脊髓胶状质内生长抑素免疫反应阳性结构与一级传入纤维之间的突触连接

本文用单纯免疫电镜及免疫电镜与溃变(后根切断术)相结合的方法,研究了一级传入纤维与脊髓胶状质内生长抑素(SOM)阳性结构之间的突触连结。结果在脊髓胶状质内观察到SOM阳性的胞体、轴突、树突及溃变的轴突,以上结构间形成了几种不同类型的突触连结:(1)Ⅰ型或Ⅱ型突触球的中央成份(CⅠ或CⅡ末梢)是溃变的或是SOM免疫反应阳性的,它们与周围的树突形成轴树突触、轴轴突触或树轴突触,其中有一些周围的树突还是SOM阳性的。(2)某些简单的轴突(不参与构成突触球的轴突)呈暗型溃变,并与SOM阳性的树突形成轴树突触。(3)简单的SOM阳性的致密型轴突与含SOM的树突或核周质形成轴树或轴体突触。(4)简单的SOM阳性的亮型轴突与含SOM的树突形成轴树突触。这些突触关系提示脊髓胶状质内SOM阳性树突和胞体可直接从一级传入纤维或脊髓后角固有神经元接受冲动,其中有一些一级传入纤维和脊髓后角固有神经元也是SOM阳性的。这表明在脊髓固有神经元与一级传入纤维之间及脊髓固有神经元本身都存在着自调节突触。本实验结果为SOM参与感觉信息的调节提供了超微结构证据。     

大鼠粒细胞内质网的电镜细胞化学反应

本实验用电镜细胞化学方法观察了大鼠骨髓粒细胞发育过程中内质网的髓过氧化物酶(MPO)反应和葡萄糖-6-磷酸酶(G-6-P)反??应。结果表明:MPO除定位于内质网、核膜,还出现在高尔基体和颗粒,它是粒细胞内质网的合成产物。G-6-P只在内质网、核膜中出现,它是内质网膜的结构成分。MPO反应的超微结构定位随粒细胞发育而变,利用这种变化作标志可以划分不同发育阶段的粒细胞;G-6-P反应定位不随发育而变,但反应强度与内质网的多寡、功能状态相对应。实验还表明核膜与内质网在结构、功能上的一致性;尤其在成熟粒细胞内质网很少的情况下,核膜可能代替了内质网的功能。     

新疆医科大学基础医学院组织胚胎学教研室

目的:观察国人胚胎三叉神经节细胞分化及发育过程。方法:取水囊引产18-36周国人胎儿三叉神经节,HE染色及透射电镜观察。结果:18-20周胎儿三叉神经节神经元排列紧密,胞质少,可见到数量不多的线粒体,且其内几乎看不到嵴,其它细胞器少。25周时,线粒体嵴变长,粗面内质网雏形出现,有纵形小管出现;27周时可观察到成熟的高尔基复合体,32周后,线粒体、粗面内质网等细胞器发育趋于成熟。到33周电镜下可见溶酶体;36周时细胞内各种细胞器结构和功能基本完善。结论:人胚胎三叉神经节细胞发育过程中随胎龄增加,其结构和功能逐步完善,32～36周(8～9月)是细胞的分化发育重要时期。     

6-OHDA制备的帕金森病大鼠黑质神经元的超微结构改变

目的观察6-羟多巴胺(6-OHDA)单侧注射制备的帕金森病(PD)大鼠多巴胺(DA)能神经元的超微结构改变。方法单侧微量注射6-OHDA制备PD大鼠模型,用免疫荧光组织化学方法观察正常侧与6-OHDA注射侧黑质酪氨酸羟化酶(TH)阳性神经细胞及神经纤维的变化;并利用免疫电镜技术观察大鼠正常侧与注射侧黑质致密部DA能神经元的超微结构。结果免疫荧光法显示注射侧黑质致密部TH阳性细胞数和网状部TH阳性纤维面积与正常侧的百分比平均值分别为21.83%,23.19%。免疫电镜显示:TH免疫反应阳性产物表达于PD大鼠正常侧DA能神经元的高尔基复合体质膜面及胞质内,电子密度较高,注射侧很少见或几乎未见,且注射侧线粒体嵴有不同程度的溶解,呈空泡样变或髓样变,粗面内质网脱颗粒。结论6-OHDA可引起DA能神经元发生凋亡的超微结构改变。     

脊髓背角深层痛敏神经元与胶质层SP,Clu和GABA能末梢的突触联系

应用整体猫单细胞生理特性鉴定和细胞内注射辣根过氧化物酶标记法,显示了一些脊髓背角深层广动力范围型痛敏神经元有背侧树突延伸至背角浅层.并结合包埋后免疫,电镜显示这种神经元可通过分布于背角胶质层的树突接受大量P物质和谷氨酸免疫反应阳性纤维末梢的支配.由于后者主要来源于C类纤维,由此可以推测在背角浅层C类纤维介导的部分痛信息,可直接以单突触方式转送至背角深层的痛敏神经元.背角浅层的GABA免疫反应阳性轴突可与标记的远端树突形成突触,支持通过突触后抑制对脊髓痛觉传递发挥调制作用.     

玉米幼苗根不同发育区细胞中高尔基体的变化

玉米根细胞的三个发育区——分裂区、延伸区和成熟区高尔基体的变化:分裂区先由部分内质网碎片转化为潴泡,再由潴泡叠加构成具六个潴泡结构的高尔基器;延伸区高尔基器进行大量合成分泌物质,使大部分潴泡变成分泌泡而排出细胞外,导致高尔基器大量减少;成熟区高尔基器相当少,分泌能力一般。     

猫丘脑腹后外侧核的超微结构

采用电镜技术观察了猫丘脑腹后外侧核的超微结构。该核内的神经元可分为大小两种类型，大型直径在１５—４０μｍ，小型小于１５μｍ，其胞质内容无明显差别。树突较多见，直径从１—１０μｍ不等。轴突可分为三种类型：含圆形小泡的小终末、终末及扁平小泡的终末。突触类型主要为轴树突触，此外还可见到轴体、轴轴、轴轴树、树树突触以及以树突为中心的突触复合体。在树突之间、树突与胞体之间还存在有非突触的丝状连接。     

烫伤对大鼠下丘脑视上核、室旁核AVP神经元的影响──免疫电镜观察及形态计量分析

为研究加压素与应激的关系,我们曾应用免疫细胞化学（ＰＡＰ）方法结合图像分析技术观察到烫伤应激后２小时视上核、室旁核加压素神经元免疫反应阳性物质的总体积减小最明显。本文采用免疫电镜技术,进一步观察了烫伤后２小时视上核、室旁核加压素神经元超微结构的变化,并运用体视学方法定量分析了对照组及烫伤后２小时组视上核、室分校加压素神经元各２４０张照片的粗面内质网、高尔基复合体及线粒体的体积密度（Ｖｖ）、面积密度（Ｓｖ）、面数密度（Ｎａ）等。结果显示：烫伤后２小时组视上核、室旁核加压素神经元的粗面内质网的Ｖｖ．Ｓｖ显著增大,说明合成功能已开始增强,但是,高尔基复合体的Ｖｖ、Ｓｖ及阳性分泌颗粒却显著减少,因而引起总体积的缩小。从超微结构水平进一步证实加压素参与应激过程。     

豚鼠脊髓前角神经元线状溶酶体的电镜酶细胞化学研究

本研究采用电镜金属盐法──三偏磷酸酶（ＴＭＰａｓｅ）细胞化学方法探讨了豚鼠脊髓前角神经无线状溶酶体（ＮＬＹ）的存在及其酶细胞化学特点。ＴＭＰａｓｅ是港酶体的标志酶之一。本研究首次以偏磷酸钠代替三偏磷酸钠为ＴＭＰａｓｅ的底物,很好地显示了ＮＬＹ的结构。ＴＭＰａｓｅ反应产物虽高电子密度的黑色铅盐沉淀,不仅分布于圆形溶酶体,也可见于ＮＬＹ,同时,在高尔基复合体的部分板层也有酶活性分布,可能酶是经高尔基复合体加工后输送至溶酶体。ＮＬＹ在神经元胞体,突起及突触中均有分布,并且从胞体到神经终末均有ＮＬＹ和线粒体相贴现象,提示酶是由依赖于线粒体提供运动能量的ＮＬＹ从胞体输送到神经终末,这可能和ＮＬＹ参与神经递质的降解及神经元代谢物质的处理密切相关。     

大鼠脊髓胶状质内GABA能神经元突触联系的超微结构研究

本文用免疫电镜方法对脊髓胶状质内ＧＡＢＡ能神经元的突触联系进行了超微结构研究。结果表明;脊髓胶状质内有许多ＧＡＢＡ能神经元胞体和末梢分布;标记的ＧＡＢＡ能神经末梢可作为突触前成分与未标记的ＧＡＢＡ形成输一树突触。未标记的末梢可与标记的ＧＡＢＡ末梢形成输一轴突触。此外,标记的ＧＡＢＡ能神经末梢还可作为突触前成分与标记的ＧＡＢＡ能轴突、树突或胞体形成输－轴、轴－树或轴－体突触,即自调节突触。上述结果揭示：ＧＡＢＡ能末梢可对脊髓胶状质内其它神经元产生抑制或脱抑制作用。值得注意的是胶状质内含ＧＡｎＡ的神经结构可形成各种形式的自调节突触,并借此实现其对脊髓功能的复杂调节。     

内质网及其标志酶在离体培养脊髓神经元中的发育变化

In an attempt to elucidate the relationship between synapse formation and cell development, the morphology and cytochemistry of the endoplasmic reticulum and its enzymic marker, glucose-6-phosphatase (G-6-Pase), in cultured mouse spinal neurons were investigated ultrastructurally. It was found that in the early period of the development, neurons were characterized by scarceness of organelles; only a few of granular or agranular endoplasmic reticulum and mitochondria were seen. The endoplasmic reticulum and nuclear envelope were packed specifically with G-6-Pase resection product but the product was weak. After a period of culture, most of the neurons had well-developed endoplasmic reticulum, Golgi apparatus, mitochondria and microtubules, etc. The Golgi apparatus was relatively large, having some cisternae associated with vesicles. Either concave of convex face of the saccules was labeled by thiamine pyrophosphatase (TPPase) specifically. GERL, labeled by cytidine monophosphatase (CMPase), was also seen close to the inner or outer face of some Golgi apparatus. The endoplasmic reticulum at this stage was distributed throughout the cytoplasm, including that in dendrites; its enzyme marker (G-6-Pase) localized consistently within the lumen of all endoplasmic reticulum, nuclear space and subsurface cisternae, and frequently in the concave saccules of the Golgi apparatus. After a long-term culture, some neurons became "aged". The endoplasmic reticulum cisternae enlarged and G-6-Pase reaction reduced. Along with the neuronal development, especially maturation of the endoplasmic reticulum and its enzymic marker, synapse formation was begun at the neuropile area. The axo-dendritic synapses always occurred between the axonal terminals and dendrites where the endoplasmic reticulum had showed positive G-6-Pase reactions. Considering the fact, it suggests that the appearance and change of these specific enzymes may be related to the maturation of the neurons in vitro, and also related to the synapse formation between neurons.     

Ultrastructural localization of phosphatase activity in the guinea pig pineal gland by the cerium technique

Thiamine pyrophosphatase (TPPase), nucleoside diphosphatase (NDPase), and glucose-6-phosphatase (G-6-Pase) were localized by the cerium technique in guinea pig pinealocytes and compared with the corresponding lead technique. NDPase and TPPase were also compared at different pH values using the cerium technique. Vibratome sections of perfusion-fixed tissue were incubated with cerium chloride or lead nitrate. Substrates used were thiamine pyrophosphate (for TPPase), sodium inosine diphosphate (NDPase), and disodium glucose-6-phosphate (G-6-Pase). The 1-2 trans saccules of the Golgi apparatus showed TPPase and NDPase activity but none for G-6-Pase. The endoplasmic reticulum (ER) cisternae and perinuclear space had NDPase and G-6-Pase activity but not TPPase. The abluminal plasmalemma of endothelial cells and the plasmalemma of Schwann cells demonstrated TPPase and NDPase activity but the luminal plasmalemma of the endothelial cells and the plasmalemma of pinealocyte processes showed only NDPase activity. TPPase was active at all pH values tested, but NDPase was most active at pH values of 6.5 and 7.0. Lead phosphate precipitate was frequently seen in nuclei, perinuclear space, ER cisternae, and "synaptic" vesicles when lead was used as the capturing agent. These sites were usually not labeled when cerium was used.     

Ultrastructural Changes in Maturing Sporangia of Albugo Candida

Maturation of sporangia in Albugo sp. involved considerableinternal differentiation. There was a burst of activity in sporangiasoon after their formation when the numbers of mitochondria,and the amounts of endoplasmic reticulum increased. Perinuclearvesicles and smooth surfaced cisternae differentiated into well-developedgolgi apparatus which remained secretory until completion ofmaturation. The cisternae of rough endoplasmic reticulum arrangedthemselves in parallel stacked arrays. Maturing sporangia hadautophagic vacuoles containing various cell organelles. Nucleardegeneration and mitosis proceeded simultaneously. All activitiesdeclined towards the end of sporangial maturation: Golgi dictyosomesbecame quiescent and numbers of mitochondria and amounts ofendoplasmic reticulum decreased. There was a three-fold increasein the thickness of the sporangial wall during maturation.     

Albumin secreted by rat liver bypasses Golgi apparatus cisternae

Albumin was isolated immunologically from various subcellular fractions from livers of adult male rats receiving an intraperitoneal injection of [³H]leucine to investigate the kinetics and pathway of subcellular transfer of newly synthesized albumin during secretion. At appropriate time intervals, livers were excised and fractionated into endoplasmic reticulum and Golgi apparatus. Golgi apparatus were further subfractionated into cisternae and secretory vesicles. In endoplasmic reticulum fractions, labeled albumin appeared within 7.5 min of injection of isotope, followed by a rapid decline in specific activity. Albumin in Golgi apparatus was labeled and concentrated in secretory vesicles over 25 min. The radioactivity in albumin per mg total protein was highest in secretory vesicles and insignificant in the cisternal fraction. Labeled albumin was present in serum by 30 min and radioactivity in serum albumin reached a plateau within 60–90 min after injection of isotope. Results provide evidence for the migration of albumin from its site of synthesis on endoplasmic reticulum membrane-bound polyribosomes to its site of secretion into the circulation via the Golgi apparatus. The pathway of albumin transport to secretory vesicles is suggested to involve peripheral elemenst of the Golgi apparatus. Secretory vesicle formation and maturation required 20 to 30 min for completion, via a mechanism whereby the inner spaces of the central saccules may be bypassed.     

Cytochemical localization of glucose-6-phosphatase in rabbit mononuclear phagocytes during differentiation

Cytochemical and biochemical investigations have revealed glucose-6-phosphatase (G-6-Pase) activity in Kupffer cells of the liver. To determine whether other mononuclear phagocytes are also reactive for G-6-Pase, rabbit bone marrow, blood, and alveolar macrophages were tested for G-6-Pase by a modified Wachstein-Meisel method and prepared for electron microscopy. Some mononuclear phagocytes from all three tissues were intensely reactive; others were unreactive. In promonocytes, monocytes, and alveolar macrophages, reaction product for the enzyme was localized throughout all cisternae of the endoplasmic reticulum (ER) and the perinuclear cisternae, but it was absent from the Golgi complex, lysosomes, and occasional smooth tubular channels. These results indicate that mononuclear phagocytes at all stages of development contain cytochemically demonstrable G-6-Pase and that the distribution of the enzyme is not altered during their differentiation from immature cells in the bone marrow to mature macrophages in the lung.     

Golgi apparatus, GERL, and secretory granule formation within neurons of the hypothalamo-neurohypophysial system of control and hyperosmotically stressed mice

The vasopressin-producing neurons of the hypothalamo-neurohypophysial system are a particularly good model with which to consider the relationship between the Golgi apparatus nd GERL and their roles in secretory granule production because these neurons increase their synthesis and secretion of vasopressin in response to hyperosmotic stress. Enzyme cytochemical techniques for acid phosphatase (AcPase) and thiamine pyrophosphatase (TPPase) activities were used to distinguish GERL from the Golgi apparatus in cell bodies of the supraoptic nucleus from normal mice, mice hyperosmotically stressed by drinking 2% salt water, and mice allowed to recover for 5-10 d from hyperosmotic stress. In nonincubated preparations of control supraoptic perikarya, immature secretory granules at the trans face of the Golgi apparatus were frequently attached to a narrow, smooth membrane cisterna identified as GERL. Secretory granules were occasionally seen attached to Golgi saccules. TPPase activity was present in one or two of the trans Golgi saccules; AcPase activity appeared in GERL and attached immature secretory granules, rarely in the trans Golgi saccules, and in secondary lysosomes. As a result of hyperosmotic stress, the Golgi apparatus hypertrophied, and secretory granules formed from all Golgi saccules and GERL. Little or no AcPase activity could be demonstrated in GERL, whereas all Golgi saccules and GERL-like cisternae were TPPase positive. During recovery, AcPase activity in GERL returned to normal; however, the elevated TPPase activity and secretory granule formation seen in GERL-like cisternae and all Golgi saccules during hyperosmotic stress persisted. These results suggest that under normal conditions GERL is the predominant site for the secretory granule formation, but during hyperosmotic stress, the Golgi saccules assume increased importance in this function. The observed cytochemical modulations in Golgi saccules and GERL suggest that GERL is structurally and functionally related to the Golgi saccules.     

Relationship between the golgi apparatus, gerl, and secretory granules in acinar cells of the rat exorbital lacrimal gland

The method of secretory granuleformation in the acinar cells of the rat exorbital lacrimal gland was studied by electron microscope morphological and cytochemical techniques. Immature secretory granules at the inner face of the Golgi apparatus were frequently attached to a narrow cisternal structure similar to GERL as described in neurons by Novikoff et al. (Novikoff, P. M., A. B. Novikoff, N. Quintana, and J.-J. Hauw. 1971. J. Cell Bio. 50:859-886). In the lacrimal gland. GERL was located adjacent to the inner Golgi saccule, or separated from it by a variable distance. Portions of GERL were often closely paralleled by modified cisternae of rough endoplasmic reticulum (RER), which lacked ribosomes on the surface adjacent to GERL. Diaminobenzidine reaction product of the secretory enzyme peroxidase was localized in the cisternae of the nuclear envelope, RER, peripheral Golgi vesicles, Golgi saccules, and immature and mature secretory granules. GERL was usually free of peroxidase reaction product or contained only a small amount. Thiamine pyrophosphatase reaction product was present in two to four inner Golgi saccules; occasionally, the innermost saccule was dilated and fenestrated, and contained less reaction product than the next adjacent saccule. Acid phosphatase (AcPase) reaction product was present in GERL, immature granules, and, rarely, in the innermost saccule, but not in the rest of the Golgi saccules. Thick sections of AcPase preparations viewed at 100 kV revealed that GERL consisted of cisternal, and fenestrated or tublular portions. The immature granules were attached to GERL by multiple connections to the tublular portions. These results suggest that, in the rat exorbital lacrimal gland, the Golgi saccules participate in the transport of secretory proteins, and that GERL is involved in the formation of secretory granules.     

Ultrastructural changes in the MP3 neuron of the mollusk Lymnaea stagnalis after cryopreservation of the isolated brain

Investigation of a possibility of long-term storage of frozen (-196 degrees C) viable neurons and nervous tissue is one of the central present day problems. In this study ultrastructural changes in neurons of frozen-thawed snail brain were examined as a function of time. We studied the influence of cryopreservation, cryoprotectant (Me2SO), cooling to 4-6 degrees C, and a prolonged incubation in physiological solution at 4-6 degrees C on dictyosomes of Golgi apparatus, endoplasmic reticulum (ER) cisternae and mitochondria. It has been found that responses of these intracellular structures of cryopreserved neurons to the above influences are similar: dissociation of Golgi dictyosomes, swelling of endoplasmic reticulum cisternae and mitochondrial cristae. Both freezing-thawing and cryoprotectant were seen to cause an increase in the number of lysosomes, liposomes, myelin-like structures, and to form large vacuoles. The structural changes in molluscan neurons caused by cryopreservation with Me2SO (2 M) were reversible.     

An ultrastructural study of osmiophilia in normal human oesophageal epithelium

Summary Oesophageal biopsies were obtained from patients with normal oesophagi during fibre-optic endoscopy for upper gastro-intestinal symptoms. They were studied with the prolonged osmication technique. The forming face of the Golgi apparatus was demonstrated in the basal and lower prickle cells. These cells also showed osmium deposition in their mitochondria, endoplasmic reticulum, perinuclear cisternae and lysosomes. The capillary endothelial cells also showed osmium deposition in their Golgi apparatus and endoplasmic reticulum.     

Electron microscopic and cytochemical studies of the mouse subcommissural organ

Summary In mice most of the ependymal cells of the subcommissural organ (SCO cells) are densely packed with dilated cisternae of the endoplasmic reticulum (ER) containing either finely granular or flocculent materials. The well developed supra-nuclear Golgi apparatus consists of stacks of flattened saccules and small vesicles; the two or three outer Golgi saccules are moderately dilated and exhibit numerous fenestrations; occasional profiles suggesting the budding of coated vesicles and formation of membrane-bound dense bodies from the ends of the innermost Golgi saccules are seen. A few coated vesicles and membrane-bound dense bodies of various sizes and shapes are also found in the Golgi region.The contents of the dilated ER cisternae are stained with periodic acid-silver methenamine techniques. In the Golgi complex the two or three inner saccules are stained as deeply as the dense bodies, and the outer saccules are only slightly stained. The stained contents of ER cisternae are more electron opaque than those of the outer but less opaque than those of the inner Golgi saccules and the dense bodies.Acid phosphatase activities are localized in the dense bodies, some of the coated vesicles in the Golgi region, and in the one or two inner Golgi saccules.On the basis of these results the following conclusions have been reached: (1) In mouse SCO cells the finely granular and the flocculent materials in the lumen of ER cisternae contain a complex carbohydrate(s) which is secreted into the ventricle to form Reissner's fiber; (2) the secretory substance is assumed to be synthesized by the ER and stored in its cisternae, and the Golgi apparatus might play only a minor role, if any, in the elaboration of the secretory material; (3) most of the dense bodies in the mouse SCO cells are lysosomal in nature instead of being so-called dark secretory granules.Sponsored by the National Science Council, Republic of China.