大鼠中缝大核向脊髓投射神经元与神经降压素能终末的突触联系

神经降压素(NT)是中枢下行抑制系统的重要神经活性物质。本研究运用免疫组织化学与逆行追踪法相结合的双标技术,在电镜下观察NT能终末与中缝大核(NRM)向脊髓投射神经元的突触联系。在光镜下可见NT阳性纤维和终末散在分布于NRM,但未见NT阳性神经元;将HRP注入腰髓背角后,在NRM内可见比较密集的HRP逆标神经元。在电镜下可见NT阳性终末与HRP逆标神经元的胞体和树突形成以非对称性为主的轴-体突触和轴-树突触。上述结果说明NT可能调控NRM向脊髓背角投射神经元的活动,借此对伤害性信息向中枢的传递发挥抑制效应。     

Ciliated neurons in supraoptic nucleus of rat hypothalamus during neonatal period

Summary Cilia 9+0 have been found in differentiating neurosecretory neurons of the hypothalamic supraoptic nuclei of Wistar rats. These ciliated neurosecretory cells were always observed during the neonatal period of the rat and no more than one cilium per cell has been encountered.Single cilia arising from typical basal bodies were usually located in deep invaginations of the neuronal perikaryon, but can also be seen in superficial positions. Their basal bodies were commonly found in the vicinity of Golgi complexes, and associated structures such as striated rootlets and alar sheets were also present. In addition, single centrioles frequently appeared in these neurons, occurring close to basal bodies but also in centrosomatic areas.The respective roles of these morphological features are suggested and their possible ontogenetic significance is briefly discussed.     

Neurogenesis of GABAergic neurons in the rat dentate gyrus: a combined autoradiographic and immunocytochemical study

Neurogenesis of GABAergic neurons in the rat area dentata was studied combining [3H]thymidine autoradiography with immunostaining for glutamate decarboxylase (GAD), the gamma-aminobutyric acid (GABA) synthesizing enzyme. GAD immunocytochemistry stained many neurons located mainly in the hilar region but also in the granular and molecular layers. Granule cells were not immunoreactive. On embryonic day (E) 14, [3H]thymidine injection labelled 12.8% of GAD-positive (+) neurons in sections of the area dentata processed at an age of 40 days postnatally. This proportion decreased to 1.8% on E17 and to 1% on E18. No GAD (+) neurons were labelled by thymidine injection on E19, while non-immunoreactive granule cells and CA4 pyramids were still labelled, indicating persisting neurogenesis of those cells.     

Ultrastructural studies of medullary synaptic inputs to vasopressin-immunoreactive neurons in the supraoptic nucleus of the rat hypothalamus.

Direct projections from the A1/C1 catecholaminergic cell group in the caudal ventrolateral medulla oblongata to neurons containing vasopressin (VP) in the supraoptic nucleus (SON) were studied electron microscopically by a double-labeling technique which combines anterograde tracing after injection of wheat germ agglutinin-conjugated horseradish peroxidase (WGA-HRP) into the A1/C1 cell group with VP immunocytochemistry. WGA-HRP-labeled axon terminals originating from neurons in the A1/C1 cell group were found to make synaptic contacts with VP-immunoreactive cell bodies and dendrites in the SON, most often forming axo-dendritic synapses. This indicates that VP-containing neurosecretory neurons in the SON receive monosynaptic catecholaminergic input from the A1/C1 cell group.     

电刺激大鼠小脑顶核对下丘脑神经元放电活动的影响

目的:研究电刺激小脑顶核(fastigial nucleus,FN)及微电泳Glu(glutamic acid)、MK-801对大鼠下丘脑(hypothalamus,HT)神经元自发放电活动的影响,探讨电刺激FN治疗脑卒中大鼠的机制。方法:应用细胞外记录的方法,记录电刺激FN及微电泳药物对HT神经元放电的影响。结果:电刺激频率为20Hz(低频)时,50%的HT神经元的放电频率增高(P0.01),电刺激频率为100Hz(高频时),80%的HT神经元的放电频率增高(P0.01);Glu对HT有紧张性兴奋作用,其拮抗剂MK-801能够明显抑制Glu诱致的兴奋作用;70%HT神经元在微电泳MK-801的基础上进行100Hz电刺激FN时,高频刺激诱发的兴奋作用被明显削弱。结论:采用电刺激FN治疗脑卒中,其可能机制是通过Glu的兴奋作用来调节HT的异常活动。     

糖尿病大鼠下丘脑视上核nNOS免疫阳性神经元的变化

目的：观察糖尿病大鼠下丘脑视上核神经元型一氧化氮合酶(nNOS)免疫阳性神经元数量的变化。方法：用链脲佐菌素诱导建立糖尿病大鼠模型;免疫细胞化学染色显示nNOS免疫阳性神经元,并进行定量分析。结果：糖尿病视上核nNOS免疫阳性神经元着色深浅不一,着色较深的阳性神经元散在分布,神经元的形态多样,突起较少。对照组大鼠视上核nNOS免疫阳性神经元较稀疏,各时期无明显改变。糖尿病2w,nNOS免疫阳性神经元数量与对照组无显著差异;7w,nNOS阳性神经元较密集,明显多于对照组;12w,nNOS免疫阳性神经元数量略低于7w,但仍多于对照组。结论：糖尿病大鼠下丘脑视上核nNOS免疫阳性神经元数量明显增多。     

Localization of the spinal nucleus of accessory nerve in rat: a horseradish peroxidase study

The spinal nucleus of the accessory nerve (SNA) comprises the group of somata (perikarya) of motor neurons that supply the sternocleidomastoid and trapezius muscles. There are many conflicting views regarding the longitudinal extent and topography of the SNA, even in the same species, and these disagreements prompted the present investigation. Thirty Sprague-Dawley rats (15 males, 15 females) were used. The SNA was localized by retrograde axonal transport of horseradish peroxidase. Longitudinally, the SNA was found to be located in the caudal part (caudal 0.9-1.2 mm) of the medulla oblongata, the whole lengths of cervical spinal cord segments C1, C2, C3, C4, C5 and rostral fourth of C6. In the caudal part of the medulla oblongata, the SNA was represented by a group of perikarya of motor neurons lying immediately ventrolateral to the pyramidal fibres that were passing dorsolaterally after their decussation. In the spinal cord, the motor neuronal somata of the SNA were located in the dorsomedial and central columns at C1, in the dorsomedial, central and ventrolateral columns at C2 and in the ventrolateral column only at C3, C4, C5 and rostral quarter of C6. The perikarya of motor neurons supplying the sternocleidomastoid were located in the caudal part (caudal 0.9-1.2 mm) of the medulla oblongata ventrolateral to the pyramidal fibres that were passing dorsolaterally after their decussation. They were also located in the dorsomedial and central columns at C1, in the dorsomedial, central and ventrolateral columns at C2 and only in the ventrolateral column at the rostral three-quarters of C3. The perikarya of motor neurons supplying the trapezius muscle were located in the ventrolateral column only in the caudal three-quarters of C2, the whole lengths of C3, C4 and C5, and in the rostral quarter of C6.     

Activity-dependent synaptic plasticity in the supraoptic nucleus of the rat hypothalamus

Activity-dependent long-term synaptic changes were investigated at glutamatergic synapses in the supraoptic nucleus (SON) of the rat hypothalamus. In acute hypothalamic slices, high frequency stimulation (HFS) of afferent fibres caused long-term potentiation (LTP) of the amplitude of AMPA receptor-mediated excitatory postsynaptic currents (EPSCs) recorded with the whole-cell patch-clamp technique. LTP was also obtained in response to membrane depolarization paired with mild afferent stimulation. On the other hand, stimulating the inputs at 5 Hz for 3 min at resting membrane potential caused long-term depression (LTD) of excitatory transmission in the SON. These forms of synaptic plasticity required the activation of NMDA receptors since they were abolished in the presence of d -AP5 or ifenprodil, two selective blockers of these receptors. Analysis of paired-pulse facilitation and trial-to-trial variability indicated that LTP and LTD were not associated with changes in the probability of transmitter release, thereby suggesting that the locus of expression of these phenomena was postsynaptic. Using sharp microelectrode recordings in a hypothalamic explant preparation, we found that HFS also generates LTP at functionally defined glutamatergic synapses formed between the organum vasculosum lamina terminalis and SON neurons. Taken together, our findings indicate that glutamatergic synapses in the SON exhibit activity-dependent long-term synaptic changes similar to those prevailing in other brain areas. Such forms of plasticity could play an important role in the context of physiological responses, like dehydration or lactation, where the activity of presynaptic glutamatergic neurons is strongly increased.     

Effect of male sex hormones on specific uptake and release of3H-serotonin by the rat hypothalamus in vitro

Laboratory of Hormonal Regulation, N. K. Kol'tsov Institute of Developmental Biology, Russian Academy of Medical Sciences, Moscow. (Presented by Academician of the Russian Academy of Medical Sciences A. P. Avtsyn.) Translated from Byulleten' Éksperimental'noi Biologii i Meditsiny, Vol. 113, No. 6, pp. 653–655, June, 1992.     

Vasoactive intestinal polypeptide (VIP)-containing neurons in the spinal cord of the rat and their projections

The distribution of vasoactive intestinal polypeptide (VIP)-like immunoreactive structures in the rat spinal cord and their projections were investigated by means of an immunofluorescent method. In the normal rat, a small number of VIP-positive fibers were observed in the superficial layer of the dorsal horn and in the lateral funiculus. With colchicine pretreatment, VIP-positive neurons were demonstrated in the lateral spinal nucleus (lsn) and in the lamina X (Rexed). Transections of the spinal cord at various levels revealed that some of the VIP neurons in the lsn might project to supraspinal areas via lateral funiculus.     

新生大鼠脊髓少突胶质细胞体外培养与鉴定

本研究探索利用新生大鼠脊髓培养和纯化少突胶质细胞的方法。取新生大鼠全脊髓,胰酶消化并吹打分散细胞,用含20％胎牛血清的DMEM培养液原代混合细胞培养,细胞铺满瓶底后传代培养。用抗半乳糖脑苷脂抗体和抗胶质原纤维酸性蛋白抗体进行细胞分类免疫组化鉴定。结果显示:少突胶质细胞纯度可达98％以上,表明新生大鼠脊髓是少突胶质细胞体外培养的理想取材部位。本操作简单易行,可以在短时间内获得足量的纯化的少突胶质细胞。     

Magnocellular tuberomammillary nucleus input to the supraoptic nucleus in the rat: anatomical and in vitro electrophysiological investigations

Anatomical and electrophysiological methods were used to investigate the existence and role of inputs from the magnocellular tuberomammillary nucleus to the supraoptic nucleus. After injecting either Fluoro-Gold or rhodamine-labeled latex microspheres into the supraoptic nucleus, consistent patterns of retrogradely labeled neurons within the tuberomammillary nucleus were observed. The results indicate that both subdivisions of the supraoptic nucleus, the tuberal and the anterior, receive input from the tuberomammillary nucleus. Injections into the tuberal supraoptic nucleus tended to label more cells in the contralateral tuberomammillary nucleus, while injections into the anterior supraoptic nucleus may label more cells on the ipsilateral side. The in vitro intracellular electrophysiological results support the anatomical findings and extend them in several ways. Some tuberomammillary neurons were found to project to the supraoptic nuclei on both sides of the brain. Intracellular Lucifer Yellow injections into tuberomammillary cells after electrophysiological recording revealed labeled axons that were traceable into the supraoptic nucleus, where apparent varicosities (possible en passant terminals) were seen. Magnocellular tuberomammillary nucleus neurons had characteristic passive and active membrane properties and morphology, similar to histaminergic neurons in this area studied by other workers. Finally, in two of the 21 cases, Lucifer Yellow injection into one neuron revealed dye-coupled pairs of tuberomammillary neurons. Previous work by others has shown that histamine excited cells in the tuberal subdivision of the supraoptic nucleus, stimulating vasopressin release, and that the tuberomammillary nucleus provides histaminergic input to the anterior portion of the supraoptic. The present findings show that the tuberomammillary nucleus supplies input to both subdivisions of the supraoptic nucleus and that this input is provided bilaterally. Taken together with previous work, these data suggest that the tuberomammillary nucleus provides histaminergic input to the supraoptic nucleus and may be involved specifically with vasopressin release.     

Nitric oxide modulates the firing rate of the rat supraoptic magnocellular neurons

In vitro, nitric oxide (NO) inhibits the firing rate of magnocellular neurosecretory cells (MNCs) of hypothalamic supraoptic and paraventricular nuclei and this effect has been attributed to GABAergic activation. However, little is known about the direct effects of NO in MNCs. We used the patch-clamp technique to verify the effect of l-arginine, a precursor for NO synthesis, and N(omega)-nitro-l-arginine methyl ester hydrochloride (l-NAME), an inhibitor of NOS, on spontaneous electrical activity of MNCs after glutamatergic and GABAergic blockade in Wistar rat brain slices. 6-Cyano-7-nitroquinoxaline-2,3-dione (CNQX) (10 muM) and dl-2-amino-5-phosphonovaleric acid (dl-AP5) (30 muM) were used to block postsynaptic glutamatergic currents, and picrotoxin (30 muM) and saclofen (30 muM) to block ionotropic and metabotropic postsynaptic GABAergic currents. Under these conditions, 500 muM l-arginine decreased the firing rate from 3.7+/-0.6 Hz to 1.3+/-0.3 Hz. Conversely, 100 muM l-NAME increased the firing rate from 3.0+/-0.3 Hz to 5.8+/-0.4 Hz. All points histogram analysis showed changes in resting potential from -58.1+/-0.8 mV to -62.2+/-1.1 mV in the presence of l-arginine and from -59.8+/-0.7 mV to -56.9+/-0.8 mV by l-NAME. Despite the nitrergic modulator effect on firing rate, some MNCs had no significant changes in their resting potential. In those neurons, hyperpolarizing after-potential (HAP) amplitude increased from 12.4+/-1.2 mV to 16.8+/-0.7 mV by l-arginine, but without significant changes by l-NAME treatment. To our knowledge, this is the first demonstration that NO can inhibit MNCs independent of GABAergic inputs. Further, our results point to HAP as a potential site for nitrergic modulation.     

Ca++-dependent serotonin secretion from the rat hypothalamus during ontogeny

Laboratory of Hormonal Regulation, N. K. Kol'tsov Institute of Developmental Biology, Academy of Sciences of the USSR, Moscow. (Presented by Academician of the Academy of Medical Sciences of the USSR V. N. Orekhovich.) Translated from Byulleten' Éksperimental'noi Biologii i Meditsiny, Vol. 108, No. 8, pp. 166–169, August, 1989.     

Noradrenergic innervation of vasopression-containing neurons in the rat hypothalamic supraoptic nucleus

The noradrenergic innervation of vasopressin (VP)-containing neurons in the supraoptic nucleus (SON) of the rat hypothalamus was studied electron microscopically by using double-labeling immunocytochemistry combining the pre-embedding peroxidase-anti-peroxidase method with post-embedding immunocolloidal gold staining. Noradrenaline-like immunoreactive axon terminals were found to make synaptic contacts with neurophysin II-like immunoreactive neurons in the SON. This study provides morphological evidence for noradrenergic control of neuronal activity of VP-containing neurons at the SON level.     

不同神经示踪剂组合对大鼠脊髓运动神经元的逆行标记效率比较

目的:探讨神经示踪剂荧光金(FG)、真蓝(TB)和荧光红(FR)两两组合对脊髓运动神经元的标记效率差异,为再生神经重支配准确性研究奠定基础.方法;采用大鼠胫神经示踪模型,采取神经内注射与神经横断后近侧断端浸泡(20 min)2种方式,分别对FG、TB和FR的两两组合进行示踪试验.示踪术后5d,取脊髓腰膨大段冷冻纵切,共聚焦显微镜进行显微成像和计数.结果:FG联合TB示踪标记的运动神经元数量最多,其次为FG联合FR,而FR联合TB组标记细胞数最少,双标比例也最小.神经断端浸泡方式使用示踪剂时标记效率仅为神经内注射的2/3左右.结论:FG联合TB以及FG联合FR示踪对脊髓运动神经元的标记效果较好,且神经内注射使用示踪剂效果优于持续20 min的神经断端浸泡.     

Enzyme-histochemical studies on the nonsecretory neurons of the rat supraoptic nucleus with the application of karyometry and electronmicroscopy

Detailed histochemical studies were conducted on the distribution of SDH, G6PD, and TPPase as well as the Nissl substance and Gomori-positive material in the nonsecretory neurons of the supraoptic nucleus (SO) of the adult Wistar strain rats. Karyometry and statistical analysis were performed to identify those neurons. Electron microscopy confirmed the cytological characteristics indicated by the histochemical results. Based on the classification of SO neurons by the Golgi-Cox method and the present results concerning the Nissl pattern, shape, size, and number, these nonsecretory neurons appear to be intercalated neurons. Weak SDH and G6PD activity in the perikaryon with a few mitochondria indicate that they belong to the category of ordinary neurons with a low level of carbohydrate metabolism. The TPPase reaction revealed heterogeneous Golgi apparatus (GA) with poor development. In addition, it was difficult to find profiles of GA in many ultrathin sections. These results indicate that the GA may not undergo cyclic activity and lacks the capacity for secretion. No Gomori-positive material was detected in the perikaryon, whereas the Nissl substance was densely distributed throughout the entire perikaryon, where many free ribosomal rosettes and junctions of cisternae of abundant granular reticulum were evenly dispersed. The nonsecretory neurons reflect an active phase of cyclic activity of protein synthesis. However, other nonsecretory neurons with less active protein synthesis are very likely to be present.     

Somatotopic organization of lumbar muscle-innervating neurons in the ventral horn of the rat spinal cord

The ventral horn of the rat spinal cord was investigated with respect to the somatotopic organization of the motor neurons that innervate the lumbar muscles. Neurotracer 1,1′‐dioctadecyl‐3,3,3′,3′‐tetramethylindocarbocyanine perchlorate (DiI) was applied to specific sites in lumbar muscles. Spinal cord segments at L1 through L4 levels were cut into 40‐μm serial transverse sections. Labeled neurons were located in the ventromedial nucleus (VM) and lateromedial nucleus (LM) nuclei of Rexed’s lamina IX. Motor neurons innervating the m. interspinales lumborum and m. multifidus were without exception present in the VM, whereas all motor neurons innervating the m. rectus abdominis were present in the LM. Forty percent of motor neurons innervating the m. quadratus lumborum were present in the VM and the other 60% were in the LM. Although most of the motor neurons innervating the m. psoas major were present in the LM, a few labeled neurons existed in the VM. These results suggest that the border zone demarcating the areas of innervation of the dorsal and ventral rami of spinal nerves crosses the m. quadratus lumborum.     

Light and electron microscopic localization of glutamate immunoreactivity in the supraoptic nucleus of the rat hypothalamus

The distribution of glutamate immunoreactivity was mapped within the supraoptic nucleus of the rat hypothalamus utilizing a specific anti-glutamate antibody. Magnocellular neuroendocrine cells of the supraoptic nucleus showed intense immunoreactivity for glutamate which varied with the conditions of fixation. Within the perikarya, reaction product was found associated with the endoplasmic reticulum but not the mitochondria, Golgi, dense bodies or neurosecretory granules. A relatively high density of glutamate-immunoreactive terminals was found in the supraoptic nucleus. These terminals were less affected by fixation condition and were generally found contacting large, glutamate-immunoreactive processes within the ventral dendritic neuropil of the supraoptic nucleus. The pattern and characteristics of glutamate immunoreactivity in the supraoptic nucleus suggested the presence of two distinct glutamate pools. The magnocellular neuroendocrine cells may contain a large, labile metabolic pool of glutamate. These cells, in turn, appear to receive glutamate synaptic input from a more stable pool consistent with suggestions that glutamate may be used as a transmitter within this system.     

Possible morphological bases for synchronisation of neuronal firing in the rat supraoptic nucleus during lactation

Oxytocin-containing neurones in the supraoptic and paraventricular nuclei of lactating rats display a periodic activation which results in a pulsatile release of hormone before each reflex milk ejection induced by suckling. This electrical activity occurs in an all-or-none fashion and is synchronised in the whole population of oxytocin neurones in both nuclei. The present report describes changes in the ultrastructure of the supraoptic nucleus of lactating animals which may serve as morphological bases for such a functional synchronisation.In the supraoptic nuclei of normal rats, neurosecretory neurones are usually separated by elements of the neuropil, particularly glial processes. At rare intervals, adjacent neurosecretory somata, and dendrites, are seen to be in direct apposition. The only specialisations apparent between the contiguous membranes are occasional attachment plates. In nuclei of lactating rats, quantitative analysis indicated that 34% of profiles of the sectioned neurosecretory cell bodies were in direct contact with each other and 22% with profiles of dendrites, a 5-fold increase over the corresponding frequencies observed in normal male and virgin female animals. Such contacts involved 10% of the total measured soma surface membrane (compared to 1.5% in the controls). The number of attachment plates supporting the apposing membranes also increased significantly as did the mean size of the individual appositions. There was also a higher incidence of presynaptic terminals contacting more than one post-synaptic element (soma or dendrite) in the same plane of section, a rare phenomenon in the normal nucleus. No further increases were evident in these appositional relations in virgin female and lactating rats deprived of water for one day, a stimulus which enhances vasopressin release.It is postulated that the structural reorganisation observed in the nuclei of lactating animals may lead to electrical interactions between the neurosecretory cells and may thus be one of the factors supporting the synchronisation of neuronal activity during the episodic release of oxytocin.