THE ULTRASTRUCTURE OF LICHENS. I. A GENERAL SURVEY

The fine structure of 10 lichens was examined. A comparison was made of the storage products of the algal symbiont (Trebouxia) in situ in the desiccated and hydrated states of the lichens. All the Trebouxia phycobionts, with the exception of that in Usnea strigosa, had lipid-containing globules in the pyrenoid. The globules were present in both the hydrated and desiccated conditions. Trebouxia in the hydrated condition contained starch granules in the chloroplast as well as the lipid-containing globules in the pyrenoid. The cell wall of Trebouxia consists of an outer electron-dense layer and an inner electron-light layer. Fungal haustoria (in Lecanora rubina) rupture the outer layer of the algal cell wall and invaginate the inner layer. A thick polysaccharide fibrillar material surrounds the fungal cells. Many bacteria were observed within this material. Septa and lomasomes are described. Ellipsoidal bodies, which appear to be an integral and unique part of the lichen fungal ultrastructure, were observed associated with membrane profiles.     

Ultrastructural Changes During Encystment of Schizopyrenus russelli*

Ultrastructural changes associated with the encystment of Schizopyrenus russelli have been studied by electron microscopy. Before encystment small “black bodies” appear in the cytoplasm and later migrate toward the periphery. The outer cyst wall is secreted at this stage as a thin discontinuous layer which thickens and subsequently becomes continuous. Concomitant with this, the endoplasmic reticulum surrounds the mitochondria. The inner cyst wall later appears as a multilayered structure which presumably is cast off from the plasma membrane. Between the inner and outer layers of the cyst wall, there is a middle, less electron-dense layer wherein extruded cytoplasmic material is found embedded at certain places.     

The fine structure of ascospore wall formation in Sordaria fimicola

Summary The fine structure of ascopore wall development in the pyrenomycete Sordaria fimicola has been studied in asci fixed in either glutaraldehyde-OsO₄ or KMnO₄. Three distinct wall layers are deposited between the outer spore investing membrane and the inner spore plasma membrane which initially delimit each of the eight ascopores. Primary wall deposition occurs initially, followed by the deposition of secondary wall material to the outside of the primary wall. The tertiary wall is initiated as an electron dense layer along the interface between the primary and secondary walls. Pigment accumulates in this region. Increase in overall thickness of the ascospore wall occurs mainly in the secondary and tertiary layers, the former becoming fibrous and gelationous, and the latter multilayered, at maturity.     

ELECTRON MICROSCOPY OF WOOD OF CALLIXYLON AND CORDAITES

Replicas and ultrathin sections of the wood of two Paleozoic genera, Callixylon and Cordaites, were examined with the electron microscope. The pattern of wall layering of Callixylon closely resembles that of extant plants. An electron-dense compound middle lamella markedly thickened at the corners of cells, a thin, electron-transparent S₁ layer of the secondary wall, and a thick, electron-dense, partially decayed S₂ layer of the secondary wall are evident in transverse sections of tracheids. No S₃ layer seems to be present. The structure of the bordered pit-pairs of Callixylon is described in detail. The slitlike outer pit apertures are conspicuously narrower and shorter than the inner pit apertures. Both sections and replicas of the bordered pit-pairs display pit membranes lacking tori. Microfibrillar structure is obscure in both sections and replicas of Callixylon wood. Replicas of the bordered pits of Cordaites wood are very similar to those of Callixylon. Pit membranes lack tori, and microfibrillar structure is not very discernible. Knowledge about the evolution of the torus is summarized. It is postulated that the type of pit membrane of Callixylon and Cordaites, which is very homogeneous in structure and lacks a torus, represents a primitive condition among gymnosperms from which structurally more complex pit membranes and the torus later evolved.     

LIGHT AND ELECTRON MICROSCOPE STUDIES OF THE CELL WALL STRUCTURE OF THE ROOT HAIRS OF RAPHANUS SATIVUS

Dawes , Clinton J., and Edwin Bowler . (U. of California, Los Angeles.) Light and electron microscope studies of the cell wall structure of the root hairs of Raphanus sativus. Amer. Jour. Bot. 46(8): 561–565. Illus. 1959.—The structure and development of the cell wall of the root hair of Raphanus sativus were studied under the light and electron microscopes. The outer layer of the root hair consists of mucilage which covers the entire hair and forms a thick cap at the tip. Beneath the mucilage a thin cuticle covers the inner layers of the cell wall. These layers consist of cellulose microfibrils, varying in pattern, in a granular matrix, presumably pectic in nature. The microfibrils of the outer layer, apparently laid down at the tip, are reticulate in arrangement. In mature regions of the root hair, the wall is thickened by an inner layer of parallel and longitudinally orientated microfibrils. Pores in the cellulose wall are evident and increase in number and size near the base of the hair.     

THE PECTIC LAYER OF THE CELL WALL OF SCENEDESMUS QUADRICAUDA

Further evidence from shadow casting techniques of the empty cells of Scenedesmus quadricauda confirms the structure of the pectic layer presented in an earlier work which was based entirely on reconstruction from thin sections. The structure of the net and props and their relationship are clearly seen and the inner boundary of the pectic layer is demonstrated by staining techniques.     

The chitin-glucan complex ofSaccharomyces cerevisiae

Differentiation of the cell wall ofSaccharomyces cerevisiae at the site of the future bud was followed. A lentil-like structure originates on the inner side of the cell wall during the first phase. At the same time, an electron-dense layer occurs at the boundary between the inner layer of the cell wall and the lentil-like structure. During the second phase granular material is accumulated at the lower side of the lentil-like structure. During the third phase the lentil-like structure is split apart due to proliferation of the granular material resulting in formation of the base of the encircling region. The marked electron-dense layer observed from the first phase is attached to the surface of the encircling region during differentiation of the latter. During the budding proper the outer layers of the cell wall protrude and the end of the encircling region, together with the adjacent electron-dense layer, acquire their definitive appearance of rings, observed as marked electron-transparent and electron-dense tears on ultrathin sections.     

The fungal bladders of the endocyanosisGeosiphon pyriforme,aGlomus-related fungus: cell wall permeability indicates a limiting pore radius of only 0.5 nm

Summary Geosiphon pyriforme, a consortium of aGlomiw-like fungus andNostoc spp., forms syncytial, up to 2 mm long bladders accommodating the endosymbiotic cyanobacteria. The bladders are bordered by an elastic cell wall and have a turgor of about 0.6 MPa, as measured by piercing them with oil filled microcapillaries within different osmolarities of sorbitol. In the presence of certain organic osmolytes in the surrounding medium, the bladders collapsed, i.e., showed cytorrhysis. We studied systematically the cytorrhytic effectivity of the diverse osmolytes in relation to their hydrodynamic molecule radii by a solute-exclusion method with living bladders and those which have been extracted by different methods. The results suggest that the cell wall of the bladders has an unusually small limiting pore size thus representing an effective diffusion barrier for glucose and is virtually impermeable for sucrose for at least 8 h. The pore radii of the cell wall are estimated to be about 0.5 nm. Na₂CO₃ extraction, frequently used to partially extract pectic substances from plant cell walls, strongly increases wall permeability. Electron microscopic observations show an electron-dense outer cell wall layer, perhaps responsible for the low permeability. The finding that the cell wall of theGeosiphon bladders represents an effective osmotic barrier provides not only new insights into the cell physiology ofGeosiphon but may also contribute more generally to a better understanding of the mechanisms of selectivity of transport across the cell walls of AM fungi.Abbreviations AM arbuscular mycorrhiza - DMSO dimethyl sulfoxyde - EDTA ethylenediaminetetraacetic acid - PEG polyethylene glycol - res Einstein-Stokes hydrodynamic radius     

ULTRASTRUCTURAL STUDY ON MICROSPORE WALL MORPHOGENESIS IN ISOETES JAPONICA (ISOETACEAE)

Spore wall morphogenesis of the microspore of Isoetes japonica was studied by transmission electron microscopy. The microspore wall consists of four layers: the perispore, outer exospore, inner exospore, and endospore. The perispore consists of electron-dense materials. The exospore is divided into outer and inner sections, with a large gap between the two. The outer exospore appears as an undulating plate consisting of tripartite lamellae with homogeneous sporopollenin. The inner exospore consists of an accumulation of tripartite lamellae on the microspore cell membrane. Immediately after meiosis, the tripartite lamellae of the outer exospore forms around the microspore. The lamellated inner exospore forms next, which adheres to the cell membrane of the microspore. The deposition of homogeneous sporopollenin material on the tripartite lamellae causes the plates of the outer exospore to thicken. Some homogeneous material may also be deposited on the inner exospore. Lastly, the electron-dense perispore is deposited on the outer exospore, and the electron-lucent endospore forms beneath the inner exospore. We conclude that the lamellae of the outer exospore, inner exospore, and endospore are formed and derived, in that order, from the gametophytic microspore cytoplasm. The homogeneous sporopollenin material of the outer exospore and perispore may be derived from the sporophytic tapetal cytoplasm.     

Ultrastructural aspects of wheat straw degradation by Phanerochaete chrysosporium and Trametes versicolor

The ultrastructural patterns characterizing wheat straw degradation by the ligninolytic fungi Phanerochaete chrysosporium and Trametes versicolor were studied. During fungal attack, the less lignified tissues were degraded first, whereas the xylematic and sclerenchymatic fibers underwent a delayed attack. In straw samples degraded by T. versicolor, partial delignification, defibrillation and swelling of cell walls, often causing separation between primary and secondary walls, were observed. By contrast, the formation of erosions and fissures, with minor lignin removal, characterized the attack to the cell wall by P. chrysosporium. At an advanced stage of decay, KMnO₄ staining demonstrated abundant electron-dense material around hyphae and in the proximity of the cell-wall surface. In the case of P. chrysosporium, spherical black bodies were found in the erosions and fissures produced during fungal attack.     

Yeast Glucan in the Cyst Wall of Pneumocystis carinii

Ultrastructurally, the cyst wall of Pneumocystis carinii consists of an electron-dense outer layer, an electron-lucent middle layer, and an innermost plasmalemma. This is similar in appearance to the cell wall of some yeasts, e.g. Saccharomyces cerevisiae , which consists of an outer dense layer of mannan, a middle lucent layer of β−1,3-glucan (yeast glucan) and an innermost plasmalemma. The cyst wall P. carinii , as well as the cell wall of S. cerevisiae , can be labeled by a variety of methods which stain polysaccharides, such as Gomori's methenamine silver (GMS) and by Aniline blue, a dye which selectively stains β-1,3-glucan. The treatment of P. carinii cysts with Zymolyase, which the key enzyme is β,3-gIucan laminari-pentaohydrolase, results in lysis of the outer 2 layers of the cyst wall and the loss of positive staining by both GMS and Aniline blue. The lysis of elements of the cyst wall of P. carinii is achieved under the same conditions and concentration at which Zymolyase lyses the outer 2 layers of the cell wall of viable cells of S. cerevisiae . These observations indicate that a major component of the cyst wall of P. carinii is β-1,3-glucan.     

Yeast glucan in the cyst wall of Pneumocystis carinii

Ultrastructurally, the cyst wall of Pneumocystis carinii consists of an electron-dense outer layer, an electron-lucent middle layer, and an innermost plasmalemma. This is similar in appearance to the cell wall of some yeasts, e.g. Saccharomyces cerevisiae, which consists of an outer dense layer of mannan, a middle lucent layer of beta-1,3-glucan (yeast glucan) and an innermost plasmalemma. The cyst wall of P. carinii, as well as the cell wall of S. cerevisiae, can be labeled by a variety of methods which stain polysaccharides, such as Gomori's methenamine silver (GMS) and by Aniline blue, a dye which selectively stains beta-1,3-glucan. The treatment of P. carinii cysts with Zymolyase, which the key enzyme is beta-1,3-glucan laminaripentaohydrolase, results in lysis of the outer 2 layers of the cyst wall and the loss of positive staining by both GMS and Aniline blue. The lysis of elements of the cyst wall of P. carinii is achieved under the same conditions and concentration at which Zymolyase lyses the outer 2 layers of the cell wall of viable cells of S. cerevisiae. These observations indicate that a major component of the cyst wall of P. carinii is beta-1,3-glucan.     

Evidence against the presence of fibres or chemically distinct layers in the cell wall ofSaccharomyces

The gross chemical composition of material extracted from yeast cell walls with various solvents or enzymes was studied. Attempts were made to locate these materials in situ by comparing electron micrographs of negatively stained and sectioned cell walls with those of the residues of the extraction procedures. There are at least two chemically distinct species of carbohydrate polymers which can be extracted with strong alkali: one yielding mainly mannose and some amino acid on hydrolysis and the other yielding mannose, glucose and amino acid. The alkali-insoluble material also yielded glucose, mannose and amino acid on hydrolysis but the glucose/mannose ratio was much higher. It was shown that none of these polymers constituted a physically distinct layer in the yeast cell wall. However, there does seem to be a region at the outer surface with distinctive properties. This is not fibrillar in nature and after extraction with ethylene diamine forms a double-layered structure. Materials which react with KMnO₄ to produce an electron-dense material are located throughout the wall but tend to be concentrated in the outer and inner regions. Procedures which remove this material also remove up to 80% of the mannose, 40% of the glucose and 35 % of the protein of the original wall material. It was shown that fibres do not constitute a major fraction of the normal cell wall, except possibly in the region of the bud scars but may be produced fairly readily by certain specific treatments. The classical view of the yeast cell wall with the structural integrity being maintained by a fibrous network of 1–3, 1–6 linked glucose residues is challenged and evidence to support an alternative view is presented.The results in wthis paper were presented to the University of Manchester Institute of Science and Technology by JKB in a Thesis for the degree of M.Sc. (Bowden, 1966). The authors are indebted to Miss C. Backhouse and Miss B. Murphy for help in preparing the electron micrographs.     

MORPHOLOGY AND FINE STRUCTURE OF FISCHERELLA AMBIGUA1

Fischerella ambigua is a branching blue-green alga, the filamentous nature of which is maintained almost entirely by sheath material. Cell division in this organism most closely resembles the septal division found in most unicellular organisms. In all filamentous blue-green algae previously examined with the electron microscope, cell division has resulted from the imagination of the plasma membrane and inner wall layer only; both the middle wall and the outer wall layers remain continuous throughout the length of the filament. In Fischerella, by contrast, the plasma membrane and the inner wall layer invaginate to produce initially 2 cells. However, the middle wall layer, outer wall layer, and sheath also invaginate to separate the daughter cells. The sheath alone remains continuous throughout the length of the filament.     

Electron microscope studies on Leucothrix mucor

Summary Electron microscopic studies of thin sections of filaments, knots, resettes, gonidia, and gonidial-forming filaments of Leucothrix mucor were carried out. The cell wall is typical of gram-negative bacteria, with a double outer layer of variable thickness, a single thin middle layer which is probably peptidoglycan, and a double inner layer which is the cell membrane. The transverse septa of these filaments show two peptidoglycan layers, and no clearly demarked outer layer. During gonidial formation, there is a gradual rounding up of the cells, and the transverse septa become part of the gonidial wall. The cell membrane contains many invaginations, both along the outer wall and along the transverse septa. Thin sections through rosettes show the holdfast as material which is a heavily-staining amorphous material peripheral to the outer wall layer. Sections through knots show highly contorted cell walls, closely appressed. Fibrillar nuclear material, ribosomes, and storage granules can be seen within the cytoplasmic matrix.     

The electron microscopic observation of haustoria of Erysiphe graminis hordei

The fine structure of haustoria ofErysiphe graminis hordei was studied using samples fixed with 3 per cent KMnO₄ or 2 per cent OsO₄. The cell wall of the infected leaves of barley seedlings was extremely electron-dense around the penetration point of this fungus. This may be due to chemical change of components in cell wall by the enzymatic action of the fungus. The cell wall was invaginated towards the cytoplasm at the point of penetration and formed a sheath around the infection hypha. Unknown electron-dense substances were accumulated around the infection hypha outside the sheath. The haustorial cell wall was surrounded with encapsulation and distinguished clearly from the cytoplasm of epidermal cell. The cell wall of the haustorium was very thin and electron-transparent, when compared with that of conidia and hyphae. A septum with a septal pore was observed between the infection hypha and the haustorium. Besides the nucleus, mitochondria, endoplasmic reticula and the like, many kinds of vesicles and specific coiled membraneous structure were found in the haustorium. The origin and the function of the encapsulation remain obscure.

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Zusammenfassung Die Feinstruktur von Haustorien vonErysiphe graminis hordei war untersucht, indem Stücke mit 3 % KMnO₄ oder 2 % OsO₄ fixiert worden sind. Die Zellwand der infizierten Blätter der Gerstenkeimlinge war elektron-dicht um die Eindringungsstelle des Pilzes. Dies mag die Folge der chemischen Veränderung der Komponenten in der Zellwand durch die enzymatische Wirkung des Pilzes sein. Die Zellwand war an der Eindringungsstelle zum Zytoplasma gebogen und hat eine Hülle um die Infektionshyphe gebildet. Unbekannte, elektron-dichte Substanzen waren um die Infektionshyphe außerhalb der Hülle angesammelt. Die Haustorialzellwand war abgegrenzt und war vom Zytoplasma der Epidermalzelle unterscheidbar. Die Zellwand des Haustoriums war dünn und elektron-durchsichtig im Vergleich mit denen der Konidien und Hyphen. Ein Septum mit einer Septalpore war zwischen der Infektionshyphe und dem Haustorium beobachtet. Neben dem Nucleus, Mitochondrien, endoplasmatischen Netz sind mancherlei Blister, spezifische, eingerollte Membranstruktur im Haustorium gefunden worden. Die Herkunft und die Funktion dieser Strukturen blieb ungeklärt.

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Contribution No. 232     

STRUCTURE AND DEVELOPMENT OF WALLS IN FUNARIA STOMATA

The development and structure of the guard cell walls of Funaria hygrometrica Hedw. (Musci) were studied with the light and electron microscopes. The stoma consists of only one, binucleate guard cell as the pore wall does not extend to the ends of the cell. The guard cell wall is thinnest in the dorsal wall near the outer wall but during movement is most likely to flex at thin areas of the outer and ventral walls. The mature wall contains a mottled layer sandwiched between two, more fibrillar layers. The internal wall layer has sublayers with fibrils in axial and radial orientations with respect to the pore. During substomatal cavity formation, the middle lamella is stretched into an electron dense network and into strands and sheets. After stomatal pore formation, the subsidiary cell walls close to the guard cell become strikingly thickened. The functional implications of these results are discussed.     

Fine Structure of Bacillus subtilis : I. Fixation

The fine structure of Bacillus subtilis has been studied by observing sections fixed in KMnO₄, OsO₄, or a combination of both. The majority of examinations were made in samples fixed in 2.0 per cent KMnO₄ in tap water. Samples were embedded in butyl methacrylate for sectioning. In general, KMnO₄ fixation appeared to provide much better definition of the boundaries of various structures than did OsO₄. With either type of fixation, however, the surface structure of the cell appeared to consist of two components: cell wall and cytoplasmic membrane. Each of these, in turn, was observed to have a double aspect. The cell wall appeared to be composed of an outer part, broad and light, and an inner part, thin and dense. The cytoplasmic membrane appeared (at times, under KMnO₄ fixation) as two thin lines. In cells fixed first with OsO₄ solution, and then refixed with a mixture of KMnO₄ and OsO₄ solutions, the features revealed were more or less a mixture of those revealed by each fixation alone. A homogeneous, smooth structure, lacking a vacuole-like space, was identified as the nuclear structure in a form relatively free of artifacts. Two unidentified structures were observed in the cytoplasm when B. subtilis was fixed with KMnO₄. One a tortuous, fine filamentous element associated with a narrow light space, was often found near the ends of cells, or attached to one end of the pre-spore. The other showed a special inner structure somewhat similar to cristae mitochondriales.     

Differences in protodermal cell wall structure in zygotic and somatic embryos of <Emphasis Type="Italic">Daucus carota</Emphasis> (L.) cultured on solid and in liquid media

The ultrastructure, cuticle, and distribution of pectic epitopes in outer periclinal walls of protodermal cells of Daucus carota zygotic and somatic embryos from solid and suspension culture were investigated. Lipid substances were present as a continuous layer in zygotic and somatic embryos cultured on solid medium. Somatic embryos from suspension cultures were devoid of cuticle. The ultrastructure of the outer walls of protodermis of embryos was similar in zygotic and somatic embryos from solid culture. Fibrillar material was observed on the surface of somatic embryos. In zygotic embryos, in cotyledons and root pectic epitopes recognised by the antibody JIM5 were observed in all cell walls. In hypocotyls of these embryos, these pectic epitopes were not present in the outer periclinal and anticlinal walls of the protodermis. In somatic embryos from solid media, distribution of pectic epitopes recognised by JIM5 was similar to that described for their zygotic counterparts. In somatic embryos from suspension culture, pectic epitopes recognised by JIM5 were detected in all cell walls. In the cotyledons and hypocotyls, a punctate signal was observed on the outside of the protodermis. Pectic epitopes recognised by JIM7 were present in all cell walls independent of embryo organs. In zygotic embryos, this signal was punctate; in somatic embryos from both cultures, this signal was uniformly distributed. In embryos from suspension cultures, a punctate signal was detected outside the surface of cotyledon and hypocotyl. These data are discussed in light of current models for embryogenesis and the influence of culture conditions on cell wall structure.     

The cell envelope of Mycobacterium smegmatis: cytochemistry and architectural implications

In sections stained for localizing both carbohydrates (Thiery's method) and lipids (the O.T.O. method), the cell envelope of Mycobacterium smegmatis appeared to consists of an asymmetric cytoplasmic membrane surrounded by a three-layered cell wall. The outer layer of the cytoplasmic membrane was found to contain more glycoconjugate molecules (probably phosphatidyl inositol mannosides) than the inner one. The cell wall consists of the peptidoglycan (the innermost layer) surrounded by a layer containing both arabinogalactan and mycolates (the electron-dense layer), whereas the outermost layer was unstainable. There is clearly a difficulty in reconciling such a cell wall organization with the models so far proposed.