Bacterial peptidoglycan (PG) is a mesh like structure comprising glycan strands cross-linked by peptide stems. Since PG is a specific and essential component of bacterial cells it is an attractive and validated target for antibacterial agents. Indeed, the first antibiotic in clinical use - the β-lactam penicillin - targets the enzymes catalyzing the final transpeptidation step of PG synthesis - the Penicillin-Binding-Proteins (PBPs). A prevalent mechanism of resistance to β-lactams is the production of β-lactamases (βLs) that inactivate the drugs. A first generation of β-lactamase inhibitors (BLIs) was based on the β-lactam core followed by diazabicyclooctanes (DBOs), which entered the market in 2015 with avibactam. Emergence of mutations compromising the efficacy of DBOs prompted us to study a series of triazole-substituted DBOs that were obtained by click chemistry. The triazole ring was found to be disfavored due to the absence of a hydrogen bond connecting the carboxamide of marketed DBOs to the conserved N132 residue of βLs. However, functionalization of the triazole partially restored inhibition efficacy without impairing drug penetration. Besides the major cross-links formed by PBPs, alternative cross-links are formed by the structurally distinct l,d-transpeptidases (LDTs) mediating resistance to several β-lactams. We investigated the mechanisms of insertion of new subunits into the expanding PG mesh by developing a method based on labeling with heavy isotopes and mass spectrometry. We report the modes of PG polymerization in strains relying on PBPs and LDTs for PG cross-linking in the presence or absence of β-lactams together with the extent of PG recycling.