Phenylalanine ammonia-lyase and chalcone synthase in glands ofPrimula kewensis (W. Wats): immunofluorescence and immunogold localization

Phenylalanine ammonia-lyase (PAL) and chalcone synthase (CHS) were localized by indirect immunofluorescence and immunogold labeling in glands ofPrimula kewensis. Both enzymes were exclusively present in the head cells of the glands. Phenylalanine ammonialyase was located in the regions of the dense tubular endoplasmic reticulum and occasionally found in more or less spherical organelles that have not yet been identified. Furthermore, an appreciable proportion of the enzyme protein was associated with the plasmalemma and the cell wall of the head cell. In contrast, the occurrence of CHS was restricted to the spherical, unidentified cell compartments. Our findings indicate that the gland cells have the potential for flavonoid biosynthesis. When a mutant ofP. kewensis forming structurally intact glands but incapable of farina excretion was studied, neither PAL nor CHS were found in the head cells.Abbreviations CHS chalcone synthase - IgG immunoglobulin G - PAL phenylalanine ammonia-lyase Financial support from the Deutsche Forschungsgemeinschaft and the Fonds der Chemischen Industrie is gratefully acknowledged. We are grateful to Mrs. Karin Schlattmann and Mrs. Susanne Otter for preparing the ultrathin sections and to Mrs. Marianne Opalka for taking the photographs.     

In situ localization of antigens of Histoplasma capsulatum using colloidal gold immune electron microscopy

Histoplasma capsulatum contains multiple antigens, among them the H antigen and M antigen, which are useful in serologic testing for histoplasmosis. We prepared 7 mouse monoclonal antibodies (5 IgG, 2 IgM) to histoplasmin, and compared these with polyclonal histoplasmin antibodies raised in rabbits and mice. Both monoclonal and polyclonal antibodies were high titered by ELISA. Colloidal gold immune electron microscopy (CGIEM) showed that polyclonal antibodies to histoplasmin or H antigen bound at multiple sites in the cell wall, cytoplasm, and nucleus of Histoplasma yeast cells. In contrast, antibodies to M antigen selectively label the cell membrane and antibodies to alkali soluble cell wall antigen label only the cell wall. Polyclonal antibodies cross reacted extensively with other fungi, both by ELISA and CGIEM. Monoclonal antibodies stained only cytoplasmic epitopes, but also cross reacted with other fungi by electron microscopy. Only periodate treated H antigen elicited polyclonal antibodies which were more specific than those of untreated H antigen or histoplasmin.     

Differentiation of the membrane system in the cells of imaginai discs

Summary Imaginal discs from developing larvae of the fly Calliphora erythrocephala fixed in permanganate or osmium tetroxide and embedded in Epon 812 were observed by electron microscopy. When the larval growth ceases, the differentiation manifests itself through an enlargement of the endoplasmic reticulum, by which continuous membrane contact is established between all cell organelles. During the same time mitochondria swell up and transform into lipid granules and the intercellular contacts weaken.I am indebted to Mrs Mariann Carleson and Miss Brita Nilsson for technical aid.     

Antifungal mechanism of antibacterial peptide, ABP-CM4, from Bombyx mori against Aspergillus niger

Antibacterial peptide, CM4 (ABP-CM4), a 35 amino acid peptide from Chinese silkworm—Bombyx mori, displayed a strong antifungal activity against Aspergillus niger, Trichoderma viride and Gibberella saubinetii. Scanning electron microcopy showed that the morphology of conidia became more irregular and swelled when treated with ABP-CM4 at its minimal inhibitory concentration (MIC) of 8 μM. A cell wall regeneration assay indicated that the plasma membrane was the prime target of ABP-CM4 action. Confocal laser scanning microscopy showed that the cytoskeleton of A. niger was destroyed when treated with ABP-CM4 at 8 μM. Furthermore, transmission electron microscopy showed that the membrane and the cellular organelles of fungus were disrupted and there were many vacuoles in the fungal cellular space after the treatment with ABP-CM4. A gel-retardation assay showed that ABP-CM4 bound the DNA of A. niger. Our results suggest that ABP-CM4 exerts its antifungal activity by disrupting the structure of cell membranes and the cytoskeleton and interacts with the organelles, such as the mitochondrion and with the DNA in the fungal cell, subsequently resulting in cell death.     

Ultrastructure of the epithelium from the ovary wall of Dendrochirus brachypterus (Pteroidae,Teleostei)

Summary The inner epithelium of the ovary wall in Dendrochirus brachypterus does not take part in egg production, as it does in other teleosts. The epithelium consists of columnar cells rich in mitochondria and secretory organelles. The distal ends of these cells hang free in the ovary lumen, separated from each other and densely covered by large microvilli. During reproduction the epithelium secretes large amounts of mucus that forms an envelope around the eggs produced from a spongy stroma of the ovary, and keeps the spawn afloat for 24 h.Thanks are due to Mrs. H. Segal and Mr. N. Sharon for technical assistance, and Mr. D. Fridman, for help during the collection of the fish. Also appreciation is given to the technicians of the Electron Microscopy Laboratory of Tel-Aviv University for help in preparation of electron and scanning microscope figures     

Die Feinstruktur vonChloromonas rosae Ettl

Zusammenfassung Die Feinstruktur vonChloromonas rosae wird sowohl mit dem Lichtals auch mit dem Elektronenmikroskop untersucht und verglichen. Diese Art ist lichtoptisch schon lange gut bekannt, so daß ein Vergleich der taxonomischen Merkmale mit den elektronenmikroskopischen Aufnahmen ohne Schwierigkeiten möglich ist. Im Elektronenmikroskop kommen viele Details zum Vorschein, vor allem die Struktur der Membran und der Papille, die Geißelinsertion und die Anordnung der übrigen Organellen. Diese Details können aber die Taxonomie der GattungChloromonas vorläufig nicht weitgehend beeinflussen. Für die Taxonomie bleibt auch weiterhin die mit dem Lichtmikroskop feststellbare Zellmorphologie maßgebend. Untersuchungen mit dem Elektronenmikroskop können jedoch bei äußerst kleinen Arten von besonderem Wert sein, wo es gilt, Organellen deutlicher zu zeigen.

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Summary The fine structure ofChloromonas rosae as shown by light optical as well as electron optical investigations is compared. Light microscopically, this species has been known well for a long time, so that taxonomic features may be compared to electron microscopic photographs without difficulty. In the electron microscope many details show up, especially the structures of membrane and papilla, the insertion of the flagella and the arrangement of the other organelles. For the present, however, these details cannot have much influence on the taxonomy of the genusChloromonas. Cell morphology as established by light microscopy will be decisive for taxonomy until further notice. It is with extremely small species that electron microscopic investigations can be of special value, where the main point is to show organelles more clearly.

     

Comparative observations of ultrastructure of five species of Candida

An electron microscopic comparison was made of five species ofCandida, namely:C. guilliermondii, C. krusei, C. parapsilosis, C. stellatoidea andC. tropicalis. The cell wall, plasma membrane and the cytoplasm with its organelles were described. The cell wall ofC. tropicalis was twice as thick as the cell wall in the other species.C. krusei appeared with distinct, rather elaborate wall sculpturing, a feature not pronounced in the other four species. A single nucleus with nucleolus appeared only in micrographs ofC. guilliermondii andC. krusei. At the same time, large central electron-luscent area (vacuole) appeared in the cells ofC. guilliermondii, C. parapsilosis andC. stellatoidea. The cytoplasm ofC. tropicalis was characterized by a granular appearance. Budding cells and pseudohyphae appeared similar to single cells in their general organelles. Such organelles in species studied were similar to these reported for other yeasts. These include: mitochondria, lipid granules, endoplasmic reticulum, ribosomes and vacuoles.Southwest Foundation for Research and Education, San Antonio, Texas.In partial fulfillment of the requirement of course work for Master of Science, Incarnate Word College, San Antonio.     

Immunohistochemical characterization of the thymic microenvironment

Summary The epithelial framework of the human thymus has been studied in parallel by immunohistochemical methods at the light- and electron-microscopic levels. Different monoclonal antibodies were used, reacting with components of the major histocompatibility complex, keratins, thymic hormones and other as yet antigenically undefined substances, which show specific immunoreactivities with human thymus epithelial cells.The electron-microscopic immunocytochemical observations clearly confirm microtopographical differences of epithelial cells not only between the thymic cortex and medulla, but also within the cortex itself. At least four subtypes of epithelial cells could be distinguished: 1) the cortical surface epithelium; 2) the main cortical epithelial cells and thymic nurse cells; 3) the medullary epithelial cells; and 4) the epithelial cells of Hassall's corpuscles.The various epithelial cell types of the thymus display several common features like tonofilaments, desmosomes and some surface antigens as demonstrated by anti-KiM3. In other respects, however, they differ from each other. The cortical subtype of thymic epithelial cells including the thymic nurse cells shows a distinct pattern of surface antigens reacting positively with antibodies against HLA-DR (anti-HLA-DR) and anti-21A62E. Electron-microscopic immunocytochemistry with these antibodies clearly reveals a surface labeling and a narrow contact to cortical thymocytes particularly in the peripheral cortical regions. An alternative staining pattern is realized by antibodies to some antigens associated with other subtypes of thymic epithelial cells. Medullary epithelial cells as well as the cortical surface epithelium react likewise positively with antibodies to special surface antigens (anti-Ep-1), to special epitopes of cytokeratin (anti-IV/82), and to thymic hormones (anti-FTS). The functional significance of distinct microenvironments within the thymus provided by different epithelial cells is discussed in view of the maturation of T-precursor cells.Glossary of Abbreviations Anti-X anti-X antibody - APUD-cells amine precursor uptake and decarboxylation (gastro-intestinal endocrine cells) - DAB diamino-benzidine - DMSO dimethyl sulfoxide - FTS facteur thymique sérique - HLA-A, B, C human leucocyte antigen, A, B, C-region related - HLA-DR human leucocyte antigen, D-region related - IDC interdigitating cell - MHC major histocompatibility gene complex - PBS phosphate-buffered saline - TNC thymic nurse cell This investigation was supported by grants from the Deutsche Forschungsgemeinschaft, and its Sonderforschungsbereich 111Fellow of the Alexander von Humbold-Stiftung, Institute of Pathology, University of Würzburg, Federal Republic of GermanyThe authors appreciate the contribution of human thymus tissue from Professor Alexander Bernhard, Abteilung kardiovasculäre Chirurgie der Universität Kiel; the gift of monoclonal antibodies from Dr. M.J.D. Anderson, Dr. M. Dardenne and Dr. H.J. Radzun; and the excellent technical assistence of Mrs. O.M. Bracker, Mrs. H. Hansen, Mrs. R. Köpke, Mrs. M. v. Kolszynski, Mrs. J. Quitzau, Mrs. H. Siebke, and Mrs. H. Waluk     

Accumulation of organelles at the ends of interrupted axons

Summary Proximal and distal stumps of the sciatic nerve of rats were examined with the light and electron microscope in the course of 48 hours following nerve crush. On both sides of the lesion organelles accumulate in axons beyond regions disorganized by injury. A stretch of clear axoplasm filled with fine granules usually separates the cone of accumulating particles from the damaged part of the fibre. From two hours onwards closely packed vesicles, tubules, mitochondria and other organelles form dense pellets which fill up the whole lumen of the fibre. Further away from the fibre tip organelles are stranded at the circumference only, whereas the central core is occupied by neurofilaments. In a number of fibres no pellets are observed and only a moderately increased network of axoplasmic reticulum is seen at the fibre ends.Measurements on isolated fibres have shown that the length of the pellet increases with time on both sides of the lesion up to 18 hours after crush; thereafter the elongation is arrested in the distal stump, while in the proximal stump it continues further at a slower rate.The authors wish to acknowledge gratefully the technical assistance of Mrs. M. Sobotková, Mr. M. Doubek, Mrs. J. Waryszewska and Mrs. B. Lwowska.     

The cytoplasmic organization of hyphal tip cells in the fungusAllomyces macrogynus

Summary Light and transmission electron microscopy were used to examine hyphal tip cells of the fungusAllomyces macrogynus (Chytridiomycetes). A well defined apical body, i.e., Spitzenkörper, was observed at the extreme apex of hyphal cells. This distinctive, spherical cytoplasmic region consisted of a granular matrix devoid of ribosomes and most organelles. To our knowledge this is the first report describing such a structure in hyphae of an aseptate fungus. Vesicles (45–65 nm diameter) were concentrated in the peripheral cytoplasm of the apex, while relatively few were observed within the Spitzenkörper. Filasomes, spherical patches of dense fibrillar material containing a microvesicle core, were abundant in the apical regions near the plasma membrane. Microtubules traversed the Spitzenkörper at various angles and were in close association with the plasma membrane. Microfilaments were observed as individual elements in the cytoplasm or were organized into bundles. Individual microfilaments were frequently in close association with the plasma membrane, vesicles and microtubules. In the immediate subapical region mitochondria, multivesicular bodies, microbodies, Golgi equivalents and nuclei were abundant.Abbreviations CW cell wall - F filasome - M mitochondria - N nucleus - PM plasma membrane - TEM transmission electron microscopy     

Die Feinstruktur der Zellwand und Cytoplasmamembran von Clostridium nigrificans,dargestellt mit Hilfe der Gefrierätz- und Ultradünnschnittechnik

Zusammenfassung Der mit Hilfe der Gefrierätztechnik dargestellte Feinbau der Zellwand und Cytoplasmamembran von Clostridium nigrificans wurde mit den Ergebnissen der chemischen Fixation verglichen. Die Zellwand von chemisch fixierten Zellen zeigt einen Aufbau aus drei stark und zwei schwach elektronenstreuenden Schichten, wobei die innerste, der Cytoplasmamembran angrenzende Schicht nicht immer darstellbar ist. Die Cytoplasmamembran hat eine asymmetrische Elementarmembran-Struktur. Mit Hilfe der Gefrierätztechnik konnte die Zellwand in drei Schichten aufgespalten werden: Einer äußeren aus globulären, rechtwinkelig geordneten, etwa 9 nm messenden Partikeln aufgebauten Schicht und zwei darunter liegenden, 15 und 5 nm dicken Schichten. Die Cytoplasmamembran wird in jungen Kulturen vollkommen, in alten teilweise mit 5–15 nm großen Teilchen bedeckt. An Stellen wo die Teilchen abgespalten wurden oder entsprechend locker angeordnet waren, konnte die Oberfläche der Cytoplasmamembran sichtbar gemacht werden. Sie ist sowohl auf der der Zellwand als auch auf der dem Cytoplasma zugekehrten Seite mit systemlos verteilten, scheinbar verschieden tief eingebetteten Teilchen bedeckt.

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The fine structure of the cell wall and cytoplasmic membrane of Clostridium nigrificans demonstrated by means of freeze-etching and chemical fixation techniques

Summary A comparison was made between the results obtained using the freeze-etching technique in demonstrating the fine structure of the cell wall and the cytoplasmic membrane of Clostridium nigrificans with those using the chemical fixation technique. In chemically fixed cells, the cell wall appears to consist of three dense layers separated by two layers of low electron scattering power, whereby it is not always possible to observe that layer immediately bordering on the cytoplasmic membrane. The cytoplasmic membrane has an asymmetrical unit membrane structure. It was possible, to separate the cell wall in three distinct layers using the freeze-etching technique. The outermost is composed of globular, rectangularly arranged particles, approximataly 9 nm in size, the two inner layers are 15 and 5 nm wide respectively. The cytoplasmic membrane is covered with particles 5 to 15 nm in size, in younger cultures completely, in older cultures partially. On those places where the particles have been split off or where they are loosly arranged, it was possible to observe the surface of the cytoplasmic membrane. It appears to be covered with unsystematically scattered particles imbedded at different depths, not only on that side turned to the cell wall but also on that facing the cytoplasm.

     

猕猴桃茎尖超低温保存过程中超微结构观察

应用透射电镜观察了猕猴桃组培苗茎尖细胞在玻璃化法超低温保存过程中的超微结构变化.研究发现:在预培养、PVS2脱水处理过程中,茎尖细胞内液泡逐渐变多、变小,质壁分离愈加显著,表明细胞的抗冻力增强;在随后的冷冻和解冻过程中,部分细胞的质壁分离更加严重,细胞壁与细胞膜之间出现液腔,细胞器变得模糊,有些细胞的细胞膜、甚至细胞壁撕裂,细胞腔内留下破碎的细胞膜和细胞残片,细胞结构破坏严重,这可能是导致材料在恢复培养中死亡的原因之一;部分细胞经过7d的恢复培养后,细胞器清晰,细胞膜完好并紧贴细胞壁,细胞中央出现较大的液胞,具有与对照相似的结构特征,最终存活下来并能够再生植株.     

Assembly of the subcellular parts of <Emphasis Type="Italic">Bryopsis hypnoides</Emphasis> Lamouroux into new protoplasts

The chloroplasts, mitochondria, and protoplasm devoid of mature chloroplasts (PMC) of Bryopsis hypnoides Lamouroux were isolated by low-speed and sucrose density centrifugation. The PMC aggregated in artificial seawater, and then protoplasts without mature chloroplasts (PtMCs) were formed. Transmission electron microscopy and cytochemical studies indicated that there were mitochondria, nuclei, vesicles, and other small cell organelles in the PtMCs. Scanning electron microscopy showed that there were holes on the surface of 1-h PtMCs and then fewer holes on the surface of 24-h PtMCs, suggesting that a healing process occurred. The plasma membrane was formed over the surface of the PtMCs. However, the cell wall was not regenerated, and the newly formed PtMCs were ruptured and died in 3 days. Light intensity during alga maintenance before use influenced significantly (one-way ANOVA, P < 0.0001) on the number of PtMCs formed; the highest number of PtMCs was formed at 20μmol/(m² s). When isolated chloroplasts were transferred into seawater, there were only two or three chloroplasts aggregated together. However, isolated mitochondria and the mixed six layers of cell organelles (separated by sucrose density centrifugation) could not aggregate in the artificial seawater. This indicates that the conjunction of cell organelles is important for their aggregation. Published in Russian in Fiziologiya Rastenii, 2009, Vol. 56, No. 1, pp. 123–130. The text was submitted by the autors in English.     

Fine Structure of the Fat Body and its Bacteroids in Blattella germanica (Blattodea)

The abdominal fat body of the cockroach Blattella germanica contains three characteristic cell types—trophocytes, bacteriocytes and urate cells—which have been investigated by electron microscopy. The trophocytes are rich in lipid droplets of different sizes; glycogen, rough endoplasmic reticulum and mitochondria are also abundant. In females immediately after eclosion, the trophocytes contain a greater number of lipid droplets, some of which have different electron density; glycogen and cytoplasmic organelles are clearly reduced. The bacteriocytes hold rod-like and spherical bacteroids, which are encapsulated by a vacuolar membrane; they show a thin cytoplasmic membrane and an evident cell wall surrounded by a membrane-like outer envelope. The bacteroids appear to be dividing either by transverse partition or by budding. The urate cells, adjacent to the bacteriocytes, are characterized by complex urate vacuoles delimited by a double layer-structure.     

Regions of lead uptake inLemna minor plants and localization of this metal within selected parts of the root

Investigations were carried out to determine the sites of lead uptake within the frond and the root ofLemna minor. With the sodium rhodizonate four regions favoured in lead uptake were distinguished: the frond region between the base and the node, the basal part of the root, and the regions at the proximal and distal ends of the root cap. For analysis in electron microscope only the root regions were chosen. The highest rate of lead uptake was found in the basal part of the root. Lead was present in the apoplast of this region after 5 min of exposure and was observed in the stelar cells after 30 min of incubation. Lead deposits were detected mostly in the cell walls adjacent to the plasma membrane and in the lumen of several endomembrane compartments - the endoplasmic reticulum (ER), dictyosomal vesicles, nuclear envelope and the vacuoles. Lead induced changes of cell ultrastructure; an increase in the number of membraneous structures, swelling of ER cisternae and distortion of the dictyosomal cisternae were observed after 2 to 6 h of exposure. We wish to thank Mrs. G. Winiecka for her technical assistance in preparing the photographs.     

THE DEMONSTRATION OF THE SUCCINIC DEHYDROGENASE SYSTEM IN BACILLUS SUBTILIS USING TETRANITRO-BLUE TETRAZOLIUM COMBINED WITH TECHNIQUES OF ELECTRON MICROSCOPY

Activity of the succinic dehydrogenase system was studied in Bacillus subtilis utilizing combined techniques of cytochemistry and electron microscopy. Organisms were incubated in a medium containing tetranitro-blue tetrazolium (TNBT) which served as an electron acceptor. Enzymatic activity, as evidenced by deposition of TNBT-formazan, was found on membranous organelles associated with the cytoplasmic membrane and septal plasma membrane, the nuclear area, and the plasma membrane. Flagella, ~190 A in diameter, with thorn-like projections protruded through the cell wall. Tangential-oblique sections of the cell wall showed many pores ~220 A in diameter with a center-to-center spacing of ~450 A.     

Morphology and phylogeny of a new wall‐less freshwater volvocalean flagellate,Hapalochloris nozakii gen. et sp. nov. (Volvocales,Chlorophyceae)

New strains of a wall‐less unicellular volvocalean flagellate were isolated from a freshwater environment in Japan. Observations of the alga, described here as Hapalochloris nozakii Nakada, gen. et sp. nov., were made using light, fluorescence, and electron microscopy. Each vegetative cell had two flagella, four contractile vacuoles, and a spirally furrowed cup‐shaped chloroplast with an axial pyrenoid, and mitochondria located in the furrows. Based on the morphology, H. nozakii was distinguished from other known wall‐less volvocalean flagellates. Under electron microscopy, fibrous material, instead of a cell wall and dense cortical microtubules, was observed outside and inside the cell membrane, respectively. Based on the phylogenetic analyses of 18S rRNA gene sequences, H. nozakii was found to be closely related to Asterococcus, Oogamochlamys, Rhysamphichloris, and “Dunaliella” lateralis and was separated from other known wall‐less flagellate volvocaleans, indicating independent secondary loss of the cell wall in H. nozakii. In the combined 18S rRNA and chloroplast gene tree, H. nozakii was sister to Lobochlamys.     

伊曲康唑对皮肤癣菌形态学影响研究

目的观察皮肤癣菌在伊曲康唑作用下的形态学变化。方法应用美国CLSI制订的标准M38-A方案进行伊曲康唑对皮肤癣菌的体外药敏试验,测定最小抑菌浓度（MIC）,将伊曲康唑作用前后的皮肤癣菌分别制成标本,在光学显微镜、扫描电子显微镜和透射电子显微镜下观察形态学变化。结果伊曲康唑作用于皮肤癣菌后,在光学显微镜下菌丝变得弯曲、短粗,顶端和局部出现膨大;扫描电子显微镜下菌丝变得弯曲、短粗、干瘪,顶端和局部出现膨大,有不规则分支,表面粗糙,有大小不等的凹陷;透射电子显微镜下菌丝变得皱缩,有凹陷,双层细胞壁结构消失或不完整,细胞膜不连续,皱缩细胞膜和细胞壁之间及胞浆内出现许多小的高电子密度颗粒,细胞器也变得不清晰。结论伊曲康唑使皮肤癣菌的形态发生明显变化。     

The Ultrastructure of Polytomella agilis*

SYNOPSIS Motile cells and cysts of Polytomella agilis, obtained over the entire growth cycle, were examined by electron microscopy. In typical late log phase cells there is a concentric arrangement of the internal organelles around the centrally located nucleus. Lying just beneath the plasma membrane is a peripheral band of elongate mitochondria. Numerous well defined Golgi bodies are also distributed around the nucleus. Vesicles associated with the Golgi body increase in size with distance from the secretory edges of the organelle. Cytoplasmic membranes with associated ribosomes are found between the mitochondrial and Golgi regions. A layer of slender membrane-limited structures is located near the mitochondrial layer. These organelles, which resemble proplastids, become highly branched during late log and early stationary phase, reaching maximum development in late stationary and early pre-cyst stages. Large storage granules of varying density are found within the cell. The PAS-positive granules have been isolated and shown to contain starch. There is an increase in the amount of this storage material as the cells enter the stationary phase. The remainder of the cytoplasmic matrix is finely granular and contains numerous free ribosomes except in the region of the anterior papilla. Four flagella arise from basal bodies at the anterior end of the cell. The cyst is characterized by a thick multi-layered cell wall whose electron density obscures the limiting plasma membrane. Large storage granules are located close to and often in contact with the periphery of the cell, suggesting their involvement in the process of cell wall deposition. Altho mitochondria can still be seen in the mature cyst, other cytoplasmic organelles often appear atypical. The mature cyst has an irregular profile possibly due to shrinkage from dehydration.     

Electron Microscopy of Young Candida albicans Chlamydospores

One- to three-day-old cultures of Candida albicans bearing chlamydospores were grown and harvested by a special technique, free of agar, and prepared for ultramicrotomy and electron microscopy. These young chlamydospores exhibited a subcellular structure similar to that of the yeast phase, e.g., cytoplasmic membrane, ribosomes, and mitochondria. Other structural characteristics unique to chlamydospores were a very thick, layered cell wall, the outer layer of which was continuous with the outer layer of the suspensor cell wall and was covered by hair-like projections; membrane bound organelles; and large lipoid inclusions. Only young chlamydospores less than 3 to 4 days old exhibited these ultrastructural characteristics.