The present invention relates to endophytes, plants infected with endophytes, products produced by the endophytes and related methods.
Microbes represent an invaluable source of novel genes and compounds that have the potential to be utilised in a range of industrial sectors. Scientific literature gives numerous accounts of microbes being the primary source of antibiotics, immune-suppressants, anticancer agents and cholesterol-lowering drugs, in addition to their use in environmental decontamination and in the production of food and cosmetics.
A relatively unexplored group of microbes known as endophytes, which reside in the tissues of living plants, offer a particularly diverse source of novel compounds and genes that may provide important benefits to society, and in particular, agriculture.
Endophytes often form mutualistic relationships with their hosts, with the endophyte conferring increased fitness to the host, often through the production of defense compounds. At the same time, the host plant offers the benefits of a protected environment and nutriment to the endophyte.
Other microbes, such as bacteria which can reside in the tissues of living plants, are also relatively unexplored in this setting. Plant-borne bacteria offer similar benefits.
The Brachiaria-Urochloa species complex is a component of the grass family Poaceae, with representatives distributed throughout tropical regions, particularly in Africa. Genetic diversity analysis based on internal transcribed spacer (ITS) nuclear ribosomal DNA sequence data indicates a strong affinity between Urochloa and Brachiaria, supporting morphological and anatomical studies that show a continuous gradation between these grass genera. Some Brachiaria-Urochloa species are economically significant tropical forage grasses that have been released as commercial cultivars and include B. brizantha, B. decumbens, B. humidicola, and B. ruziziensis, as well as corresponding interspecific and intraspecific hybrids.
Methods for the identification and characterization of novel endophytes and their deployment in Brachiaria-Urochloa plant improvement programs have been discussed in WO2012/174585, the disclosure of which is hereby incorporated herein in its entirety. Strains of endophytic fungi were isolated from Brachiaria-Urochloa species. These Brachiaria fungal endophytes were genetically diverse. Some of these endophytes exhibited broad spectrum anti-fungal activity and may play a role in protecting Brachiaria-Urochloa from fungal pathogens, such as Drechslera spp., which cause leaf spots.
There remains a general lack of information and knowledge of the fungal endophytes of the Brachiaria-Urochloa species complex as well as of methods for the identification and characterisation of novel endophytes and their deployment in Brachiaria-Urochloa plant improvement programs.
There is also a general lack of information and knowledge of the bacterial endophytes of the Brachiaria-Urochloa species complex as well as of methods for the identification and characterisation of novel bacterial organisms and their deployment in Brachiaria-Urochloa plant improvement programs.
Furthermore, although widely used for pasture-based agriculture in tropical regions of South America, Asia and Australia, Brachiaria-Urochloa exhibits a number of shortcomings that constrain both its use and genetic enhancement.
Forage grasses, including Brachiaria-Urochloa, have also been recognised in recent years for implications in nitrogen pollution. A major concern of modern production in agriculture is the high level of nitrogen (N) pollution and low efficiency of N utilisation. N losses from denitrification results in environmental pollution and inefficient use of both soil N and applied N (as fertiliser).
Nitrification is carried out primarily by two groups of chemo-lithotrophic bacteria (Nitrosomonas sp. and Nitrobacter spp), ubiquitous components of the soil microbial population. For example, nitrifying soil bacteria, such as Nitrosomonas spp convert ammonium (NH4+) to nitrate (NO3−). Nitrate can also be converted to nitrous oxide (N2O) gas. Inhibition of nitrification may keep N in soil for longer and improve nitrogen use efficiency (NUE).
A bioluminescence assay using a recombinant strain of Nitrosomonas europaea has been developed to detect nitrification inhibitors released from plant roots, making it possible to determine and compare the biological nitrification inhibition (BNI) capacity of different crops and pastures (Subbarao et al., 2006).
The concept of plants releasing inhibitory compounds that suppress soil nitrification has previously been suggested. Several researchers have observed a slow rate of nitrification in soils of certain tropical grassland and forest soils. BNI is the ability of certain plant species to release organic compounds from their roots that have a targeted suppressive effect on soil nitrifying bacteria (Subbarao et al., 2006 2009).
Brachialactone is the major nitrification inhibitor released from roots of B. humidicola (Subbarao et al. 2009). Brachialactone belongs to a group of diterpenes called Fusicoccanes. Fusicoccanes have been identified and isolated from a diverse range of plants, fungi and bacteria. Brachialactone has been shown to exhibit biocidal activity against Nitrosomonas spp (Subbarao et al. 2009). N is then available to plant, increasing pasture performance. Literature has suggested that this compound is produced by the plant in response to ammonium in the root environment (Subbarao et al. 2009).
It is an object of the present invention to overcome, or at least alleviate, one or more of the difficulties or deficiencies associated with the prior art.
In one aspect, the present invention provides a method for isolating, selecting and/or characterising an endophyte strain, said method including:
By an endophyte strain is meant a bacterial or fungal strain that is closely associated with a plant, preferably a plant of the Brachiaria-Urochloa species complex. By ‘associated with’ in this context is meant that the bacteria or fungus lives on, in or in close proximity to the plant. For example, it may be endophytic, for example living within the internal tissues of the plant, or epiphytic, for example growing externally on the plant.
The plant material used to prepare the samples is from a plant of the Brachiaria-Urochloa species complex. More particularly, the plant of the Brachiaria-Urochloa species complex is selected from the group consisting of Brachiaria brizantha, Brachiaria decumbens, Brachiaria humidicola, Brachiaria stolonifera, Brachiaria ruziziensis, Urochloa brizantha, Urochloa decumbens, Urochloa humidicola, Urochloa mosambicensis, Brachiaria marlothii, Brachiaria nigropedata, Urochloa dictyoneura, Urochloa oligotricha, Urochloa panicoides, Brachiaria obtusiflora, Brachiaria serrifolia, Urochloa advena, Urochloa arrecta, Urochloa brachyura, Urochloa eminii, Urochloa mollis, Urochloa xantholeuca, Urochloa oligotricha, Urochloa panicoides, Urochloa plantaginea, Urochloa platynota, Urochloa xantholeuca, Brachiaria holosericea, Brachiaria reptans, Brachiaria milliformis, and Brachiaria distachya, as well as interspecific and intraspecific hybrids of Brachiaria-Urochloa species complex.
In a particularly preferred embodiment, the plant of the Brachiaria-Urochloa complex is selected from the group consisting of Brachiaria brizantha, Brachiaria decumbens, Brachiaria humidicola, Brachiaria ruziziensis and Urochloa mosambicensis.
Preferably, the samples of plant material are selected from the group consisting of leaf, stem, root and seed material. Even more preferably, samples of leaf, stem and root types are provided. Alternatively, samples of seed are provided. In another preferred embodiment samples of leaf, stem, root and seed material are provided.
By ‘subjecting said samples to metagenomic analysis’ as used herein is meant that metagenomic sequence data is generated from the plant material. More particularly, genetic material recovered from the plant samples is analysed to produce bacterial and/or fungal sequence data.
The term ‘recovering genetic material’ includes the extraction of genetic material, including DNA, from the sample of plant material.
The genetic material recovered from the plant samples may be enriched for DNA from endophytic strains (such as bacterial and/or fungal DNA) closely associated with the plant, as part of the process of recovering the genetic material from the sample of plant material.
Accordingly, in a preferred embodiment, the step of providing samples of plant material from plant species of the Brachiaria-Urochloa species complex includes the steps of:
In this aspect of the invention, preferably the plant material is plant seed. Preferably the plant material is roughly ground. Preferably the alcohol is ethanol, more preferably 100% ethanol. Preferably the ground plant material is washed multiple times, for example two times with alcohol. Preferably the nucleic acid is DNA.
Applicants have surprisingly found that it is possible to reduce the amount of plant nucleic acid, e.g. plant seed nucleic acid and/or enrich for nucleic acid from endophytic strains by roughly grinding the plant tissue, e.g. seed, and then washing this in alcohol, preferably ethanol. While applicants do not wish to be restricted by theory, it is thought that the alcohol acts to preserve the microbe component of the plant material, particularly seed. Extracting nucleic acid, e.g. DNA from the alcohol, e.g. ethanol, wash reduces the amount of host plant nucleic acid and enriches for microbe nucleic acid. This overcomes or at least alleviates the problem of one or more prior art methods, including those which generate large numbers of sequence reads to capture the microbial component or use differences in nucleic acid, e.g. DNA methylation density to distinguish between host and microbial nucleic acid.
In a preferred embodiment, universal polymerase chain reaction (PCR) primers for profiling bacterial microbiome and/or fungal microbiome may be used to generate the sequence data. For example, primers directed to the 16S rDNA gene, more particularly the V4 region of the 16S rDNA gene, may be used for profiling bacterial microbiome. For example, primers directed to the internal transcribed spacer (ITS) region of rDNA genes, more particularly the ITS2 region of rDNA genes, may be used for profiling fungal microbiome.
In one embodiment, bacterial sequence data is produced using universal primers directed to the V4 region of the 16S rDNA gene and the fungal sequence data is produced using universal primers directed to the ITS2 region of the rDNA genes.
Metagenomic sequence data may be assembled to create the bacterial and/or fungal operational taxonomic units (OTUs). Preferably, the metagenomic sequence data may be quality trimmed and then paired using a paired-end assembler for sequences, such as PANDAseq, to create the bacterial and/or fungal OTUs.
The OTUs may be aligned against a bacterial database, such as the GreenGenes bacterial database, and/or a fungal database, such as the UNITE fungal database, to assign taxonomy.
The number of sequences associated with OTUs may be calculated for each sample.
By comparing the OTUs present in each sample species, core, supplemental and unique microbiomes may be identified. By a ‘microbiome’ is meant the collective genomes of the bacteria and/or fungi. By a ‘core microbiome’ is meant OTUs that are found across all or substantially all Brachiaria-Urochloa species tested. By a ‘supplemental microbiome’ is meant OTUs that are found across a subset of the Brachiaria-Urochloa species tested. By a ‘unique microbiome’ is meant OTUs associated with specific Brachiaria-Urochloa species.
Endophytes having a desired core, supplemental or unique microbiome may then be selected. For example, endophytes with a broad host range may be selected as candidates for delivery of traits into plants of the Brachiaria-Urochloa species complex. For example, endophytes with a narrow or specific host range may be selected as candidates for specific traits of interest, for example for production of compounds that provide beneficial properties such as improved tolerance to water and/or nutrient stress, or improved resistance to pests and/or diseases in the plant with which the endophyte is associated. In a preferred embodiment, the beneficial properties include insecticidal or insect repellent activity. In a further preferred embodiment, the improved resistance to pests and/or diseases includes antifungal activity. In a particularly preferred embodiment the compound may be an inhibitory compound, such as a nitrification inhibitor, for example a fusicoccane such as brachialactone.
In a second aspect of the present invention there is provided a substantially purified or isolated endophyte selected from the group consisting of Hypocrea sp./Acremonium sp., Acremonium sp., Microsphaeropsis arundis, and Sarocladium sp./Acremonium sp., as described herein. Preferably said endophyte is isolated, selected and/or characterised by a method as hereinbefore described.
Representative samples, namely Hypocrea sp./Acremonium sp. 2.15.A.2, Acremonium sp. 2.3.C.1, Microsphaeropsis arundis 2.10.D.1, Sarocladium sp./Acremonium sp. 2.12.B.1, Sarocladium sp./Acremonium sp. 2.10.C.2 and Sarocladium sp./Acremonium sp. 2.11.B.1 were deposited at The National. Measurement Institute on 22 Sep. 2015 with accession numbers V15/028236, V15/028237, V15/028238, V15/028239, V15/028240, V15/028241 and V15/028242, respectively.
By ‘substantially purified’ is meant that the endophyte is free of other organisms. The term therefore includes, for example, an endophyte in axenic culture. Preferably, the endophyte is at least approximately 90% pure, more preferably at least approximately 95% pure, even more preferably at least approximately 98% pure, even more preferably at least approximately 99% pure. Preferably the endophyte is in axenic culture.
The term ‘isolated’ means that the endophyte is removed from its original environment (e.g. the natural environment if it is naturally occurring). For example, a naturally occurring endophyte present in a living plant is not isolated, but the same endophyte separated from some or all of the coexisting materials in the natural system, is isolated.
In its natural environment, the endophyte may live mutualistically within a plant. Alternatively, the endophyte may be an epiphyte, i.e. grow attached to or upon a plant. The endophyte may be a fungal endophyte or a bacterial endophyte.
The endophyte of the present invention may, in its natural environment, be associated with a plant of the Brachiaria-Urochloa species complex. More particularly, the plant of the Brachiaria-Urochloa species complex is selected from the group consisting of Brachiaria brizantha, Brachiaria decumbens, Brachiaria humidicola, Brachiaria stolonifera, Brachiaria ruziziensis, Urochloa brizantha, Urochloa decumbens, Urochloa humidicola, Urochloa mosambicensis, Brachiaria marlothii, Brachiaria nigropedata, Urochloa dictyoneura, Urochloa oligotricha, Urochloa panicoides, Brachiaria obtusiflora, Brachiaria serrifolia, Urochloa advena, Urochloa arrecta, Urochloa brachyura, Urochloa eminii, Urochloa mollis, Urochloa xantholeuca, Urochloa oligotricha, Urochloa panicoides, Urochloa plantaginea, Urochloa platynota, Urochloa xantholeuca, Brachiaria holosericea, Brachiaria reptans, Brachiaria milliformis, and Brachiaria distachya, as well as interspecific and intraspecific hybrids of Brachiaria-Urochloa species complex.
In a particularly preferred embodiment, the plant of the Brachiaria-Urochloa complex is selected from the group consisting of Brachiaria brizantha, Brachiaria decumbens, Brachiaria humidicola, Brachiaria ruziziensis and Urochloa mosambicensis.
By ‘associated with’ in this context is meant that the endophyte lives on, in or in close proximity to the plant. For example, it may be endophytic, for example living within the internal tissues of the plant, or epiphytic, for example growing externally on the plant.
The fungus may be a heterotroph that uses organic carbon for growth, more particularly a saprotroph that obtains nutrients by consuming detritus.
In a further aspect, the present invention provides a plant inoculated with an endophyte as hereinbefore described, said plant comprising an endophyte-free host plant stably infected with said endophyte. Preferably, said plant is a plant with which the endophyte is not naturally associated.
In a preferred embodiment, the plant with which the endophyte is associated has improved resistance to pests and/or diseases relative to an uninoculated control plant. Preferably, the improved resistance to pests and/or diseases includes insecticidal or insect repellent activity. In a further preferred embodiment, the improved resistance to pests and/or diseases includes antifungal activity.
In a preferred embodiment, the endophyte or plant with which the endophyte is associated may produce one or more compounds that provide beneficial properties such as improved tolerance to water and/or nutrient stress, or improved resistance to pests and/or diseases in the plant with which the fungus is associated. In a preferred embodiment, the beneficial properties include insecticidal or insect repellent activity. In a further preferred embodiment, the improved resistance to pests and/or diseases includes antifungal activity.
In a particularly preferred embodiment, the endophyte or plant with which the endophyte is associated may produce an inhibitory compound, such as a nitrification inhibitor, for example a fusicoccane such as brachialactone.
In a preferred embodiment, the host plant may be inoculated with more than one endophyte strain according to the present invention.
Preferably, the plant is an agricultural plant such as a grass species, preferably forage, turf or bioenergy grasses, or a grain crop or industrial crop grass.
The forage, turf or bioenergy grass may be those belonging to the Brachiaria-Urochloa species complex (panic grasses) including Brachiaria brizantha, Brachiaria decumbens, Brachiaria humidicola, Brachiaria stolonifera, Brachiaria ruziziensis, B. dictyoneura, Urochloa brizantha, Urochloa decumbens, Urochloa humidicola, Urochloa mosambicensis as well as interspecific and intraspecific hybrids of Brachiaria-Urochloa species complex, and those belonging to the genera Lolium and Festuca, including L. perenne (perennial ryegrass) and L. arundinaceum (tall fescue) and L. multiflorum (Italian ryegrass).
The grain crop or industrial crop grass may be those belonging to the genus Triticum, including T. aestivum (wheat), those belonging to the genus Hordeum, including H. vulgare (barley), those belonging to the genus Zea, including Z. mays (maize or corn), those belonging to the genus Oryza, including O. sativa (rice), those belonging to the genus Saccharum including S. officinarum (sugarcane), those belonging to the genus Sorghum including S. bicolor (sorghum), those belonging to the genus Panicum, including P. virgatum (switchgrass), and those belonging to the genera Miscanthus, Paspalum, Pennisetum, Poa, Eragrostis and Agrostis.
Preferably, the plant is infected with the endophyte by a method selected from the group consisting of inoculation breeding, crossing, hybridization, transduction, transfection, transformation and/or gene targeting; and combinations thereof.
The endophyte-infected plants may be cultured by known techniques. The person skilled in the art can readily determine appropriate culture conditions depending on the plant to be cultured.
In a further aspect, the present invention provides a plant, plant seed or other plant part derived from a plant of the present invention and stably infected with an endophyte of the present invention. Preferably, the plant, plant seed or other plant part with which the endophyte is associated has improved resistance to pests and/or diseases relative to an uninoculated control plant, plant seed or other plant part. In a preferred embodiment, the improved resistance to pests and/or diseases includes insecticidal or insect repellent activity. In a further preferred embodiment, the improved resistance to pests and/or diseases includes antifungal activity.
In a particularly preferred embodiment, endophyte or plant with which the endophyte is associated may produce an inhibitory compound, such as a nitrification inhibitor, for example a fusicoccane such as brachialactone.
Preferably, the plant cell, plant, plant seed or other plant part is from a grass, more preferably a forage, turf, bioenergy, grain crop or industrial crop grass.
The forage, turf or bioenergy grass may be those belonging to the Brachiaria-Urochloa species complex (panic grasses), including Brachiaria brizantha, Brachiaria decumbens, Brachiaria humidicola, Brachiaria stolonifera, Brachiaria ruziziensis, B. dictyoneura, Urochloa brizantha, Urochloa decumbens, Urochloa humidicola, Urochloa mosambicensis as well as interspecific and intraspecific hybrids of Brachiaria-Urochloa species complex such as interspecific hybrids between Brachiaria ruziziensis x Brachiaria brizantha, Brachiaria ruziziensis x Brachiaria decumbens, [Brachiaria ruziziensis x Brachiaria decumbens] x Brachiaria brizantha, [Brachiaria ruziziensis x Brachiaria brizantha] x Brachiaria decumbens and those belonging to the genera Lolium and Festuca, including L. perenne (perennial ryegrass) and L. arundinaceum (tall fescue) and L. multiflorum (Italian ryegrass).
The grain crop or industrial crop grass may be those belonging to the genus Triticum, including T. aestivum (wheat), those belonging to the genus Hordeum, including H. vulgare (barley), those belonging to the genus Zea, including Z. mays (maize or corn), those belonging to the genus Oryza, including O. sativa (rice), those belonging to the genus Saccharum including S. officinarum (sugarcane), those belonging to the genus Sorghum including S. bicolor (sorghum), those belonging to the genus Panicum, including P. virgatum (switchgrass), and those belonging to the genera Miscanthus, Paspalum, Pennisetum, Poa, Eragrostis and Agrostis.
By ‘plant cell’ is meant any self-propagating cell bounded by a semi-permeable membrane and containing plastid. Such a cell also required a cell wall if further propagation is desired. Plant cell, as used herein includes, without limitation, seeds suspension cultures, embryos, meristematic regions, callus tissue, leaves, roots, shoots, gametophytes, sporophytes, pollen and microspores.
In a further aspect, the present invention provides use of an endophyte as hereinbefore described to produce a plant stably infected with said endophyte. Preferably, the plant with which the endophyte is associated has improved resistance to pests and/or diseases relative to an uninoculated control plant. In a preferred embodiment, the improved resistance to pests and/or diseases includes insecticidal or insect repellent activity. In a further preferred embodiment, the improved resistance to pests and/or diseases includes antifungal activity.
In a preferred embodiment, the endophyte or plant with which the endophyte is associated may produce one or more compounds that provide beneficial properties such as improved tolerance to water and/or nutrient stress, or improved resistance to pests and/or diseases in the plant with which the fungus is associated. In a preferred embodiment, the beneficial properties include insecticidal or insect repellent activity. In a further preferred embodiment, the improved resistance to pests and/or diseases includes antifungal activity.
In a particularly preferred embodiment, the endophyte or plant with which the endophyte is associated may produce an inhibitory compound, such as a nitrification inhibitor, for example a fusicoccane, such as brachialactone.
In another preferred embodiment, the plant with which the endophyte is associated is a forage, turf, bioenergy, grain crop or industrial crop grass as hereinbefore described.
In a further aspect of the present invention, there is provided a method of increasing resistance to pests and/or diseases in a plant, said method including inoculating said plant with an endophyte as hereinbefore described. Preferably, the plant with which the endophyte is associated has improved resistance to pests and/or diseases relative to an uninoculated control plant. In a preferred embodiment, the improved resistance to pests and/or diseases includes insecticidal or insect repellent activity. In a further preferred embodiment, the improved resistance to pests and/or diseases includes antifungal activity.
In yet another preferred embodiment, the plant with which the endophyte is associated is a forage, turf, bioenergy, grain crop or industrial crop grass as hereinbefore described.
In another aspect, the present invention provides a method of producing a fusicoccane, said method including
Preferably the endophyte is an endophyte as hereinbefore described.
Preferably, the fusicoccane is compound of formula I:
otherwise known as bracialactone, or a derivative, an isomer and/or a salt thereof.
Preferably, the plant of the Brachiaria-Urochloa species complex is selected from the group consisting of Brachiaria brizantha, Brachiaria decumbens, Brachiaria humidicola, Brachiaria stolonifera, Brachiaria ruziziensis, Urochloa brizantha, Urochloa decumbens, Urochloa humidicola, Urochloa mosambicensis, Brachiaria marlothii, Brachiaria nigropedata, Urochloa dictyoneura, Urochloa oligotricha, Urochloa panicoides, Brachiaria obtusiflora, Brachiaria serrifolia, Urochloa advena, Urochloa arrecta, Urochloa brachyura, Urochloa Urochloa mollis, Urochloa xantholeuca, Urochloa oligotricha, Urochloa panicoides, Urochloa plantaginea, Urochloa platynota, Urochloa xantholeuca, Brachiaria holosericea, Brachiaria reptans, Brachiaria milliformis, and Brachiaria distachya, as well as interspecific and intraspecific hybrids of Brachiaria-Urochloa species complex.
Preferably the endophyte is grown in a culture medium including a source of carbohydrates.
The source of carbohydrates may be a starch/sugar-based agar or broth such as potato dextrose agar, potato dextrose broth or half potato dextrose agar or a cereal-based agar or broth such as oatmeal agar or oatmeal broth. Other sources of carbohydrates can include endophyte agar, Murashige and Skoog with 20% sucrose, half V8 juice/half PDA, water agar and yeast malt extract agar.
In a preferred embodiment, the endophyte may be cultured in a culture medium including potato dextrose or oatmeal, for example potato dextrose agar, half potato dextrose agar, oatmeal agar, potato dextrose broth or oatmeal broth. Most preferably, the fungus may be cultured in a culture medium including oatmeal.
The endophyte may be cultured under aerobic or anaerobic conditions.
The endophyte may be cultured for a period of approximately 1 to approximately 100 days, more preferably from approximately 1 to approximately 50 days more preferably from approximately 1 to approximately 10 days.
In a preferred embodiment, the endophyte may be cultured in a bioreactor. By a ‘bioreactor’ is meant a device or system that supports a biologically active environment, such as a vessel in which is carried out a chemical process involving fungi of the present invention and/or products thereof. The chemical process may be aerobic or anaerobic. The bioreactor may have a volume ranging in size from milliliters to cubic metres, for example from approximately 50 millilitres to approximately 50,000 litres. The bioreactor may be operated via batch culture, batch feed culture, perfusion culture or continuous culture, for example continuous culture in a stirred-tank bioreactor. Endophytes cultured in the bioreactor may be suspended or immobilised.
The method includes the step of recovering one or more organic compounds including the fusicoccane from endophyte cells, from the culture medium, or from air space associated with the culture medium or endophyte.
For example, the organic compound(s) may be recovered from intracellular tissues, from the culture medium into which the endophyte may secrete liquids, or from the air space into which the endophyte may secrete vapours.
Vapours may arise directly from the endophyte or from the secreted liquids which transition between vapour and liquid phases.
The step of recovering the organic compound(s) is preferably done by separating cells from the culture medium or capturing vapours associated with the culture medium or endophyte.
Preferably the organic compound(s) is then isolated or purified by a method selected from the group consisting of gas chromatography, liquid chromatography, fractional distillation, cryogenic distillation, membrane separation and absorption chromatography, such as pressure, vacuum or temperature swing adsorption.
By an ‘organic compound’ is meant a chemical compound, the molecules of which contain the element carbon.
In a preferred embodiment, the organic compound may be a hydrocarbon such as a volatile hydrocarbon or a liquid hydrocarbon. Most preferably, the organic compound may be a volatile hydrocarbon.
By a ‘hydrocarbon’ is meant an organic compound comprising the elements carbon and hydrogen.
The term ‘volatile’ in this context is meant an organic compound which can evaporate or sublimate at standard laboratory temperature and pressure. Volatile organic compounds include those with a high vapour pressure, low boiling point and/or low molecular weight.
In a further aspect of the present invention there is provided a method of producing a fusicoccane in a plant of the Brachiaria-Urochloa species complex, said method including:
Preferably, the plant of the Brachiaria-Urochloa species complex is selected from the group consisting of Brachiaria brizantha, Brachiaria decumbens, Brachiaria humidicola, Brachiaria stolonifera, Brachiaria ruziziensis, Urochloa brizantha, Urochloa decumbens, Urochloa humidicola, Urochloa mosambicensis, Brachiaria marlothii, Brachiaria nigropedata, Urochloa dictyoneura, Urochloa oligotricha, Urochloa panicoides, Brachiaria obtusiflora, Brachiaria serrifolia, Urochloa advena, Urochloa arrecta, Urochloa brachyura, Urochloa Urochloa mollis, Urochloa xantholeuca, Urochloa oligotricha, Urochloa panicoides, Urochloa plantaginea, Urochloa platynota, Urochloa xantholeuca, Brachiaria holosericea, Brachiaria reptans, Brachiaria milliformis, and Brachiaria distachya, as well as interspecific and intraspecific hybrids of Brachiaria-Urochloa species complex.
Preferably, the plant is infected with the endophyte by a method selected from the group consisting of inoculation, breeding, crossing, hybridization, transduction, transfection, transformation and/or gene targeting; and combinations thereof.
The endophyte-infected plants may be cultured by known techniques. The person skilled in the art can readily determine appropriate culture conditions depending on the plant to be cultured.
In a further aspect, the present invention provides a plant, plant seed or other plant part derived from a plant produced by the method of the present invention and stably infected with an endophyte of the present invention. Preferably, the plant, plant seed or other plant part with which the endophyte is associated has improved resistance to pests and/or diseases relative to an uninoculated control plant, plant seed or other plant part. In a preferred embodiment, the improved resistance to pests and/or diseases includes insecticidal or insect repellent activity. In a further preferred embodiment, the improved resistance to pests and/or diseases includes antifungal activity.
In a particularly preferred embodiment, the endophyte or plant with which the endophyte is associated may produce an inhibitory compound, such as a nitrification inhibitor, for example a fusicoccane such as brachialactone.
Preferably, the plant cell, plant, plant seed or other plant part is from a grass, more preferably a forage, turf, bioenergy, grain crop or industrial crop grass.
The forage, turf or bioenergy grass may be those belonging to the Brachiaria-Urochloa species complex (panic grasses), including Brachiaria brizantha, Brachiaria decumbens, Brachiaria humidicola, Brachiaria stolonifera, Brachiaria ruziziensis, B. dictyoneura, Urochloa brizantha, Urochloa decumbens, Urochloa humidicola, Urochloa mosambicensis as well as interspecific and intraspecific hybrids of Brachiaria-Urochloa species complex such as interspecific hybrids between Brachiaria ruziziensis x Brachiaria brizantha, Brachiaria ruziziensis x Brachiaria decumbens, [Brachiaria ruziziensis x Brachiaria decumbens] x Brachiaria brizantha, [Brachiaria ruziziensis x Brachiaria brizantha] x Brachiaria decumbens and those belonging to the genera Lolium and Festuca, including L. perenne (perennial ryegrass) and L. arundinaceum (tall fescue) and L. multiflorum (Italian ryegrass).
The grain crop or industrial crop grass may be those belonging to the genus Triticum, including T. aestivum (wheat), those belonging to the genus Hordeum, including H. vulgare (barley), those belonging to the genus Zea, including Z. mays (maize or corn), those belonging to the genus Oryza, including O. sativa (rice), those belonging to the genus Saccharum including S. officinarum (sugarcane), those belonging to the genus Sorghum including S. bicolor (sorghum), those belonging to the genus Panicum, including P. virgatum (switchgrass), and those belonging to the genera Miscanthus, Paspalum, Pennisetum, Poa, Eragrostis and Agrostis.
In another aspect, the present invention provides a method of inoculating a plant of the Brachiaria-Urochloa species complex with one or more endophytes, said method including
While Applicant does not wish to be restricted by theory, it is thought that conducting the method of the present invention under aseptic conditions ensures endophytes are inoculated into host plants that are substantially free of microbial organisms, thereby facilitating a high frequency of successful inoculation. Further, it is thought that the use of different media prior to inoculation to allow the host plant to establish, such as root growth promoting media, also facilitates high inoculation frequency. The use of a sterile environment also enables analysis of the microbiome without contamination.
For example the inoculation frequency may be between approximately 25% and approximately 100%, more preferably between approximately 50% and approximately 100%, even more preferably between approximately 75% and approximately 100%. The inoculation frequency may be higher than conventional methods.
Preferably, the plant of the Brachiaria-Urochloa species complex is of a species as hereinbefore described.
Preferably said one or more endophytes are selected from the endophytes as hereinbefore described. The one or more endophytes may be bacterial or fungal or a mixture thereof. In a preferred embodiment, the step of germinating the seed under aseptic conditions to produce host plants may include growing the germinated seed on shoot multiplication medium such as M3B and root multiplication medium such as MS+NAA. Preferably, the germinated seed may be grown on shoot multiplication medium, splitting the resulting shoots into single tillers and then transferring them to root multiplication medium. The single tillers may be grown on the root multiplication medium for approximately 1 to approximately 6 weeks, more preferably approximately 2 to approximately 3 weeks, to promote root growth. The resulting plantlets may again be split into single tillers for endophyte inoculation.
In a preferred embodiment, the step of inoculating the host plants with the one or more endophytes may include removal of the outer sheath to reveal shoot initial, creation of a wound in the shoot meristem and inoculation into the wound.
In a preferred embodiment, the method may include the further step of retaining the plantlets on sterile media following inoculation, preferably for a period of approximately 1 to approximately 6 weeks, more preferably approximately 2 to approximately 3 weeks.
In a preferred embodiment, the method may include the still further step of transferring the inoculated plants thus produced to soil or similar medium for further growth, for example under glasshouse conditions.
The present invention will now be more fully described with reference to the accompanying Examples and drawings. It should be understood, however, that the description following is illustrative only and should not be taken in any way as a restriction on the generality of the invention described above.
The endophytic microbiomes of five Brachiaria-Urochloa species were profiled using metagenomics. Species included B. brizantha, B. humidicola, B. ruziziensis, B. decumbens and U. mosambicensis. A total of three plants were profiled per species. Three organs were profiled from each plant (roots, stem and leaves). A total of two replicates were prepared per organ, per plant. Plant material (approximately 100 mg) was surface sterilised by soaking in 70% ethanol for 30 seconds, followed by 4.2% NaOCl (bleach) for 2 minutes, and then rinsed three to five times in sterile MilliQ water to ensure the sterilant had been completely removed. Samples were freeze-dried for 48 hours at −58° C. and 0.014 mBar. DNA was extracted using the Qiagen DNeasy plant mini kit according to manufacturer's instructions. Endophytic bacteria and fungi were evaluated in the metagenomics analyses using the universal PCR primers 515f and 806r for profiling the bacterial microbiome (V4 region of the 16S rDNA gene, approx. 350 base pairs), and 58A2F and ITS4 for the fungal microbiome (ITS2 region of the rDNA genes, approx. 400 base pairs), with associated Illumina adapters. Paired end libraries were prepared and loaded according to the corresponding Illumina user guide. Metagenomic sequence data was quality trimmed and paired using PANDSEQ to create operational taxonomic units (OTU), which were aligned against the GreenGenes bacterial database and the UNITE fungal database to assign taxonomy (OTU: 97% sequence identity, e-value <10e-110). The number of sequences associated with OTUs was calculated across all samples, and normalised as a percentage.
A total of 361 bacterial operational taxonomic units (OTUs) were identified across all Brachiaria-Urochloa species, comprising 25 bacterial Phyla, 56 Classes, 121 Families and 170 Genera (including candidate taxonomic groups) (Table 1). The analyses identified the core microbiome (OTUs found across all Brachiaria-Urochloa species) and the unique microbiome (OTUs associated with specific Brachiaria-Urochloa species), along with bacterial OTUs only associated with Brachiaria-Urochloa species known to produce brachialactone (B. humidicola and B. ruziziensis) (Table 1). The analyses also provided cross validation of the presence of endophytes isolated from these Brachiaria-Urochloa species.
In addition, 84 fungal OTUs were identified, comprising 5 Phyla, 14 Classes, 32 Families and 44 Genera (Table 2). The analyses identified the core microbiome (OTUs found across all Brachiaria-Urochloa species) and the unique microbiome (OTUs associated with specific Brachiaria-Urochloa species), along with fungal OTUs only associated with Brachiaria-Urochloa species known to produce brachialactone (B. humidicola and B. ruziziensis) (Table 2). The analyses also provide cross validation of the presence of endophytes isolated from these Brachiaria-Urochloa species.
Brachiaria-Urochloa species (361 OTUs), including identification of the core microbiome,
Enterobacteriaceae sp
Rhodospirillaceae sp
Comamonadaceae sp
Agrobacterium sp
Alicyclobacillaceae sp
Sphingobacteriaceae sp
Mycobacterium sp
Bacillus sp
Chitinophagaceae sp
Pseudomonas sp
Caulobacteraceae sp
Rhodoplanes sp
Rhizobium sp
Rhizobiales sp
Janthinobacterium sp
Cellulomonas sp
Herbaspirillum sp
Flavobacterium sp
Xanthomonadaceae sp
Solirubrobacterales sp
Dyella
spginsengisoli
Betaproteobacteria sp 1
Opitutus sp
Aquicella sp
Candidatus_
Xiphinematobacter sp
Microbacterium sp
Flavobacterium
spsuccinicans
Kiloniellales sp
Alphaproteobacteria sp 1
Devosia sp
Planctomyces sp
Sphingomonadaceae sp
Isosphaeraceae sp
Asticcacaulis
spbiprosthecium
Pirellulaceae sp 1
Myxococcales sp 1
Gammaproteobacteria sp
Mycobacterium
spvaccae
Chitinophaga sp
Dechloromonas sp
Streptomyces sp
Desulfosporosinus
spmeridiei
Rhodocyclaceae sp
Novosphingobium sp
Oxalobacteraceae sp
Opitutaceae sp
Hyphomicrobium sp
Legionellaceae sp
Rhodanobacter sp
Sinobacteraceae sp
Sphingobium sp
Nocardioidaceae sp
Azospirillum sp
Acidobacteria sp 1
Alphaproteobacteria sp 2
Klebsiella sp
Pleomorphomonas
sporyzae
Rhizobiaceae sp
Bacillus
spginsengihumi
Rhodobacteraceae sp
Cytophagaceae sp
Bradyrhizobium sp
Methylotenera
spmobilis
Microbacterium
spchocolatum
Acidobacteria sp 2
Rhodobacter sp
Coxiellaceae sp
Acidimicrobiales sp 1
Mesorhizobium sp
Cellvibrio sp
Methylibium sp
Rubrivivax
spgelatinosus
Clostridium sp
Erythrobacteraceae sp
Pedosphaerales sp 1
Microbacteriaceae sp
Thermomicrobia sp
Hyphomicrobiaceae sp
Sphingobacteriales sp
Bradyrhizobiaceae sp
Acetobacteraceae sp
Phaeospirillum
spfulvum
Legionella sp
Dyella sp
Gemmata sp
Hydrogenophaga sp
Betaproteobacteria sp 2
Rhodanobacter
splindaniclasticus
Pedobacter sp
Asticcacaulis sp
Magnetospirillum sp
Prosthecobacter sp
Paenibacillus sp
Sphingomonas
spwittichii
Methylophilaceae sp
Sphingomonas sp
Chryseobacterium sp
Chloroflexi sp 1
Propionivibrio sp
Phenylobacterium sp
Delftia sp
Bacillales sp
Erwinia sp
Limnohabitans sp
Cohnella sp
Denitrobacter sp
Kaistia sp
Dyadobacter sp
Alphaproteobacteria sp 3
Sphingomonas
spazotifigens
Actinomycetales sp
Pirellulaceae sp 2
Fluviicola sp
Shinella sp
Spirochaeta
spaurantia
Brucellaceae sp
Agrobacterium
spsullae
Fibrobacteria sp
Alteromonadales sp 1
Nakamurellaceae sp
Alcaligenaceae sp
Desulfovibrio sp
Sediminibacterium sp
Cryocola sp
Sphingopyxis sp
Burkholderia sp
Gaiellaceae sp
Niastella sp
Rathayibacter sp
Pandoraea sp
Burkholderiales sp
Thermomonas sp
Novosphingobium
spcapsulatum
Pseudomonas
spnitroreducens
Lachnospiraceae sp
Caldilineaceae sp
Micrococcaceae sp
Geobacillus sp
Salinibacterium sp
Rickettsiales sp
Cyanobacteria sp 1
Hyphomonadaceae sp
Salinispora
sptropica
Bdellovibrio sp
Caulobacter sp
Salinispora sp
Sulfurospirillum sp
Uliginosibacterium sp
Bdellovibrio
spbacteriovorus
Chloroflexi sp 2
Ruminococcaceae sp
Anaerolineae sp 1
Kyrpidia sp
Rhodoferax sp
Aurantimonadaceae sp
Curtobacterium sp
Cupriavidus sp
Nocardioides sp
Legionellales sp
Coprococcus sp
Pseudomonadaceae sp
Emticicia sp
Procabacteriaceae sp
Aeromonadaceae sp
Cytophaga sp
Haliangiaceae sp
Chloroflexi sp 3
Gemmatimonadetes sp 1
Betaproteobacteria sp 3
Demequina sp
Cyanobacteria sp 2
Moraxellaceae sp
Chlorobi sp 1
Bacteriovoracaceae sp
Paludibactersp
Burkholderia
spbryophila
Porphyromonadaceae sp
Leptothrix sp
Gemmataceae sp
Aminobacter sp
Desulfovibrio
spmexicanus
Flavihumibacter sp
Ramlibacter sp
Neisseriaceae sp
Asteroleplasma sp
Edaphobacter
spmodestum
Verrucomicrobiaceae sp
Patulibacteraceae sp
Arthrospira sp
Achromobacter sp
Desulfobulbus sp
Pelomonas sp
Zoogloea sp
Desulfovibrio
spputealis
Salmonella
spenterica
Acidimicrobiales sp 2
Phyllobacteriaceae sp
Dokdonella sp
Pedosphaerales sp 2
Variovorax
spparadoxus
Armatimonadetes sp
Bacteroidales sp
Chloroflexi sp 4
Geobacter sp
Deltaproteobacteria sp 1
Sulfuricurvum
spkujiense
Phaeospirillum sp
Tatlockia sp
Terriglobus sp
Pelosinus sp
Thermomonas
spfusca
Gemmata
spobscuriglobus
Telmatospirillum sp
Luteibacter
sprhizovicinus
Acidisoma sp
Fimbriimonas sp
Janibactersp
Anaerolineae sp 2
Chloroflexi sp 5
Thermoanaerobacterium
spsaccharolyticum
Luteolibacter sp
Leadbetterella sp
Afifella sp
Microthrixaceae sp
Chlorobi sp 2
Ancylobacter sp
Steroidobacter sp
Singulisphaera sp
Luteimonas sp
Gemmatimonadetes sp 2
Bosea
spgenosp.
Salinibacterium
spamurskyense
Pedosphaerales sp 3
Phycicoccus sp
Spirosoma sp
Chromatiales sp
Rathayibacter
spcaricis
Treponema sp
Holophagaceae sp
Anaerovorax sp
Desulfobulbaceae sp
Reichenbachiella sp
Nannocystis sp
Polyangiaceae sp
Haererehalobacter
spsalaria
Streptomyces
splanatus
Aquitalea
spmagnusonii
Erwinia
spsoli
Trabulsiella sp
Pilimelia sp
Clostridia sp
Ammoniphilus sp
Paenibacillaceae sp
Streptosporangiaceae sp
Methylocystaceae sp
Solibacterales sp
Acidobacteria sp 3
Frankiaceae sp
Acidovorax
spdelafieldii
Piscirickettsiaceae sp
Candidatus_Solibacter sp
Parvibaculum sp
Betaproteobacteria sp 4
Acidobacteria sp 4
Cellulomonas
spuda
Chloroflexi sp 6
Brevibacillus
spreuszeri
Blastomonas sp
Streptomycetaceae sp
Sphingomonas
spechinoides
Polaromonas sp
Cellulomonadaceae sp
Armatimonadia sp
Cyanobacteria sp 3
Comamonas sp
Gracilibacteraceae sp
Cenarchaeaceae sp
Acidovorax sp
Janthinobacterium
splividum
Acinetobacter sp
Ruminococcus sp
Simplicispira sp
Rheinheimera sp
Pseudomonas
spstutzeri
Acidobacteriaceae sp
Kouleothrixaceae sp
Azospira sp
Chromatiaceae sp
Pseudomonas
spviridiflava
Staphylococcus
spaureus
Alteromonadaceae sp
Aeromicrobium sp
Chthoniobacter sp
Saprospiraceae sp
Bacillus
spcoagulans
Frankia sp
Kineosporiaceae sp
Alicyclobacillus sp
Sporolactobacillaceae sp
Pedosphaerales sp 4
Nocardia sp
Planctomycetes sp
Syntrophobacteraceae sp
Xanthobacteraceae sp
Saprospirales sp
Geobacillus
spthermodenitrificans
Paenibacillus
spchondroitinus
Mycoplana sp
Corynebacterium sp
Microbacterium
spaurum
Nostocaceae sp
Thermoanaerobacterium
Peptococcaceae sp
Clostridiales sp
Ochrobactrum sp
Myxococcales sp 2
Pseudomonas
spalcaligenes
Methanobacterium sp
Methylophilales sp
Enterobacter sp
Niabella sp
Bacillaceae sp
Balneimonas sp
Schlegelella sp
Deltaproteobacteria sp 2
Chthoniobacteraceae sp
Acidobacteria sp 5
Inquilinus sp
Myxococcaceae sp
Prosthecobacter
spdebontii
Dermacoccus sp
Jonesiaceae sp
Actinoplanes sp
Clostridium
spbowmanii
Chromobacterium sp
Tolumonas sp
Alteromonadales sp 2
Corynebacterium
spkroppenstedtii
Cloacibacterium sp
Thermogemmatispora sp
Staphylococcus
spepidermidis
Sporomusa sp
Azovibrio sp
Alteromonadales sp 3
Erwinia
spdispersa
Acinetobacter
spjohnsonii
Bacteroides sp
Anaerococcus sp
Peptoniphilus sp
Acidocella sp
Desulfovibrionaceae sp
Urochloa species (84 OTUs), including identification of the core microbiome, the unique
B. decumbens (Bd).
Dothideomycetes sp
(Microdochium bolleyi)
Fusarium
proliferatum
Lecythophora sp
Chaetosphaeriales sp
Sarocladium
strictum
Chaetomium sp 1
Sordariomycetes sp
Hypocrea sp
Coniochaeta sp
Microsphaeropsis
arundinis
Chrysosporium sp 1
Acremonium sp
Podospora sp 1
Fusarium sp
Fusarium
oxysporum
f
Rhizophagus sp
Cryptococcus
laurentii
Flagelloscypha
minutissima
Podospora
communis
Cladosporium
cladosporioides
Exophiala
cancerae
Rhizophagus
irregularis
Myrmecridium
schulzeri
Urediniomycete sp
Rhizophagus
irregularis
Paraglomus
brasilianum
Parascedosporium
putredinis
Chaetomium
thermophilum
Candida
tropicalis
Conlarium sp
Arthrobotrys sp
Candida sp
Trichoderma
harzianum
Pseudeurotium sp
Chaetomium sp 2
Doratomyces sp
Zopfiella
marina
Monographella
cucumerina
Clitopilus
scyphoides
Acephala sp
Trichurus sp
Corynascus sp
Trichoderma
asperellum
Gibberella
fujikuroi
Fusarium sp
Fusarium
oxysporum
Peziza
ostracoderma
Pseudallescheria
boydii
Pseudogymnoascus sp
Claroideoglomus sp
Leptosphaeria sp
Herpotrichiellaceae
Haptocillium
sinense
Piriformospora
indica
Exophiala sp
Neotyphodium sp FaTG 2
Podospora sp 2
Meira sp
Leptosphaerulina
chartarum
Chrysosporium sp 2
llyonectria sp
Gibberella
intricans
Ophiostoma
stenoceras
Microbotryomycetes sp
Cryptococcus
podzolicus
Microbial diversity was greatest in the roots of Brachiaria-Urochloa species accounting for 359 bacterial species (99.4%) and 83 fungal species (98.8%) (Tables 1 and 2). The microbial diversity in the stem and leaf was significantly lower than the roots, accounting for 5-20 bacterial or fungal OTUs.
The core microbiome consisted of 130 bacterial OTUs and 14 fungal OTUs (Tables 1, 2, and 3). The core bacterial microbiome contained a diverse array of taxa, while the core fungal microbiome predominantly contained Sordariomycetes species (8). The OTUs associated with the core microbiome were also the most abundant OTUs across all Brachiaria-Urochloa species. The number of OTUs unique to Brachiaria-Urochloa species ranged from 5 to 27 for bacteria and 2 to 12 for fungi, and were predominantly found in low abundance in their respective species.
B.
B.
B.
U.
B.
brizantha
decumbens
humidicola
mosambicensis
ruziziensis
Microbial Species Associated with B. humidicola and B. decumbens
The number of bacterial and fungal OTUs associated with B. humidicola was 189 and 48 respectively. B. humidicola had the highest fungal diversity, approximately 15% higher than any other Brachiaria-Urochloa species. Conversely, B. humidicola had the second lowest bacterial diversity, approximately 31% lower than B. decumbens (highest bacterial diversity). As with all other Brachiaria-Urochloa species the greatest microbial diversity was observed in the roots, while there was very low microbial diversity in the stems and leaves.
The number of bacterial and fungal OTUs associated with B. decumbens was 276 and 37 respectively. B. decumbens had the highest bacterial diversity, approximately 3 to 33% higher than any other Brachiaria-Urochloa species. Conversely, B. decumbens had the second lowest fungal diversity, approximately 23% lower than B. humidicola. As with all other Brachiaria-Urochloa species the greatest microbial diversity was observed in the roots, while there was very low microbial diversity in the stems and leaves.
The top five fungal and bacterial OTUs associated with both B. humidicola and B. decumbens show sequence homology to isolates from NCBI that have been predominantly been identified as endophytes, including endophytes of other Poaceae species (e.g. Oryzae sativa, Triticum aestivum), mycorrhizae (e.g. Glomus species) or rhizobacteria (Rhizobiales species). The fungal pathogen Fusarium proliferatum was also present, which is a seed-borne pathogen of a range of agricultural crop species (Tables 4 and 5).
Dothidiomycetes
Trillium
tschonoskii
Holcus
lanatus
Microdochium
Triticum
bolleyi
aestivum
Sporobolus
cryptandrus
Chaetosphaeriales
Chaetosphaeriales
Populus
trichocarpa
Chaetosphaeriaceae
Populus
deltoides
Fusarium
Fusarium
Dendrobium
proliferatum
proliferatum
Fusarium sp.
Saccharum
officinarum
Allium
cepa
L.
Glomus sp.
Sequoiadendron
Glomeromycota
giganteum
Enterobacteriaceae
Enterobacter
Oryza
sativa
oryziphilus
Kosakonia
Saccharum
sacchari
officinarum
Pseudomonas sp
Pseudomonas
Oryza
sativa
fulva
Pseudomonas
—
protegens Pf-5
Pseudomonas
−
Soil
entomophila
Agrobacterium sp
Agrobacterium
—
tumefaciens
Rhizobium
Astragalus
vignae
dahuricus
Rhizobium
Lemna
paknamense
aequinoctialis
Comamonadaceae
Ottowia
shaoguanensis
Comamonas
—
granuli
Comamonas
testosteroni
Herbaspirillum sp
Herbaspirillum
Miscanthus
frisingense
sacchariflorus
Herbaspirillum
huttiense
Oxalicibacterium
horti
Microbial Diversity Associated with Brachialactone Producing Brachiaria-Urochloa Species
A total of 45 bacterial and 29 fungal OTUs were identified only in the Brachiaria-Urochloa species found to produce brachialactone, B. humidicola and/or B. ruziziensis (Tables 1 and 2). The OTUs associated with brachialactone producing Brachiaria-Urochloa species represent a range of diverse bacterial and fungal taxa.
A total of 97 fungal endophyte isolates derived from 11 Brachiaria-Urochloa species were identified in a global study of 281 accessions from 23 countries. The internal transcribed spacer ITS sequence was used for further characterisation. The entire region of nuclear ribosomal DNA which comprises both internal transcribed spacers ITS1 and ITS2 and the 5.8S subunit was PCR-amplified using primers ITS5 and ITS4 (White et al. 1990). Purified PCR amplification products were sequenced using Sanger sequencing technology. Isolated subcultured endophytes were then grouped based on ITS sequence identity. Ribosomal DNA (rDNA) sequence analysis based on the internal transcribed spacer (ITS) and 18S coding regions shows that Brachiaria endophyte isolates are genetically diverse, representing at least 10 distinct taxonomic groups (
Sequence data was used in BLASTN analysis to identify matches in the NCBI database. Brachiaria endophytes discovered are genetically novel. Comparison of each isolates ITS sequence to those in publically available databases did not identify any fungal strains with >90% identity. Phylogenetic analysis confirmed that isolates from different ITS clusters belonged to diverse genera. In several accessions, multiple endophytes isolated from a single plant belonged to different rDNA specific clusters, suggesting co-existence of multiple fungal endophyte species in the same plant (Table 6).
B. decumbens
U. mosambicensis
B. holosericea
B. reptans
B. reptans
B. miliiformis
B. ruziziensis
B. ruziziensis
U. panicoides
U. mosambicensis
U. oligotricha
B. humidicola
U. panicoides
U. oligotricha
U. mosambicensis
B. humidicola
B. brizantha
B. decumbens
B. humidicola
B. humidicola
B. decumbens
U. mosambicensis
U. mosambicensis
B. decumbens
B. humidicola
B. distachya
B. miliiformis
The rDNA-ITS region sequence for selected isolated and culturable fungal endophyte strains was used to identify their presence/absence in the microbiomes of 5 Brachiaria-Urochloa species (Bb—B. brizantha; Bh—B. humidicola; Bd—B. decumbens; Um—U. mosambicensis; Ur—U. ruziensis) (
Mature plants of Brachiaria-Urochloa grass-endophyte associations that had been maintained in a controlled environment were subjected to metabolic profiling analysis. Four individual plants (biological replicates) from each of three Brachiaria-Urochloa species (B. humidicola, U. mosambicensis, B. ruziziensis) were analysed for the presence of brachialactone using liquid chromatography-mass spectrometry (LC-MS). Freeze-dried pseudostem samples were prepared for LC-MS analysis using an 80% methanol extraction procedure. The compound brachialactone was identified in the root tissues of Brachiaria-endophyte associations (B. humidicola, B. ruziensis) (
Brachiaria-Urochloa
B. humidicola
U. mosambiciensis
B. decumbens
B. ruziziensis
A host panel comprising commercially relevant Brachiaria-Urochloa germplasm was established to enable inoculation of genetically novel and highly diverse endophyte isolates into a single host genotype. An optimised method for endophyte inoculation into host plants free of microbial organisms in axenic conditions was developed, facilitating a high frequency of successful inoculation (Table 8). Four fungal endophytes representing four of the rDNA sequence-defined clades were identified as candidates for inoculation and characterisation into the Brachiaria-Urochloa host panel.
Sterilised Brachiaria seed are germinated under aseptic conditions to remove microbial organisms from the host plants to be used for inoculation. Microbe-free donor plantlets are grown on shoot multiplication media (M3B) under sterile conditions. Donor shoots are split into single tillers and transferred to root multiplication media (MS+NAA). Single tillers are grown for 2-3 weeks to promote root growth, plantlets are then again split into single tillers and the outer sheath is removed to reveal shoot initial. Shoot initials with intact roots are transferred to water agar for inoculation of endophyte mycelia. For endophyte inoculation, a small cut is made across the shoot meristem, and endophyte is inoculated into the wound. Following inoculation, plantlets are retained on ½ MS media for 2 weeks. They are then transferred to soil and grown under glasshouse conditions for 8 weeks before testing for endophyte presence using a diagnostic set of strain specific SSR markers (
Endophyte inoculation frequency was determined for each candidate endophyte, approximately 6 months post inoculation, using a diagnostic (i.e. specific allele sizes at each SSR loci for each endophyte) set of simple sequence repeat (SSR) markers for each endophyte isolate.
Successful inoculation was achieved for representative endophytes from each of the ribosomal DNA sequence-defined clades (Table 8). Variation between endophyte isolates representing different ITS groups was observed. ITS5 (2.15.A.2)>ITS7 (2.10.C.2)>ITS2 (12.1.B)>ITS1 (5.1.B). Cross species compatibility was also observed. Endophyte isolate 2.15.A.2 (58 to 83%) and 2.10.C.2 (38% to 83%) exhibit broad species compatibility compared to the moderately compatible 12.1.B (8 to 76%) and narrow host compatibility of 5.1.B (0 to 7%). As would be expected, each endophyte strain shows highest inoculation frequency for the species from which it was originally isolated.
Variation in inoculation ability of the host was also observed. U. mosambicensis forms stable associations with a broad range of fungal endophytes at a very high frequency of successful inoculation (60%). Also of note is that U. mosambicensis forms associations with multiple, highly diverse fungal endophytes (FIG. 1; Table 6). Endophyte strains representing 6 of the 7 ITS groups identified in Brachiaria were isolated from this species (
A significant challenge in plant microbiome studies is that in order to analyse the endophytic component of a plant microbiome, it is necessary to extract DNA from plant tissues. The presence of a high proportion of plant DNA:microbe DNA (in the order of 20:1 for bacteria and 1:1 for fungi) in DNA extracted affects downstream sequence analysis. In previous studies, one way this has been dealt with is to generate large numbers of sequence reads to achieve a target number of microbiome reads.
In this example, a method was developed to enrich for the microbiome (both bacterial and fungal DNA) when extracting DNA from plant seed. The method is not limited in application to plant seed, and may be applied to any plant tissue from any species of interest, including leaf, stem and/or root plant material.
Seed-associated endophytic microbes are of interest as they may be exploited in a molecular breeding scenario whereby the microbe and host plant are co-selected for a particular trait of interest. Further, the presence of endophytic microbes in both root and seed microbiomes is of particular interest as seed associated microbes that are distributed throughout the plant may be associated with enhanced performance traits, such as pest and disease resistance, or biological nitrification inhibition (BNI) through the production of brachialactone.
Variation in host seed colonisation may be an indicator of host-endophyte co-evolution and specialisation
Once isolated and purified, individual components of the endophytic seed microbiome can be genome sequenced and characterised for molecular marker development, taxonomic identification and phylogenomic analyses. Selected microbiome component organisms can also be phenotypically assessed singly and in combination to identify microbes that confer enhanced production traits, for example BNI, to a range of commercially significant Brachiaria species. There is potential to further exploit the biological properties of the Brachiaria microbiome across a broad range of crop species to the benefit of sustainable agriculture and the environment.
A method was developed to enrich for the microbiome (bacterial and fungal DNA) component in Brachiaria seed (
Fifty grams of seed from each of the ten selected accessions (Table 9) was surface sterilised (5% [w/v] NaHCl and Tween 20) for 30 min with shaking. Seed samples were then rinsed eight to ten times in sterile MilliQ water to ensure the sterilant had been completely removed. Seed were dried on sterile filter paper under aseptic conditions overnight. Dried seeds were partially ground using a genogrinder (SPEX SamplePrep 2010 Geno/Grinder®, Metuchen, USA). Ground seeds were then washed twice for 12 hrs with absolute ethanol and continuous shaking. Following washes, samples were allowed to settle and the supernatant containing the seed associated endophytic microbiome collected. The supernatant was then completely evaporated under sterile conditions. DNA was extracted from the final crude (what was left following ethanol evaporation) using the Qiagen DNeasy plant mini kit according to manufacturer's instructions.
Simultaneously, DNA was also extracted from surface sterilised seeds (10 seeds from each accession) using the Qiagen DNeasy plant mini kit according to manufacturer's instructions. Bacteria and fungi were evaluated in the metagenomics analyses using the universal PCR primers 515f (Wang & Qian, 2009) and 806r (McBain et al, 2003) for profiling the bacterial microbiome (V4 region of the 16S rDNA gene, approx. 350 base pairs), and 58A2F (Martin & Rygiewicz, 2005) and ITS4 (White et al, 1990) for the fungal microbiome (ITS2 region of the rDNA genes, approx. 400 base pairs), with associated Illumina adapters. Ribosomal RNA gene amplicons were prepared and sequenced on the MiSeq (Illumina) according to the corresponding user guide.
Brachiaria species used in this example.
Brachiaria species
B. brizantha
B. humidicola
B. decumbens
B. ruziziensis
The endophytic (bacterial and fungal) seed microbiomes of four selected Brachiaria-Urochloa species were profiled using metagenomics with the aim of identifying microbes associated with a particular species and or/trait, such as pest and disease resistance, or biological nitrification inhibition (BNI) through the production of brachialactone.
Brachiaria species examined included three species—B. humidicola, B. ruziziensis, B. decumbens—previously documented to produce biological nitrification inhibition (BNI) compounds, and B. brizantha which does not produce BNI compounds (Table 9).
The data is then analysed to identify the seed associated endophytic microbiome of Brachiaria:
It is to be understood that various alterations, modifications and/or additions may be made without departing from the spirit of the present invention as outlined herein.
As used herein, except where the context requires otherwise, the term “comprise” and variations of the term, such as “comprising”, “comprises” and “comprised”, are not intended to be in any way limiting or to exclude further additives, components, integers or steps.
Reference to any prior art in the specification is not, and should not be taken as, an acknowledgment or any form of suggestion that this prior art forms part of the common general knowledge in Australia or any other jurisdiction or that this prior art could reasonably be expected to be ascertained, understood and/or regarded as relevant by a person skilled in the art.
Number | Date | Country | Kind |
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2015903909 | Sep 2015 | AU | national |
2016903174 | Aug 2016 | AU | national |
Number | Date | Country | |
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Parent | 15762988 | Mar 2018 | US |
Child | 17518882 | US |