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神经激肽3受体在视上核加压素和催产素神经元中的作用。

Role of neurokinin 3 receptors in supraoptic vasopressin and oxytocin neurons.

作者信息

Howe Heather E, Somponpun Suwit J, Sladek Celia D

机构信息

Department of Physiology and Biophysics, University of Colorado Health Sciences Center, Denver, Colorado 80262, USA.

出版信息

J Neurosci. 2004 Nov 10;24(45):10103-10. doi: 10.1523/JNEUROSCI.3164-04.2004.

Abstract

Neurokinin 3 receptors (NK3-Rs) are expressed in the supraoptic nucleus (SON), and SON is innervated by substance P (SP)-expressing A1 neurons in the medulla. Because SP stimulates vasopressin (VP) and oxytocin release from explants of the hypothalamo-neurohypophyseal system (HNS), two hypotheses were tested: (1) SP-stimulated VP release is mediated by NK3-Rs, and (2) stimulation of the A1 pathway by hypotension activates SON NK3-Rs. Senktide, an NK3-R agonist, stimulated VP release from HNS explants, but neither a neurokinin 1 receptor antagonist [L732,138 (N-acetyl-L-tryptophan 3,5-bis(tri-fluoromethyl)benzyl ester)] nor two NK3-R antagonists (SB222200 and SB235375) prevented SP-stimulated VP release. Because the affinity of these antagonists for rat NK-Rs may limit their efficacy, NK3-R internalization was used to assess the ability of SP to activate SON NK3-Rs. Senktide, SP, or vehicle was microinjected above SON. The brain was perfused 5 min after injection and stained for NK3-R immunoreactivity. Using confocal microscopy, the number of NK3-R-immunoreactive (-IR) endosomes was counted in a 5.6(2) mu region of cytoplasm in SON neurons. Senktide, but not SP or vehicle, significantly increased the number of NK3-R-IR endosomes in the cytoplasm. When hypotension was induced with hydralazine, NK3-R internalization was observed within 5 min (p < 0.005). A decrease in cytoplasmic NK3-R immunoreactivity was observed within 15 min of hypotension. Unexpectedly, both senktide and hypotension resulted in translocation of NK3-R-IR immunoreactivity to the nucleus. Thus, although these studies do not identify SP as the NK3-R ligand, they do provide evidence for hypotension-induced release of an endogenous tachykinin in SON and evidence suggesting a role for NK3-Rs in transcription regulation.

摘要

神经激肽3受体(NK3-Rs)在下丘脑视上核(SON)中表达,并且延髓中表达P物质(SP)的A1神经元支配视上核。由于SP刺激下丘脑-神经垂体系统(HNS)外植体释放血管加压素(VP)和催产素,因此对两个假说进行了验证:(1)SP刺激的VP释放由NK3-Rs介导,以及(2)低血压对A1通路的刺激激活视上核NK3-Rs。NK3-R激动剂senktide刺激HNS外植体释放VP,但神经激肽1受体拮抗剂[L732,138(N-乙酰-L-色氨酸3,5-双(三氟甲基)苄酯)]和两种NK3-R拮抗剂(SB222200和SB235375)均不能阻止SP刺激的VP释放。由于这些拮抗剂对大鼠NK-Rs的亲和力可能会限制其效力,因此使用NK3-R内化来评估SP激活视上核NK3-Rs的能力。将senktide、SP或赋形剂微量注射到视上核上方。注射后5分钟对大脑进行灌注,并对NK3-R免疫反应性进行染色。使用共聚焦显微镜,在视上核神经元细胞质的5.6(2)μm区域内计数NK3-R免疫反应性(-IR)内体的数量。senktide可显著增加细胞质中NK3-R-IR内体的数量,而SP或赋形剂则无此作用。当用肼屈嗪诱导低血压时,5分钟内观察到NK3-R内化(p<0.005)。低血压15分钟内观察到细胞质中NK3-R免疫反应性降低。出乎意料的是,senktide和低血压均导致NK3-R-IR免疫反应性向细胞核移位。因此,尽管这些研究未将SP鉴定为NK3-R配体,但它们确实提供了低血压诱导视上核释放内源性速激肽的证据,以及表明NK3-Rs在转录调节中起作用的证据。

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