Development of a competitive fluorescence-based synaptosome binding assay for brevetoxins

被引:19
作者
McCall, Jennifer R. [1 ]
Jacocks, Henry M. [1 ]
Baden, Daniel G. [1 ]
Bourdelais, Andrea J. [1 ]
机构
[1] Univ N Carolina, Ctr Marine Sci, Wilmington, NC 28409 USA
关键词
BODIPY; Brevetoxin; Competition binding assay; Fluorescence assay; DINOFLAGELLATE KARENIA-BREVIS; SENSITIVE SODIUM-CHANNELS; FLORIDA RED TIDE; AEROSOLIZED BREVETOXINS; RAT-BRAIN; LIGANDS; ACTIVATORS; RECEPTORS; SHELLFISH; NEURONS;
D O I
10.1016/j.hal.2012.06.003
中图分类号
Q17 [水生生物学];
学科分类号
071004 ;
摘要
Brevetoxins are a family of ladder-frame polyether toxins produced during blooms of the marine dinoflagellate Karenia brevis. Inhalation of brevetoxins aerosolized by wind and wave action can lead to asthma-like symptoms in beach goers. Consumption of either shellfish or finfish exposed to K. brevis blooms can lead to the development of neurotoxic shellfish poisoning. The toxic effects of brevetoxins are due to activation of voltage-sensitive sodium channels (VSSCs) in cell membranes. Binding of brevetoxin analogs and competitors to site 5 on these channels has historically been measured using a radioligand competition assay that is fraught with difficulty, including slow analysis time, production of radioactive waste, and cumbersome and expensive methods associated with the generation of radioactive labeled ligands. In this study, we describe the development of a novel fluorescent synaptosome binding assay for the brevetoxin receptor. BODIPY (R)-conjugated to PbTx-2 was used as the labeled ligand. The BODIPY (R)-PbTx-2 conjugate was found to displace [H-3]-PbTx-3 from its binding site on VSSCs on rat brain synaptosomes with an equilibrium inhibition constant of 0.11 nM. We have shown that brevetoxin A and B analogs are all able to compete for binding with the fluorescent ligand. Most importantly, this assay was validated against the current site 5 receptor binding assay standard, the radioligand receptor assay for the brevetoxin receptor using [H-3]-PbTx-3 as the labeled ligand. The fluorescence based assay yielded equilibrium inhibition constants comparable to the radioligand assay for all brevetoxin analogs. The fluorescence based assay was quicker, far less expensive, and did not generate radioactive waste or need radioactive facilities. As such, this fluorescence-based assay can be used to replace the current radioligand assay for site 5 on voltagesensitive sodium channels and will be a vital tool for future experiments examining the binding affinity of various ligands for site 5 on sodium channels. (c) 2012 Elsevier B.V. All rights reserved.
引用
收藏
页码:85 / 91
页数:7
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