The effect of pH and K+ on appressorium formation byUromyces appendiculatus urediospore germlings

Uromyces appendiculatus germlings attached to a plastic surface and differentiating in response to contact with inductive ridges formed appressoria most efficiently in the pH range 5.5–6.5. Formation of appressoria was inhibited by increased concentrations of Ca²⁺ and K⁺.     

Cytoskeletal organization during xylem cell differentiation

The water and mineral conductive tube, the xylem vessel and tracheid, is a highly conspicuous tissue due to its elaborately patterned secondary-wall deposition. One constituent of the xylem vessel and tracheid, the tracheary element, is an empty dead cell that develops secondary walls in the elaborate patterns. The wall pattern is appropriately regulated according to the developmental stage of the plant. The cytoskeleton is an essential component of this regulation. In fact, the cortical microtubule is well known to participate in patterned secondary cell wall formation. The dynamic rearrangement of the microtubules and actin filaments have also been recognized in the cultured cells differentiating into tracheary elements in vitro. There has recently been considerable progress in our understanding of the dynamics and regulation of cortical microtubules, and several plant microtubule associated proteins have been identified and characterized. The microtubules have been observed during tracheary element differentiation in living Arabidopsis thaliana cells. Based on this recently acquired information on the plant cytoskeleton and tracheary element differentiation, this review discusses the role of the cytoskeleton in secondary cell wall formation.     

Regulation of melanin biosynthesis during appressorium formation inColletotrichum lagenarium

Regulation of melanin biosynthesis in relation to appressorium differentiation ofColletotrichum lagenarium was investigated. When spores of the parent strain 104-T were incubated at 24°C, appressorial pigmentation started at 6 h of incubation and was preceded by appressorim swelling; appressoria were darkly pigmented at 12 h of incubation. The same time course of appressorial pigmentation was observed in albino mutant 79215 when scytalone, a natural precursor of melanin biosynthesis, was applied before the swelling of appressoria. In accordance with this result, [¹⁴C]scytalone was not incorporated into germlings of albino mutant 79215 before the swelling of appressoria. Cycloheximide applied 1 h or more after incubation of spores of the parent strain 104-T, or of albino mutant 79215 treated with scytalone, inhibited neither appressorium formation nor appressorial pigmentation. These results indicate that enzymes involved in melanin biosynthesis subsequent to scytalone are preexisting enzymes or synthesized as inactive forms during 1 h of incubation, and that they are activated during appressorium differentiation. In addition, an early step(s) prior to scytalone in the melanin biosynthesis of appressoria was temperature sensitive; when colorless appressoria of the parent strain 104-T formed during 6 h of incubation at 24°C were postincubated at 32°C, the appressoria did not melanize, whereas application of scytalone to the postincubation at 32°C permitted melanization of the appressoria. Also, albino mutant 79215 formed melanized appressoria during postincubation at 32°C in the presence of scytalone. These results indicate that high temperatures inhibit melanin biosynthesis by inhibiting one or more steps prior to scytalone synthesis.     

Cytoskeletal organization at the postsynaptic complex

Postsynaptic densities and the adjacent cytoskeleton were examined in deep-etched, unfixed slices of guinea pig anteroventral cochlear nucleus. The postsynaptic density seen in conventional thin sections corresponds to a meshwork of 4-nm filaments associated with intramembrane particles at the postsynaptic active zone of inhibitory as well as excitatory synapses. These filaments intermesh with a lattice of 8- to 9-nm microfilaments, tentatively identified as F- actin, that is concentrated under the postsynaptic density. We postulate that the meshwork of 4-nm filaments anchors receptors to the adjacent microfilament lattice; this extended postsynaptic complex may limit the mobility of receptors and help maintain the curvature of the postsynaptic membrane.     

Cytoskeletal pattern changes during branch formation in a centrifugedAdiantum protonema

A protonemal branch was induced on a side wall of a fern filamentous protonema by cell centrifugation and subsequent polarized-red light irradiation as described in a previous paper (Wada 1995, J. Plant Res. 108: 501–509). Changes in microtubule (MT) and microfilament (MF) patters during the branch development were observed under fluorescence microscopy. A ring-like band of cortical MTs (MT-ring) and MFs similar to a preprophase band or a subapical ring structure (Murataet al. 1987) appeared transiently at the future branching site before cell swelling, the first visible step of branch formation. At this stage, the nucleus was located far from the branching site and the MT-ring appeared to be connected to the nucleus by endoplasmic MFs as well as with endoplasmic MTs. The MT-ring disappeared when cell wall swelling occurred. When the cell wall swelling began, a fan-like pattern of cortical MTs emanating from the new growing tip was established and the MTs reached the opposite flank of the protonema. When a new branch started to elongate and the nucleus moved into the branch, a faint subapical ring of MTs appeared at the subapical part of the new branch. Strands of MTs and MFs emanating from the nuclear front end reached a part of the subapical ring.     

Modeling the formation of root apices

The formation of new root apices from small groups of cells with different cellular patterns has been simulated using an existing model based on growth tensors. To generate an apex, a steady growth field was used. The pattern of cells evolved to approach the steady state. Two extreme types of progressions have been obtained : one leading to an apex with a single or a few apical cells, and the other to an apex with a quiescent centre. The change of structure while applying a steady growth tensor indicates that development may involve a succession of discrete growth tensors.     

Electron microscopic observation of cell wall structure during appressorium formation in Colletotrichum lagenarium

Summary The formation of cell walls during the appressorium formation inColletotrichum lagenarium was observed by electron microscope on the materials prepared by replicas and sectioning. The outer layer of conidia cell walls ruptured at the time of germination and the inner layer bulged out to form a germ tube. The germ tubes and primordia of appressoria had smooth surface and were consisted of one-layered cell wall. However, as the appressorium matured, the electron dense materials appeared on the outer surface of the cell wall which grew into granules. These granules are believed to form the outer layer of appressoria. The under side of the appressorium in contact with the glass surface showed a round pore.Contribution No. 191.     

Cytoskeletal organization of a cloned hemopoietic stromal cell line during attachment and spreading

The cell membrane of a cloned murine bone marrow stromal cell line D2XRII was extracted in situ using Triton X-100 detergent and the cytoskeletal structure studied during the process of adherence and spreading. During this process, three zones can be identified in the cytoplasm: the perinuclear zone, which was the fixed part of the cell; the peripheral mixed filamentous zone, which formed the core of long cytoplasmic projections; and an outer zone, which formed the boundary of cytoplasmic projections and contained only intermediate filaments. The process of spreading appeared to originate from very long strips of microfilaments emanating from the second zone, crossing the width of the outer zone, and extending beyond for a long distance. The second and third zones then appeared to "stream out" around the axis of this strip, and in this fashion the cytoplasm spreads over the substratum.     

Cytoskeletal organization: whirling to the beat

Dense populations of microtubules driven by axonemal dynein form large vortices, providing insights into how simple interactions between individuals can give rise to large-scale coordinated movement, such as that seen in schools of fish and flocks of birds.     

Cytoskeletal changes during generative cell division and sperm formation inTradescantia virginiana

Summary Cytoskeletal organization and chromosome behavior were studied inTradescantia generative cells prior to and during sperm formation using in vitro grown pollen tubes and fluorescence staining methods. Before pollen germination, the crescent-shaped generative cell contains a reticulate microtubule (Mt) system. The cell elongates dramatically after germination, and its Mts assume a helical to longitudinal arrangement. Chromosome condensation is evident approximately 3hr after germination. Kinetochores appear as dark interruptions in the Mt array, and thus seem to attach directly to interphase fibers. No metaphase plate typical of other cells is observed with either DAPI or anti-tubulin staining. Instead, the chromosomes adopt a twisted or braided arrangement, with kinetochores distributed along the length of the cell and kinetochore fibers linked to each other and to surrounding fibers. Anaphase is characterized by a staggered, overlapping separation of chromosomes and by elongation of Mt branches connecting opposing kinetochore fibers. Cytokinesis appears to utilize a furrowing process; a phragmoplast or cell plate was never seen. As a result of these events, the sperm directly inherit their cytoskeleton from generative cell Mts involved in division. No actin fibers are observed at any stage using rhodamine-phalloidin staining. The results are discussed in terms of other reports on sperm formation, possible mitotic and cytokinetic mechanisms, and past distinctions between Mt arrays in higher plant somatic cells.Abbreviations CD cytochalasin D - DAPI 46-diamidino-2-phenyl-indole - DMSO dimethylsulfoxide - K-fiber kinetochore fiber - Mf microfilament - Mt microtubule - PPB preprophase Mt band - RP rhodamine phalloidin     

Proteome analysis of rice blast fungus (Magnaporthe grisea) proteome during appressorium formation

We used two-dimensional gel electrophoresis (2-DE) to identify the proteins that are induced in the rice blast fungus Magnaporthe grisea during appressorium formation. Proteins were extracted from conidia that had germinated on hydrophilic glass plates or from germinated and appressoria-forming conidia on leaf wax-coated hydrophobic glass plates after 4, 8, and 12 h of incubation. Differentially expressed protein spots during appressorium formation were confirmed from gels after 2-DE analysis where proteins had been labeled with (35)S methionine and stained with silver. Internal amino acid sequencing identified five proteins among several proteins induced during appressorium formation. Two denoted as M. grisea proteasome homolgues (MgP1 and MgP5) were 20S proteasome alpha subunits. The remaining three were scytalone dehydratase (SCD), and serine carboxypeptidase Y (CPY). None of the five have been reported previously in the rice blast fungus apart from SCD. We further investigated the role the alpha subunit of 20S proteasome plays in appressorium formation. We confirmed by Western blot analysis that MgP5 is highly expressed during appressorium formation and found that it is also markedly induced by nitrogen- and carbon-starvation, in particular by the former. These observations suggest that the 20S proteasome may be involved in remobilizing storage proteins, which then help to build the appressorium. Thus, fungal proteome analysis may provide important clues about developmental changes such as the generation of the appressorium.     

MoCDC14 is important for septation during conidiation and appressorium formation in Magnaporthe oryzae

As a typical foliar pathogen, appressorium formation and penetration are critical steps in the infection cycle of Magnaporthe oryzae. Because appressorium formation and penetration are closely co‐regulated with the cell cycle, and Cdc14 phosphatases have an antagonistic relationship with cyclin‐dependent kinases (CDKs) on proteins related to mitotic exit and cytokinesis, in this study, we functionally characterized the MoCDC14 gene in M. oryzae. The Mocdc14 deletion mutant showed significantly reduced growth rate and conidiation. It was also defective in septum formation and nuclear distribution. Septation was irregular in Mocdc14 hyphae and hyphal compartments became multi‐nucleate. Mutant conidia often showed incomplete septa or lacked any septum. During appressorium formation, the septum delimiting appressoria from the rest of the germ tubes was often formed far away from the neck of the appressoria or not formed at all. Unlike the wild‐type, some mutant appressoria had more than one nucleus at 24 h. In addition to appressoria, melanization occurred on parts of the germ tubes and conidia, depending on the irregular position of the appressorium‐delimiting septum. The Mocdc14 mutant was also defective in glycogen degradation during appressorium formation and appressorial penetration of intact plant cells. Similar defects in septum formation, melanization and penetration were observed with appressorium‐like structures formed at hyphal tips in the Mocdc14 mutant. Often a long fragment of mutant hyphae was melanized, together with the apical appressorium‐like structures. These results indicate that MoCDC14 plays a critical role in septation, nuclear distribution and pathogenesis in M. oryzae, and correct septum formation during conidiogenesis and appressorium formation requires the MoCdc14 phosphatase.     

Cytology of teliospore germination and basidiospore formation inUromyces appendiculatus var.appendiculatus

Summary The cytology of teliospore germination and basidiospore formation inUromyces appendiculatus var.appendiculatus was characterized with light and fluoroscence microscopy. Meiosis of the diploid nucleus occurred in the metabasidium. The four haploid daughter nuclei migrated into the basidiospore initials where they underwent a post meiotic mitosis. Each basidiospore was delimited from the meatabasidium by a septum at the apex of the sterigma. Seventy-five percent of mature basidiospores were binucleate, 24.5% uninucleate, and 0.5% trinucleate. Mature, released basidiospores measured 16×9 m, were smooth-surfaced, and reniform to ovate-elliptical in shape.This study represents portion of a dissertation submitted by the senior author to the Faculty of Biology of the University of Constance in March, 1983, in partial fulfillment of the requirements for the degree of Doctor of Natural Sciences (Dr. rer. nat.).     

Calcium-regulated appressorium formation of the entomopathogenic fungusZoophthora radicans

Summary The fungusZoophthora radicans (Zygomycetes: Entomophthorales) requires external Ca²⁺ for appressorium formation but not for conidial germination. The number of appressoria formed depends on the Ca²⁺ concentration of the medium. At low [Ca²⁺] (100 pM) nuclear division and germ tube growth are significantly reduced compared to higher Ca²⁺ concentrations (10 and 1,000 M). By contrast, neither external K⁺ nor external Cl^– is needed for germination or appressorium formation. Treatment of conidia with a Ca²⁺-antagonist, Nd³⁺, and a Ca²⁺-channel blocker, nifedipine, inhibits appressorium formation, showing that a Ca²⁺ influx is required for appressorium formation. Furthermore, the partial yet saturating inhibition by nifedipine and complete inhibition by Nd³⁺ indicates that at least two kinds of Ca²⁺ channels are involved in appressorium formation. A contribution of intracellular Ca²⁺ to the signal transduction chain for the formation of appressoria is demonstrated by the inhibitory effect of the intracellular Ca²⁺ antagonist TMB-8. The calmodulin antagonists R24571, TFP, W-7, and W-5 inhibit appressorium formation at concentrations which have no effect on germination. The data presented in this paper are consistent with the hypothesis that a Ca²⁺/calmodulin system is involved in regulating appressorium formation. However, since the direct effects of the drugs were not specifically tested on their proposed binding sites, we leave room for alternative hypotheses that have yet to be formulated.Abbreviations A-9-C 9-anthracenecarboxylic acid - DAPI 4,6 diamino-2-phenylindole - EGTA ethylene glycol bis(-aminoethylether)-N,N-tetraacetic acid - HEPES N-2-hydroxyethylpiperazine-N-2-ethanesulfonic acid - H-7 N-(2-methylamino)ethyl-5-isoquino-linesulphonamide dihydrochloride - IC₅₀ concentration of inhibitor that causes 50% inhibiton - R24571 (calmidazolium) 1-[bis-(4-chlorophenyl)methyl]-3-[2,4-dichloro--(2,4-dichlorobenzyloxy)phenethyl]-imidazolium chloride - TEA tetraethylammonium - TFP (trifluoperazine) 10-[3-(4-methylpiperazine-1-yl)-propyl]-2-trifluomethylphenothiazine - TMB-8 8-(diethylamino)octyl 3,4,5-trimethoxybenzoate hydrochloride - W-5 N-(6-aminohexyl)-1-naphthalene-sulfonamide - W-7 N-(6-aminohexyl)-5-chloro-1-naphthalenesulfonamide     

Ultrastructural changes associated with the haustorial mother cell septum during haustorium formation inUromyces phaseoli var.vignae

Protoplasma - The ultrastructural features of developing haustoria and associated haustorial mother cell septa were examined in the cowpea rust fungus,Uromyces phaseoli var.vignae. Significant...