Solubilization and characterization of [3H] 5HT high affinity binding sites (5HT1 and 5HT3).

Journal de pharmacologie Pub Date : 1985-10-01
J C Rousselle, G Gillet, G Fillion
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Abstract

The solubilization of the serotonergic 5HT1 and 5HT3 sites was performed with digitonin and sodium cholate at 1% (final concentration). Two binding sites for [3H]5HT were observed on rat or horse brain synaptosomal membranes solubilized with these detergents. The corresponding dissociation constants (KD) were 1-3 nM and 13-30 nM respectively. These values were closely similar to those corresponding to 5HT1 and 5HT3 sites located in intact membranes. The solubilized sites specifically bound 5HT. The effect of GTP decreasing the binding to 5HT1 sites was lost on solubilized 5HT1 sites; it was recovered, however, by addition of phospholipids (asolectin 0,2%). The apparent molecular weights of these sites were determined using the gel filtration method (438 and 235 K daltons). The photoactivation of [3H]5HT by U.V. light was used to label 5HT1 and 5HT3 sites irreversively in membranes. The binding of [3H]5HT following U.V. irradiation was not dissociated after dilution; it was saturable and prevented by serotonergic drugs and not by adrenergic or dopaminergic antagonists. Moreover, GTP added prior to the irradiation reduced it markedly thus showing that 5HT1 sites were labelled. Electrophoretic and fluorographic analyses of the labelled material evidenced a 60 K dalton-band specifically labelled with [3H]5HT (5 or 20 nM). These results tend to indicate that the 60 K dalton-proteic band might represent a proteic subunit constituting part of 5HT1 and 5HT3 sites.

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[3H] 5HT高亲和结合位点(5HT1和5HT3)的增溶和表征。
用1%(终浓度)的洋地黄苷和胆酸钠对血清素能5HT1和5HT3位点进行增溶。在大鼠或马脑突触体膜上观察到两个[3H]5HT的结合位点。相应的解离常数(KD)分别为1 ~ 3 nM和13 ~ 30 nM。这些值与位于完整膜上的5HT1和5HT3位点对应的值非常相似。可溶性位点特异性结合5HT。GTP降低5HT1位点结合的作用在可溶性5HT1位点上消失;然而,通过添加磷脂(asolectin 0,2%)可以回收。用凝胶过滤法测定了这些位点的表观分子量(438和235 K道尔顿)。利用紫外光对[3H]5HT的光活化作用,对膜中的5HT1和5HT3位点进行了不可逆标记。紫外线照射后[3H]5HT的结合在稀释后不解离;它是饱和的,并由血清素能药物而不是肾上腺素能或多巴胺能拮抗剂阻止。此外,在辐照前添加的GTP显著降低了5HT1位点,从而表明5HT1位点被标记。标记材料的电泳和荧光分析证明了60 K道尔顿带,专门标记为[3H]5HT(5或20 nM)。这些结果倾向于表明60k道尔顿蛋白带可能代表构成5HT1和5HT3位点一部分的蛋白质亚基。
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