Teliospores of smut fungi teliospore walls and the development of ornamentation studied by electron microscopy

Summary The walls of mature teliospores and the development of ornamentation, as seen by transmission electron microscopy, are described for 37 genera of smut fungi, based on observations of ca. 120 species and on literature. Structural diversity of mature teliospore walls is due to differences in spore wall layers forming the spore wall (endosporium, middle layer, exosporium, ornamentation) and to different elements forming the ornamentation (exosporium, ornaments, sheath, hyphal wall, adjacent fungal cells, material of the host). During teliosporogenesis the outer layers are usually deposited first. At the beginning of the formation of the ornamentation the plasma membrane may be smooth or undulated carrying the developing ornaments on its tips or in its depressions. The ornamentation of some genera appears similar when seen by scanning electron microscopy, but can be the product of different developmental patterns (e.g., warts of species ofFarysia, Tilletia, andUstilago), however, warty and reticulate ornamentation can both be produced by similar developmental processes (shown, e.g., for species ofCintractia andTilletia). Typical structures of the mature teliospore wall and developmental patterns based on homologous similarities are described for the following groups of genera or species:Macalpinomyces, Melanopsichium, Sporisorium, andUstilago infecting members of the family Poaceae;Kuntzeomyces, Testicularia, andTrichocintractia; Anthracoidea, Cintractia, Heterotolyposporium piluliforme, andTolyposporium junci; Glomosporium, Sorosporium, andThecaphora; Conidiosporomyces, Erratomyces, Ingoldiomyces, Neovossia, Oberwinkleria, andTilletia; Entyloma, and genera of the Doassansia group;Liroa, Microbotryum, Sphacelotheca, Ustilago infecting dicotyledons, andZundeliomyces; Aurantiosporium, Fulvisporium, andUstilentyloma. Special characteristics of the teliospore wall were observed for the generaDermatosorus, Doassinga, Entorrhha, Farysia, Mycosyrinx, Rhamphospora, and some species ofTolyposporium.Part 165 in the series Studies in Heterobasidiomycetes from the Botanical Institute, University of Tübingen     

Teliospores of smut fungi general aspects of teliospore walls and sporogenesis

Summary The concept and nomenclature for the elements of teliospore walls in smut fungi are presented and a survey of teliosporogenesis is given, as seen by light and transmission electron microscopy. Four developmental types are distinguished: the Ustilago, Microbotryum, Tilletia, and Entorrhiza type. In the Ustilago type, sporogenous hyphae are completely segmented into teliospore initials which are embedded in a hyaline matrix formed by gelatinised hyphal walls (found in species ofAnthracoidea, Cintractia, Heterotolyposporium, Kuntzeomyces, Macalpinomyces, Melanopsichium, Sporisorium, Testicularia, Tolyposporium junci, Trichocintractia, and species ofUstilago infecting members of the family Poaceae). In the Microbotryum type, septate sporogenous hyphae are also completely segmented into teliospore initials, however, they are not surrounded by a hyaline matrix (Microbotryum, Sphacelotheca, Ustilago spp. infecting dicotyledons). A yeast-like budding of teliosporogenic cells is observed for some species ofMicrobotryum, Sphacelotheca, andUstilago infecting dicotyledons. In the Tilletia type, teliospores differentiate locally in the sporogenous hyphae, in an apical or intercalary position, without a hyaline matrix (Conidiosporomyces, Doassinga, Entyloma, Erratomyces, Ingoldiomyces, Neovossia, Oberwinkleria, Rhamphospora, Tilletia). In all these types, the teliospore initials first develop a hyaline sheath under which the ornamentation, the exosporium, sometimes a middle layer, and the endosporium are successively deposited by the fungal cell. In the Entorrhiza type, the teliospores develop inside vital host cells with the wall of the sporogenous hypha included into the teliospore wall. The fungus develops a middle layer and an electron-transparent endosporium inside the hyphal wall while a layer forming the ornamentation is deposited onto the hyphal wall, probably by vesicles of dictyosomes of the host cell.Part 164 in the series Studies in Heterobasidiomycetes from the Botanical Institute, University of Tübingen     

Effect of liming on spore germination,germ tube growth and root colonization by vesicular-arbuscular mycorrhizal fungi

Summary The effect of soil acidity on spore germination, germ tube growth and root colonization of vesicular-arbuscular mycorrhizal (VAM) fungi was examined using a Florida Ultisol. Soil samples were treated with 0, 4, 8 and 12 meq Ca/MgCO₃/100 g soil and each lime level received 0, 240, and 720 ppm P as superphosphate. Corn (Zea mays L.) was planted in the soil treatments, inoculated with eitherGlomus mosseae orGigaspora margarita spores and grown for 31 days. Acid soil inhibits mycorrhizal formation byG. mosseae through its strong fungistatic effect against the spores. The dolomitic lime increased mycorrhizal formation by both fungal species.G. margarita is much less sensitive to acidic conditions thanG. mosseae. Al ions are a very important component of the fungistatic property against the VAM symbiosis. VAM fungus adaptation may be important for plants growing on infertile acid soils if soil inoculation with these fungi is to contribute significantly to low-input technology for tropical agricultural systems.     

Effect of cytochalasin A on actin distribution in the fission yeastSchizosaccharomyces pombe studied by fluorescent and electron microscopy

Summary Actin distribution and ultrastructure of the fission yeastSchizosaccharomyces pombe treated with cytochalasin A (CA) were investigated by fluorescence microscopy using rhodamine-conjugated phalloidin (rh-ph) and freeze substitution electron microscopy. Among the cytochalasins tested, CA was most effective and at 5 g/ ml inhibited the appearance of the actin ring at the cell equator at the stage prior to septum formation and the accumulation of actin dots at the septum-forming site both in wild-type cells and the mutantcdc 11, which is defective in septum formation at restrictive temperature. Freeze substitution electron microscopy of CA-treated cells revealed the displacement and morphological alteration of cytoplasmic vesicles and dictyosomes within 30 min and the appearance of dense bodies in the cytoplasm. A sub-population of cytoplasmic vesicles and dictyosomes were insensitive to CA and maintained their original structure. An electron less dense layer containing filamentous material was noted beneath the plasma membrane and thought to be the area of heavy actin patches stained with rh-ph at the cells ends. These results suggest that CA disrupted an actin network that normally maintains the organization of the secretory pathway involving dictyosomes and vesicles.     

The granule-containing cell somata in the superior cervical ganglion of the rat,as studied by a serial sampling method for electron microscopy

Summary The surface of 4 granule-containing cells, in a cluster within the rat superior cervical ganglion, was studied by a serial sampling technique for electron microscopy. The result shows that all the 4 cells receive one, or three afferent synaptic boutons from the preganglionic fibers impinging upon their somata, and a somatic efferent synapse exists at two locations on each soma of the 2 of these cells. The postsynaptic element of the efferent synapse is observed to be represented by non-vesiculated and vesiculated segments of dendrites, soma and a possible axon collateral of the adrenergic principal neuron of the ganglion. There is a remarkably constant development of the attachment plaque between the granule-containing cells themselves, representing 1.7–2.3% of surface area for each cell. The surface area exposed to the extracellular space (covered only by a basal lamina) varies from 0.1 to 2.3% of the total perikaryal surface of the 4 cells. A tendency is noted that those cells without efferent synapses possess a more extensive area exposed to extracellular space than those forming somatic efferent synapse to the postganglionic elements.It is a pleasure to acknowledge the advice and encouragement of Professor A. Yamauchi throughout this work. I thank Mr. K. Kumagai and Miss K. Tsushida for their technical assistance.     

Gonadotropin production and release in female goldfish (Carassius auratus) after administration of pimozide and an LHRH analogue as studied by electron microscopy and radioimmunoassay

Summary The effect of pimozide and an LHRH-analogue (LHRH-A) on gonadotropic cells of the goldfish pituitary gland were described qualitatively and quantitatively. A scale of four categories was devised to reflect various ultrastructural appearances of the cells. Experimental animals were divided into a control group, a group injected with LHRH-A alone, pimozide alone, and groups receiving these two substances in combination. Fish injected with the single substance were killed 12 h after injection while the groups receiving the combined treatments were killed at 4, 12 and 48 h. Serum levels of gonadotropin measured by radioimmunoassay were used to indicate whether an increase in hormone release had occurred. An immunocytochemical technique, the protein A-gold procedure, assured that the cells studied were gonadotropes. The control group showed variation in the profiles of gonadotropic cells. The single treatment groups showed some increase in secretory inclusions. At 4 h after injection the combined treatment caused a significant increase in hormone granules; at 12 and 48 h there was a gradual decrease in content of secretory products, and an increase in vacuolization. The results indicate that the combined pimozide and LHRH-A treatment stimulated gonadotropin production as well as release.     

Early developmental stages of two actinosporeans,Raabeia and Aurantiactinomyxon (Myxozoa), as detected by light and electron microscopy

The development of actinosporeans in their oligochaete host proceeding pansporocyst formation is relatively well documented, however, phases preceding it are not as well known. The initial stages in the development of two actinosporeans, Raabeia type 1 of Oumouna et al. [Parasitol. Res. 2002] and Aurantiactinomyxon pavinsis (Ormières, 1968) Marquès [Languedoc, Universite des Sciences et Techniques, Dissertation, 1984] from schizogony to gametogony and sporogony are described. Both actinosporeans begin their development as multinucleate stages near the basal lamina of the oligochaete intestine. Proximal to these stages and between the host epithelium cells are uninucleate cells whose nuclei divide to produce binucleate cells. These divide mitotically to produce cells with four nuclei which then undergo plasmotomy to yield a tetracellular stage and the first phase in pansporocyst formation. From the uninucleate stage to the tetranucleate stage, the cell membrane of the parasite is associated closely via finger-like projections with the intestinal epithelial and glandular cells of the host.     

Effects of two mitosis inhibitors (Colchicine and Vinblastine) on the distribution and axonal transport of noradrenaline storage particles,studied by fluorescence and electron microscopy

Summary The lumbar sympathetic ganglia and the interganglionic interconnecting nerves of untreated rats and rats treated with Colchicine (COL) or Vinblastine (VIN) were studied with the help of the Falck-Hillarp fluorescence technique and electron microscopy. Both in untreated and drug treated rats there was a good correlation between the distribution of noradrenaline (NA) specific fluorescence and granular vesicles supporting the previous view that the granular vesicles represent the main intraneuronal NA storage sites. The granular vesicles were present both in the cell bodies—mainly in the peripheral part of the cytoplasm— and in the axons of untreated rats. After local application of COL or VIN on the ganglia there was a marked increase in fluorescence intensity and number of granular vesicles in many cell bodies. Often increased number of granular vesicles were found in the neighbourhood of the Golgi apparatus, in which region only few such vesicles are found in untreated rats. In some cell bodies high numbers of granular vesicles could be found all over the cytoplasm.When applied locally to axons the mitosis inhibitors caused a marked accumulation of fluorescence and granular vesicles—and other cell organelles like mitochondria and tubules of the endoplasmic reticulum-proximal to the site of application.A prominent feature both in cell bodies and axons of drug treated rats were large bundles of neurofilaments running through the cytoplasm. In the axons these filaments were often localized to the central part of the axon and surrounded by vesicles and tubules. Microtubules, on the other hand, which are rather numerous in cell bodies and axons of untreated rats seemed to be reduced in number after COL or VIN treatment, especially in those axons in which large amounts of subcellular organelles had accumulated.The present findings are discussed with respect to intraneuronal transport of NA and possible mechanisms behind this transport. It is suggested that the accumulation of fluorescence and granular vesicles after application of mitosis inhibitors is due to an interruption of the centrifugal transport of NA granules. The increased numbers of granular vesicles in the neighbourhood of the Golgi apparatus suggest that granular vesicles are produced in this part of the cytoplasm. This does not exclude a local formation of granular vesicles in other parts of the neuron. Furthermore, the possibility is discussed that the interruption of the transport is related to the increased number of neurofilaments and a possible decrease or disarrangement of microtubules. This discussion is based on previous suggestions that microtubules are involved in intracellular transport mechanisms and on recent findings that COL and VIN bind to proteins specific for microtubules.This study has been supported by grants from the Swedish Medical Research Council (B70-14X-2887-01; B71-14X-2887-02A; B71-14P-3262-01 A; B70-14X-2207-04; B71-14X-2207-05A; K70-40P-3045-01A), from Magnus Bergwalls Foundation, from Wilhelm and Martina Lundgrens Foundation, from the Medical Faculty, University of Göteborg.For generous supply of vinblastine (Velbe^®) we thank Eli Lilly Ltd.The skilful technical assistance of Mrs Kirsten Collin, Mrs Waldraut Hiort and Mr Pär-Anders Larsson is gratefully acknowledged.     

Study of ectoparasitism of ultramicrobacteria of the genus <Emphasis Type="Italic">Kaistia</Emphasis>, strains NF1 and NF3 by electron and fluorescence microscopy

Transmission electron and fluorescence microscopy was used to study the character of the interaction of free-living ultramicrobacterial (UMB) strains NF1 and NF3, affiliated with the genus Kaistia, and seven species of gram-positive and gram-negative heterotrophic bacteria. Strains NF1 and NF3 were found to exhibit parasitic activity against gram-positive Bacillus subtilis and gram-negative Acidovorax delafildii. UMB cells are tightly attached to the envelopes of the victim cells and induce their lysis, thus demonstrating the features of typical ectoparasitism. The selectivity of parasitism of the studied UMB to the victim bacteria has been shown: only two soil microorganisms of the seven test objects, B. subtilis ATCC 6633 and an aerobic gramnegative bacterium A. delafildii 39, were found to be sensitive to UMB attack. Other bacteria (Micrococcus luteus VKM Ac-2230, Staphylococcus aureus 209-P, Pseudomonas putida BS394, Escherichia coli C 600, and Pantoea agglomerans ATCC 27155) were not attacked by UMB. It was established for the first time that free-living UMB may be facultative parasites not only of phototrophic bacteria, as we have previously demonstrated [1], but of heterotrophic bacteria as well. The UMB under study seem to play an important role in the regulation of the quantity of microorganisms and in the functioning of microbial communities in some natural ecotopes.