Your search keyword '"Oded Yarden"' showing total 17 results

1. AlteringNeurospora crassaMOB2A exposes its functions in development and affects its interaction with the NDR kinase COT1

Author

Oded Yarden, Liran Aharoni-Kats, She Chen, and Einat Zelinger

Subjects

0301 basic medicine, NDR kinase, Kinase, 030106 microbiology, Mutant, Crassa, Conidiation, Biology, biology.organism_classification, Microbiology, Cell biology, Neurospora crassa, law.invention, 03 medical and health sciences, 030104 developmental biology, law, Phosphorylation, Suppressor, Molecular Biology

Abstract

The Neurospora crassa Mps One Binder (MOB) proteins MOB2A and MOB2B physically interact with the Nuclear Dbf2 Related (NDR) kinase COT1 and have been shown to have overlapping functions in various aspects of asexual development. Here, we identified two N. crassa MOB2A residues, Tyr117 and Tyr119, which are potentially phosphorylated. Using phosphomimetic mob-2a mutants we have been able to establish that apart from their previously described roles, MOB2A/B are involved in additional developmental processes. Enhanced conidial germination, accompanied by conidial agglutination, in the phosphomimetic mutants indicated that MOB2A is a negative regulator of germination. Thick-section imaging of perithecia revealed slow maturation and a lack of asci alignment in the mutant strains demonstrating a role for MOB2A in sexual development. We demonstrate that even though MOB2A and MOB2B have some overlapping functions, MOB2B cannot compensate for the roles MOB2A has in conidiation and germination. Altering Tyr residues 117 and 119 impaired the physical interactions between MOB2A and COT1, most likely contributing to some of the observed effects. As cot-1 and the phosphomimetic mutants share an extragenic suppressor (gul-1), we concluded that at least some of the effects imposed by altering Tyr117 and Tyr119 are mediated by the NDR kinase.

Published

2018

2. Differences in the responses of melon accessions to fusarium root and stem rot and their colonization byFusarium oxysporumf. sp.radicis-cucumerinum

Author

Marcel Maymon, Uzi Saar, Stanley Freeman, Yaakov Tadmor, Menahem Edelstein, Eduard Belausov, Oded Yarden, G. Orgil, Yosef Burger, R. Cohen, and Meital Elkabetz

Subjects

Fusarium, biology, Melon, Inoculation, food and beverages, Xylem, Plant Science, Horticulture, biology.organism_classification, Fusarium oxysporum, Botany, Genetics, Colonization, Cultivar, Stem rot, Agronomy and Crop Science

Abstract

Fusarium root and stem rot caused by the fungus Fusarium oxysporum f. sp. radicis-cucumerinum is a major disease in greenhouse cucumbers. Over the past decade, the disease has been documented in melon greenhouses in Greece, and recently it has been sporadically recorded in greenhouse melons in Israel. Variations in disease response were found among 41 melon accessions artificially inoculated with the pathogen: 10 accessions were highly susceptible (90–100% mortality), 23 exhibited an intermediate response (20–86%) and eight were resistant (0–4%). Two melon accessions – HEM (highly resistant) and TAD (partially resistant) – were crossed with the susceptible accession DUL. The responses of the three accessions and F1 crosses between the resistant and susceptible parents were evaluated. HEM contributed higher resistance to the F1 hybrid than TAD. Roots of susceptible and resistant accessions were 100 and 79% colonized, respectively, following artificial inoculation. However, only susceptible plants showed colonization of the upper plant tissues. Microscopic evaluation of cross sections taken from the crown region of the susceptible DUL revealed profuse fungal growth in the intercellular spaces of the parenchyma and in xylem vessels. In the resistant cultivar HEM, very little fungal growth was detected in the intercellular spaces of the parenchyma, and none in the xylem or any other vascular tissue. Finding resistant accessions may create an opportunity to study the genetics of resistance inheritance and to develop molecular markers that will facilitate breeding resistant melon cultivars.

Published

2014

3. Changes in atmospheric CO2influence the allergenicity ofAspergillus fumigatus

Author

Oded Yarden, Jordan Peccia, Yinon Rudich, Karen C. Dannemiller, Naama Lang-Yona, and Yishai Levin

Subjects

Fungal growth, Allergy, Nitrogen, Climate Change, Fungus, Real-Time Polymerase Chain Reaction, medicine.disease_cause, Mass Spectrometry, Microbiology, Conidium, Aspergillus fumigatus, Fungal Proteins, chemistry.chemical_compound, Allergen, Respiration, medicine, Humans, Environmental Chemistry, skin and connective tissue diseases, Antibodies, Fungal, General Environmental Science, Global and Planetary Change, Growth medium, Ecology, biology, Antibodies, Monoclonal, Allergens, Carbon Dioxide, Immunoglobulin E, Spores, Fungal, biology.organism_classification, medicine.disease, Carbon, Gene Expression Regulation, chemistry, Chromatography, Liquid

Abstract

Increased susceptibility to allergies has been documented in the Western world in recent decades. However, a comprehensive understanding of its causes is not yet available. It is therefore essential to understand trends and mechanisms of allergy-inducing agents, such as fungal conidia. In this study, we investigated the hypothesis that environmental conditions linked to global atmospheric changes can affect the allergenicity of Aspergillus fumigatus, a common allergenic fungal species in indoor and outdoor environments and in airborne particulate matter. We show that fungi grown under present-day CO2 levels (392 ppm) exhibit 8.5 and 3.5 fold higher allergenicity compared to fungi grown at preindustrial (280 ppm) and double (560 ppm) CO2 levels, respectively. A corresponding trend is observed in the expression of genes encoding for known allergenic proteins and in the major allergen Asp f1 concentrations, possibly due to physiological changes such as respiration rates and the nitrogen content of the fungus, influenced by the CO2 concentrations. Increased carbon and nitrogen levels in the growth medium also lead to a significant increase in the allergenicity. We propose that climatic changes such as increasing atmospheric CO2 levels and changes in the fungal growth medium may impact the ability of allergenic fungi such as A. fumigatus to induce allergies.

Published

2013

4. Inactivation of Snt2, a BAH/PHD-containing transcription factor, impairs pathogenicity and increases autophagosome abundance in Fusarium oxysporum

Author

Stanley Freeman, Oded Yarden, and Youlia Denisov

Subjects

Subtraction hybridization, fungi, Mutant, Crassa, Soil Science, Virulence, Plant Science, Biology, biology.organism_classification, Microbiology, Neurospora crassa, Gene product, Fusarium oxysporum, Agronomy and Crop Science, Molecular Biology, Wilt disease

Abstract

The soil-borne, asexual fungus Fusarium oxysporum f.sp. melonis (FOM) is a causal agent of muskmelon wilt disease. The current study focused on the most virulent race of FOM-race 1,2. The tagged mutant D122, generated by Agrobacterium tumefaciens-mediated transformation, caused the delayed appearance of initial wilt disease symptoms, as well as a 75% reduction in pathogenicity. D122 was impaired in the gene product homologous to the Snt2-like transcription factor of Schizosaccharomyces pombe. Involvement of snt2 in the early stage of FOM pathogenesis and its requirement for host colonization were confirmed by targeted disruption followed by quantitative reverse transcription-polymerase chain reaction analysis of snt2 expression in planta. Δsnt2 mutants of FOM and Neurospora crassa exhibited similar morphological abnormalities, including a reduction in conidia production and biomass accumulation, slower vegetative growth and frequent hyphal septation. In N. crassa, snt-2 is required for sexual development, as Δsnt-2 mutants were unable to produce mature perithecia. Suppressive subtraction hybridization analysis of the D122 mutant versus wild-type isolate detected four genes (idi4, pdc, msf1, eEF1G) that were found previously in association with the target of rapamycin (TOR) kinase pathway. Expression of the autophagy-related idi4 and pdc genes was found to be up-regulated in the Δsnt2 FOM mutant. In N. crassa, disruption of snt-2 also conferred a significant over-expression of idi4.

Published

2011

5. Pleurotus ostreatus manganese-dependent peroxidase silencing impairs decolourization of Orange II

Author

Oded Yarden, Tomer M. Salame, and Yitzhak Hadar

Subjects

Pleurotus, biology, Bioengineering, biology.organism_classification, Applied Microbiology and Biotechnology, Biochemistry, Molecular biology, Reverse genetics, Gene expression, biology.protein, Gene family, Pleurotus ostreatus, Versatile peroxidase, Gene, Biotechnology, Peroxidase

Abstract

Decolourization of azo dyes by Pleurotus ostreatus, a white‐rot fungus capable of lignin depolymerization and mineralization, is related to the ligninolytic activity of enzymes produced by this fungus. The capacity of P. ostreatus to decolourize the azo dye Orange II (OII) was dependent and positively co‐linear to Mn2+ concentration in the medium, and thus attributed to Mn2+‐dependent peroxidase (MnP) activity. Based on the ongoing P. ostreatus genome deciphering project we identified at least nine genes encoding for MnP gene family members (mnp1–9), of which only four (mnp1–4) were previously known. Relative real‐time PCR quantification analysis confirmed that all the nine genes are transcribed, and that Mn2+ amendment results in a drastic increase in the transcript levels of the predominantly expressed MnP genes (mnp3 and mnp9), while decreasing versatile peroxidase gene transcription (mnp4). A reverse genetics strategy based on silencing the P. ostreatus mnp3 gene by RNAi was implemented. Knock‐down of mnp3 resulted in the reduction of fungal OII decolourization capacity, which was co‐linear with marked silencing of the Mn2+‐dependent peroxidase genes mnp3 and mnp9. This is the first direct genetic proof of an association between MnP gene expression levels and azo dye decolourization capacity in P. ostreatus, which may have significant implication on understanding the mechanisms governing lignin biodegradation. Moreover, this study has proven the applicability of RNAi as a tool for gene function studies in Pleurotus research.

Published

2009

6. Cell elongation and branching are regulated by differential phosphorylation states of the nuclear Dbf2-related kinase COT1 inNeurospora crassa

Author

Rena Gorovits, Oded Yarden, Stephan Seiler, Carmit Ziv, Galia Kra-Oz, and Sabine März

Subjects

inorganic chemicals, Hyphal growth, 0303 health sciences, biology, Kinase, 030302 biochemistry & molecular biology, macromolecular substances, biology.organism_classification, Microbiology, Phosphorylation cascade, Neurospora crassa, Cell biology, 03 medical and health sciences, Biochemistry, Phosphorylation, Protein phosphorylation, Kinase activity, Molecular Biology, Actin, 030304 developmental biology

Abstract

Dysfunction of the Neurospora crassa nuclear Dbf2-related kinase COT1 leads to cessation of tip extension and massive induction of new sites of growth. To determine the role phosphorylation plays in COT1 function, we mutated COT1 residues corresponding to positions of highly conserved nuclear Dbf2-related phosphorylation sites. Analyses of the point-mutation cot-1 strains (mimicking non- and constitutively phosphorylated states) indicate the involvement of COT1 phosphorylation in the regulation of hyphal elongation and branching as well as asexual development by altering cell wall integrity and actin organization. Phosphorylation of COT1's activation segment (at Ser417) is required for proper in vitro kinase activity, but has only a limited effect on hyphal growth. In marked contrast, even though phosphorylation of the C-terminal hydrophobic motif (at Thr589) is crucial for all COT1 functions in vivo, the lack of Thr589 phosphorylation did not significantly affect in vitro COT1 kinase activity. Nevertheless, its regulatory role has been made evident by the significant increase observed in COT1 kinase activity when this residue was substituted in a manner mimicking constitutive phosphorylation. We conclude that COT1 regulates elongation and branching in an independent manner, which is determined by its phosphorylation state.

Published

2009

7. Two NDR kinase-MOB complexes function as distinct modules during septum formation and tip extension inNeurospora crassa

Author

Stephan Seiler, Oliver Valerius, Sabine Maerz, Anne Dettmann, Carmit Ziv, Yi Liu, and Oded Yarden

Subjects

0303 health sciences, Fungal protein, NDR kinase, Protein-Serine-Threonine Kinases, Kinase, 030302 biochemistry & molecular biology, Signal transducing adaptor protein, Conidiation, Biology, biology.organism_classification, Microbiology, Cell biology, Neurospora crassa, 03 medical and health sciences, Biochemistry, Protein kinase domain, Molecular Biology, 030304 developmental biology

Abstract

NDR kinases are important for growth and differentiation and require interaction with MOB proteins for activity and function. We characterized the NDR kinases and MOB activators in Neurospora crassa and identified two NDR kinases (COT1 and DBF2) and four MOB proteins (MOB1, MOB2A, MOB2B and MOB3/phocein) that form two functional NDR-MOB protein complexes. The MOB1-DBF2 complex is not only essential for septum formation in vegetative cells and during conidiation, but also functions during sexual fruiting body development and ascosporogenesis. The two MOB2-type proteins interact with both COT1 isoforms and control polar tip extension and branching by regulating COT1 activity. The conserved region directly preceding the kinase domain of COT1 is sufficient for the formation of COT1-MOB2 heterodimers, but also for kinase homodimerization. An additional N-terminal extension that is poorly conserved, but present in most fungal NDR kinases, is required for further stabilization of both types of interactions and for stimulating COT1 activity. COT1 lacking this region is degraded in a mob-2 background. We propose a specific role of MOB3/phocein during vegetative cell fusion, fruiting body development and ascosporogenesis that is unrelated to the three other MOB proteins and NDR kinase signalling.

Published

2009

8. Gene silencing of mannose 6-phosphate reductase in the parasitic weedOrobanche aegyptiacathrough the production of homologous dsRNA sequences in the host plant

Author

Oded Yarden, Benjamin Steinitz, Daniel M. Joel, Hila Cholakh, Anna Naglis, Diana Leibman, Aaron Zelcer, Amit Gal-On, and Radi Aly

Subjects

Parasitic plant, Molecular Sequence Data, Mannose, Orobanche aegyptiaca, Plant Science, Plant Roots, Host-Parasite Interactions, chemistry.chemical_compound, Solanum lycopersicum, Gene Expression Regulation, Plant, Botany, Genetically modified tomato, Gene Silencing, RNA, Messenger, RNA, Small Interfering, RNA, Double-Stranded, Base Sequence, biology, Orobanche, fungi, food and beverages, Plants, Genetically Modified, biology.organism_classification, RNA silencing, chemistry, RNA, Plant, Weed, Sequence Alignment, Agronomy and Crop Science, Solanaceae, Sugar Alcohol Dehydrogenases, Biotechnology

Abstract

Orobanche spp. (broomrape) are parasitic plants which subsist on the roots of a wide range of hosts, including tomato, causing severe losses in yield quality and quantity. Large amounts of mannitol accumulate in this parasitic weed during development. Mannose 6-phosphate reductase (M6PR) is a key enzyme in mannitol biosynthesis, and it has been suggested that mannitol accumulation may be very important for Orobanche development. Therefore, the Orobanche M6PR gene is a potential target for efforts to control this parasite. Transgenic tomato plants were produced bearing a gene construct containing a specific 277-bp fragment from Orobanche aegyptiaca M6PR-mRNA, in an inverted-repeat configuration. M6PR-siRNA was detected in three independent transgenic tomato lines in the R1 generation, but was not detected in the parasite. Quantitative RT-PCR analysis showed that the amount of endogenous M6PR mRNA in the tubercles and underground shoots of O. aegyptiaca grown on transgenic host plants was reduced by 60%-80%. Concomitant with M6PR mRNA suppression, there was a significant decrease in mannitol level and a significant increase in the percentage of dead O. aegyptiaca tubercles on the transgenic host plants. The detection of mir390, which is involved with cytoplasmic dsRNA processing, is the first indication of the existence of gene-silencing mechanisms in Orobanche spp. Gene silencing mechanisms are probably involved with the production of decreased levels of M6PR mRNA in the parasites grown on the transformed tomato lines.

Published

2009

9. Differential protein expression in Colletotrichum acutatum: changes associated with reactive oxygen species and nitrogen starvation implicated in pathogenicity on strawberry

Author

Stanley Freeman, Natan Gollop, Oded Yarden, Aida Zveibil, Eduard Belausov, Sigal Horowitz Brown, and Songbi Chen

Subjects

Proteomics, Nitrogen, Molecular Sequence Data, Glyoxylate cycle, Soil Science, Plant Science, Fragaria, Malate dehydrogenase, Fungal Proteins, Superoxide dismutase, Colletotrichum acutatum, Tandem Mass Spectrometry, Colletotrichum, Electrophoresis, Gel, Two-Dimensional, Molecular Biology, chemistry.chemical_classification, Appressorium, Reactive oxygen species, Fungal protein, biology, fungi, Original Articles, biology.organism_classification, chemistry, Biochemistry, Catalase, Host-Pathogen Interactions, biology.protein, Reactive Oxygen Species, Agronomy and Crop Science, Chromatography, Liquid

Abstract

The cellular outcome of changes in nitrogen availability in the context of development and early stages of pathogenicity was studied by quantitative analysis of two‐dimensional gel electrophoresis of Colletotrichum acutatum infecting strawberry. Significant alterations occurred in the abundance of proteins synthesized during appressorium formation under nitrogen‐limiting conditions compared with a complete nutrient supply. Proteins that were up‐ or down‐regulated were involved in energy metabolism, nitrogen and amino acid metabolism, protein synthesis and degradation, response to stress and reactive oxygen scavenging. Members belonging to the reactive oxygen species (ROS) scavenger machinery, superoxide dismutase and glutathione peroxidase, were up‐regulated at the appressorium formation stage, as well as under nitrogen‐limiting conditions relative to growth with a complete nutrient supply, whereas abundance of bifunctional catalase was up‐regulated predominantly at the appressorium formation stage. Fungal ROS were detected within germinating conidia during host pre‐penetration, penetration and colonization stages, accompanied by plant ROS, which were abundant in the apoplastic space. Application of exogenous antioxidants quenched ROS production and reduced the frequency of appressorium formation. Up‐regulation in metabolic activity was detected during appressorium formation and nutrient deficiency compared with growth under complete nutrient supply. Enhanced levels of proteins related to the glyoxylate cycle and lipid metabolism (malate dehydrogenase, formate dehydrogenase and acetyl‐CoA acetyltransferase) were observed at the appressorium formation stage, in contrast to down‐regulation of isocitrate dehydrogenase. The present study demonstrates that appressoria formation processes, occurring under nutritional deprivation, are accompanied by metabolic shifts, and that ROS production is an early fungal response that may modulate initial stages of pathogen development.

Published

2008

10. Trifluralin herbicide-induced resistance of melon to fusarium wilt involves expression of stress- and defence-related genes

Author

Nurit Katzir, Vitaly Portnoy, Oded Yarden, Ron Cohen, Yosef Burger, and Maya Lotan-Pompan

Subjects

Fusarium, biology, Inoculation, Melon, food and beverages, Soil Science, Trifluralin, Plant Science, Fungi imperfecti, biology.organism_classification, Fusarium wilt, Microbiology, chemistry.chemical_compound, chemistry, Suppression subtractive hybridization, Botany, Fusarium oxysporum, Agronomy and Crop Science, Molecular Biology

Abstract

SUMMARY To identify genes involved in trifluralin herbicide-induced resistance of melon to Fusarium oxysporum f. sp. melonis, suppression subtractive hybridization (SSH) and cDNA-amplified fragment-length polymorphism (cDNA-AFLP) were used. A total of 123 clones-60 of which have never been isolated from melon-were isolated, sequenced and annotated. A significant proportion (35%) of the total 123 clones exhibited similarity to genes that have been formerly described as stress- or defence-related. Thirty-two selected clones were subjected to a detailed expression analysis, one-third of which were found to be up-regulated in response to trifluralin treatment and/or fusarium inoculation. The putative roles of seven of these clones in stress are discussed. Furthermore, the expression of four stress-related and up-regulated genes was enhanced when the plants were subjected to salinity stress, suggesting that trifluralin induces a general stress response which protects the plant against fusarium wilt.

Published

2007

11. The global nitrogen regulator, FNR1, regulates fungal nutrition-genes and fitness during Fusarium oxysporum pathogenesis

Author

Carmit Ziv, Oded Yarden, Robert Fluhr, Hege Hvattum Divon, and Olga Davydov

Subjects

Zinc finger, biology, fungi, Mutant, Crassa, food and beverages, Soil Science, Plant Science, biology.organism_classification, Microbiology, Neurospora crassa, Fusarium oxysporum, Gibberella fujikuroi, Agronomy and Crop Science, Molecular Biology, Pathogen, Gene

Abstract

SUMMARY Fusarium oxysporum is a soil-borne pathogen that infects plants through the roots and uses the vascular system for host ingress. Specialized for this route of infection, F. oxysporum is able to adapt to the scarce nutrient environment in the xylem vessels. Here we report the cloning of the F. oxysporum global nitrogen regulator, Fnr1, and show that it is one of the determinants for fungal fitness during in planta growth. The Fnr1 gene has a single conserved GATA-type zinc finger domain and is 96% and 48% identical to AREA-GF from Gibberella fujikuroi, and NIT2 from Neurospora crassa, respectively. Fnr1 cDNA, expressed under a constitutive promoter, was able to complement functionally an N. crassa nit-2(RIP) mutant, restoring the ability of the mutant to utilize nitrate. Fnr1 disruption mutants showed high tolerance to chlorate and reduced ability to utilize several secondary nitrogen sources such as amino acids, hypoxanthine and uric acid, whereas growth on favourable nitrogen sources was not affected. Fnr1 disruption also abolished in vitro expression of nutrition genes, normally induced during the early phase of infection. In an infection assay on tomato seedlings, infection rate of disruption mutants was significantly delayed in comparison with the parental strain. Our results indicate that FNR1 mediates adaptation to nitrogen-poor conditions in planta through the regulation of secondary nitrogen acquisition, and as such acts as a determinant for fungal fitness during infection.

Published

2006

12. Microwave-assisted extraction of bioactive saponins from chickpea (Cicer arietinum L)

Author

Zohar Kerem, Oded Yarden, and Hilla German-Shashoua

Subjects

Antifungal, chemistry.chemical_classification, Fusarium, Penicillium digitatum, Nutrition and Dietetics, biology, medicine.drug_class, Butanol, Extraction (chemistry), Saponin, biology.organism_classification, Microwave assisted, chemistry.chemical_compound, chemistry, Botany, medicine, Food science, Agronomy and Crop Science, Legume, Food Science, Biotechnology

Abstract

Growing interest in plant secondary metabolites has brought with it the need for economical, rapidandefficientextractionprotocols.Microwave-assistedextraction(MAE)wasusedtoextractsaponins from chickpea (Cicer arietinum). Several MAE conditions were tested, and the method proved to be superior to Soxhlet extraction with regard to amounts of solvents required, time and energy expended. The use of a butanol/H2O mixture showed selectivity towards saponin extraction. Using TLC, two distinct saponins were observed in the various chickpea extracts. The identification of the major saponin as a DDMP-conjugated saponin was verified using 1 Ha nd 13 CN MR, for the fi rst time in chickpea. The MAE procedure most likely contributed to the conservation of the heat-sensitive DDMP moiety. The pure chickpea saponin exhibited significant inhibitory activity against Penicillium digitatum and additional filamentous fungi. Two Fusarium strains tested were highly tolerant to the saponin. The potential for using MAE for the efficient extraction of natural products may assist in expediting the chemical analysis and characterization of the biological activities of such compounds.  2004 Society of Chemical Industry

Published

2005

13. Quantification of the arbuscular mycorrhizal fungus Glomus intraradices in host tissue using real‐time polymerase chain reaction

Author

Oded Yarden, Vijay Gadkar, Joel Coburn, Noam Alkan, and Yoram Kapulnik

Subjects

Chalcone synthase, biology, Hypha, Physiology, fungi, food and beverages, Plant Science, biology.organism_classification, Medicago truncatula, Lycopersicon, law.invention, Microbiology, Arbuscular mycorrhiza, Real-time polymerase chain reaction, law, biology.protein, Mycorrhiza, Polymerase chain reaction

Abstract

Summary •A rapid method to quantify the colonization of the arbuscular mycorrhizal fungus (AMF) Glomus intraradices in planta using quantitative real-time polymerase chain reaction (qRT-PCR) technique. • Specific PCR primers for the fungus (28S rDNA sequence) and host root tissue (chitinase and chalcone synthase gene) were developed and their respective specificity determined. • The plant specific primers for Lycopersicon esculentum , Medicago truncatula amplified linearly over a concentration range of: 6.4 pg to 20 ng. The G. intraradices specific primer amplified as low as 1 pg of its target DNA, which allowed us to detect a single spore of the fungus. High degrees of correlation were obtained when threshold cycle (Ct) was plotted against vesicular, hyphal and total colonization using microscopically quantified host roots. • This is the first report of the application of the qRT-PCR technique for quantification of AMF colonization in planta . The success of its application should open up the possibility of its wider application in AM research.

Published

2004

14. The N-terminal region of theNeurospora NDR kinase COT1 regulates morphology via its interactions with MOB2A/B

Author

Carmit Ziv, Liran Aharoni-Kats, Yi Liu, Oded Yarden, Daria Feldman, and She Chen

Subjects

Hyphal growth, Fungal protein, NDR kinase, Protein-Serine-Threonine Kinases, Kinase, Hyphal tip, Conidiation, Biology, biology.organism_classification, Molecular Biology, Microbiology, Neurospora, Cell biology

Abstract

Summary Nuclear Dbf2p-related (NDR) protein kinases are important for cell differentiation and polar morphogenesis in various organisms, yet some of their functions are still elusive. Dysfunction of the Neurospora crassa NDR kinase COT1 leads to cessation of tip extension and hyperbranching. NDR kinases require the physical interaction between the kinase's N-terminal region (NTR) and the MPS1-binding (MOB) proteins for their activity and functions. To study the interactions between COT1 and MOB2 proteins, we mutated several conserved residues and a novel phosphorylation site within the COT1 NTR. The phenotypes of these mutants suggest that the NTR is required for COT1 functions in regulating hyphal elongation and branching, asexual conidiation and germination. Interestingly, while both MOB2A and MOB2B promote proper hyphal growth, they have distinct COT1-dependent roles in regulation of macroconidiation. Immunoprecipitation experiments indicate physical association of COT1 with both MOB2A and MOB2B, simultaneously. Furthermore, the binding of the two MOB2 proteins to COT1 is mediated by different residues at the COT1 NTR, suggesting a hetero-trimer is formed. Thus, although MOB2A/B may have some overlapping functions in regulating hyphal tip extension, their function is not redundant and they are both required for proper fungal development.

Published

2013

15. cot-1, a gene required for hyphal elongation in Neurospora crassa, encodes a protein kinase

Author

M Plamann, Oded Yarden, Daniel J. Ebbole, and Charles Yanofsky

Subjects

Genes, Fungal, Molecular Sequence Data, Restriction Mapping, Hyphal tip, General Biochemistry, Genetics and Molecular Biology, Neurospora crassa, Sequence Homology, Nucleic Acid, Amino Acid Sequence, Cloning, Molecular, DNA, Fungal, Molecular Biology, Gene, Genetics, Base Sequence, General Immunology and Microbiology, biology, General Neuroscience, fungi, Structural gene, Wild type, RNA, Fungal, Temperature-sensitive mutant, biology.organism_classification, Cell biology, Complementation, Cosmid, Protein Kinases, Research Article, Plasmids

Abstract

Neurospora crassa is a filamentous fungus that grows on semisolid media by forming spreading colonies. Mutations at several loci prevent this spreading growth. cot-1 is a temperature sensitive mutant of N.crassa that exhibits restricted colonial growth. At temperatures above 32 degrees C colonies are compact while at lower temperatures growth is indistinguishable from that of the wild type. Restricted colonial growth is due to a defect in hyphal tip elongation and a concomitant increase in hyphal branching. We have isolated a genomic cosmid clone containing the wild type allele of cot-1 by complementation. Sequence analyses suggested that cot-1 encodes a member of the cAMP-dependent protein kinase family. Strains in which we disrupted cot-1 are viable but display restricted colonial growth. Duplication, by ectopic integration of a promoter-containing fragment which includes the first one-third (209 codons) of the structural gene, unexpectedly resulted in restricted colonial growth. Our results suggest that an active COT1 kinase is required for one or more events essential for hyphal elongation.

Published

1992

16. A rapid bioassay for the determination of carbendazim residues in soil

Author

Oded Yarden, Nadav Aharonson, and Jaacov Katan

Subjects

Penicillium digitatum, Residue (complex analysis), food.ingredient, Chromatography, biology, Carbendazim, Extraction (chemistry), Plant Science, Horticulture, biology.organism_classification, complex mixtures, Agar plate, chemistry.chemical_compound, food, chemistry, Soil water, Genetics, Bioassay, Agar, Agronomy and Crop Science

Abstract

A simple and rapid bioassay for the direct determination of carbendazim residues in soil was developed. Pellets composed of mixtures of soil (200–500 mg) and agar were placed on an agar medium pre–inoculated with the test organism Penicillium digitatum. After cold pre–incubation followed by incubation at 27°C, the size of the inhibition zone was determined. The lowest detectable concentrations of carbendazim and thiabendazole in a sandy soil were 0.25 and 10 μg/g, respectively. The lowest detectable concentration was higher in heavy soils. In a study of carbendazim degradation in soil, chemical analysis and the pellet bioassay technique yielded similar results. This technique requires only small quantities of soil, without the need for soil extraction.

Published

1985

17. Paclobutrazol and other plant growth-retarding chemicals increase resistance of melon seedlings to fusarium wilt

Author

Oded Yarden, R. Cohen, Jaacov Katan, J. Riov, and N. Lisker

Subjects

biology, food and beverages, Benomyl, Wilting, Plant Science, Horticulture, biology.organism_classification, Fusarium wilt, Paclobutrazol, chemistry.chemical_compound, Agronomy, chemistry, Seedling, Germination, Fusarium oxysporum, Genetics, Gibberellin, Agronomy and Crop Science

Abstract

Studies were made of plant growth retardation and effects on resistance of melon to fusarium wilt by soil application of paclobutrazol, other ergosterol biosynthesis inhibitors, the fungicide benomyl and the herbicide dinitramine. Paclobutrazol and ancymidol delayed the onset of wilting and were the most effective in reducing wilt incidence. A relationship between effectiveness in retarding seedling elongation and increasing resistance to fusarium wilt was observed. No chemical had a significant effect on pathogen population level in the plant, as determined by stem colonization and direct assessment tests in seedlings grown in soil treated with the chemicals. Excluding benomyl, and to a lesser extent dinitramine, leaf and stem extracts had no inhibitory effect on conidial germination. Gibberellins GA4+7, when applied to seedlings inoculated after germination in paclobutrazol-treated soil, nullified growth retardation and increased disease incidence. We suggest that disease incidence reduction by paclobutrazol is due to an effect on plant metabolic processes and not to direct fungitoxicity of the compound.

Published

1987