脉红螺神经细胞和胶质细胞光镜及电镜观察

脉红螺(Rapana venosa)神经节存在三种细胞,它们是神经细胞、星形胶质细胞和无突胶质细胞。从结构上看,神经细胞与后鳃类软体动物海兔(Aplysia)的神经细胞不尽相同。电镜观察表明,脉红螺右足神经节细胞体区的星形胶质细胞与海兔腹神经节内包围神经细胞体的星形胶质细胞很相似。但在脉红螺,星形胶质细胞的突起与神经细胞之间的拓朴学关系尚不清楚。无突胶质细胞在脉红螺神经节内广泛存在,它的核类似于海兔神经细胞的核。这类细胞的功能尚不清楚。     

枸杞胚性细胞分化的超微结构和ATP酶的细胞化学定位研究

枸杞的胚性细胞多由愈伤组织表层的薄壁细胞分化而来,与愈伤组织中未分化的细胞相比,胚性细胞呈卵圆形,细胞核大,核仁明显,细胞质浓厚并含有丰富的细胞器,细胞壁较薄,细胞间有胞间连丝相通;胚性细胞发育到晚期细胞壁加厚,胞间连丝逐渐消失,细胞核向一端偏移,有大液泡形成;胚性细胞的第一次分裂多为均等分裂,形成二细胞原胚,继续分裂形成多细胞原胚;组成多细胞原胚胚体的细胞核大,核形状不规则,细胞质浓厚,细胞器丰富,在质体中出现淀粉的积累。在胚性细胞发育的早期,ATP酶活性主要位于质膜上,随后在液泡内和细胞核中都出现ATP酶活性的分布;随着胚性细胞壁的加厚,细胞壁加厚处和细胞间隙中也出现ATP酶活性反应;当多细胞原胚形成后,ATP酶活性反应主要定位于液泡膜上。由此分析了结构特征、ATP酶活性定位变化与胚性细胞分化的关系。     

小白鼠精母细胞的核内环状片层

环状片层(annlulate lamellae)是存在于细胞质或细胞核内的一种片层结构,在细胞发育和分化的一定阶段出现。这种细胞器最初是在生殖细胞中发现的,现已普遍见于生殖细胞、胚胎细胞、肿瘤细胞以及其他一些细胞,甚至在包括神经细胞在内的某些高度分化的细胞和植物细胞中也都观察到了这种结构。细胞质环状片层较为常见,已有许多报道;核     

果蝇胶质细胞在神经系统的功能研究进展

胶质细胞是一类广泛存在于神经系统的细胞,但其在神经系统的功能作用尚不太清楚。果蝇神经系统中也存在多种的胶质细胞,包括表面胶质细胞(Surface glia)、皮质胶质细胞(Cortex glia)、类星形胶质细胞(Astrocyte-like glia)、神经节包裹型胶质细胞(Ensheathing glia)和轴突包裹型胶质细胞(Wrapping glia)。本综述介绍果蝇胶质细胞研究的近期进展,研究表明果蝇胶质细胞能激活神经干细胞分裂,维持神经干细胞的存活,促进视叶神经上皮细胞的增殖。胶质细胞还能维持神经元的存活,以及促进轴突的形成、聚束和正常的投射。此外,胶质细胞还具有清除凋亡神经细胞的作用。     

细胞的起源和进化(二)

（续１９９８年第３３卷第６期第１４页）３内共生学说真核细胞除了有细胞核外,细胞质中还有多种细胞器,这些细胞器的起源和进化同样是细胞进化的重要事件。其中研究得最多,争论也最大的是线粒体和叶绿体的起源和进化。作为经典的学说,一直有人认为线粒体和叶绿体是原...     

胶质瘢痕对神经系统损伤的保护作用

胶质瘢痕是神经系统损伤后由反应性星形胶质细胞,小胶质细胞及其分泌的细胞外基质组成。早期的研究多集中于胶质瘢痕在抑制轴突生长,神经细胞再生等方面的作用。而最新的研究表明胶质瘢痕的形成对损伤急性期神经细胞具有重要的保护作用。本文从瘢痕组织在损伤缝合和组织重构、局部免疫调节、神经再生等方面对神经损伤的保护作用进行综述。     

体外培养的鸡胚神经元迁移的光镜和扫描电镜的研究

用鸡胚神经细胞为材料,建立神经细胞体外培养技术,相差显微镜观察到鸡胚神经元可以沿着神经胶质细胞纤维运动。扫描电子显微镜揭示体外培养神经元与胶质细胞的关系。     

玉米螟幼虫侧单眼的神经鞘和胶质细胞

用透射电镜观察了欧洲玉米螟Ostrinia nubilalis(Hbner)5龄幼虫侧单眼神经的神经围膜、周神经细胞和其他神经胶质.神经围膜与若干周神经细胞包围若42根轴突.周神经细胞的原生质膜在它们的侧面和内面高度卷曲,并与相邻细胞交错对插,这是细胞与细胞间的特殊连接方式;它们的外面以桥粒和半桥粒固定在神经围膜内面.周神经细胞由神经胶质细胞演化而来,所形成的膜称神经束膜,它与神经围膜组成围在侧单眼神经外面的神经鞘.侧单眼神经内的神经胶质细胞大而平整,具有许多突起物(相当于脊椎动物的少突神经胶质细胞),每一个突起物包被一个感光轴突.神经胶质细胞包被轴突的形式有三种不同的类型:一种是相邻轴突间插入15层神经胶质细胞突起物所形成的普通轴系膜形式,另两种是神经胶质细胞突起物在一个轴突的周围,由一些褶所形成的不同形式.最后,对这些神经胶质细胞以不同形式包被轴突的功能意义进行了讨论.     

菜豆胚乳游离核中的线粒体(简报)

在植物细胞中,细胞核以及具DNA的细胞器——质体和线粒体,在结构上通常各具自身的被膜而独立存在。关于核与这两种细胞器以及两种细胞器之间通过外膜的连接在一些植物中已有报道。最近,Yu和Russell在烟草中发现了细胞核中存在线粒体的现象。本     

植物叶片原生质体分离的可能机制

分析了植物叶片在分离液环境中形成原生质体的过程,文中提出,分离液配方中的酸性物质使植物叶片处于酸性环境中并导致植物正常细胞首先发生细胞壁酸性降解,随后出现原生质体脱离细胞壁进入分离液,继而又进一步发生质膜的酸性降解,使细胞核和细胞器进入分离液中,最终分离液中的细胞器以细胞核为中心进行细胞器重组,最后产生外貌形态一致的新的原生质体.植物细胞壁和质膜是植物细胞的包被系统.植物细胞包被系统的酸性降解使植物细胞器重组并产生新的原生质体成为可能.     

Organotypic Slice Cultures to Study Oligodendrocyte Dynamics and Myelination

NG2 expressing cells (polydendrocytes, oligodendrocyte precursor cells) are the fourth major glial cell population in the central nervous system. During embryonic and postnatal development they actively proliferate and generate myelinating oligodendrocytes. These cells have commonly been studied in primary dissociated cultures, neuron cocultures, and in fixed tissue. Using newly available transgenic mouse lines slice culture systems can be used to investigate proliferation and differentiation of oligodendrocyte lineage cells in both gray and white matter regions of the forebrain and cerebellum. Slice cultures are prepared from early postnatal mice and are kept in culture for up to 1 month. These slices can be imaged multiple times over the culture period to investigate cellular behavior and interactions. This method allows visualization of NG2 cell division and the steps leading to oligodendrocyte differentiation while enabling detailed analysis of region-dependent NG2 cell and oligodendrocyte functional heterogeneity. This is a powerful technique that can be used to investigate the intrinsic and extrinsic signals influencing these cells over time in a cellular environment that closely resembles that found in vivo.     

Migration of neurons between ganglia in the metamorphosing insect nervous system

Migration of neurons over long distances occurs during the development of the adult central nervous system of the sphinx moth Manduca sexta, and the turnip moth Agrotis segetum. From each of the suboesophageal and three thoracic ganglia, bilaterally-paired clusters of immature neurons and associated glial cells migrate posteriorly along the interganglionic connectives, to enter the next posterior ganglion. The first sign of migration is observed at the onset of metamorphosis, when posterio-lateral cell clusters gradually separate from the cortex of neuronal cell bodies and enter the connectives. Cell clusters migrate posteriorly along the connective to reach the next ganglion over the first three days (approximately 15%) of pupal development. During migration, each cell cluster is completely enveloped by a single giant glial cell spanning the entire length of the connective between two adjacent ganglia. Intracellular cobalt staining reveals that each migrating neuron has an ovoid cell body and an extremely long leading process which extends as far as the next posterior ganglion; this is not a common morphology for migrating neurons that have been described in vertebrates. Once the cells arrive at the anterior cortex of the next ganglion, they rapidly intermingle with the surrounding neurons and so we were unable to determine the fate of the migrating neurons at their final location.     

The development of the insect nervous system. I. An analysis of postembryonic growth in the terminal ganglion of Acheta domesticus

This study describes the post-embryonic growth of the terminal ganglion in Acheta domesticus in terms of volume and cell number. All measurements were made at the beginning of each instar from hatching until the final moult on animals reared under controlled conditions. The terminal ganglion increases about 40-fold in volume from 2 × 10⁶ μ³ in the first instar to 85 × 10⁶ μ³ in the adult. A double logarithmic plot of ganglion volume against body weight shows that the ganglion volume is a function of body weight to the 0.56 power. Initially the neuropile grows at a greater rate than the cortex; in later stages they increase at the same rate. Increase in cell number was determined from serial sections. The total number of cells, based on corrected nuclear counts, increases from 3,400 to 20,000. There is little or no increase in the number of neurons. There are approximately 2,000 association neurons and 100 motor neurons in all stages. The number of glial cells increase from 1,000 to 17,000. Their multiplication rate appears to be related to the increase in neuron volume. Despite the increase in glial cell number, increase in cell volume is primarily responsible for the increase in total volume of the ganglion.     

Structure of the intramural nerves of the rat bladder

The bladder of adult female rats receives ～16,000 axons (i.e., is the target of that many ganglion neurons) of which at least half are sensory. In nerves containing between 40 and 1200 axons cross-sectional area is proportional to number of axons; >99% of axons are unmyelinated. A capsule forms a seal around nerves and ends abruptly where nerves, after branching, contain ～10 axons. A single blood vessel is present in many of the large nerves but never in nerves of <600 axons. The number of glial cells was estimated through the number of their nuclei. There is a glial nucleus profile every 76 axonal profiles. Each glial cell is associated with many axons and collectively covers ～1,000 μm of axonal length. In all nerves a few axonal profiles contain large clusters of vesicles independent of microtubules. The axons do not branch; they alter their relative position along the nerve; they vary in size along their length; none has a circular profile. All the axons are fully wrapped by glial cells and never contact each other. The volume of axons is larger than that of glial cells (55%–45%), while the surface of glial cell is twice as extensive as that of axons; there are ～2.27 m² of axolemma and ～4.60 m² of glial cell membrane per gram of nerve. Of the mitochondria of a nerve ～3/4 are in axons and ～1/4 in glial cells.     

Stability of neuron and glial number in the parabigeminal nucleus of the ageing mouse

The number of neurons and glia in the albino mouse parabigeminal nucleus remains constant between 6 and 31 months of age. The presence of a small number of mitotic and pyknotic cells in the parabigeminal nucleus indicates a slow turnover of the glial population throughout life. Examination of the superior colliculus showed that degenerating neurons were present from 6 months of age and neurons appeared to be much more sparsely scattered in the superficial layers of aged mice than in young adults. The stability of the neuron number in the parabigeminal nucleus may be due to the reciprocal innervation of neurons of the superior colliculi and parabigeminal nuclei protecting each other from transneuronal degeneration which might otherwise occur as a consequence of loss of retinal ganglion cells. Alternatively, since each neuron in the parabigeminal nucleus probably synapses with many tectal neurons, the loss of only some of its target neurons would probably not lead to transneuronal degeneration.     

Morphology of neuroglia in the hypothalamus of the opossum (Didelphis virginiana), armadillo (Dasypus novemcinctus mexicanus) and cat (Felis domestica)

The hypothalamus of the opossum (Didelphis virginiana), the armadillo (Dasypus novemcinctus mexicanus), and the cat (Felis domestica) was studied using Del Rio Hortega's silver carbonate technique, as modified by Scharenberg ('60). This technique demonstrates astrocytes, oligodendroglia, and neuronal perikarya, but does not impregnate microglia. The morphology of macroglia was observed in ten comparable nuclei in each of the three species. The subpial and subependymal areas were also examined. Astrocytes display more cell body angularity and have more processes in most hypothalamic regions of the cat when compared to similar regions of the opossum and armadillo. In the anterior hypothalamic nucleus, the ventromedial and the dorsomedial hypothalamic nuclei, and the medial mammillary nucleus of all three species, astrocytes send processes to neurons, but neuronal and astrocytic perikarya are usually not directly contiguous. However, oligodendrocytes in a perisomatic position on neurons are a consistent feature in these nuclei. A closer relationship appears to exist between astrocytes and neurons in the neurosecretory nuclei. In the supraoptic nucleus and paraventricular nucleus of all three species a basket-like structure, designated a ?pericellular envelope”? was observed surrounding neuronal perikarya. This structure is composed of astrocytic and oligodendroglial cell bodies and processes, and is most highly developed in the cat. A dense astrocytic plexus was observed in the suprachiasmatic nucleus of the cat, and in the comparable nuclei of the armadillo and opossum. The most prominent macroglial cell type of the lateral hypothalamic and lateral mammillary nuclei of all three species is the interfascicular oligodendrocyte. The posterior hypothalamic nucleus of each species has many perisomatic oligodendrocytes, and in the armadillo and cat astrocytes are closely related to the larger neurons. A subpial plexus, consisting of a palisade of small glial cells with many processes, is present in the hypothalamus of the three species. Ependymal cells have long projecting processes throughout the length of the third ventricle in the armadillo hypothalamus, but such processes are only apparent in the region of the infundibular nucleus and median eminence in the opossum and cat.     

Localization of axonally transported 125I-wheat germ agglutinin beneath the plasma membrane of chick retinal ganglion cells

The distribution of 125I-wheat germ agglutinin (WGA) transported by axons of chick retinal ganglion cells to layer d of the optic tectum was studied by electron microscopic autoradiography. We found that 52% of the radioactivity was located in axons and axon terminals in the contralateral optic tectum 22 h after intravitreal injection of affinity-purified 125I-WGA. Axons comprised 43% of the volume of layer d. Dendrites, glial cells, and neuron cell bodies contained 20%, 17%, and 3% of the label, whereas these structures comprised 24%, 21%, and 2% of the tissue volume, respectively. We also measured the distances between the autoradiographic silver grains and the plasma membranes of these profiles, and compared observed distributions of grains to theoretical distributions computed for band-shaped sources at various distances from the plasma membranes. This analysis revealed that the radioactive source within axons was distributed in a band of cytoplasm extending in from the plasma membrane a distance of 63 nm. Because WGA is known to bind to specific membrane glycoconjugates, we infer that at least some glycoconjugates may be concentrated within an annular region of cytoplasm just beneath the axonal plasma membrane after axoplasmic transport from the neuron cell body.     

ELECTRON MICROSCOPIC OBSERVATIONS OF RAT AND MOUSE CEREBELLUM IN TISSUE CULTURE

Closely ordered stages of myelin formation in cultures of newborn rat and mouse cerebellum, selected by direct light microscopy, were studied with the electron microscope. Electron micrographs of these cultures reveal the presence of neurons, axons, neuroglia, microglia, and ependymal cells. The appearance of the neuron is identical to that previously described in vivo. The neuroglial cell has long, branching processes, and its cytoplasm is characterized by packets of long, narrow fibrils. During myelin formation, a glial cell process surrounds the axon. This process may form an internal mesaxon and may spiral for several turns around the axon. Other glial cell processes may interdigitate with or overlay the innermost process to contribute to the multilamellated structure. The glial processes flatten and the cytoplasmic surfaces of the cell membrane come into contact to form the lamellae of the myelin sheath. These adhesions may be temporarily incomplete as evidenced by sequestered islands of glial cytoplasm among the myelin lamellae. Ultimately, a compact, apparently spiral, myelin sheath is formed. These findings are discussed in relation to in vivo central myelin formation.     

Fine structure of glial cells in the central nervous system of the tapeworm Grillotia erinaceus (Cestoda: Trypanorhyncha)

The problem of glial cells existing in parasitic and free living flatworms is correlated with organization of parenchyma in platyhelmintes. In the contrary to the widespread opinion that myelin-like envelopes and glial cells do not exist in the nervous system of parasitic flatworms, it has been shown by ultrastructural researches that Amphilina foliacea (Cestoda, Amphilinidea) has well developed glial cells and myelin-like envelopes in the ganglia and main cords, which include both glial cells and intercellular components. The aim of our research was to reveal and investigate in details structural components corresponding to the concept of the glial cell in the CNS of Grillotia erinaceus (Cestoda: Trypanorhyncha). Three types of glial cells have been found. The first type is the fibroblast-like glial cells; cells locate in the cerebral ganglion, contain in cytoplasm and extract out fibrillar matrix, form desmosomes and have supporting function. The glial cells of the second type form myeline-like envelope of the giant axons and bulbar nerves in scolex and have laminar cytoplasm. These cells are numerous and exceed in number the neurons bodies into the nerve. The glial cells of the third type form multilayer envelopes in the main nerve cords; extra cellular fibers and gap-junctions take place between the layers. There are contacts between the glial cells of the third type and excretory epithelium but specialized contacts with neurons have been not found. The existing of glial cells in free living and parasitic flatworms is discussed.     

The ultrastructure of the Sertoli cell of the vervet monkey, Chlorocebus aethiops

The ultrastructure of the Sertoli cell of the vervet monkey was studied using both scanning and transmission electron microscopic techniques. SEM micrographs revealed perforated sleeve-like processes which encased mature elongated spermatids which are ready for spermiation. TEM micrographs showed a large Sertoli cell nucleus characterized by many lobes (4–5) and consisting of a homogenous nucleoplasm and a distinctive nucleolus. The nucleus occupies a significant portion of the basal region of the cell. The distribution of chromatin clearly shows high activity of these cells. Lipid droplets and free ribosomes are also found scattered throughout the cytoplasm. Well-developed Golgi apparatus is found in the basal region of the cell. There is phagocytic activity in the Sertoli cells as revealed by the presence of numerous phagosomes. Numerous mitochondria with well-developed tubular cristae are found on the basal side of the nucleus, whereas few mitochondria are located on the apical side of the nucleus. Distinct desmosomes are located between cells. A well-developed smooth endoplasmic reticulum and granular endoplasmic reticulum are frequently found in the cytoplasm of the Sertoli cells. The results of this investigation showed that Sertoli cells of the vervet monkey are almost similar to those of humans and show many similarities with other mammalian species.