Abstract
Protein lysine carbamylation is an irreversible post-translational modification resulting in generation of homocitrulline (N-ε-carbamyllysine), which no longer possesses a charged ε-amino moiety. Two distinct pathways can promote protein carbamylation. One results from urea decomposition, forming an equilibrium mixture of cyanate (CNO−) and the reactive electrophile isocyanate. The second pathway involves myeloperoxidase (MPO)-catalyzed oxidation of thiocyanate (SCN−), yielding CNO− and isocyanate. Apolipoprotein A-I (apoA-I), the major protein constituent of high-density lipoprotein (HDL), is a known target for MPO-catalyzed modification in vivo, converting the cardioprotective lipoprotein into a proatherogenic and proapoptotic one. We hypothesized that monitoring site-specific carbamylation patterns of apoA-I recovered from human atherosclerotic aorta could provide insights into the chemical environment within the artery wall. To test this, we first mapped carbamyllysine obtained from in vitro carbamylation of apoA-I by both the urea-driven (nonenzymatic) and inflammatory-driven (enzymatic) pathways in lipid-poor and lipidated apoA-I (reconstituted HDL). Our results suggest that lysine residues within proximity of the known MPO-binding sites on HDL are preferentially targeted by the enzymatic (MPO) carbamylation pathway, whereas the nonenzymatic pathway leads to nearly uniform distribution of carbamylated lysine residues along the apoA-I polypeptide chain. Quantitative proteomic analyses of apoA-I from human aortic atheroma identified 16 of the 21 lysine residues as carbamylated and suggested that the majority of apoA-I carbamylation in vivo occurs on “lipid-poor” apoA-I forms via the nonenzymatic CNO− pathway. Monitoring patterns of apoA-I carbamylation recovered from arterial tissues can provide insights into both apoA-I structure and the chemical environment within human atheroma.
Highlights
High-density lipoprotein (HDL) is a heterogeneous particle varying in composition of protein, lipids, size, density, and electrophoretic mobility [1, 2]
We sought to examine the extent of protein-bound lysine carbamylation on apolipoprotein A-I (apoA-I) recovered from human atherosclerotic plaque
In panel B, a parallel SDS-PAGE gel was run, and proteins transferred onto a membrane probed with high-affinity antihuman apoA-I-specific antibody for Western blot analysis
Summary
High-density lipoprotein (HDL) is a heterogeneous particle varying in composition of protein, lipids, size, density, and electrophoretic mobility [1, 2]. Displayed using the same X-axis (lysine location in apoA-I) is the summary of the patterns of site-specific apoA-I carbamylation observed in vitro using either the CNO− or MPO systems, for lipid-poor apoA-I and rHDL (Fig. 6A).
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