ABSTRACT
Metarhizium spp. is used as a biocontrol agent but is limited because of low tolerance to abiotic stress. Metarhizium robertsii is an excellent study model of fungal pathogenesis in insects, and its tolerance to different stress conditions has been extensively investigated. Priming is the time-limited pre-exposure of an organism to specific stress conditions that increases adaptive response to subsequent exposures. Congo red is a water-soluble azo dye extensively used in stress assays in fungi. It induces morphological changes and weakens the cell wall at sublethal concentrations. Therefore, this chemical agent has been proposed as a stressor to induce priming against other stress conditions in entomopathogenic fungi. This study aimed to evaluate the capacity of Congo red to induce priming in M. robertsii. Conidia were grown on potato dextrose agar with or without Congo red.The tolerance of conidia produced from mycelia grown in these three conditions was evaluated against stress conditions, including osmotic, oxidative, heat, and UV-B radiation. Conidia produced on medium supplemented with Congo red were significantly more tolerant to UV-B radiation but not to the other stress conditions assayed. Our results suggest that Congo red confers trans-priming to UV-B radiation but not for heat, oxidative, or osmotic stress.
Subject(s)
Metarhizium , Metarhizium/physiology , Congo Red , Ultraviolet Rays , Spores, Fungal/physiologyABSTRACT
Soybean, corn, and cotton crops are afflicted by several noctuid pests and the development of bioinsecticides could help control these pests. The fungus Metarhizium rileyi has the greatest potential because its epizootics decimate caterpillar populations in the absence of insecticide applications. However, insect-pathogenic fungi when used for insect control in agriculture have low survival mainly due to the deleterious effects of ultraviolet radiation and heat from solar radiation. In this study, fourteen isolates of M. rileyi were studied and compared with isolates ARSEF 324 and ARSEF 2575 of Metarhizium acridum and Metarhizium robertsii, respectively, whose sensitivity to UV-B radiation had previously been studied. Conidia were exposed at room temperature (ca. 26 °C) to 847.90 mWm-2 of Quaite-weighted UV-B using two fluorescent lamps. The plates containing the conidial suspensions were irradiated for 1, 2, and 3 h, providing doses of 3.05, 6.10, and 9.16 kJ m2, respectively. A wide variability in conidial UV-B tolerance was found among the fourteen isolates of M. rileyi. Isolate CNPSo-Mr 150 was the most tolerant isolate (germination above 80% after 2 h exposure), which was comparable to ARSEF 324 (germination above 90% after 2 h exposure), the most tolerant Metarhizium species. The least tolerant isolates were CNPSo-Mr 141, CNPSo-Mr 142, CNPSo-Mr 156, and CNPSo-Mr 597. Nine M. rileyi isolates exhibited similar tolerance to UV-B radiation as ARSEF 2575 (germination above 50% after 2 h exposure). In conclusion, the majority of M. rileyi isolates studied can endure 1 or 2 h of UV-B radiation exposure. However, after 3 h of exposure, the germination of all studied isolates reduced below 40%, except for CNPSo-Mr 150 and ARSEF 324.
Subject(s)
Metarhizium , Animals , Ultraviolet Rays , Spores, Fungal , InsectaABSTRACT
Polyamines are ubiquitous polycationic molecules with multiple effects. Spermidine was present in all the life stages of Phycomyces blakesleeanus, fulfilled the physiological requirement for polyamines during germination, and became most abundant at the emergence of germinating tubes. Putrescine was not found in resting spores or in stationary cultures, but was synthesized during apical growth and greatly exceeded spermidine in fast-growing stages of the vegetative and sexual life cycles. Changes in the polyamines did not correlate with the various stages of sporulation. Ornithine decarboxylase was so strongly inhibited in vitro by its product, putrescine, that it would completely block the enzyme if not compartmentalized away. 1,4-Diamino-2-butanone inhibited mycelial growth throughout the vegetative cycle without killing the cells. The inhibition was counteracted very effectively by putrescine, which acts as a close analog of the inhibitor, and very little by spermidine. Four independent spe mutants were obtained by a procedure that selected for resistance to diaminobutanone among functionally-uninucleate spores that survived exposure to N-methyl-N'-nitro-N-nitrosoguanidine. The stability of the enzyme, in vivo and in vitro, and its inhibition by diaminobutanone in vitro were the same in the wild type and in the mutants. Two of these were hypomorph mutants, with lower affinity of their ornithine decarboxylase for its substrate, ornithine, and lower maximal velocity. The other two were hypermorph transport mutants; we propose that they are affected in a protein that binds putrescine and its analogs for transport across the plasmalemma and sequestration away from the active enzyme. The transport mutants concentrated the exogenous diaminobutanone and the endogenous putrescine in inactive compartments; the highest enzyme activity was reached when the plasmalemma of the mutants was permeabilized with diethylaminoethyl dextran.
Subject(s)
Ornithine Decarboxylase , Polyamines , Growth and Development , Ornithine Decarboxylase/genetics , Ornithine Decarboxylase/metabolism , Phycomyces , Polyamines/metabolism , Putrescine/pharmacology , Spermidine/pharmacologyABSTRACT
The fungal species Trichoderma is frequently found in soil antagonizing plant-pathogenic fungi as well as parasitizing plant-pathogenic nematodes. Metarhizium species are insect-pathogenic fungi that are used throughout the world to control agricultural insect pests. Here, we determine whether the antagonism (A) of Trichoderma atroviride to Metarhizium robertsii during growth and spore formation can impact the stress biology of M. robertsii conidia. Cultures of M. robertsii were either produced without exposure to T. atroviride (control) or in the presence of T. atroviride. M. robertsii was grown in dual culture with T. atroviride on potato dextrose agar (PDA) using the following treatments: 1) Trichoderma inoculated at the same time with Metarhizium (A0); 2) Trichoderma inoculated two days after the inoculation of Metarhizium (A2); 3) Trichoderma inoculated four days after Metarhizium (A4); 4) Trichoderma inoculated 6 d after Metarhizium (A6); 5) M. robertsii grown alone on PDA medium (control); and 6) M. robertsii grown alone on minimal medium (Czapek-Dox medium without sucrose) (MM). Germination of M. robertsii conidia from all six treatments was then assessed under osmotic, oxidative, UV-B, and thermal stress. M. robertsii conidia produced on MM were the most tolerant to all stress conditions. For all stress conditions, conidia from treatments A0 and A2 were not viable. For osmotic stress, conidia produced in treatment A4 were the most tolerant, followed by conidia from treatment A6, which were both more tolerant than the control. For oxidative stress, conidia produced in both A4 and A6 treatments were similarly tolerant and more tolerant than conidia produced in the control. For thermal stress, conidia produced in treatments A4, A6, and control (PDA) were similarly heat-tolerant. For UV-B stress, conidia produced in treatments A4 and A6 were equally tolerant and more tolerant than conidia produced in the control. The germination speed of conidia produced in all treatments, A0, A2, A4, and A6 was also tested. Conidia produced on MM germinated faster than the other treatments. Conidia produced in the A4 treatment were the second fastest, followed by conidia produced in treatment A6. Both A4 and A6 conidia germinated faster than conidia produced in the control treatment. Conidia produced in the treatments A0 and A2 did not germinate in 24 h. In summary, moderate levels of biotic stress from a fungal competitor or low-nutrient conditions can enhance the stress tolerance of M. robertsii conidia.
Subject(s)
Hypocreales , Metarhizium , Microbial Interactions , Hot Temperature , Hypocreales/physiology , Metarhizium/physiology , Osmotic Pressure , Spores, Fungal/physiology , Time FactorsABSTRACT
Plants and fungi use light and other signals to regulate development, growth, and metabolism. The fruiting bodies of the fungus Phycomyces blakesleeanus are single cells that react to environmental cues, including light, but the mechanisms are largely unknown [1]. The related fungus Mucor circinelloides is an opportunistic human pathogen that changes its mode of growth upon receipt of signals from the environment to facilitate pathogenesis [2]. Understanding how these organisms respond to environmental cues should provide insights into the mechanisms of sensory perception and signal transduction by a single eukaryotic cell, and their role in pathogenesis. We sequenced the genomes of P. blakesleeanus and M. circinelloides and show that they have been shaped by an extensive genome duplication or, most likely, a whole-genome duplication (WGD), which is rarely observed in fungi [3-6]. We show that the genome duplication has expanded gene families, including those involved in signal transduction, and that duplicated genes have specialized, as evidenced by differences in their regulation by light. The transcriptional response to light varies with the developmental stage and is still observed in a photoreceptor mutant of P. blakesleeanus. A phototropic mutant of P. blakesleeanus with a heterozygous mutation in the photoreceptor gene madA demonstrates that photosensor dosage is important for the magnitude of signal transduction. We conclude that the genome duplication provided the means to improve signal transduction for enhanced perception of environmental signals. Our results will help to understand the role of genome dynamics in the evolution of sensory perception in eukaryotes.
Subject(s)
Evolution, Molecular , Gene Duplication , Genome, Fungal , Mucor/genetics , Phycomyces/genetics , Signal Transduction/genetics , Light , Mucor/radiation effects , Multigene Family , Perception , Phycomyces/radiation effects , Transcription, Genetic/radiation effectsABSTRACT
The oxidative cleavage of ß-carotene in the Mucorales produces three fragments of 18, 15, and 7 carbons, respective heads of three families of apocarotenoids: the methylhexanoids, the trisporoids, and the cyclofarnesoids (named after their 1,6-cyclofarnesane skeleton). The apocarotenoids are easily recognized because they are absent in white mutants unable to produce ß-carotene. In cultures of Phycomyces blakesleeanus we detected thirty-two apocarotenoids by LC, UV absorbance, and MS. With additional IR and NMR we identified two methylhexanoids and the eight most abundant cyclofarnesoids. Four of them were previously-unknown natural compounds, including 4-dihydrocyclofarnesine S, the most abundant cyclofarnesoid in young cultures. We arranged the apocarotenoids of the Mucorales in a scheme that helps classifying and naming them and suggests possible metabolites and biosynthetic pathways. We propose specific biosynthetic pathways for cyclofarnesoids and methylhexanoids based on structural comparisons, the time course of appearance of individual compounds, and the bioconversion of ß-apo-12-carotenol, an early precursor, to three more oxygenated cyclofarnesoids by the white mutants. Some of the reactions occur spontaneously in the increasingly acidic culture media. Mating increased the contents of methylhexanoids and cyclofarnesoids by ca. threefold in young cultures and ca. twelvefold in old ones (five days); cyclofarnesine S, the most abundant cyclofarnesoid in old cultures, increased over one hundredfold. We found no differences between the sexes and no activity as sexual pheromones, but we suggest that methylhexanoids and cyclofarnesoids could mediate species-specific physiology and behavior.
Subject(s)
Carotenoids/chemistry , Carotenoids/metabolism , Mucorales/metabolism , Phycomyces/chemistry , beta Carotene/chemistry , Biosynthetic Pathways , Culture Media/chemistry , Nuclear Magnetic Resonance, Biomolecular , Sex Attractants/metabolismABSTRACT
Mating and sexual development in fungi are controlled by molecular mechanisms that are specific for each fungal group. Mating in Phycomyces blakesleeanus and other Mucorales requires pheromones derived from ß-carotene. Phycomyces mutants in gene carS accumulate large amounts of ß-carotene but do not enter the sexual process. We show that carS encodes a ß-carotene-cleaving oxygenase that catalyzes the first step in the biosynthesis of a variety of apocarotenoids, including those that act as pheromones. Therefore carS mutants cannot stimulate their sexual partners, although they respond to them. CarS catalyzes the biosynthesis of a ß-ring-containing apocarotenoid that inhibits the activity of the carotenogenic enzyme complex in vegetative cells and provides a feedback regulation for the ß-carotene pathway. The carS gene product is a keystone in carotenogenesis and in sexual reproduction.
Subject(s)
Carotenoids/metabolism , Metabolic Networks and Pathways , Pheromones/biosynthesis , Phycomyces/genetics , Phycomyces/metabolism , Amino Acid Sequence , DNA, Fungal/chemistry , DNA, Fungal/genetics , Molecular Sequence Data , Oxygenases/genetics , Oxygenases/metabolism , Sequence Analysis, DNA , Sequence Homology, Amino AcidABSTRACT
Mixed cultures of strains of opposite sex of the Mucorales produce trisporic acids and other compounds arising from cleavage of ß-carotene, some of which act as signals in the mating process. The genome of Phycomyces blakesleeanus contains five sequences akin to those of verified carotenoid cleavage oxygenases. All five are transcribed, three of them have the sequence traits that are considered essential for activity, and we have discovered the reactions catalysed by the products of two of them, genes carS and acaA. The transcripts of carS became more abundant in the course of mating, and its expression in ß-carotene-producing Escherichia coli cells led to the formation of ß-apo-12'-carotenal, a C25 cleavage product of ß-carotene. Joint expression of both genes in the same in vivo system resulted in the production of ß-apo-13-carotenone, a C18 fragment. In vitro, AcaA cleaved ß-apo-12'-carotenal into ß-apo-13-carotenone and was active on other apocarotenoid substrates. According to these and other results, the first reactions in the apocarotenoid pathway of Phycomyces are the cleavage of ß-carotene at its C11'-C12' double bond by CarS and the cleavage of the resulting C25-fragment at its C13-14 double bond by AcaA.
