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通过非洲爪蟾卵母细胞中受控制的受体表达来测定亲和常数(KA)值。

Determination of KA values by controlled receptor expression in Xenopus oocytes.

作者信息

Murakoshi H, Nunoki K, Ishii K, Taira N

机构信息

Department of Pharmacology, Tohoku University School of Medicine, Sendai, Japan.

出版信息

Br J Pharmacol. 1995 Oct;116(3):2062-6. doi: 10.1111/j.1476-5381.1995.tb16412.x.

Abstract
  1. In the present study we estimated the KA value of endothelin-1 (ET-1) for ETA-receptors by a new method in which the level of expression of ETA-receptors in Xenopus oocytes was altered in a controlled way. 2. Kvl.2 (a delayed rectifier type K channel) c RNA at the fixed concentration of 0.2 micro g micro l(-1) was mixed with ETA-receptor cRNA at various concentration ratios (10(-3)-3). Oocytes were examined 2-4 days after the injection of the cRNA mixtures. 3. In these oocytes, ET-1 suppressed the amplitude of Kvl.2 current in a dose-dependent manner in the range of 0.1-100 nM; the maximum inhibition produced by ET-1 was larger and the EC50 value for the inhibition by ET-1 was smaller as the mixture ratio was increased. Double-reciprocal plots of equiactive concentrations of ET-1 in 1/1- and 1/30-injected oocytes yielded a KA for ET-1 of 7.4 nM. The number of ETA-receptors in 1/30-injected oocytes was 13% of that in 1/1-injected oocytes, whereas the inhibition of the current in 1/30-injected oocytes was about 60% of that in 1/1-injected oocytes. This suggests the presence of spare receptors of ETA in the latter. 4. A saturation binding experiment estimated a KD value of 0.1 nM for ET-1 at ETA-receptors and the number of ETA-receptors in 1/30-injected oocytes was 23% of that in 1/1-injected ones. This value was not significantly different from that estimated by the above new method. However, there was a discrepancy between KA and KD, which could be due to factors unique to the expression system employed in the present study.
摘要
  1. 在本研究中,我们通过一种新方法估计了内皮素 -1(ET -1)对ETA受体的KA值,该方法可控制非洲爪蟾卵母细胞中ETA受体的表达水平。2. 将固定浓度为0.2μg/μl(-1)的Kvl.2(一种延迟整流型钾通道)cRNA与不同浓度比(10(-3)-3)的ETA受体cRNA混合。在注射cRNA混合物2 - 4天后检查卵母细胞。3. 在这些卵母细胞中,ET -1在0.1 - 100 nM范围内以剂量依赖性方式抑制Kvl.2电流;随着混合比例增加,ET -1产生的最大抑制作用更大,ET -1抑制的EC50值更小。对1/1和1/30注射卵母细胞中ET -1等效活性浓度的双倒数作图得出ET -1的KA为7.4 nM。1/30注射卵母细胞中ETA受体的数量是1/1注射卵母细胞中的13%,而1/30注射卵母细胞中电流的抑制约为1/1注射卵母细胞中的60%。这表明后者中存在ETA的备用受体。4. 饱和结合实验估计ET -1在ETA受体处的KD值为0.1 nM,1/30注射卵母细胞中ETA受体的数量是1/1注射卵母细胞中的23%。该值与上述新方法估计的值无显著差异。然而,KA和KD之间存在差异,这可能是由于本研究中使用的表达系统所特有的因素。

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本文引用的文献

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Br J Pharmacol Chemother. 1956 Dec;11(4):379-93. doi: 10.1111/j.1476-5381.1956.tb00006.x.
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Proc R Soc Lond B Biol Sci. 1983 Dec 22;220(1219):141-62. doi: 10.1098/rspb.1983.0093.

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