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大鼠脑中血管活性肠肽受体的特性与分布

Properties and distribution of vasoactive intestinal polypeptide receptors in the rat brain.

作者信息

Ogawa N, Mizuno S, Mori A, Nukina I, Yanaihara N

出版信息

Peptides. 1985;6 Suppl 1:103-9. doi: 10.1016/0196-9781(85)90017-8.

DOI:10.1016/0196-9781(85)90017-8
PMID:2995938
Abstract

Vasoactive intestinal polypeptide (VIP) interaction with the rat brain synaptic membrane was examined using 125I-labeled VIP as a tracer molecule. Ion, pH and incubation time significantly influenced VIP receptor binding. Scatchard analysis suggested that the rat brain membrane had a single binding site with an apparent dissociation constant (Kd) of 9.8 X 10(-9) M. The receptor activity was sensitive to trypsin and phospholipase A digestion, and heating at 100 degrees C for 5 min completely destroyed the binding activity. This indicates that protein and phospholipid moieties are essential for VIP binding. Thiol reagents reduced receptor binding activity, suggesting that an intrachain disulfide bond might be an important constituent of the VIP binding site. High levels of binding were found in the hippocampus, striatum and cerebral cortex, and binding was very low in the medulla/pons and cerebellum. The receptor density did not always parallel the brain distribution of immunoreactive VIP (IR-VIP) concentration. The cerebral cortex had the highest ratio of IR-VIP-to-receptor, and the striatum had the lowest ratio of IR-VIP-to receptor. Although intra-nigral or intra-striatal injection of 6-hydroxydopamine had no effect on striatal VIP-binding, an intra-striatal injection of kainic acid resulted in a substantial lowering of striatal VIP receptors. The neurotoxic effects of kainic acid have been shown to be dependent on the corticostriatal tract, and this suggests that the striatum receives the VIPergic innervation from the cerebral cortex. Our findings indicate that endogenous VIP and VIP receptors might act as a neurotransmission modulator of extrapyramidal function in the striatum.

摘要

以125I标记的血管活性肠肽(VIP)作为示踪分子,研究了其与大鼠脑突触膜的相互作用。离子、pH值和孵育时间对VIP受体结合有显著影响。Scatchard分析表明,大鼠脑膜有一个单一结合位点,其表观解离常数(Kd)为9.8×10(-9)M。受体活性对胰蛋白酶和磷脂酶A消化敏感,在100℃加热5分钟会完全破坏结合活性。这表明蛋白质和磷脂部分对VIP结合至关重要。硫醇试剂降低了受体结合活性,提示链内二硫键可能是VIP结合位点的重要组成部分。在海马、纹状体和大脑皮层中发现高水平的结合,而在延髓/脑桥和小脑中结合非常低。受体密度并不总是与免疫反应性VIP(IR-VIP)浓度的脑部分布平行。大脑皮层的IR-VIP与受体的比例最高,而纹状体的IR-VIP与受体的比例最低。虽然脑内注射6-羟基多巴胺对纹状体VIP结合没有影响,但脑内注射 kainic 酸会导致纹状体VIP受体大量减少。已证明kainic酸的神经毒性作用依赖于皮质纹状体束,这表明纹状体接受来自大脑皮层的VIP能神经支配。我们的研究结果表明,内源性VIP和VIP受体可能作为纹状体锥体外系功能的神经传递调节剂。

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