First, we created a hypermethylated DIA assay library by DDA acquisitions of 6 SCX fractions from Gnmt -/- mouse livers. We supplemented this library with a DDA acquisition of a methyl-Lys immunoprecipitation from a hepatoma cell line derived from Gnmt -/- mice. This gave us an assay library of 808 methyl Arg and Lys peptides. We further supplemented the library with DDA acquisitions of a ‘one-pot’ acetyl-Lys and succinyl-Lys immunoaffinity enrichment of mitochondrial extract and whole liver lysate isolated from WT mouse liver which provided us with 2428 succinylated peptides and 2547 acetylated peptides. We then assayed whole liver cellular lysate from Mat1a -/- and Gnmt -/- and their WT littermates against this hypermethylated Arg and Lys peptide assay library acquired in both 4 Dalton and 12 Dalton precursor mass windows on the Orbitrap Fusion Lumos.