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血管紧张素II刺激下丘脑-脑干神经元培养物中去甲肾上腺素的摄取。

Angiotensin II stimulates norepinephrine uptake in hypothalamus-brain stem neuronal cultures.

作者信息

Sumners C, Raizada M K

出版信息

Am J Physiol. 1986 Feb;250(2 Pt 1):C236-44. doi: 10.1152/ajpcell.1986.250.2.C236.

DOI:10.1152/ajpcell.1986.250.2.C236
PMID:3513605
Abstract

In this study we have characterized the uptake of [3H]norepinephrine (NE) into neuronal co-cultures of rat hypothalamus and brain stem and have examined the effects of angiotensin II (ANG II) on this uptake. Neuronal co-cultures prepared from the brains of 1-day-old Sprague-Dawley (SD) or Wistar-Kyoto (WKY) rats exhibited sodium-dependent and sodium-independent portions of the total [3H]NE uptake. The sodium-dependent uptake was abolished by blockers such as maprotiline, desmethylimipramine, and xylamine (0.1-100 microM) and is presumably neuronal uptake. The sodium-independent uptake was unaffected by these drugs and is presumably non-neuronal, since nonneuronal co-cultures from SD rats exhibited no significant sodium-dependent or blocker-sensitive uptake. In SD or WKY neuronal co-cultures, ANG II (0.1 nM-10 microM) caused increased [3H]NE uptake during short-term incubations (1-5 min). This stimulatory effect of ANG II was on neuronal NE uptake. Furthermore, it was inhibited by preincubation with saralasin (1-10 microM). Construction of saturation curves and kinetic analyses revealed that ANG II caused an increase in the maximal velocity of uptake of neuronal [3H]NE, but the affinity of the transporter for NE was not altered. With longer-term incubations (15-30 min), ANG II caused a reduction in neuronal [3H]NE uptake. This effect was also blocked by saralasin. However, reliable kinetic analysis was not possible with the longer-term incubations, and it is likely that the inhibitory action of the peptide represents a stimulation of NE release. Therefore, using neuronal co-cultures, we have identified a previously unseen stimulatory action of ANG II on neuronal [3H]NE uptake, which precedes the already documented inhibitory actions.

摘要

在本研究中,我们对[3H]去甲肾上腺素(NE)摄取到大鼠下丘脑和脑干的神经元共培养物中的情况进行了表征,并研究了血管紧张素II(ANG II)对这种摄取的影响。从1日龄的斯普拉格-道利(SD)或Wistar-Kyoto(WKY)大鼠的大脑制备的神经元共培养物表现出总[3H]NE摄取的钠依赖性和非钠依赖性部分。钠依赖性摄取被诸如马普替林、去甲丙咪嗪和二甲苯胺(0.1 - 100 microM)等阻滞剂所消除,推测为神经元摄取。非钠依赖性摄取不受这些药物影响,推测为非神经元摄取,因为来自SD大鼠的非神经元共培养物未表现出明显的钠依赖性或阻滞剂敏感性摄取。在SD或WKY神经元共培养物中(0.1 nM - 10 microM),ANG II在短期孵育(1 - 5分钟)期间导致[3H]NE摄取增加。ANG II的这种刺激作用是对神经元NE摄取的作用。此外,预先用沙拉新(1 - 10 microM)孵育可抑制这种作用。饱和曲线的构建和动力学分析表明,ANG II导致神经元[3H]NE摄取的最大速度增加,但转运体对NE的亲和力未改变。在较长时间孵育(15 - 30分钟)时,ANG II导致神经元[3H]NE摄取减少。这种作用也被沙拉新阻断。然而,较长时间孵育时无法进行可靠的动力学分析,并且该肽的抑制作用可能代表对NE释放的刺激。因此,使用神经元共培养物,我们发现了ANG II对神经元[3H]NE摄取的一种先前未见到的刺激作用,该作用先于已记录的抑制作用。

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