Locomotion of Physarum polycephalum amoebae is guided by a short range interaction with E. coli

Studies of the behavior of Physarum polycephalum amoebae have shown that locomotion of these cells is guided by surfaces composed of aggregated bacteria. Amoebae move readily on both E. coli and agar surfaces. However, when a cell migrating on bacteria encounters an edge of the bacterial surface, the orientation of cell movement changes so that the cell maintains contact with bacteria. Time-lapse cinemicrographic studies employing wild type and mutant cells show that this behavior involves short range interactions between amoebae and bacteria, that it is not dependent on variations in the rate of phagocytosis, and that it is not a simple result of constraints on cell movement imposed by adhesive bonds between amoebae and bacteria. These results provide evidence that guidance of cell locomotion depends on active regulation of the cellular force generating system as the amoebae contact surfaces of varying characteristics and, therefore, suggest that this system is amenable to detailed studies of process involved both in cell-cell recognition and in linking such recognition to regulation of cell movement.     

Formation of cellulose fibrils by gram-negative bacteria and their role in bacterial flocculation

Summary Exocellular fibrils, consisting of true cellulose, were found to be produced by many bacteria. These bacteria have been selected out of a large number of strains isolated from activated sludge on the basis of their flocculent growth habit in liquid medium.The amount of cellulose, present in the bacterial flocs, varied from 1.0 to 4.0%. In addition to strains isolated from activated sludge, like Pseudomonas, Achromobacter, Alcaligenes and Aerobacter, also strains of the genera Rhizobium, Agrobacterium and Azotobacter were found to give flocculent growth due to the formation of cellulose fibrils.Bacterial flocculation in pure cultures of the strains examined was mainly caused by the production of exocellular fibrils. Apparently, the formation of cellulose fibrils seems to be a common property of Gram-negative, floc-forming bacteria, and may not be restricted to Acetobacter xylinum.     

Unequal distribution of DNA-containing organelles in generative and sperm cells of Erythrina crista-galli (Fabaceae)

The generative cell at anthesis in the mature pollen grain of Erythrina crista-galli (Fabaceae) was examined by 4,6-diamidino-2-phenylindole(DAPI)-fluorescence microscopy using the squash method. An unequal, polarized distribution of DNA-containing organelles (plastids and/or mitochondria) within the generative cell was observed in every mature pollen grain examined. Polarization of DNA-containing organelles is obvious when generative cells are freed and assume a spherical shape soon after microspore mitosis, as revealed by fluorescence-microscopic observations of specimens embedded in Technovit 7100 resin and thin-sectioned at different developmental stages. Early establishment of polarized localization of organelles in young generative cells of E. crista-galli and maintenance of this unequal distribution until pollen maturation strongly suggests that the organelles may still be clustered at pollen mitosis. Production of a dimorphic pair of sperm cells, as has been reported in Plumbago zeylanica, was observed in some pollen tubes germinated in vitro. The differentiation of the two sperm cells is discussed in relation to possible preferential double fertilization in angiosperms. Received: 28 July 1999 / Revision accepted: 8 November 1999     

Imperfect repeats in the functional amyloid protein FapC reduce the tendency to fragment during fibrillation

Functional amyloid (FA) is widespread in bacteria and serves multiple purposes such as strengthening of biofilm and contact with eukaryotic hosts. Unlike pathological amyloid, FA has been subjected to evolutionary optimization which is likely to be reflected in the aggregation mechanism. FA from different bacteria, including Escherichia coli (CsgA) and Pseudomonas (FapC), contains a number of imperfect repeats which may be key to efficient aggregation. Here we report on the aggregative behavior of FapC constructs which represent all single, double, and triple deletions of the protein's three imperfect repeats. Analysis of the fibrillation kinetics by the program Amylofit reveals that the removal of these repeats increases the tendency of the growing fibrils to fragment and also generally increases aggregation half‐times. Remarkably, even the mutant lacking all three repeats was able to fibrillate, although fibrillation was much more irregular and led to significantly altered and destabilized fibrils. We conclude that imperfect repeats can promote fibrillation efficiency thanks to their modular design, though the context of the imperfect repeats also plays a significant role.     

Evidence that surface fibrils expressed by Haemophilus influenzae type b promote attachment to human epithelial ceils

Hemophilus influenzae type b is a Gram-negative bacillus that initiates infection by colonizing the upper respiratory tract. Previous studies have established that H. influenzae haemagglutinating pili possess adhesive properties and influence the process of colonization. Additional studies suggest the presence of a second H. influenzae adhesin distinct from haemagglulinating pili. In the present study, we examined a non-piliated H. influenzae type b strain by transmission electron microscopy and visualized occasional short, thin, surface fibrils. Subsequently, we isolated a spontaneous mutant that lacked surface fibrils and was deficient in adherence to cultured human epithelial cells. Using a cloning strategy that exploited this mutant, we isolated a fragment of DNA that promotes in vitro adherence to human epithelial cells when expressed in laboratory strains of Escherichia coli. Mutagenesis of this fragment in a series of H. influenzae type b strains resulted in loss of expression of surface fibrils and a marked decrease in attachment. Furthermore, restoration of surface fibril expression was associated with reacquisition of wild-type levels of adherence. Our results are consistent with the conclusion that H. influenzae type b surface fibrils have adhesive capacity. We speculate that these organelles facilitate colonization of the human respiratory tract.     

Substrate Viscosity Enhances Correlation in Epithelial Sheet Movement

The movement of the epithelium plays vital roles in the development and renewal of complex tissues, from the separation of tissues in the early embryo, to turnover in the homeostasis of the gastrointestinal mucosa. Yet, despite its importance, a clear interpretation of the mechanism for collective motion in epithelial sheets remains elusive. This interpretation is prohibited by the lack of understanding of the relationship between motion and cell-cell contact, and their mediation by the mechanical properties of the underlying substrate. To better mimic physiological substrates that have inherent viscosity, we probe this relationship using polydimethylsiloxane, a substrate whose mechanical properties can be tuned from predominantly elastic to viscous by altering its cross-linking content. We therefore characterize the comparative spatiotemporal correlations in cell velocity during the movement of an epithelial monolayer as a function of the viscoelasticity of the substrate. Our results show that high correlation in cell velocity is achieved when the substrate G″(ω) is ∼0.4 × G′(ω). This correlation is driven by a balance between cell-cell contact and the adhesion and contraction of the extracellular matrix. For G″(ω) > G′(ω), this balance shifts, and contraction of the tissue drives the substrate to flow, further elevating the correlation in movement.     

An IQGAP-related gene is activated during tentacle formation in the simple metazoan Hydra

Differentiation of body column epithelial cells into tentacle epithelial cells in Hydra is accompanied by changes in both cell shape and cell-cell contact. The molecular mechanism by which epithelial cells acquire tentacle cell characteristics is unknown. Here we report that expression of a Hydra homologue of the mammalian IQGAP1 protein is strongly upregulated during tentacle formation. Like mammalian IQGAP, Hydra IQGAP1 contains an N-terminal calponin-homology domain, IQ repeats and a conserved C terminus. In adult polyps a high level of Hydra IQGAP1 mRNA is detected at the basis of tentacles. Consistent with a role in tentacle formation, IQGAP1 expression is activated during head regeneration and budding at a time when tentacles are emerging. The observations support the previous hypothesis that IQGAP proteins are involved in cytoskeletal as well as cell-cell contact rearrangements. Received: 25 January 2000 / Accepted: 2 May 2000     

Organelle movement and fibrillar elements of the cytoskeleton in the angiosperm pollen tube

Summary Continuous observation of organelles and other cytoplasmic inclusions in the older stretches of living pollen tubes of Iris pseudacorus shows that in the more attentuated parts of the protoplast they move along single, mainly longitudinally oriented fibrils, corresponding to those previously isolated from other species and shown to contain bundles of uniformly polarised actin microfilaments. The traffic associated with each fibril is unidirectional, but organelles move along them independently, sometimes with conspicuously different velocities. Larger columns of cytoplasm passing along the tube are associated with several such fibrils, as revealed in occasional discontinuities and also in columns isolated from the tube in suitable medium without fixation. The dimensions of the individual fibrils suggest that the bundles of actin microfilaments are not likely to be enclosed in a unit membrane corresponding to a tonoplast. If so, the nature of the continuous cavities traversed by numerous fibrils in the older parts of the pollen tube requires reappraisal, since these are more likely to be volumes of attentuated cytoplasm comparable with that of the central cavity of the sieve tube than vacuoles of the normal plant-cell type.     

Negative Feedback from Integrins to Cadherins: A Micromechanical Study

The coupling between cell-cell and cell-matrix adhesion systems is known to affect the stability of the adhesive status of cells, as well as tissue cohesion. In this work, we perform quantitative assays of integrin-cadherin cross talk in controlled and reproducible conditions. This is achieved by plating cells on microprinted fibronectin patterns of different sizes, and simulating the formation of an intercellular contact with a microbead coated with E-cadherin extracellular domains and brought to the cell membrane. Using an optical trap, we measure the average rigidity modulus of the E-cadherin bead-cell contact as a function of the contact incubation time and of the cell spreading area. For a given incubation time, this rigidity modulus decreases by three orders of magnitude as the cell-matrix contact area, A, increases from 100 to 700 μm². In a similar way, the dynamics of formation of the bead-cell contact gets slower as this area increases. This is clear evidence for a strong negative feedback from cell-fibronectin onto cell-cell adhesive contacts, for which we discuss some possible mechanisms.     

Variations dans ľexpression du pouvoir oncogène d'Agrobacterium tumefaciens

Variations in the expression of the oncogenic power of Agrobacterium tumefaciens due to interactions between bacteria. The effects of the virulent strain A6 of Agrobacterium tumefaciens after co-culture with non-virulent variants of the same bacterium, or even with other bacterial species (e.g. Escherichia coli), showed that interactions between different strains of bacteria exist. These interactions are expressed as a phenomenon of either enhancement or inhibition, as shown by an increase or a decrease in the weights of tumors induced in decapitated stems of Pisum sativum L. cv. Annonay. These two phenomena depend on the contact time between the bacteria in mixed cultures (type I). With a short contact time between the two bacterial types (one or two generations), infections in decapitated pea stems produced by mixed inocula caused an increase in tumor weight compared with infections induced by inocula of virulent bacteria only. If the contact time was increased to the end of the log phase, a decrease in tumor weight was observed. Clarified supernatant fluids of spent media were also used as culture media (type II) for the virulent A6 bacteria. The stimulatory or inhibitory activity of (a) substance(s) present in these supernatant fluids depended on two variables: culture time of the bacteria A6 in the supernatant fluids and the “age” of the bacterial culture used to prepare them. Weight increase of the tumors was obtained if the proliferating time of the A6 bacteria in the supernatant fluids was short (4 h), or if the super natants were obtained from “young” cultures. Inhibition of the tumor expression occurred if the contact time of A6 bacteria in the supernatant fluids was increased or if the supernatants originated from bacterial cultures at the end of their growth. The in vitro interactions between the two bacterial strains in a mixed culture (type I or type II) were suppressed in the presence of pancreatic ribonuclease. Deoxyribonuclease had no effect. This provides indirect evidence for the action of a ribonucleic acid in the expression of the oncogenic power of a bacterial population of Agrobacterium tumefaciens.     

The modulation of cellular contractility and adhesion by trypsin and EGTA

The relationship of cell to substrate and the organisation of the cellular contractile system has been studied using whole-cell mount transmission electron microscopy (TEM). The cellular response to trypsin is compared with that induced by treatment with the Ca²⁺-specific chelating agent EGTA. Trypsinisation results in a breakdown of the ordered contractile system and both cell-cell and cell-substrate adhesion. Studies with the respiratory inhibitor 2,4 dinitrophenol (DNP) have shown that cellular rounding mediated by trypsinisation is energy independent. The response to EGTA is confluence modulated. Confluent monolayers are induced to contract and detach as sheets, a response related here to the overlapping of the peripheral cytoplasm. Subconfluent cells contract centripetally withdrawing organelles to the perinuclear region. Withdrawal of organelles is accompanied by a redistribution of the contractile system. Contraction results in a rounded cell anchored to the substrate by numerous retraction fibrils. The response to EGTA is energy dependent. The observations suggest that a chelation of Ca²⁺ results in an active contraction of the actomyosin system. We propose a mechanism for this response based on ultrastructural and biochemical characterisation of the actomyosin system.     

Mixed-Species Biofilm Formation by Direct Cell-Cell Contact between Brewing Yeasts and Lactic Acid Bacteria

Mixed-species biofilm was remarkably formed in a static co-culture of Lactobacillus plantarum ML11-11 and Saccharomyces cerevisiae Y11-43 isolated from brewing samples of Fukuyama pot vinegar. Mixed-species biofilm is probably formed by direct cell-cell contact between ML11-11 and S. cerevisiae including Y11-43 and laboratory yeast strains. Scanning electron microscopic observation suggested that the mixed-species biofilm had a thick, bi-layer structure.     

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.     

Subcortical microtubule network separates the periplasm from the endoplasm and is responsible for maintaining the position of accessory nuclei in hymenopteran oocytes

Oocytes of hymenopterans are equipped with peculiar organelles termed accessory nuclei. These organelles originate from the germinal vesicle (oocyte nucleus) and gather preferentially at the anterior pole. To gain insight into the mechanism of uneven (asymmetrical) distribution of accessory nuclei, the organization of the microtubule cytoskeleton in the oocytes of two hymenopterans Chrysis ignita and Cosmoconus meridionator has been studied. It is shown that during late previtellogenesis two networks of microtubules are present along the contact zone between the oocyte and enveloping follicular epithelium. The external one is associated with belt desmosomes connecting neighbouring follicular cells. The internal network is composed of randomly orientated microtubules and separates transparent, organelle-free periplasm from the endoplasm. All cellular organelles and the germinal vesicle are localized in the endoplasm. Accessory nuclei are accumulated in the anterior endoplasm; they always lie in direct contact with the subcortical network. Treatment with colchicine results in the disappearance of the periplasm as well as in the redistribution of cellular organelles including accessory nuclei. Presented findings suggest that subcortical microtubules play an important role in the positioning of accessory nuclei throughout the ooplasm.     

Effects of the mixotrophic flagellate Ochromonas sp. on colony formation in Microcystis aeruginosa

The aim of this study was to investigate the interactions between the cyanobacteria (Microcystis aeruginosa) and the potential grazer (Ochromonas sp.) with regard to colony formation. Two kinds of treatments were carried out: (i) In the dialyse experiment Microcystis aeruginosa and Ochromonas sp. were physically separated by a dialyse tubing. (ii) In the contact experiment interactions between Microcystis aeruginosa, heterotrophic bacteria and Ochromonas sp. in different concentrations were investigated. In one treatment where the predator Ochromonas sp. came in direct contact with Microcystis, aggregates were formed.In the contact experiment, there were some interactions between the predator Ochromonas sp. and the two groups of prey, Microcystis aeruginosa and heterotrophic bacteria. When exposed to a low initial Ochromonas sp. concentration, Microcystis aeruginosa decreased and then remained stable in concentration. Ochromonas sp. switched to feed on heterotrophic bacteria and increased. At a high initial Ochromonas sp. concentration Microcystis was grazed down.     

Electron-cytochemical demonstration of acid phosphatase in saprophytic Claviceps purpurea

p-Nitrophenylphosphate in combination with lead salt technique was used for the cytochemical localization of acid phosphatase (EC 3.1.3.2) in saprophytic submerged culture of Claviceps purpurea Tul. The lead reaction product was found in capsular fibrils, in the newly formed parts of the well wall and in the vacuoles of aged cells (autolysosomes). Phosphatase activity was present also in particulate intracytoplasmatic organelles. The concentric layering of lead deposits in these organelles indicates their relationship to endoplasmic reticulum membranes.Abbreviation Used pNPP p-nitrophenylphosphate     

Microbodies und Diaminobenzidin-Reaktion in den Acetat-Flagellaten Polytomella caeca und Chlorogonium elongatum

Summary In two forms of acetate flagellates, the colourless Volvocale Polytomella caeca and the green Volvocale Chlorogonium elongatum, cell organelles can be demonstrated which are ultrastructurally similar to microbodies of higher organisms. The organelles do not have a close association with the endoplasmic reticulum and are located in the peripheral cytoplasm between the elongated mitochondria. In Polytomella they exhibit more or less spherical profiles in section and have a maximum diameter of approximately 0.2–0.25 . In Chlorogonium the organelles occasionally have an elongated shape and are larger than in Polytomella. Employing the electron microscopic cytochemical reagent diaminobenzidine (DAB)/H₂O₂ to localize the microbodial marker enzyme catalase in these organelles, it was found that no accumulation of the electron-opaque product occurs in the microbodies either at alkaline or neutral pH or at room temperature or 37° C. Only the cristae of mitochondria are stained with the DAB reaction caused by cytochrome oxidase and possibly by a cytochrome peroxidase.Organelles of Polytomella caeca containing catalase or cytochrome oxidase can be separated by rate centrifugation of a crude particulate fraction on a sucrose gradient (Gerhardt, 1971). The particles isolated from the peak of catalase activity show the same fine structural characteristics as the microbodies in situ do. But again, there is no detectable staining of these organelles by the DAB/H₂O₂ reaction.The identity of the microbody-like particles in Polytomella caeca and Chlorogonium elongatum with microbodies in general is deduced despite the negative results in cytochemical localization of catalase in these organelles.     

Inoculum Sources for the Spread of Leaf Scald Disease of Sugarcane Caused by Xanthomonas albilineans in Guadeloupe

Leaf scald of sugarcane, caused by Xanthomonas albilineans, is thought to be spread mainly in infected cuttings and transmitted on infested cutting implements. Several observations made in Guadeloupe indicated that other means of spreading also occur. The dispersal of the pathogen outside sugarcane was investigated with plants inoculated by an antibiotic-resistant marked strain of X. albilineans and with plants naturally infested with wild strains of the pathogen. The bacteria were isolated in water droplets (rain or dew) on the surface of sugarcane leaves at dawn. It was also detected on the surface of dry leaves during the day by leaf imprinting onto a selective culture medium. The bacteria were much more frequently isolated from the surface of symptomatic leaves than from symptomless ones. Aerial dispersal of X. albilineans was investigated by placing Petri dishes containing selective culture medium between sugarcane plants but without direct contact with the leaves. The pathogen was isolated in four out of 270 dishes which were randomly set 3–14 h in a diseased field. These results indicated that the pathogen exuded from the leaves and then was spread by aerial means (rain, insects, …) or by leaf contact. The bacteria were also found in roots and rhizospheric soil of infested sugarcane stools suggesting that X. albilineans could be transmitted by root to root contact or by the soil. Finally, isolations of the pathogen in sugarcane inflorescences were positive. So, fuzz transmission may also occur.     

Diversity in surface colonization behavior in marine bacteria

Using laminar flow chambers and time-lapse video imaging, colonization of surfaces by four marine bacteria revealed a diverse range of morphological characteristics and cell-cell interactions. The strain SW5 formed a compact, multilayered single- and double-cell biofilm on hydrophobic surfaces but developed long multicellular chains on hydrophilic surfaces. The morphologically similar SW8 showed unusual proximal vertical packing of cells on both substrata.Vibrio sp strain S14 exhibited cyclical colonization-detachment events on both substrata.Pseudomonas sp strain S9 initially displayed reversible and then irreversible adhesion apparently triggered by a cell density phenomenon that led to the development of regular microcolonies on both substrata with individual cells translocating between the colonies. The length of time bacteria were exposed to and their density at a surface influenced behavioral traits, with diverse and distinctive species-specific behavioral events.     

Inoculum Sources for the Spread of Leaf Scald Disease of Sugarcane Caused by Xanthomonas albilineans in Guadeloupe

Leaf scald of sugarcane, caused by Xanthomonas albilineans, is thought to be spread mainly in infected cuttings and transmitted on infested cutting implements. Several observations made in Guadeloupe indicated that other means of spreading also occur. The dispersal of the pathogen outside sugarcane was investigated with plants inoculated by an antibiotic-resistant marked strain of X. albilineans and with plants naturally infested with wild strains of the pathogen. The bacteria were isolated in water droplets (rain or dew) on the surface of sugarcane leaves at dawn. It was also detected on the surface of dry leaves during the day by leaf imprinting onto a selective culture medium. The bacteria were much more frequently isolated from the surface of symptomatic leaves than from symptomless ones. Aerial dispersal of X. albilineans was investigated by placing Petri dishes containing selective culture medium between sugarcane plants but without direct contact with the leaves. The pathogen was isolated in four out of 270 dishes which were randomly set 3-14 h in a diseased field. These results indicated that the pathogen exuded from the leaves and then was spread by aerial means (rain, insects,…) or by leaf contact. The bacteria were also found in roots and rhizospheric soil of infested sugarcane stools suggesting that X. albilineans could be transmitted by root to root contact or by the soil. Finally, isolations of the pathogen in sugarcane inflorescences were positive. So, fuzz transmission may also occur.