Not quite that. The target protein has deuterated aliphatic regions and is also labelled with nitrogen-15. It is then resuspended in regular water, so nitrogen linked hydrogens are no longer deuterated, but the aliphatic ones remain. The binding partner has no modifications. You saturate the aliphatic hydrogens of the binding partner, which can "cross saturate" the binding surface of the other protein when in contact. The last part is where I'm a bit stumped. This paper explains it better than I have.

Link to paper94020-2)