Abstract
Firefly luciferase is homologous to fatty acyl-CoA synthetases. We hypothesized that the firefly luciferase substrate d-luciferin and its analogs are fatty acid mimics that are ideally suited to probe the chemistry of enzymes that release fatty acid products. Here, we synthesized luciferin amides and found that these molecules are hydrolyzed to substrates for firefly luciferase by the enzyme fatty acid amide hydrolase (FAAH). In the presence of luciferase, these molecules enable highly sensitive and selective bioluminescent detection of FAAH activity in vitro, in live cells, and in vivo. The potency and tissue distribution of FAAH inhibitors can be imaged in live mice, and luciferin amides serve as exemplary reagents for greatly improved bioluminescence imaging in FAAH-expressing tissues such as the brain.
Publication types
-
Research Support, N.I.H., Extramural
MeSH terms
-
Amides / chemical synthesis
-
Amides / chemistry
-
Amides / metabolism*
-
Amidohydrolases / analysis
-
Amidohydrolases / antagonists & inhibitors
-
Amidohydrolases / metabolism*
-
Animals
-
Benzothiazoles / chemical synthesis
-
Benzothiazoles / chemistry
-
Benzothiazoles / metabolism*
-
CHO Cells
-
Cricetulus
-
Enzyme Assays
-
Enzyme Inhibitors / pharmacokinetics*
-
Enzyme Inhibitors / pharmacology
-
HeLa Cells
-
Humans
-
Hydrolysis
-
Luciferases, Firefly / metabolism*
-
Luminescent Agents / chemical synthesis
-
Luminescent Agents / chemistry
-
Luminescent Agents / metabolism*
-
Mice
-
Optical Imaging
-
Piperidines / pharmacokinetics*
-
Piperidines / pharmacology
-
Pyridines / pharmacokinetics*
-
Pyridines / pharmacology
-
Tissue Distribution
Substances
-
Amides
-
Benzothiazoles
-
D-luciferin
-
Enzyme Inhibitors
-
Luminescent Agents
-
PF 3845
-
Piperidines
-
Pyridines
-
Luciferases, Firefly
-
Amidohydrolases
-
fatty-acid amide hydrolase