Identification and Characterization of Acyl-Protein Thioesterase 1/Lysophospholipase I As a Ghrelin Deacylation/Lysophospholipid Hydrolyzing Enzyme in Fetal Bovine Serum and Conditioned Medium

Ghrelin contains an octanoic acid at the third residue serine, and the presence of octanoic acid on ghrelin is critical to its physiological functions. The precise mechanism for the deacylation of ghrelin in circulation remains to be clarified, although the level of deacylated ghrelin (des-acyl ghre...

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Published in:Endocrinology (Philadelphia) 2010-10, Vol.151 (10), p.4765-4775
Main Authors: Satou, Motoyasu, Nishi, Yoshihiro, Yoh, Junko, Hattori, Yoshiyuki, Sugimoto, Hiroyuki
Format: Article
Language:English
Subjects:
Acetylation - drug effects
Animals
Biological and medical sciences
Cattle
Cell culture
Cells, Cultured
Culture Media, Conditioned - chemistry
Culture Media, Conditioned - pharmacology
Deacylation
Enzymes
Fetal Blood - physiology
Fetal calf serum
Fundamental and applied biological sciences. Psychology
Ghrelin
Ghrelin - metabolism
Hep G2 Cells
Hepatocytes
Humans
Hydrolysis - drug effects
Ionization
Lipopolysaccharides
Lysophospholipase
Lysophospholipase - isolation & purification
Lysophospholipase - metabolism
Lysophospholipids - metabolism
Macrophages
Male
Mass spectrometry
Mass spectroscopy
mRNA
Octanoic acid
Protein folding
Proteins
Rats
Rats, Wistar
Serum - chemistry
Serum - physiology
Thioesterase
Vertebrates: endocrinology
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Summary:Ghrelin contains an octanoic acid at the third residue serine, and the presence of octanoic acid on ghrelin is critical to its physiological functions. The precise mechanism for the deacylation of ghrelin in circulation remains to be clarified, although the level of deacylated ghrelin (des-acyl ghrelin) is higher than that of acylated ghrelin in serum. In this study, rapid identification of ghrelin deacylation activity was achieved by matrix-assisted laser desorption/ionization time-of-flight mass spectrometry, and a ghrelin deacylation enzyme was purified 1515-fold from fetal bovine serum. Chromatographic separation showed a 24-kDa band on SDS-PAGE corresponding to ghrelin deacylation activity, and the protein band was identified as acyl-protein thioesterase 1 (APT1)/lysophospholipase I. A ghrelin deacylation enzyme in medium from HepG2 cells was also purified and identified as APT1. Although it lacks a secretion signal sequence, APT1 may be released by cells expressing APT1, mainly from liver in vivo. APT1 was originally purified as a cytosolic lysophospholipid hydrolyzing enzyme (lysophospholipase I), and recombinant APT1 exhibited deacylation activity as well as lysophospholipase activity in vitro. APT1 is released at high levels from RAW264.7 macrophage-like cells into the culture medium after stimulation with lipopolysaccharide (LPS), and LPS suppresses APT1 mRNA and protein expressions in these cells. More potent ghrelin deacylase activities were detected in sera from LPS-treated rats than in control sera. These results suggested that the serum activity of APT1 may play an important role in determination of the concentration of des-acyl ghrelin in circulation, especially under septic inflammation. Ghrelin is rapidly deacylated by acyl-protein thioesterase 1/lysophospholipase I in fetal bovine serum.
ISSN:0013-7227
1945-7170
DOI:10.1210/en.2010-0412