蓖麻蚕微孢子虫的超微结构研究

用电镜技术研究蓖麻蚕微孢子虫各发育阶段的超微结构,发现其裂殖体和母孢子具双核,其细胞核由双层单位膜所包裹,核具半圆形的纺锤空斑,细胞质中有内质网和丰富的核糖体,但无线粒体。成熟的孢子壁由外壳、内壳及孢子膜组成,孢子器具有片层结构的极质体和后液泡,极丝为10—11圈,孢质含有核糖体和一对细胞核。     

洋葱花粉母细胞细胞内、细胞间微梁骨架的超微结构观察(英文)

以洋葱(AlliumcepaL.)花粉母细胞为材料,采用DGD包埋去包埋原位技术,对花粉母细胞不同发育时期的细胞内、细胞间微梁骨架的超微结构进行了电镜观察。结果发现,花粉母细胞核内存在粗细不等的微梁骨架,与核仁和染色体紧密相连,随着发育的推移,其均一性发生改变。在核周有核纤层样的结构存在,与细胞核和胞质中的微梁骨架紧密相连,到前期结束时解体。洋葱花粉母细胞内具有发达的胞质微梁骨架,这种结构在减数分裂前期Ⅰ变化不明显。在胞间连接(胞间连丝和胞质通道)内,也有精细的微梁骨架分布,并且与两端细胞中的骨架相连。在凝线期的花粉母细胞中观察到细胞融合现象,有胞质或核内微梁骨架与穿壁转移的胞质小球和核小球内骨架相连。此时细胞核偏向一边,但细胞的其余部位仍充满了胞质微梁骨架。初步探讨了核微梁骨架与核仁和染色体之间的关系,核纤层与细胞核之间的关系,以及细胞内、细胞间微梁骨架与细胞融合之间的关系     

大麦细胞核及染色体肌球蛋白免疫细胞化学定位

对去除DNA、组蛋白和大部分非组蛋白的大麦(Hordeum vulgare)细胞核和染色体间接免疫荧光标记实验结果表明:抗肌球蛋白抗体的荧光标记弥散分布在整个细胞核和染色体上;进一步应用免疫胶体金技术分析肌球蛋白在细胞核和染色体的分布情况,发现在染色体中散布着大量的胶体金颗粒;间期细胞核中胶体金颗粒主要分布在核仁和染色质中。上述实验结果表明:肌球蛋白是细胞核及染色体非组蛋白组成成分。本文还对肌球蛋白在细胞核和染色体中的分布规律进行了讨论。     

安南龟肝脏和肾脏的组织学观察

采用常规石蜡切片对安南龟的肝脏和肾脏进行了组织学观察。研究结果发现,肝脏分为3叶,肝实质内结缔组织少。肝脏由无数肝小叶构成,肝小叶分界不清。肝细胞为多角形的腺上皮细胞,细胞核圆球形,位于中央。胆小管沿着肝细胞索向肝小叶四周放射并连成细长的微细管道。肾脏由肾小体、颈段、近曲小管、中间段、远曲小管和收集管6部分构成,肾小体由肾小球和肾小囊组成,在肾小体附近可见致密斑样结构,未见髓袢结构。肾小球由盘曲的毛细血管构成。肾小囊是肾小管的起始端,由内、外两层壁层构成,内层与肾小球的毛细血管紧贴,外层为单层扁平上皮细胞。     

阳春砂花药发育过程的组织化学研究

用环氧树脂包埋的半薄切片经PAS反应和苏丹黑染色,研究阳春砂花药发育中的多糖和脂类物质分布特征。结果发现小孢子母细胞和四分体小孢子中积累了一些脂滴,但没有淀粉。阳春砂小孢子母细胞和四分体没有胼胝质壁。晚期小孢子中除了仍有很多脂滴外,细胞核周围开始出现淀粉粒;成熟花粉粒贮存丰富的淀粉粒和脂滴,且花粉壁由多糖物质构成。阳春砂花药壁结构比较特殊:花药壁由10余层细胞组成;最内层的绒毡层细胞在小孢子时期开始解体,细胞质转变为脂滴,供花粉吸收。开花时,花药壁由表皮和几层薄壁细胞以及径向壁纤维加厚的变形细胞组成。     

洋葱花粉母细胞细胞内、细胞间微染骨架的超微结构观察

以洋葱（Allium cepa L.）花粉母细胞为材料,采用DGD包埋去包埋原位技术,对花粉母细胞不同发育时期的细胞内、细胞间微染骨架的超微结构进行了电镜观察。结果发现,花粉母细胞核内存在的粗细不等的微染骨架,与核仁和染色体紧密相连,随着发育的推移,其均一性发生改变。在核周有核纤层样的结构存在,与细胞核和胞质中的微染骨架紧密相连,到前期结束时解体。洋葱花粉母细胞内具有发达的胞质微染骨架,这种结构在减数分裂前期Ⅰ变化不明显。在胞间连接（胞间连丝和胞质通道）内,也有精细的微染骨架分布,并且与两端细胞中的骨架相连。在凝线期的花粉母细胞中观察到细胞融合现象,有胞质或核内微梁骨架与穿壁转移的胞质小球和核小球内骨架相连。此时细胞核偏向一边,但细胞的基余部位仍充满了胞质微染骨架,初步探讨了核微染骨架与核仁和染色体之间的关系,核纤层与细胞核之间的关系。以及细胞内、细胞间微染骨架与细胞融合之间的关系。     

小麦条锈菌吸器超微结构和细胞化学的研究

本文应用电镜技术和细胞化学方法,对小麦条锈菌吸器和入侵点的超微结构进行了研究。小麦条锈菌吸器由呈管状的颈部和顶端膨大的吸器体组成,颈部壁和吸器体壁相互连贯,均为两层,并且含有多糖物质。在颈部中段存在有一染色较深的颈环结构。观察发现吸器中的多核现象极为普遍。细胞化学染色结果表明:在吸器外间质内分布有多糖物质;经蛋白消酶解处理后,吸器外间质中可观察到染色较深的纤丝状物质。在入侵点部位,吸器母细胞壁因局部增厚而呈凸镜状,入侵栓壁由内、外两层构成,这两层分别与吸器母细胞壁的第六层和第五层相连接。本研究还观察到同一入侵点产生两个入侵栓的现象。     

MAR的分子结构

核基质（ｎｕｃｌｅａｒｍａｔｒｉｘ）是真核生物细胞核中存在的主要由非组蛋白性纤维蛋白组成的空间网架结构。它参与了真核生物几乎所有的细胞核功能,包括ＤＮＡ复制、ＲＮＡ的合成和调控以及ｈｎＲＮＡ的加工、染色体的功能构建、有丝分裂、甾类激素作用、病毒复制和...     

油松鳞叶中细胞核穿壁现象的初步研究

利用薄切片和超薄切片技术对油松衰老鳞叶中细胞核穿壁运动进行了观察研究。首次,细胞核内的染色质逐渐收缩集中,形成染色深的球状体,以后,细胞核逐渐与细胞壁接近。接着紧贴细胞壁的细胞核通过细胞壁上的通道或胞间连丝转移到相邻的细胞内,此外,还发现有多种其它的转移方式存在。研究结果表明细胞核的穿壁运动现象同时存在于连子植物和裸植物中,电镜观察进一步证明细胞壁道在细胞核穿壁之前已形成。     

高等动物细胞核膜和核纤层结构、功能及动态变化调控机制

细胞核是真核细胞中最大的细胞器．高等动物细胞核主要由双层核膜、核孔复合体、核纤层、染色质和核仁等组成．在细胞有丝分裂期,细胞核呈现去装配和再装配等动态变化．在细胞分裂间期,核膜、核孔复合体和核纤层构成细胞核的外周结构,为遗传物质在染色质和核仁中的代谢提供了一个相对稳定的环境,同时调控细胞核内外的物质转运,在细胞增殖、分化、个体发育和细胞衰老等许多方面发挥着重要作用．本文主要对高等动物细胞核膜和核纤层结构、功能及动态变化调控机制等方面的研究进展进行简要综述．     

Observations of in vitro gametangial copulation and oosporogenesis in Lagenidium giganteum

An in vitro liquid culture oospore production method yielding 5 × 10³ oospores/ml was used to follow the sequential events of gametangial copulation and oospore formation in Lagenidium giganteum. Observations were made with Nomarski differential interference microscopy and scanning electron microscopy. After septation and division of fungal thalli into a chain-like series of links, certain individual subthalli differentiated into gametaniga, oogonia, and antheridia. Antheridia issued a fertilization tube which made contact with, and fused to a single oogonium. Copulative behavior was relatively synchronous and necessitated physical contact between thalli. Sexual reproduction was manifested by the migration and condensation of gametes. Plasmogamy was achieved following the introduction of the male gamete into the oogonium. The fused gametes gave rise to a zygote. Small amounts of periplasm remained in the oogonium. Zygote maturation into a fully developed oospore was characterized by the deposition of a multilaminated oospore wall, the coalescence of lipids into a highly refractive central reserve globule surrounded by a layer of fine-grained cytoplasm.     

Electron Microscopy of Ultrathin Sections of Sporosarcina ureae.

Mazanec, K. (J. E. Purkyne University, Brno, Czechoslovakia), M. Kocur, and T. Martinec. Electron microscopy of ultrathin sections of Sporosarcina ureae. J. Bacteriol. 90:808-816. 1965.-Ultrathin sections of Sporosarcina ureae cells were studied by means of electron microscopy. The cell wall consists of several layers and is 340 A thick. The cytoplasm is of globular structure and includes ribosomelike structures, occasional mesosomes, and inclusions not precisely identifiable. The nuclear area has various shapes and is formed by filaments 10 to 20 A thick which proceed in various directions. Cell division occurs similarly to that of sarcinate. Both synchronic and asynchronic cell division was observed. The spores of S. ureae consist of an outer coat having several layers, a cortex, a spore wall, and cytoplasm. The results of the present investigation substantiate our previous suggestion that S. ureae should be transferred from the family Micrococcaceae to the family Bacillaceae.     

Entamoeba histolytica: cell cycle and nuclear division

The cell cycle of Entamoeba histolytica, the duration of its phases, and the details of the nuclear division stages are described in this paper. Trophozoites from clone L-6, strain HM1:IMSS, were synchronized by colchicine. Synchrony was observed immediately after treatment and cultures remained synchronous for at least three replicative cycles with synchrony indexes between 13 and 15 hr. The stages of nuclear division were studied by light and electron microscopy. Four stages of the nuclear division were defined: prophase, early anaphase, late anaphase, and telophase. No metaphase stage was observed by light or electron microscopy. One of the first events in the nuclear division was the presence of a bud close to the juxtanuclear body, which grew to a daughter nucleus. The karyosome and the nuclear membrane remained throughout the mitotic process. Bundles of intranuclear microtubules were observed forming a "V" from the center of the nucleus to one of the poles, and associated with them, 12 to 16 chromosomes-like structures appeared. The results of these studies strongly suggest that division of E. histolytica involved a pleuromitotic process which is carried out in about 120 min.     

Ultrastructural changes during sporangium formation and zoospore differentiation in Blastocladiella Emersonii

Samples from synchronized cultures of Blastocladiella emersonii were examined by electron microscopy from the late log phase to the completion of zoospore differentiation. Log-phase plants contain the usual cytoplasmic organelles but also have an unusual system of large tubules ca. 45 mμ diam that ramify in organized bundles throughout the protoplast. After induction, zoosporangium differentiation requires a 2-hr period in which the nuclei divide, a cross wall forms to separate the basal rhizoid region, and an apical papilla is produced. Nuclear division in B. emersonii is intranuclear with a typical microtubular spindle apparatus and paired, unequal, extranuclear centrioles at each pole. The papilla is formed by a process of localized cell wall breakdown and deposition of the papilla material by secretory granules. Differentiation of zoospores begins when one of the two centrioles associated with each nucleus elongates to form a basal body. The flagella fibers arise from the basal body and elongate into an expanding vesicle formed by the fusion of small secondary vesicles. The cleavage planes are formed by fusion of vesicles similar to those associated with flagellum initiation. When cleavage is complete, each sporangium contains ca. 250–260 uninucleate spore units with their flagella lying in the cleavage planes. Probable fusion of mitochondria to produce the single mitochondrion of the zoospore occurs after cleavage; the mitochondrion does not take its position around the basal body and rootlets until just before zoospore release. The ribosomal nuclear cap is organized and enclosed by a membrane formed through fusion of many small vesicles during a short period near the end of differentiation.     

Absence of “void area” in freeze-etched vesicles of the Alnus crispa var. mollis Fern. root nodule endophyte

Nitrogen-fixing root nodules of Alnus crispa var. mollis Fern. were studied by transmission electron microscopy and by freeze-etching technique. Ultrathin sectioning of septate vesicles of the actinomycetal endophyte showed an electron transparent zone, the so-called void area, between the vesicle cell wall and its encapsulation material. This void area was not observed in the freeze-etching replicas of cryoprotected nodular tissue. It is suggested that the void area is the result of the coming-off of the vesicle cell wall from the capsule and that its formation reflects difficulty in fixing the voluminous mature vesicle of the root nodule endophyte.     

Gametogenesis and auxospore development in actinocyclus (bacillariophyta)

cGametogenesis and auxospore development have been studied in detail in surprisingly few centric diatoms. We studied the development of sperm, eggs and auxospores in Actinocyclus sp., a radially symmetrical freshwater diatom collected from Japan, using LM and electron microscopy of living cultures and thin sections. Actinocyclus represents a deep branch of the 'radial centric' diatoms and should therefore contribute useful insights into the evolution of sexual reproduction in diatoms. Spermatogenesis was examined by LM and SEM and involved the formation of two spermatogonia (sperm mother-cells) in each spermatogonangium through an equal mitotic division. The spermatogonia produced a reduced 'lid' valve, resembling a large flat scale with irregular radial thickenings. Sperm formation was merogenous, producing four sperm per spermatogonium, which were released by dehiscence of the 'lid' valve. The sperm were spindle-shaped with numerous surface globules and, as usual for diatoms, the single anterior flagellum bore mastigonemes. One egg cell was produced per oogonium. Immature eggs produced a thin layer of circular silica scales before fertilization, while the eggs were still contained within the oogonium. Sperm were attracted in large numbers to each egg and were apparently able to contact the egg surface via a gap formed between the long hypotheca and shorter epitheca of the oogonium and a small underlying hole in the scale-case. Auxospores expanded isodiametrically and many new scales were added to its envelope during expansion. Finally, new slightly-domed initial valves were produced at right angles to the oogonium axis, after a strong contraction of the cell away from the auxospore wall. At different stages, Golgi bodies were associated with chloroplasts or mitochondria, contrasting with the constancy of Golgi-ER-mitochondrion (G-ER-M) units in some other centric diatoms, which has been suggested to have phylogenetic significance. Electron-dense bodies in the vacuole of Actinocyclus are probably acidocalcisomes containing polyphosphate.     

Cold-sensitive nuclear division arrest mutants of the fission yeast Schizosaccharomyces pombe

Thirteen recessive cold sensitive nuclear division arrest mutants were isolated from the fission yeast Schizosaccharomyces pombe. Twelve unlinked genes were defined; six in chromosome I, three in chromosome II and two in chromosome III. The map positions of three nuclear division arrest genes (nda1, nda2 and nda3) in chromosome II were determined precisely. Together with the previously obtained temperature-sensitive cell division cycle mutations, at least 20 genes appear to control the nuclear division of the fission yeast. Physiological studies indicated that most cold sensitive nda mutants incubated previously at 22 degrees C proceeded with a synchronously normal cell-cycle after temperature shift-up. The morphology of the nuclei and nuclear chromatin region was studied by the 4',6-diamidino-2-phenylindole staining method and by electron microscopy. Each mutant exhibited characteristic nuclear morphology at 22 degrees C, showing the specific blockages. The nda genes seem to control a pathway of structural alterations in the nuclear chromatin region with the order hemisphere, condensed ellipsoid, segregating U-form and separating hemispheres. Two genes, nda2 and nda3, pleiotropically control nuclear division, nuclear location and cell shape. The terminal phenotype of nda2-KM52 is characterized by the nuclear displacement, the absence of a spindle and abnormal locations of spindle pole bodies. The cells of nda3-KM311 were aberrant in shape and contained a partially separated chromatin region with a long spindle. Together with the results of the accompanying paper, we conclude that nda2 and nda3 genes control nuclear and cytoplasmic microtubular organization.     

Pollen development in orchids

Summary Cytokinesis in microsporocytes of moth orchids is unusual in that it occurs simultaneously after meiosis, the cytoplasm does not infurrow in the division planes, and cell plates are deposited in association with centrifugal expansion of phragmoplasts. Microtubules radiating from the nuclear envelopes appear to be of fundamental importance in establishment of division planes. Primary interzonal spindles develop between sister nuclei and interaction of radial microtubules triggers development of secondary interzonal spindles between non-sister nuclei. From three to six or more phragmoplasts, depending upon the arrangement of nuclei in the coenocyte, develop from these postmeiotic arrays. The phragmoplasts consist of co-aligned microtubules and F-actin organized into bundles that are broad proximal to the mid-plane and taper distally. Ultrastructure of the phragmoplast/cell plate reveals that abundant ER is associated with vesicle aggregation and coalescence. Cell plates are deposited in association with phragmoplasts as they expand centrifugally to join the parental wall and/or fuse with one another in the interior of the cell.Abbreviations CLSM confocal laser scanning microscope/microscopy - FITC flnorescein isothiocyanate - PPB preprophase band of microtubules - TEM transmission electron microscope/microscopy     

Wall ultrastructure of an Ediacaran acritarch from the Officer Basin, Australia

Well-preserved organic-walled microfossils referred to as acritarchs occur abundantly in Ediacaran deposits in the Officer Basin in Australia. The assemblages are taxonomically diverse, change over short stratigraphical intervals and are largely facies independent across marine basins. Affinities of this informal group of fossils to modern biota are poorly recognized or unknown, with the exception of only a few taxa. Morphological studies by use of transmitted light microscopy, geochemical analyses and other lines of evidence, suggest that some Precambrian acritarchs are related to algae (including prasinophytes, chlorophytes, and perhaps also dinoflagellates). Limitations in magnification and resolution using transmitted light microscopy may be relevant when assessing relationships to modern taxa. Scanning electron microscopy reveals details of morphology, microstructure and wall surface microelements, whereas transmission electron microscopy provides high-resolution images of the cell wall ultrastructure. In the light of previous ultrastructural studies it can be concluded that the division of acritarchs into leiospheres (unornamented) and acanthomorphs (ornamented) is entirely artificial and has no phylogenetic meaning. Examination of Gyalosphaeridium pulchrum using transmission electron microscopy reveals a vesicle wall with four distinct layers. This multilayered wall ultrastructure is broadly shared by a range of morphologically diverse acritarchs as well as some extant microalgae. The chemically resistant biopolymers forming the comparatively thick cell, together with the overall morphology support the interpretation of the microfossil as being in the resting stage in the life cycle. The set of features, morphological and ultrastructural, suggests closer relationship to green algae than dinoflagellates.     

Mitosis in the dermatophyteMicrosporum canis as revealed by freeze substitution electron microscopy

Summary Mitosis in the dermatophyteMicrosporum canis was studied by freeze substitution and electron microscopy, and analyzed by three dimensional reconstruction from serial sections of the mitotic nuclei. The interphase nucleus has associated nucleus-associated organelle (NAO) on a portion of the outer surface of the nuclear envelope, subjacent to which there was dense intranuclear material. The NAO divided and separated on the envelope, and a spindle was formed. The spindle was composed mostly of microtubules extended between opposite NAOs. Pairing of kinetochores was observed in the spindle from an early stage of development, when chromosomes were not so condensed, and remained unchanged while chromosome condensation proceeded until metaphase. Before the completion of nuclear division, daughter nuclei were connected by a narrow spindle channel, and then the nucleolus, whose structure underwent minimal change during mitosis, was eliminated into the cytoplasm.