Thermoresponsive supramolecular assemblies have been extensively explored in diverse formats, from injectable hydrogels to nanoscale carriers, for a variety of applications including drug delivery, tissue engineering and thermo-controlled catalysis. Understanding...
The propensity of broad-spectrum antibiotics to indiscriminately kill both pathogenic and beneficial bacteria has a profound impact on the spread of resistance across multiple bacterial species. Alternative approaches that narrow...
A primary
component of all known bacterial cell walls is the peptidoglycan
(PG) layer, which is composed of repeating units of sugars connected
to short and unusual peptides. The various steps within PG biosynthesis
are targets of potent antibiotics as proper assembly of the PG is
essential for cellular growth and survival. Synthetic mimics of PG
have proven to be indispensable tools to study the bacterial cell
structure, growth, and remodeling. Yet, a common component of PG, meso-diaminopimelic acid (m-DAP) at the
third position of the stem peptide, remains challenging to access
synthetically and is not commercially available. Here, we describe
the synthesis and metabolic processing of a selenium-based bioisostere
of m-DAP (selenolanthionine) and show that it is
installed within the PG of live bacteria by the native cell wall crosslinking
machinery in mycobacterial species. This PG probe has an orthogonal
release mechanism that could be important for downstream proteomics
studies. Finally, we describe a bead-based assay that is compatible
with high-throughput screening of cell wall enzymes. We envision that
this probe will supplement the current methods available for investigating
PG crosslinking in m-DAP-containing organisms.
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