成年大鼠神经元和星形胶质细胞细胞周期蛋白表达的差异研究

目的比较研究成年大鼠细胞周期蛋白在神经元和星形胶质细胞的表达差异。方法应用免疫荧光和激光扫描共聚焦显微镜观察成年大鼠生理状态下大脑皮层或海马CA1区神经元和星形胶质细胞细胞周期素D1、E、A、B1、(CyclinD1、E、A、B1)的表达。结果成年大鼠海马CA1区和大脑皮层的神经元有Cyclin D1、E、A和B1的表达,细胞核和细胞浆均有表达,以胞核为主;星形胶质细胞也有上述细胞周期蛋白的表达但细胞数目较少,并且表达这些指标的星形胶质细胞多聚集在海马CA1区。结论成年大鼠大脑皮层和海马区的神经元和星形胶质细胞均表达细胞周期蛋白,而其在神经元的表达较星形胶质细胞更为普遍。     

BRANCHING PATTERNS OF INDIVIDUAL SYMPATHETIC NEURONS IN CULTURE

The growth of single sympathetic neurons in tissue culture was examined with particular regard to the way in which the patterns of axonal or dendritic processes (here called nerve fibers), were formed. The tips of the fibers were seen to advance in straight lines and to grow at rates that did not vary appreciably with time, with their position in the cell outgrowth, or with the fiber diameter. Most of the branch points were formed by the bifurcation of a fiber tip (growth cone), apparently at random, and thereafter remained at about the same distance from the cell body. It seemed that the final shape of a neuron was the result of the reiterated and largely autonomous activities of the growth cones. The other parts of the cell played a supportive role but, apart from this, had no obvious influence on the final pattern of branches formed.     

THE FINE STRUCTURE OF SYMPATHETIC NEURONS IN X-IRRADIATED FROGS

The effects of whole body x-irradiation on the fine structure of sympathetic neurons were studied in 15 unanesthetized adult frogs (Rana pipiens), as seen at intervals ranging from 1 hour to 2 weeks after single exposures to 1000 r and 2000 r. Using standard procedures, the lumbar sympathetic ganglia of experimental and 20 control animals were prepared for electron microscope examination. Radiation produced conspicuous but irregular and variable deterioration, swelling, and clearing of neuronal lysosomes. These changes may have been due to an increased permeability of lysosomal membranes, causing the entry of fluid into lysosomes and their swelling and deterioration, but a pronounced escape of lysosomal enzymes into the cytoplasm was questionable. Less frequent were the dilatation and the parallel layering or complete fusion and tight packing of the rough-edged endoplasmic reticulum. The number of vacuoles, probably derived from Golgi cisternae, was somewhat increased. These vacuoles were conjectured to serve the "sequestration" of damaged cytoplasmic areas. Abnormal amounts of presumptive glycogen granules occupied some axons of myelinated and unmyelinated fibers, especially of presynaptic nerve fibers. This was assumed to be due to a decreased breakdown of glycogen and probably caused the interruption of the transmission of nerve impulses in presynaptic fibers. The maximal incidence of these alterations seemingly occurred 8 days after exposure to 1000 r, and 1 hour after x-irradiation with 2000 r. Signs of recovery appeared 2 weeks after exposure to 2000 r.     

ELECTRON MICROSCOPY OF CYTOPLASMIC INCLUSIONS IN CELLS INFECTED WITH ROD-SHAPED VIRUSES

Thin sections of leaf tissue infected with 12 rod-shaped viruses varying from 180 mμ to 750 mμ in length were examined in the electron microscope. Neither intranuclear nor cytoplasmic inclusions occurred in healthy tissue. Intranuclear inclusions were observed only in material infected with tobacco etch virus. Several types of cytoplasmic inclusions were induced by the group of viruses varying in length from 730 mμ to 750 mμ; however, only one type of inclusion was common to all seven viruses of this group. It is proposed that this inclusion, which appears as a pin-wheel in cross section and as a bundle in longitudinal section, is diagnostic for infection with viruses of the potato Y group, i.e., rod-shaped viruses whose lengths vary from 730 mμ to 750 mμ.     

胍基丁胺在成年大鼠组织中的表达和分布

目的观察胍基丁胺（agmatine,AGM）在成年Wistar大鼠全身组织的表达和分布。方法采用免疫组织化学法,用自制的抗胍基丁胺多克隆抗体检测胍基丁胺在成年Wistar大鼠全身组织中的表达分布情况。结果胍基丁胺在胃、十二指肠、空肠、回肠、结肠的粘膜腺上皮细胞胞质内呈强阳性表达;胍基丁胺在大脑皮层、丘脑、海马、延髓的神经元胞质和神经轴突内呈强阳性表达;胍基丁胺在子宫、输卵管、前列腺的腺上皮细胞和睾丸的生精细胞胞质内呈强阳性表达;胍基丁胺在肝细胞、肾上腺皮髓质细胞胞质内呈阳性表达,在肾脏、脾脏呈弱阳性表达;胍基丁胺在肺、阴茎的微血管平滑肌细胞胞质内呈强阳性表达,但在心脏、骨骼肌、食道、主动脉的肌细胞内未见其表达。结论胍基丁胺在成年Wistar大鼠体内广泛分布,可能具有重要的生理作用。     

西洋参胚性细胞和胚状体细胞中的核内含体与细胞质内含体

１９２１年,Ｍｏｌｉｓｈ首先在光镜下发现植物叶片细胞核中有一种晶体状的内含物（见Ｗｅｉｎｔｒａｕｂ等［１］）。后来人们陆续在某些动、植物的细胞核中观察到了这种结构［２—４］,并称之为核内含体（ｉｎｔｒａｎｕｃｌｅａｒｉｎｃｌｕｓｉｏｎｓ）。Ｂｉｇａｚｚｉ［３］曾在４５种桔梗科植物的细胞中看到了核内含体。但在离体培养的植物细胞中发现内含体的报道很少,至今仅在榛子组织培养分生细胞中看到了类似的结构［５］。我们在对西洋参体细胞胚胎发生进行超微结构研究的过程中发现,在胚性愈伤组织和胚状体细胞的核和细胞质…     

创伤后应激障碍大鼠蓝斑核神经元细胞凋亡的实验研究

目的探讨创伤后应激障碍(PTSD)大鼠蓝斑核神经元Caspase-3和Caspase-9的表达变化。方法成年健康雄性Wistar大鼠50只,随机分为连续单一刺激(single prolonged stress,SPS)模型1d、4d、7d、14d组和对照组,应用免疫组化、免疫荧光和RT-PCR方法检测PTSD大鼠蓝斑核神经元Caspase-3和Caspase-9的表达变化。结果SPS刺激后1d,4d,Caspase-9的表达逐渐增强,7d和14d逐渐下降,Caspase-3于SPS刺激后7d表达最多,14d出现下降。结论蓝斑神经元细胞凋亡可能是导致PTSD患者蓝斑功能失调的重要原因之一。     

CYTOPLASMIC FILAMENTS IN DEVELOPING AND ADULT VERTEBRATE SMOOTH MUSCLE

An extensive study of adult and developing smooth muscle has revealed the widespread occurrence of a distinct filament with an average diameter of about 100 A (termed the 100 A filament). Unlike that of myofilaments, their appearance in longitudinal section is uniform, but in transverse section they have a round profile, occasionally exhibiting a less electron-opaque core. The 100 A filaments are almost invariably preserved under a variety of fixation procedures, whereas myofilaments, particularly the thicker filaments, are preserved inconsistently. The 100 A filaments appear to be randomly oriented throughout the cytoplasm, either singly or in small groups, although they are sometimes concentrated in the juxtanuclear region of the smooth muscle cells. The intimate association of 100 A filaments with dark bodies, in both developing and adult smooth muscle cells, may indicate that these filaments either play a role in dark body formation or, at least, constitute a part of the dark body. The 100 A filaments are conspicuous in developing smooth muscle cells and occasionally form networks or clusters; they appear to decrease in relative number as maturation proceeds, but considerable numbers are still present in adult tissue.     

FINE STRUCTURE OF NERVE FIBERS AND GROWTH CONES OF ISOLATED SYMPATHETIC NEURONS IN CULTURE

The leading tips of elongating nerve fibers are enlarged into "growth cones" which are seen in tissue culture to continually undergo changes in conformation and to foster numerous transitory slender extensions (filopodia) and/or a veillike ruffling sheet. After explantation of 1-day-old rat superior cervical ganglia (as pieces or as individual neurons), nerve fibers and tips were photographed during growth and through the initial stages of aldehyde fixation and then relocated after embedding in plastic. Electron microscopy of serially sectioned tips revealed the following. The moving parts of the cone, the peripheral flange and filopodia, contained a distinctive apparently filamentous feltwork from which all organelles except membranous structures were excluded; microtubules were notably absent from these areas. The cone interior contained varied forms of agranular endoplasmic reticulum, vacuoles, vesicles, coated vesicles, mitochondria, microtubules, and occasional neurofilaments and polysomes. Dense-cored vesicles and lysosomal structures were also present and appeared to be formed locally, at least in part from reticulum. The possible roles of the various forms of agranular membranous components are discussed and it is suggested that structures involved in both the assembly and degradation of membrane are present in the cone. The content of these growing tips resembles that in sensory neuron growth cones studied by others.     

雌二醇对成年大鼠肺表面活性物质分泌的影响

采用离体非灌流肺模型,观察了雌二醇(E_2)对成年大鼠肺表面活性物质(PS)分泌的影响,并探讨了前列腺素(PG)在其中的作用。结果显示:E_2(10~(-6)mol/L)可使肺磷脂释放指数和肺磷脂释放量增多,分别为对照组的150.0％(P<0.05)及160.7％(P<0.01),表明E_2可促进成年大鼠PS的分泌;PG合成抑制剂消炎痛(10~(-5)mol/L)可以抑制E_2促进肺磷脂释放的效应,表明PG在E_2促进PS分泌中起介导作用。以上结果提示E_2可能参与成年动物PS分泌的调控。     

PTSD样大鼠蓝斑核盐皮质激素受体表达变化的研究

目的探讨PTSD样大鼠蓝斑（locus ceruleus,LC）神经元盐皮质激素受体（mineralocorticoid receptors,MR）表达的变化。方法使用连续单一应激（SPS）方法建立PTSD大鼠模型,随机分为SPS处理后24h、4d、7d、14d和28d组,非SPS刺激大鼠作为对照,应用免疫组化、免疫印迹方法分别进行各组蓝斑神经元MR表达变化的观察及检测,进行图像分析和统计学处理。结果蓝斑神经元MR的表达呈现24h急剧下调,4d、7d,14d和28d恢复性上调。结论PTSD样大鼠蓝斑神经元MR的表达变化可能直接参与了PTSD持续性精神行为障碍的发生发展过程。     

硝苯吡啶抑制豚鼠交感神经元的钙依赖性电位

应用细胞内记录技术观察了钙通道阻滞剂硝苯吡啶(nifedlpine)对离体豚鼠腹腔神经节细胞三种钙依赖性电位的可逆性作用。硝苯吡啶(0.1—1mmol/L)可剂量依赖式地抑制动作电位后超极化、强直后膜电位的变化,在无钠高钙加 TEA 溶液中,硝苯吡啶(0.1μmol/L)能抑制钙锋电位。结果表明,大剂量的硝苯吡啶可继发性抑制钙依赖性钾电导,临床治疗剂量的硝苯吡啶还直接减少钙电导。以上作用是硝苯吡啶调节交感节后神经元的兴奋性,阻滞突触前膜 ACh 的量子性释放的基础。     

NUCLEAR PROTEINS IN BRAIN OF 7-DAY-OLD AND ADULT RATS

Abstract— The incorporation of radioactive leucine into proteins of rat brain was considerably higher in the 7-day-old than in the adult rat. The greatest difference in the rate of protein synthesis between these two stages of development occurs in the mitochondrial fraction. Among the nuclear proteins the largest variation was in the histones. The only difference in the relative content of nuclear proteins between 7-day-old and adult brain was in the acidic deoxyribonucleoproteins which was higher in the younger animal. The electrophoretic profile of these proteins changed during brain development.     

CELL CYCLE PROPERTIES OF DIFFERENTIATING SPERMATOGONIA IN ADULT SPRAGUE-DAWLEY RATS

The duration of the mitotic cycle and of its components was analysed for each of the six successive generations of differentiating spermatogonia (A₁, A₂, A₃, A4, intermediate and B), using radioautographed whole mounts of seminiferous tubules from testes of adult Sprague-Dawley rats. Cell cycles were determined from two successive waves of per cent labeled metaphases obtained during the period of 81 hr after a single dose of ³H-thymidine. Except for the A₁ spermatogonia, all spermatogonial types (A₂ to B) had similar cell cycle durations of 41-42.5 hr and comparable pre-DNA synthesis phases (G₁) of 11-13 hr. Although the combined duration of DNA synthesis (S) and the post-synthesis phase (G₂) remained identical for all the cell types including A₁, there was a progressive lengthening of the S period at the expense of G₂ during the process of spermatogonial maturation. This change was most marked during the transition from A₁ to A₃ spermatogonia when the S period increased from 14 hr to 21 hr, and the G₂ phase shortened from 13 hr to 7.5 hr. This feature seems to be unique to germ cells and may be associated with an increasing amount of heterochromatin in the nucleus. Excluding the development of type A₁ cells, the entire process of spermatogonial maturation lasted for 208 hr. Combined data on cell cycle times indicated that every 313 hr or 13 days, a new sequence of spermatogonial differentiation was initiated by the A₁ cells. This was equivalent to the duration of one 'cycle' of the seminiferous epithelium as measured by other techniques.