Biosynthesis of lysine-derived elastin crosslinks in aortic cell culture

Abstract

Culture of an established line of aortic medial cells in the presence of L-[14C] lysine for 72 hours, beginning on the twenty-first day after transfer, has resulted in the incorporation of label into a residue, insoluble after autoclaving. Acid hydrolysates of this residue with or without reduction by NaBH4 were subjected to ion exchange chromatography. Several radioactive lysine-derived residues were identified, by comparison to standards, as the distinctive crosslinks of elastin, isodesmosine, desmosine, merodesmosine and lysinonorleucine. This confirms the synthesis of elastin in aortic cell culture and establishes the formation of insoluble crosslinked elastin. Differences in the heights of the peaks in the reduced and nonreduced elastin indicate the probable occurrence of dehydromerodesmosine and dehydrolysino-norleucine as well and suggest that these may be intermediates in crosslink formation. © 1975.