did find evidence that the fragment binds here as well.

 

Next, the researchers turned to the two fragments with unknown binding sites. HDX-MS revealed that these bind to the aniline binding site, though with subtly different protection patterns suggesting that they bind in slightly different regions of the pocket.

 

Finally, the researchers used their optimized HDX-MS conditions on a previously identified fragment that binds the kinase FAK with low millimolar affinity. This showed that it binds in the so-called hinge region, in agreement with crystallography. This fragment was also used as a negative control for CypD, showing that it does not bind.

 

This paper is a nice resource for those hoping to apply HDX-MS to fragments. The fact that the binding sites of such weak binders can be determined is quite remarkable. That said, the resolution is not as good as crystallography or protein-detected NMR; for FAK in particular, the ligand reduces deuterium update across a large fraction of the protein surface. And the fact that a proline-pocket binder was initially mapped to the aniline pocket also gives one pause. Perhaps the binding mode in solution really is different from that found crystallographically. It would be interesting to see whether NMR can resolve the conundrum.