大鼠腹后外侧核和相关丘脑网状核的内在组织:γ -氨基丁酸免疫金染色和凝集素偶联的辣根过氧化物酶双标记超微结构研究。

S De Biasi, C Frassoni, R Spreafico
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引用次数: 65

摘要

用电镜观察了大鼠腹后外侧核(VPL)和与体感丘脑核相关的网状丘脑核(RTN)区域的突触组织。将小麦胚芽凝集素结合辣根过氧化物酶(WGA:HRP)注射于大鼠皮层第一体感区(SI)或背柱核(DCN)。以对苯二胺-邻苯二酚(PPD-PC)为底物,观察逆行和/或顺行转运酶。在第二个系列的六个实验中,采用了一种使用特异性抗-氨基丁酸(抗- gaba)的免疫细胞化学程序。用胶体金免疫染色法对GABA包埋后定位进行超微结构观察。对注射WGA: hrp的动物的识别的VPL和RTN区域的薄片进行进一步的免疫细胞化学处理,以便在电子显微镜水平上同时定位转运酶和GABA。结果表明,来自DCN的hrp标记的末梢与VPL神经元的体细胞和近端树突接触,而SI皮质注射后标记的末梢主要位于树突的远端。同样的皮质注射也确定了与胞体接触的标记突触钮扣的存在,以及RTN神经元的近端和远端树突。与其他方法相比,在VPL中观察到的gaba免疫标记的末端数量更多,因为不仅标记了典型的F末端,而且还标记了含有圆形和/或多形性囊泡的末端。gaba能终端与VPL神经元的体细胞和近端树突接触,而在RTN细胞中主要与体细胞和近端树突进行突触接触。在双标记实验中,未观察到含有HRP和特异性免疫金GABA染色的末端。目前的数据直接证明了RTN对VPL神经元的强抑制输入的存在,以及RTN神经元中存在的自抑制。
本文章由计算机程序翻译,如有差异,请以英文原文为准。
The intrinsic organization of the ventroposterolateral nucleus and related reticular thalamic nucleus of the rat: a double-labeling ultrastructural investigation with gamma-aminobutyric acid immunogold staining and lectin-conjugated horseradish peroxidase.

An electron-microscopic investigation of the synaptic organization of the rat's ventroposterolateral nucleus (VPL) and of a reticular thalamic nucleus (RTN) area related to somatosensory thalamic nucleus was performed. In a group of 11 rats, wheatgerm agglutinin conjugated to horseradish peroxidase (WGA:HRP) was injected either in the first somatosensory area of cortex (SI) or in the dorsal column nuclei (DCN). The retrogradely and/or anterogradely transported enzyme was visualized using paraphenylenediamine-pyrocatechol (PPD-PC) as substrate. In a second series of six experiments, an immunocytochemical procedure using a specific anti-gamma-aminobutyric acid (anti-GABA) was employed. Postembedding localization of GABA was performed for ultrastructural observation by means of the colloidal gold immunostaining procedure. Thin sections of recognized VPL and RTN areas from WGA:HRP-injected animals were further processed for immunocytochemistry in order to localize simultaneously, at the electron-microscopic level, the transported enzyme and GABA. The results obtained with this procedure demonstrated that HRP-labeled terminals from DCN contacted the soma and proximal dendrites of VPL neurons, while the terminals labeled after SI cortical injections were predominantly localized to the distal portion of the dendrites. The same cortical injection also determined the presence of labeled synaptic boutons contacting the soma, and both proximal and distal dendrites of RTN neurons. GABA-immunolabeled terminals were observed in VPL in a number larger than those observed with other methods, since not only typical F terminals were labeled but also terminals containing round and/or pleomorphic vesicles. GABA-ergic terminals contacted the soma and the proximal and distal dendrites of VPL neurons, while in RTN cells they made synaptic contact mainly with the soma and proximal dendrites. In the double-labeling experiments, terminals containing both HRP and specific immunogold GABA staining were never observed. The present data provide a direct demonstration of the presence of a strong inhibitory input from RTN upon VPL neurons and of the existence of autoinhibition within RTN neurons.

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