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Proteomic analysis of human low‐density lipoprotein reveals the presence of prenylcysteine lyase,a hydrogen peroxide‐generating enzyme
Authors:Cristina Banfi Dr.  Maura Brioschi  Simona Barcella  Robin Wait  Shajna Begum  Sabrina Galli  Andrea Rizzi  Elena Tremoli
Affiliation:1. Monzino Cardiologic Center IRCCS, Milan, Italy;2. Department of Pharmacological Sciences, University of Milan, Italy;3. These authors contribute equally to this work.;4. Kennedy Institute of Rheumatology Division, Faculty of Medicine, Imperial College London, Hammersmith, London, UK
Abstract:The molecular mechanisms underlying the relationship between low‐density lipoprotein (LDL) and the risk of atherosclerosis are not clear. Therefore, detailed information on the protein composition of LDL may help to reveal its role in atherogenesis. Liquid‐phase IEF has been used to resolve LDL proteins into well‐defined fractions on the basis of pI, which improves the subsequent detection and resolution of low abundance proteins. Besides known LDL‐associated proteins, this approach revealed the presence of proteins not previously described to reside in LDL, including prenylcysteine lyase (PCL1), orosomucoid, retinol‐binding protein, and paraoxonase‐1. PCL1, an enzyme crucial for the degradation of prenylated proteins, generates free cysteine, isoprenoid aldehyde and hydrogen peroxide. Addition of the substrate farnesylcysteine to lipoprotein resulted in a time‐dependent generation of H2O2 which was stronger in very low density lipoprotein (VLDL) than in LDL or HDL, reflecting the greater protein content of PCL1 in VLDL. Farnesol, a dead end inhibitor of the PCL1 reaction, reduced H2O2 generation by VLDL. PCL1 is generated along with nascent lipoprotein, as shown by its presence in the lipoprotein secreted by HepG2 cells. The finding that an enzyme associated with atherogenic lipoproteins can itself generate an oxidant suggests that PCL1 may play a significant role in atherogenesis.
Keywords:Atherosclerosis  Hydrogen peroxide  Lipoprotein  Prefractionation techniques  Prenylcysteine lyase
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