WO2011044632A1 - Manipulation of flavonoid biosynthetic pathway - Google Patents

Manipulation of flavonoid biosynthetic pathway Download PDF

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Publication number
WO2011044632A1
WO2011044632A1 PCT/AU2010/001362 AU2010001362W WO2011044632A1 WO 2011044632 A1 WO2011044632 A1 WO 2011044632A1 AU 2010001362 W AU2010001362 W AU 2010001362W WO 2011044632 A1 WO2011044632 A1 WO 2011044632A1
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plant
polypeptide
genes
expression
gene
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PCT/AU2010/001362
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French (fr)
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Aidyn Mouradov
German Spangenberg
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Agriculture Victoria Services Pty Ltd
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Priority claimed from AU2009905058A external-priority patent/AU2009905058A0/en
Application filed by Agriculture Victoria Services Pty Ltd filed Critical Agriculture Victoria Services Pty Ltd
Priority to CA2777249A priority Critical patent/CA2777249C/en
Priority to AU2010306410A priority patent/AU2010306410B2/en
Priority to DK10822907.1T priority patent/DK2488010T3/en
Priority to NZ599243A priority patent/NZ599243A/en
Priority to US13/501,918 priority patent/US20120204289A1/en
Priority to EP10822907.1A priority patent/EP2488010B1/en
Publication of WO2011044632A1 publication Critical patent/WO2011044632A1/en

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    • C12BIOCHEMISTRY; BEER; SPIRITS; WINE; VINEGAR; MICROBIOLOGY; ENZYMOLOGY; MUTATION OR GENETIC ENGINEERING
    • C12QMEASURING OR TESTING PROCESSES INVOLVING ENZYMES, NUCLEIC ACIDS OR MICROORGANISMS; COMPOSITIONS OR TEST PAPERS THEREFOR; PROCESSES OF PREPARING SUCH COMPOSITIONS; CONDITION-RESPONSIVE CONTROL IN MICROBIOLOGICAL OR ENZYMOLOGICAL PROCESSES
    • C12Q1/00Measuring or testing processes involving enzymes, nucleic acids or microorganisms; Compositions therefor; Processes of preparing such compositions
    • C12Q1/68Measuring or testing processes involving enzymes, nucleic acids or microorganisms; Compositions therefor; Processes of preparing such compositions involving nucleic acids
    • C12Q1/6876Nucleic acid products used in the analysis of nucleic acids, e.g. primers or probes
    • C12Q1/6888Nucleic acid products used in the analysis of nucleic acids, e.g. primers or probes for detection or identification of organisms
    • C12Q1/6895Nucleic acid products used in the analysis of nucleic acids, e.g. primers or probes for detection or identification of organisms for plants, fungi or algae
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    • C12BIOCHEMISTRY; BEER; SPIRITS; WINE; VINEGAR; MICROBIOLOGY; ENZYMOLOGY; MUTATION OR GENETIC ENGINEERING
    • C12NMICROORGANISMS OR ENZYMES; COMPOSITIONS THEREOF; PROPAGATING, PRESERVING, OR MAINTAINING MICROORGANISMS; MUTATION OR GENETIC ENGINEERING; CULTURE MEDIA
    • C12N15/00Mutation or genetic engineering; DNA or RNA concerning genetic engineering, vectors, e.g. plasmids, or their isolation, preparation or purification; Use of hosts therefor
    • C12N15/09Recombinant DNA-technology
    • C12N15/63Introduction of foreign genetic material using vectors; Vectors; Use of hosts therefor; Regulation of expression
    • C12N15/79Vectors or expression systems specially adapted for eukaryotic hosts
    • C12N15/82Vectors or expression systems specially adapted for eukaryotic hosts for plant cells, e.g. plant artificial chromosomes (PACs)
    • C12N15/8241Phenotypically and genetically modified plants via recombinant DNA technology
    • C12N15/8242Phenotypically and genetically modified plants via recombinant DNA technology with non-agronomic quality (output) traits, e.g. for industrial processing; Value added, non-agronomic traits
    • C12N15/8243Phenotypically and genetically modified plants via recombinant DNA technology with non-agronomic quality (output) traits, e.g. for industrial processing; Value added, non-agronomic traits involving biosynthetic or metabolic pathways, i.e. metabolic engineering, e.g. nicotine, caffeine
    • CCHEMISTRY; METALLURGY
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    • C12NMICROORGANISMS OR ENZYMES; COMPOSITIONS THEREOF; PROPAGATING, PRESERVING, OR MAINTAINING MICROORGANISMS; MUTATION OR GENETIC ENGINEERING; CULTURE MEDIA
    • C12N15/00Mutation or genetic engineering; DNA or RNA concerning genetic engineering, vectors, e.g. plasmids, or their isolation, preparation or purification; Use of hosts therefor
    • C12N15/09Recombinant DNA-technology
    • C12N15/63Introduction of foreign genetic material using vectors; Vectors; Use of hosts therefor; Regulation of expression
    • C12N15/79Vectors or expression systems specially adapted for eukaryotic hosts
    • C12N15/82Vectors or expression systems specially adapted for eukaryotic hosts for plant cells, e.g. plant artificial chromosomes (PACs)
    • C12N15/8241Phenotypically and genetically modified plants via recombinant DNA technology
    • C12N15/8242Phenotypically and genetically modified plants via recombinant DNA technology with non-agronomic quality (output) traits, e.g. for industrial processing; Value added, non-agronomic traits
    • C12N15/8243Phenotypically and genetically modified plants via recombinant DNA technology with non-agronomic quality (output) traits, e.g. for industrial processing; Value added, non-agronomic traits involving biosynthetic or metabolic pathways, i.e. metabolic engineering, e.g. nicotine, caffeine
    • C12N15/825Phenotypically and genetically modified plants via recombinant DNA technology with non-agronomic quality (output) traits, e.g. for industrial processing; Value added, non-agronomic traits involving biosynthetic or metabolic pathways, i.e. metabolic engineering, e.g. nicotine, caffeine involving pigment biosynthesis
    • CCHEMISTRY; METALLURGY
    • C12BIOCHEMISTRY; BEER; SPIRITS; WINE; VINEGAR; MICROBIOLOGY; ENZYMOLOGY; MUTATION OR GENETIC ENGINEERING
    • C12QMEASURING OR TESTING PROCESSES INVOLVING ENZYMES, NUCLEIC ACIDS OR MICROORGANISMS; COMPOSITIONS OR TEST PAPERS THEREFOR; PROCESSES OF PREPARING SUCH COMPOSITIONS; CONDITION-RESPONSIVE CONTROL IN MICROBIOLOGICAL OR ENZYMOLOGICAL PROCESSES
    • C12Q2600/00Oligonucleotides characterized by their use
    • C12Q2600/158Expression markers

Definitions

  • the present invention relates to methods for manipulating or identifying genes involved in the flavonoid biosynthetic pathway in plants, and to related constructs, plants, plant cells, plant seeds and other plant parts.
  • Flavonoids constitute a relatively diverse family of aromatic molecules that are derived from phenyalanine and malonyl-coenzyme A (CoA, via the fatty acid pathway). These compounds include six major subgroups that are found in most higher plants: the chalcones, flavones, flavonols, flavandiols, anthocyanins and proanthocyanidins (or condensed tannins). A seventh group, the aurones, is widespread, but not ubiquitous.
  • flavonoids Some plant species also synthesize specialised forms of flavonoids, such as the isoflavonoids that are found in legumes and a small number of non-legume plants. Similarly, sorghum, maize and gloxinia are among the few species known to synthesize 3-deoxyanthocyanins (or phlobaphenes in the polymerised form).
  • the stilbenes which are closely related to flavonoids, are synthesised by another group of unrelated species that includes grape, peanut and pine.
  • flavonoids Besides providing pigmentation to flowers, fruits, seeds, and leaves, flavonoids also have key roles in signalling between plants and microbes, in male fertility of some plant species, in defense as antimicrobial agents and feeding deterrants, and in UV protection.
  • Flavonoids also have significant activities when ingested by animals, and there is great interest in their potential health benefits, particularly for compounds such as isoflavonoids, which have been linked to anticancer benefits, and stilbenes that are believed to contribute to reduced heart disease.
  • Flavonoid biosynthesis is one of the most intensively studied secondary metabolism pathways in plants. It is regulated by a complex network of signals triggered by internal metabolic cues and external signals, including visible light, ultraviolet (UV) radiation, pathogen attack, nitrogen, phosphorus and iron deficiencies, low temperature and wounding. Regulation of the flavonoid branch pathway producing the flavan-3-ols, the building blocks of proanthocyanidins (PAs) has been studied in species including Arabidopsis thaliana, legumes (Medicago sativa, M. truncatula, Desmodium uncinatum, Lotus corniculatus ), grape, apple and tobacco.
  • PAs proanthocyanidins
  • chalcone synthase CHS
  • CHI chalcone isomerase
  • F3H flavonoid 3 - hydroxylase
  • F3'H flavonoid 3'- hydroxylase
  • F3'5'H flavonoid 3'-5'- hydroxylase
  • DFR dihydroflavonol- 4-reductase
  • ANS anthocyanidin synthase
  • ANR anthocyanidin reductase
  • TT genes (TT1, TT2, TT8, TT16), two TRANSPARENT TESTA GLABRA genes ⁇ TTG1, TTG2) and PURPLE ANTHOCYANIN PIGMENTATION 1 (PAP1) encode regulatory proteins. Mutations of TT1, encoding a zinc finger protein, and TT16/ABS, encoding a MADS-box factor, affect the spatial pattern of BANYULS expression. TT16/ABS mediates the expression of BANYULS and PA accumulation in the endothelium of seed coats except for the chalazal-micropylar area. TTG2, a WRKY-box transcription factor, is involved in regulating late steps of PA biosynthesis after the leucoanthocyanidin branch point. Cooperative action of two transcription factors, TT2, an R2R3-MYB factor, and TT8, an R/B-like bHLH factor, directly regulate expression of the late biosynthesis genes (LBG) involved in PA production.
  • LBG late biosynthesis genes
  • TT12, TT19 Two TT genes (TT12, TT19) and Arabidopsis H+-ATPase 10 are involved in the compartmentalization of flavonoids.
  • the TT10 gene encoding a laccase-like enzyme thought to be involved in oxidation and condensation of PA subunits, has also been characterized.
  • the second pathway involves the sequential conversion of 2,3-flavan-3,4-diols to anthocyanidin molecules by anthocyanidin synthase (ANS, EC 1.14.11.19) and the reduction of anthocyanidins to 2,3-c/s-flavan-3-ols by anthocyanidin reductase (ANR, EC 1.3.1.77).
  • ANR anthocyanidin reductase
  • Legumes offer many opportunities for studying PAs and include species that accumulate a range of PA levels and compositions in different tissues. Extensive genetic and functional genomic resources make M. truncatula an ideal model legume for studying PA biosynthesis M. sativa and M. truncatula plants accumulate a low level of PAs in flowers, stems, roots and leaves.
  • White clover ⁇ Trifolium repens L. is a major component of temperate improved pastures, worldwide, and is a key forage plant in countries with intensive livestock production systems.
  • a low level of proanthocyanidins (3% of dry weight) in forages is beneficial in preventing pasture bloat and increasing nutrient uptake in ruminant livestock.
  • white clover plants accumulate a high level of PAs in flowers and seed coats, there is a very low level in vegetative tissues, where PAs, and/or their flavan-3-ol monomers, are restricted to trichome cells.
  • Applicants have used an extensive transcriptomics approach, in combination with biochemical analysis of selected flavonoids, for molecular dissection of the PA and ANT pathways, co-localized in epidermal cells of floral organs. Spatio-temporal profiles of flavonoid gene expression and accumulation of the corresponding metabolites suggests that components of the ANT and PA pathways may be encoded by distinct members of multigene families.
  • Applicants' gene-to-metabolite approach integrating transcriptomic and biochemical data from transgenic white clover plants in which the TrANR and TrLAR genes were down-regulated, suggests that cross-talk occurs between the ANT and PA pathways and that both the ANR- and LAR-specific branches of the PA biosynthetic pathway are active in white clover flowers. Applicants provide the first genetic evidence that LAR activity is required for 2,3-fra ?s-flavan-3-ol biosynthesis in white clover flowers.
  • Floral PAs in T. repens consist of nearly equal proportions of epigallocatechins and gallocatechins. This and the relatively high genetic transformation efficiency of white clover make it a good system for functional analysis of genes involved in biosynthesis of both 2,3-trans- flavan-3-ols and 2,3-c/s-flavan-3-ols.
  • Co-localization of the ANT and PA pathways in floral tissues is another advantage of this system, allowing the possibility of metabolic crosstalk to be investigated.
  • the present invention provides a method of identifying a gene encoding a polypeptide or polypeptide isoform which is substantially more active in either a proanthocyanidin (PA) or anthocyanin (ANT) pathway of a plant, said method including providing
  • PA proanthocyanidin
  • ANT anthocyanin
  • an oligonucleotide probe capable of hybridizing with RNA from a gene encoding a polypeptide which is active in a flavonoid biosynthetic pathway
  • the method may be performed using an electronic device, such as a computer.
  • a 'polypeptide' is meant a polymer of linked amino acids, which may be an enzyme, regulatory protein or transporter protein.
  • the enzyme may be a biosynthetic enzyme such as CHS, CHI, F3H, F3'H, F3'5'H, DFR, LAR, ANS, ANR, GST, G3T, UFGT, OlvlT, ART, ANAT or AAT.
  • the regulatory protein may be a transcription factor such as TT1, TT2, TT8, TT16, TTG1 , TTG2, MYB, bHLH, MYC, WDR or PAP1.
  • the transporter protein may be a polypeptide involved in the compartmentalisation of flavonoids, such as TT12, TT19 or H + -ATPase 10.
  • a 'polypeptide isoform' is meant one of two or more different forms of a polypeptide, which may be produced from related genes, or may arise from the same gene by alternative splicing.
  • the isoforms may be produced by single nucleotide polymorphisms (SNPs), small genetic differences between alleles of the same gene.
  • substantially more active in either a PA or ANT pathway is meant that the polypeptide or polypeptide isoform has higher activity in either the branch of the flavonoid biosynthetic pathway that produces PAs or the branch of the flavonoid biosynthetic pathway that produces ANTs, when compared with its activity in the other pathway.
  • polypeptide or polypeptide isoform has activity at least approximately 15% higher, more preferably at least approximately 25% higher, more preferably at least approximately 35% higher, more preferably at least approximately 50% higher in one pathway relative to the other pathway.
  • activity may be between approximately 15% and 100% higher, more preferably between approximately 25% and 200% higher, more preferably between approximately 35% and 300% higher, more preferably between approximately 50% and 500% higher in one pathway relative to the other pathway.
  • polypeptide or polypeptide isoform may be active in one pathway, and have no detectable activity in the other pathway.
  • polypeptide or polypeptide isoform may be substantially more active in a PA pathway relative to an ANT pathway.ln a particularly preferred embodiment, the polypeptide or polypeptide isoform may be active in the PA pathway and have no detectable activity in the ANT pathway. In a preferred embodiment, the polypeptide or polypeptide isoform may be an enzyme which is active late in the ANT pathway.
  • an “enzyme which is active late in the ANT pathway” or a “late ANT pathway enzyme” is meant an enzyme which catalyses one of the final reactions in the synthesis of anthocyganins, after the leucoanthocyanidin branch point.
  • the late ANT-pathway enzyme may be selected from the group consisting of GST, G3T, UFGT, OMT, ART, ANAT and AAT.
  • the polypeptide or polypeptide isoform may be a transcription factor.
  • the transcription factor may be selected from the group consisting of MYB, bHLH, MYC and WDR.
  • the material from said plant is preferably material from said plant at two or more developmental stages.
  • the plant material may be a plant organ or tissue, such as a flower or inflorescence, or part thereof such as a floret, petal, sepal or stamen, or other floral tissue, or a vegetative organ or part thereof such as a leaf or other plant tissue.
  • the material from said plant is floral material.
  • the floral material is at two or more developmental stages, for example immature, partially open (eg. approximately 5 to 35% open, approximately 35 to 65% open, and approximately 65- 95% open) and mature stages of development.
  • an Oligonucleotide probe is meant a short nucleic acid polymer, preferably having between approximately 5 and 200 bases, more preferably between approximately 10 and 100 bases, more preferably between approximately 20 and 50 bases.
  • 'nucleic acid' is meant a chain of nucleotides capable of carrying genetic information.
  • the term generally refers to genes or functionally active fragments or variants thereof and or other sequences in the genome of the organism that influence its phenotype.
  • the term 'nucleic acid' includes DNA (such as cDNA or genomic DNA) and RNA (such as mRNA or microRNA) that is single- or double-stranded, optionally containing synthetic, non-natural or altered nucleotide bases, synthetic nucleic acids and combinations thereof.
  • Oligonucleotide probe applies to one or more oligonucleotide molecules, either identical or non-idential, which are designed, selected, and/or otherwise able to specifically hybridize to a target RNA.
  • an oligonucleotide probe as defined herein may comprise a collection of different oligonucleotide molecules targeted to one or more target regions of the same RNA.
  • Oligonucleotide probe' as used herein may mean either the singular or the plural, such meaning being made clear by the context of usage in the present specification.
  • a pair of oligonucleotide probes is used.
  • the pair of oligonucleotide probes is selected from the pairs shown in Table 5 hereto and functionally active fragments and variants thereof.
  • fragment or variant in relation to an oligonucleotide probe is meant that the fragment or variant (such as an analogue, derivative or mutant) is capable of hybridizing with RNA from the gene encoding a polypeptide active in a flavonoid biosynthetic pathway. Additions, deletions, substitutions and derivatizations of one or more of the nucleotides are contemplated so long as the modifications do not result in loss of functional activity of the fragment or variant.
  • the functionally active fragment or variant has at least approximately 80% identity to the relevant part of the above mentioned sequence to which the fragment or variant corresponds, more preferably at least approximately 90% identity, even more preferably at least approximately 95% identity, even more preferably at least approximately 98% identity even more preferably at least approximately 99% identity.
  • the fragment has a size of between approximately 5 and 200 bases, more preferably between approximately 10 and 100 bases, more preferably between approximately 20 and 50 bases.
  • Preferred fragments and variants include those having a single addition or deletion, or substitution of a single nucleic acid, when compared with an oligonucleotide probe shown in Table 5 hereto.
  • oligonucleotide probe has a nucleotide sequence sufficiently complementary to a target RNA sequence to permit said oligonucleotide to hybridize therewith under hybridization conditions.
  • a nucleotide fragment 'capable of hybridizing' with a polynucleotide is a fragment which can hybridize with said polynucleotide under hybridization conditions which are determined in a known manner in each case.
  • the hybridization conditions are determined by means of the stringency, ie. the severity of the operating conditions. The higher the stringency at which the hybridization is carried out, the more specific the hybridization is.
  • the stringency is defined in particular according to the base composition of a probe/target duplex, and also by means of the degree of mismatching between two nucleic acids.
  • the 'stringency' can also depend on the parameters of the reaction, such as the concentration and the type of ion species present in the hybridization solution, the nature and the concentration of denaturing agents and/or the hybridization temperature.
  • the stringency of the conditions under which a hybridization reaction should be carried out will depend mainly on the target probes used. All these data are well known and the appropriate conditions can be determined by those skilled in the art.
  • high stringency conditions may be used.
  • high stringency conditions is meant the hybridization takes place at a temperature between approximately 35°C and 65°C and at a salt concentration of between approximately 0.5 to 1m, more preferably at a temperature between 50°C and 65°C and at a salt concentration of between approximately 0.8 to 1M.
  • 'RNA from a gene encoding a polypeptide which is active in a flavonoid biosynthetic pathway' is generally meant mRNA transcribed or otherwise generated from the gene.
  • the gene encoding a polypeptide which is active in a flavonoid biosynthetic pathway may encode any polypeptide which catalyses a reaction or is otherwise involved in flavonoid biosynthesis in a plant, for example an enzyme, regulatory protein or transporter protein, as hereinbefore described.
  • the polypeptide which is active in a flavonoid biosynthetic pathway is selected from the polypeptides listed in Tables 1-4 hereto.
  • RNA may be extracted from the plant material by methods known to the person skilled in the art. For example, a CTAB-based extraction method may be employed. Further purification of the extracted RNA may be carried out, again by methods known to those skilled in the art.
  • the step of hybridizing the oligonucleotide probe with the RNA may also be carried out by methods known to those skilled in the art.
  • a microarray is used to generate an expression profile.
  • an 'expression profile' is meant that the activity or level of RNA expression of the gene is measured for the material from the plant, preferably at two or more developmental stages.
  • the step of measuring PA and/or ANT levels in the plant material may be carried out qualitatively and/or quantitatively.
  • a qualitative measurement may be carried out by visualising PA and/or ANT in untreated or stained plant material.
  • plant material may be stained for the presence of PA, for example using DMACA, and then PA visualised.
  • PA visualised may be visualised in untreated plant tissues.
  • a semi-quantitative measurement of PA may be carried out using a PVPP assay.
  • PA and/or ANT levels in the plant materials may also be measured quantitatively by measuring metabolites using liquid chromatography mass spectroscopy (LCMS).
  • LCMS liquid chromatography mass spectroscopy
  • the step of comparing said expression profile with said metabolic profile may be carried out by methods known to those skilled in the art.
  • the profiles are compared to identity genes that are up- or down-regulated, the up- or down-regulation correlating with PA or ANT accumulation.
  • the step of comparing the expression profile with the metabolic profile is preferably performed using an electronic device, such as a computer.
  • the present invention provides a method of manipulating the flavonoid biosynthetic pathway in a plant, said method including identifying a gene encoding a polypeptide or polypeptide isoform which is substantially more active in either a PA or ANT pathway of said plant and up- or down-regulating expression of said gene to increase or decrease the level of PA or ANT in said plant.
  • said method includes identifying a gene encoding a polypeptide or polypeptide isoform which is substantially more active in the PA pathway and up-regulating expression of said gene.
  • said method includes identifying a gene encoding a polypeptide or polypeptide isoform which is substantially more active in the PA pathway and down-regulating expression of said gene.
  • said method includes identifying a gene encoding a polypeptide or polypeptide isoform which is substantially more active in the ANT pathway and up-regulating expression of said gene.
  • said method includes identifying a gene encoding a polypeptide or polypeptide isoform which is substantially more active in the ANT pathway and down-regulating expression of said gene.
  • said method may include down-regulating expression of a gene encoding a polypeptide or polypeptide isoform which is active late in the ANT pathway.
  • the modification may include down-regulation of late anthocyanin-specific genes.
  • Particularly preferred genes include those encoding GST, G3T, UFGT, OMT, ART, ANAT and AAT.
  • said method may include up- and/or down- regulating expression of one or more genes encoding a transcription factor.
  • the modification may include up- and/or down-regulation of genes encoding transcription factors.
  • Particularly preferred genes include those encoding MYB, bHLH, MYC and WDR.
  • flavonoid biosynthetic pathway' is meant modifying flavonoid biosynthesis in a plant relative to a control plant.
  • flavonoid biosynthesis may be modified to increase PA biosynthesis relative to ANT biosynthesis.
  • the step of identifying a gene encoding a polypeptide or polypeptide isoform which is substantially more active in a PA or ANT pathway is carried out by a method as hereinbefore described. Alternatively, in certain circumstances the gene may already be indentified and the method may omit the identification step.
  • 'up-regulating' expression of said gene is meant increasing expression of said gene and, as a result, the protein encoded by the gene, in a plant relative to a control plant.
  • 'down-regulating' expression of said gene is meant decreasing expression of said gene and, as a result, the protein encoded by the gene, in a plant relative to a control plant.
  • RNAi interfering RNA
  • the up- or down-regulation may be carried out by introducing into said plant an effective amount of a genetic construct including the gene or a modified form thereof, such as an antisense nucleic acid, a frame shifted copy of the gene or a nucleic acid encoding RNAi.
  • a genetic construct including the gene or a modified form thereof, such as an antisense nucleic acid, a frame shifted copy of the gene or a nucleic acid encoding RNAi.
  • Techniques for incorporating the genetic constructs of the present invention into plant cells are known to those skilled in the art. Such techniques include Agrobacterium mediated introduction, electroporation to tissues, cells and protoplasts, protoplast fusion, injection into reproductive organs, injection into immature embryos and high velocity projectile introduction to cells, tissues, calli, immature and mature embryos.
  • the choice of technique will depend largely on the type of plant to be transformed.
  • Cells incorporating the genetic constructs of the present invention may be selected, as described above, and then cultured in an appropriate medium to regenerate transformed plants, using techniques well known in the art. The culture conditions, such as temperature, pH and the like, will be apparent to the person skilled in the art.
  • the resulting plants may be reproduced, either sexually or asexually, using methods well known in the art, to produce successive generations of transformed plants.
  • an effective amount is meant an amount sufficient to result in an identifiable phenotypic trait in said plant, or in a plant, plant seed or other plant part derived therefrom.
  • Such amounts can be readily determined by an appropriately skilled person, taking into account the type of plant, the route of administration and other relevant factors. Such a person will readily be able to determine a suitable amount and method of administration. See, for example, Maniatis et al, Molecular Cloning: A Laboratory Manual, Cold Spring Harbor Laboratory, Cold Spring Harbor, the entire disclosure of which is incorporated herein by reference.
  • the present invention provides a method of enhancing bloat safety of a plant, said method including
  • said method may include down-regulating expression of a gene encoding a polypeptide or polypeptide isoform which is active late in the ANT pathway.
  • the modification may include down-regulation of late anthocyanin-specific genes.
  • Particularly preferred genes include those encoding GST, G3T, UFGT, OMT, ART, ANAT and AAT.
  • said method may include up- and/or down- regulating expression of one or more genes encoding a transcription factor.
  • the modification may include up- and/or down-regulation of genes encoding transcription factors.
  • Particularly preferred genes include those encoding MYB, bHLH, MYC and WDR.
  • 'enhancing bloat safety' of a plant is meant reducing the tendency of the plant to cause bloating in an animal which eats the plant.
  • the step of identifying a gene encoding a polypeptide or polypeptide isoform which is substantially more active in a PA or ANT pathway is carried out by a method as hereinbefore described.
  • the gene may already be indentified and the method may omit the identification step.
  • a genetic construct capable of manipulating the flavonoid biosynthetic pathway in a plant, said genetic construct including a gene encoding a polypeptide or polypeptide isoform which is substantially more active in either a PA or ANT pathway of said plant, or a modified form of said gene.
  • the genetic construct according to the present invention may be a vector.
  • a 'genetic construct' is meant a recombinant nucleic acid molecule.
  • a 'vector' is meant a genetic construct used to transfer genetic material to a target cell.
  • the vector may be of any suitable type and may be viral or non-viral.
  • the vector may be an expression vector.
  • Such vectors include chromosomal, non-chromosomal and synthetic nucleic acid sequences, eg. derivatives of plant viruses; bacterial plasmids; derivatives of the Ti plasmid from Agrobacterium tumefaciens; derivatives of the Ri plasmid from Agrobacterium rhizogenes; phage DNA; yeast artificial chromosomes; bacterial artificial chromosomes; binary bacterial artificial chromosomes; vectors derived from combinations of plasmids and phage DNA.
  • any other vector may be used as long as it is replicable or integrative or viable in the plant cell.
  • the genetic construct may further include a regulatory element and a terminator; said regulatory element, gene and terminator being operably linked.
  • the regulatory element, gene and terminator may be of any suitable type and may be endogenous to the target plant cell or may be exogenous, provided that they are functional in the target plant cell.
  • said regulatory element is capable of causing expression of said gene or modified form thereof in a plant cell and said terminator is capable of terminating expression of gene or modified form thereof in a plant cell.
  • said regulatory element is upstream of said gene or modified form thereof and said terminator is downstream of said gene or modified form thereof.
  • 'capable of causing expression of said gene' is meant that the gene or modified form thereof and the regulatory element, such as a promoter, are linked in such a way as to permit expression of said gene under appropriate conditions, for example when appropriate molecules such as transcriptional activator proteins are bound to the regulatory sequence.
  • the regulatory element is a promoter.
  • promoters which may be employed in the vectors of the present invention are well known to those skilled in the art. Factors influencing the choice of promoter include the desired tissue specificity of the vector, and whether constitutive or inducible expression is desired and the nature of the plant cell to be transformed (eg. monocotyledon or dicotyledon). Particularly suitable constitutive promoters include the Cauliflower Mosaic Virus 35S (CaMV 35S) promoter.
  • CaMV 35S Cauliflower Mosaic Virus 35S
  • terminators which may be employed in the vectors of the present invention are also well known to those skilled in the art.
  • the terminator may be from the same gene as the promoter sequence or a different gene.
  • Particularly suitable terminators are polyadenylation signals, such as the CaMV 35S polyA and other terminators from the nopaline synthase (nos) and the octopine synthase (ocs) genes.
  • the genetic construct in addition to the regulatory element, the gene or modified form thereof and the terminator, may include further elements necessary for expression of the gene or modified form thereof, in different combinations, for example vector backbone, origin of replication (ori), multiple cloning sites, spacer sequences, enhancers, introns (such as the maize Ubiquitin Ubi intron), antibiotic resistance genes and other selectable marker genes [such as the neomycin phosphotransferase (npt2) gene, the hygromycin phosphotransferase (hph) gene, the phosphinothricin acetyltransferase (bar or pat) gene], and reporter genes (such as beta-glucuronidase (GUS) gene (gusA)].
  • the genetic construct may also contain a ribosome binding site for translation initiation.
  • the genetic construct may also include appropriate sequences for amplifying expression.
  • the presence of the genetic construct in transformed cells may be determined by other techniques well known in the art, such as PGR (polymerase chain reaction), Southern blot hybridisation analysis, histochemical assays (e.g. GUS assays), thin layer chromatography (TLC), northern and western blot hybridisation analyses.
  • PGR polymerase chain reaction
  • Southern blot hybridisation analysis histochemical assays (e.g. GUS assays)
  • TLC thin layer chromatography
  • TLC thin layer chromatography
  • Those skilled in the art will appreciate that the various components of the genetic construct are operatively linked, so as to result in expression of said gene or modified form thereof.
  • Techniques for operatively linking the components of the genetic construct of the present invention are well known to those skilled in the art. Such techniques include the use of linkers, such as synthetic linkers, for example including one or more restriction enzyme sites.
  • the genetic construct is substantially purified or isolated.
  • the genetic construct is free of the genes, which, in the naturally-occurring genome of the organism from which the nucleic acid or promoter is derived, flank the nucleic acid or promoter.
  • the term therefore includes, for example, a genetic construct which is incorporated into a vector; into an autonomously replicating plasmid or virus; or into the genomic DNA of a prokaryote or eukaryote; or which exists as a separate molecule (eg. a cDNA or a genomic or cDNA fragment produced by PCR or restriction endonuclease digestion) independent of other sequences. It also includes a genetic construct which is part of a hybrid gene encoding additional polypeptide sequence.
  • the substantially purified genetic construct is at least approximately 90% pure, more preferably at least approximately 95% pure, even more preferably at least approximately 98% pure.
  • isolated means that the material is removed from its original environment (eg. the natural environment if it is naturally occurring).
  • a naturally occurring nucleic acid present in a living plant is not isolated, but the same nucleic acid separated from some or all of the coexisting materials in the natural system, is isolated.
  • nucleic acids could be part of a vector and/or such nucleic acids could be part of a composition, and still be isolated in that such a vector or composition is not part of its natural environment.
  • the gene included in the genetic construct of the present invention is identified by a method as hereinbefore described.
  • the gene may encode a polypeptide or polypeptide isoform which is active late in the ANT pathway.
  • the late ANT-pathway enzyme may be selected from the group consisting of GST, G3T, UFGT, OMT, ART, ANAT and AAT.
  • the gene may encode a transcription factor.
  • the transcription factor may be selected from the group consisting of MYB, bHLH, MYC and WDR.
  • a transgenic plant cell, plant, plant seed or other plant part with modified flavonoid biosynthetic characteristics relative to an untransformed control plant said plant cell, plant, plant seed or other plant part including a genetic construct or vector according to the present invention.
  • modified flavonoid biosynthetic characteristics is meant that the transformed plant exhibits increased flavonoid biosynthesis and/or contains increased levels of soluble carbohydrate relative to an untransformed control plant.
  • said transformed plant exhibits increased PA biosynthesis and/or contains increased levels of PA relative to an untransformed control plant.
  • the transgenic plant cell, plant, plant seed or other plant part with modified flavonoid biosynthetic characteristics has an increase in soluble carbohydrate, preferably an increase in PA, of least approximately 15%, more preferably at least approximately 25%, more preferably at least approximately 35%, more preferably at least approximately 50% relative to an untransformed control plant.
  • soluble carbohydrate preferably PA
  • soluble carbohydrate may be increased by between approximately 15% and 500%, more preferably between approximately 25% and 300%, more preferably between approximately 35% and 200%, more preferably between approximately 50% and 100% relative to an untransformed control plant.
  • transgenic plant cell, plant, plant seed or other plant part is produced by a method according to the present invention.
  • the present invention also provides a transgenic plant, plant seed or other plant part derived from a plant cell of the present invention and including a genetic construct or vector of the present invention.
  • the present invention also provides a transgenic plant, plant seed or other plant part derived from a plant of the present invention and including a genetic construct or vector of the present invention.
  • the plant cell, plant, plant seed or other plant part may be from any suitable species, including dicotyledons, moncotyledons and gymnosperms.
  • the plant cell, plant, plant seed or other plant part may be from a dicotyledon, preferably forage legume species such as clovers (Trifolium species) and medics (Medicago species), more preferably white clover (Trifolium repens), red clover (Trifolium pratense), subterranean clover (Trifolium subterraneum) and alfalfa (Medicago sativa).
  • the transgenic plant cell, plant, plant seed or other plant part is a clover species, more preferably white clover, or an alfalfa species.
  • the present invention enables the production of clover plants with increased PA in leaf blades, for improved nutrition for grazing animals.
  • Plant cell is meant any self-propagating cell bounded by a semi-permeable membrane and containing a plastid. Such a cell also requires a cell wall if further propagation is desired.
  • Plant cell includes, without limitation, algae, cyanobacteria, seeds suspension cultures, embryos, meristematic regions, callus tissue, leaves, roots, shoots, gametophytes, sporophytes, pollen and microspores.
  • transgenic is meant any cell which includes a DNA sequence which is inserted by artifice into a cell and becomes part of the genome of the organism which develops from that cell.
  • the transgenic organisms are generally transgenic plants and the DNA (transgene) is inserted by artifice into either the nuclear or plastidic genome.
  • the methods of the present invention may be applied to a variety of plants, including monocotyledons [such as grasses (e.g. forage and bioenergy grasses including perennial ryegrass, tall fescue, Italian ryegrass, red fescue, reed canarygrass, big bluestem, cordgrass, napiergrass, wildrye, wild sugarcane, Miscanthus, switchgrass), corn or maize, rice, wheat, barley, sorghum, sugarcane, rye, oat) and energy crops (e.g.
  • grasses e.g. forage and bioenergy grasses including perennial ryegrass, tall fescue, Italian ryegrass, red fescue, reed canarygrass, big bluestem, cordgrass, napiergrass, wildrye, wild sugarcane, Miscanthus, switchgrass
  • corn or maize rice, wheat, barley, sorghum, sugarcane, rye, oat
  • energy crops
  • energy cane energy cane, energy sorghum
  • dicotyledons such as Arabidopsis, tobacco, soybean, canola, alfalfa, potato, cassava, clovers (e.g. white clover, red clover, subterranean clover), vegetable brassicas, lettuce, spinach] and gymnosperms.
  • the methods are applied to alfalfa and clover, more preferably white clover.
  • Figure 1 Accumulation of Proanthocyanidins and Anthocyanins in White Clover Organs and Tissues at Different Stages of Development.
  • A to ( ) 4- Dimethylaminocinnemaldehyde staining of PA in inflorescences and flowers.
  • N to (P) Staining of PA in vegetative organs.
  • Q to (W) Visualisation of anthocyanins in florets and leaves, ab-abaxial; ad-adaxial; c-carpels; s-sepals, st-stamens; 1 -standard petal; 2- lateral wing petals; 3-keel petals.
  • FIG. 1 Analysis of Flavonoid Levels in White Clover Inflorescences.
  • A Appearance of white clover inflorescences and flowers at six stages of development.
  • B Proanthocyanidin level.
  • C Level and composition of free 2,3-flavan-3-ols. Black bars- GC, open bars-EGC.
  • D Level and composition of anthocyanins. Open bars-A1, black bars- A2.
  • E Level and composition of flavonol glycosides. Open bars-F1 , black bars-F2, grey bars-F3, cross-hatched bars-F4. GC-gallocatechin, EGC- epigallocatechin.
  • FIG. 3 Normalized Expression Data from Genes Differentially-Expressed (p> 0.05).
  • A Line plot showing gene expression patterns across 6 developmental stages of white clover flowers. The black lines represent genes up-regulated at stages 1-3 and down- regulated at stages 4-6. The medium grey lines represent genes down-regulated at stages 1-3 and up-regulated at stages 4-6. The light grey lines represent genes constitutively expressed.
  • B Heat map derived from hierarchical clustering of genes showing similar expression patterns across the six developmental stages. For each of the stages represented the darker to grey colour depicted the higher the observed gene expression.
  • C A self organising map with 7 X 8 output nodes organising genes into 56 clusters of similar gene expression.
  • Figure 4. Transcript Levels of Selected Genes at Six Stages of White Clover Flower Development. Normalized relative transcript levels of indicated genes determined by real-time RT-PCR are shown as bars (scale on the left) and microarray results (scale on the right), as lines. Numbers on the x-axes represent developmental stages.
  • Figure 5 Organ-Specific Expression of Selected Genes at Developmental Stages 3, 4, 5 and 6 of White Clover Flower Development. Normalized relative transcript levels of indicated genes were determined by real-time RT-PCR. Black bars represent expression in inner whorls (petals, carpel and stamens). Grey bars represent expression in sepals. Numbers on the x-axes represent developmental stages.
  • FIG. 6 Phenotypes of Flowers from White Clover Lines Containing a dsRNAi Construct Targeting TrANR.
  • A to (C) 50% open inflorescences and flowers of TrANR dsRNAi lines showing white (6-1 OA), pink (6-8A) and red (6-14D) flower phenotypes, respectively.
  • D Inflorescence of the 6-14D line at stages 5 and 6.
  • E Individual flowers of the 6-14D line at different developmental stages.
  • F Immature inflorescences at stage 3 of the wild-type (left) and 6-14D line (right).
  • G Standard petals of wild-type (upper image) and line 6-14D (lower image) at stage 3.
  • TrLAR Transcript levels of the TrLAR gene in TrLAR dsRNAi lines.
  • C Transcript levels of the TrLAR and TrANR genes in TrANR-TrLAR dsRNAi lines. Normalized relative transcript levels were determined in 50% open inflorescences of the indicated lines by real-time RT-PCR. Black bars: TrANR, open bars: TrLAR. WT-wild- type.
  • Figure 9 A Model for Flavonoid Biosynthesis in White Clover Flowers Based on Biochemical and Transcriptomic Data.
  • RED reductase-epimerase- dehydrogenase
  • FLS flavonol synthases
  • IFR isoflavone reductases
  • IFRL isoflavone reductase-like proteins
  • PBER phenylcoumaran benzylic ether reductases
  • (+)-pinoresinol/(+)-lariciresinol reductase protein (PLR) flavanone 3-hydroxylases (F3H), leucoanthocyanidin reductases (LAR), anthocyanidin reductases (ANR) and anthocyanidin reductase-like proteins (ANRL) involved in flavonoid biosynthesis.
  • FLS flavonol synthases
  • IFR isoflavone reductases
  • IFRL isoflavone reductase-like proteins
  • PBER phenylcoumaran benzylic ether reductases
  • the phylogenetic tree was constructed from a ClustalW alignment using the neighbor-joining method in the MEGA4.0.2 package.
  • VITV-V/ ' f/ ' s vinifera PINTA- Pinus taeda, LOTCO-Lotus corniculatus, TR ⁇ RE-Trifolium repens, MEDTR-Medicago truncatula, PHACO-Phaseolus coccineus, ORYSA-Oryza sativa, ORVU-Hordeum vulgare, GOSAR-Gossypium arboretum, GOSRA-Gossypium raimondii, VITSH-V/i/s shuttleworthii , MALDO-Malus x domestica, ARAY -Arabidopsis thaliana, DESUN- Desmodium uncinatum, ZEAMA-Zea mays, CAMSI-Came///a sinensis FORI -
  • accession numbers are as follows. Swissprot: Q84V83.1 , Q00016.1. P5 110.1. Genbank: CAI56335.1 , CAI56334.1, CAI56333.1 , CAI56332.1 , CAI56330.1, CAI56331.1 , AAC49608.1, AAF64174.1 , CAD91910.1, CAI56323.1 , CAI56324.1 , CAI56319.1 , CAI56325.1 , CAI56320.1 , AAN77735.1 , CAI56327.1 , CAI56328.1 , FJ842544, FJ842546, CAD91909.1, CAI56322.1, CAI56321.1 , CAD91911.1 , CAI56326.1 , CAI26310.1 , CAI26308.1 , CAA28734.1, AAZ79363.1 , AAZ79364.1, AAZ79365.1 , BAB92999.1 , AAT68773.1 , ABC71337.1 , A
  • Figure 11 Normalised gene expression data from genes showing a significantly different expression (p> 0.05) in flowers of 3 TrANR dsRNAi lines in comparison to 3 wild-type white clover plants. Grey dots represent genes up-regulated in TrANR dsRNAi lines compared to wild-type plants. Black dots represent genes down-regulated in TrANR dsRNAi lines compared to wild-type plants.
  • Wild type and transgenic white clover lines were vernalised in a controlled growth room for 6 weeks at 5°C with an 8 h photoperiod and a light intensity of 41+/-5 ⁇ - ⁇ "1 -3 "1 at canopy height.
  • Flowering was then induced in a controlled growth cabinet (Enconair) by growing plants for 4 weeks at 22°C with a 16 hour photoperiod and a light intensity of 240+/-30 ⁇ - ⁇ "1 -8 "1 at canopy height.
  • Transgenic white clover plants (Trifolium repens L. cv Mink) were generated by Agrobacterium-medlated transformation using cotyledonary explants and selection with 50 mg/L kanamycin sulfate as previously described (Ding et al., 2003). DNA was extracted from leaf tissue of putative transgenic lines using the Wizard DNA purification kit (Promega) and screened by real-time PCR for the presence of the npt2 selectable marker gene using the primers 5'-GGCTATGACTGGGCACAACA-3' and 5'- ACCGGACAGGTCGGTCTTG-3'.
  • PCR mixtures were set up in a laminar flow hood with aerosol-free pipette tips using SYBR Green PCR Master Mix (cat# 4309155, Applied Biosystems), according to the manufacturers instructions, using at least 2 technical replicates and a 25 ⁇ reaction volume.
  • Thermal cycling was performed with a MX3000P thermal cycler (Stratagene) using the following cycling conditions for the detection of the npt2 gene: 10 mins at 95°C; 40 cycles of 30 sec at 95°C, 30 sec at 60°C and 30 sec at 72°C; 1 min at 95°C, 30 sec at 55°C and 30 sec at 95°C.
  • Plant material was stained for the presence of proanthocyanidins and monomeric flavan-3-ols using 0.01% (w/v) 4-dimethylaminocinnemaldehyde (DMACA) in absolute ethanol containing 1% (w/v) concentrated hydrochloric acid (McMurrough and McDowell, 1978). Anthocyanins were visualized in untreated white clover tissues. Images were captured using a Leica MZFLIII light microscope (Leica Microsystems) fitted with a CCD camera.
  • DMACA 4-dimethylaminocinnemaldehyde
  • a semi-quantitative PVPP-butanol-HCI assay was used to measure total proanthocyanidin levels in 5 -10 mg samples of freeze-dried, finely ground white clover material (Ray et al., 2003). Samples were analyzed using a spectrophotometer (Nanodrop) and final values were normalized against the mass of individual samples. Three biological replicates were performed. Flavonol glycosides, flavan-3-ols and anthocyanins were identified and quantified by LC-MS analysis. Three technical replicates of freeze dried, finely ground plant material (approximately 5 mg) were extracted three times in 0.5 ml aliquots of 80% methanol in water.
  • the combined extracts were dried with gentle warming under a stream of nitrogen and reconstituted in 200 ⁇ L ⁇ of 80% methanol/water.
  • An Agilent 1100 series HPLC system (Waldbronn) equipped with a quaternary gradient pump, column heater, autosampler with sample cooler (maintained at 4°C), and diode array detector (data acquired over 190-800 nm), coupled to a Thermo Electron LTQ ion trap mass spectrometer was used for LC-MS analysis. 5 ⁇ aliquots of each sample were injected onto a 150 x 2.1 mm id., 3 ⁇ , Thermo BDS Hypersil C18 column maintained at 40°C.
  • the mobile phase consisted of two components: A (water with 0.1% formic acid) and B (acetonitrile with 0.1% formic acid); and followed the gradients at a flow rate of 0.2 ml/min: Gradient 1: 0-5 min, 98% A; 5-25 min, 62% A; 26-35 min, (0.3ml/min) 98% A.
  • LC-MS For identification of metabolites, LC-MS was run in polarity switching mode with MS" data acquired in both negative and positive modes. Analysis of the ESI negative mode MS and MS" data allowed the identification of four flavonol glycosides, and analysis of the ESI positive mode MS and MS n data along with the PDA data allowed the identification of two anthocyanins.
  • LC-MS data was acquired in ESI negative mode with a mass range limited to 200 to 1000 amu. Prior to data acquisition the system was tuned using a 20 ⁇ g/ml standard of epicatechin (EC). Standard curves for EC and epigallocatechin (EGC) were prepared by serial dilution of stock solutions and analysed in conjunction with the samples.
  • results were linear over the range examined (8-285 ng for EGC, 5-81 ng for GC). Standards for the flavonol glycosides and anthocyanins were not obtained and absolute quantitation was not possible. Results were based on relative levels of the metabolites in each sample, based on the area of the peak for the [M-H] " ion for the flavonols and for the UV-Vis absorption (500-550 nm) peak area for the anthocyanins.
  • cDNA clones containing the white clover ANR and LAR genes were identified using the sequences of the Arabidopsis thaliana BANYULS gene and the Desmodium unicinatum LAR gene as input data for BLAST searches of a white clover EST database (Altschul et al., 1997; Sawbridge et al. 2003).
  • the deduced protein sequences of the white clover ANR and LAR genes were compared to sequences of related genes in the reductase- epimerase-dehydrogenase (RED) superfamily by constructing a phylogenetic tree with bootstrapping from a ClustalW alignment using the neighbor-joining method in the MEGA4.0.2 package (Tamura et al., 2007; Kumar et al., 2008). Preparation of Constructs for Plant Transformation
  • TrANR and TrLAR cDNA clones in pGEM-T Easy were previously generated as part of an EST discovery project (Sawbridge et al., 2003).
  • the characterized TrANR and TrLAR cDNA clones were used as templates for PCR reactions.
  • a 331 bp fragment from the 3' end of TrANR was amplified using the primers 5'-attB1-ATGCAGTTTCTGTCGGGTTC-3' and 5'-attB2- ATCAAAATCTAATTCTTC AGTGC-3' .
  • TrLAR dsRNAi and TrLAR dsRNAi were amplified using the primers 5'-attB1 -TGAATGAGCTTGCTTCTTTGTG-3' and 5'-attB2- TAGATCCACCTCAGGTGAACC-3'.
  • PCR products were inserted into pDONR221 and fully sequenced clones were introduced into a GATEWAY®-enabled plant expression vector containing TrANR and TrLAR in hairpin constructs under the control of an enhanced CaMV 35S promoter and the 35S terminator and named TrANR dsRNAi and TrLAR dsRNAi, respectively.
  • TGAACCTTTTCAACAGGAAGC-3' were used as a template for a secondary PCR reaction using the GATEWAY primers 5'-attB1 -ATGCAGTTTCTGTCGGGTTC-3' and 5'-attB2-TAGATCCACCTCAGGTGAACC-3'.
  • Proprietary Combimatrix CustomArray software was used to design single oligonucleotide probes of 35 to 40 bases in length for each white clover unigene. The resulting probe set was then assigned to a Combimatrix Custom 12k array.
  • RNAs were extracted using the CTAB-based method of Chang et al. (1993) and were further purified using an RNeasy ® Mini kit following the manufacturer's protocol (QIAGEN).
  • RNA samples were amplified and labelling was performed using the MessageAmpTMll aRNA Amplification Kit (Ambion) and Biotin-ULS aRNA Fluorescent Labelling Kit (Kreatech), according to the manufacturers' instructions. Each sample was hybridized to a separate array following the protocol recommended by the manufacturer (CombiMatrix). Slides were labeled, post-hybridisation, with streptavidin-cy5 according to the manufacturer's protocols (http://www.combimatrix.com). Slides were re-used up to 4 times and were stripped between uses with the Combimatrix stripping reagent as per http://www.combimatrix.com. The hybridized arrays were scanned with an Axon GenePix4000B instrument. Data was extracted using Combimatrix Microarray Imager software (http://webapps.combimatrix.com/customarrav/customarravHome.isp).
  • RNA Reverse transcription of 1 ⁇ g of RNA was performed using Transcriptor First Strand cDNA Synthesis kit (Roche) according to the manufacturer's recommendations.
  • a list of the primers is shown in Table S5.
  • Duplicate controls included RT-PCR reactions lacking reverse transcriptase or no template.
  • GPDH glyceraldehyde-3P-dehydrogenase
  • EF1 elongation factor 1 -alpha
  • SAMS S-adenosylmethionine
  • Proanthocyanidins and Anthocyanins are Co-Localized in Floral Epidermal Cells
  • PAs and their monomers were histochemically stained in white clover organs and tissues using DMACA ( Figure 1). Floral organs stained strongly indicating that a high level of PA and 2,3-flavan-3-ol monomers were present. Accumulation of PAs in inflorescences at immature, partially (50%) open and mature stages of development is shown in Figure 1 (A-G). The accumulation of PAs appeared to be developmental ⁇ regulated within all three developmental stages as indicated by intense staining of the oldest florets located at the base of each inflorescence ( Figure 1B, D,E,G). White clover flowers have a calyx that consists of 5 fused sepals in which PAs or their monomers were detected only in multicellular trichomes (Figure 1H).
  • the white or pale pink asymmetrical corolla contains 5 petals: a single large standard petal and two lateral wing petals, which enclose two interior keel petals (Figure 11).
  • PA accumulation was most clearly seen in the standard petal (Figure 1J- K), followed by the inner, wing and keel petals.
  • PA accumulation appeared to start in epidermal cells located on the abaxial side of the petal and proceed to epidermal cells on the adaxial side during development (Figure 1J-K).
  • the bases of all five petals are fused to a tube of 10 stamens.
  • a mosaic pattern of PA accumulation was detected on the abaxial side of stamen filaments ( Figure 1 L).
  • a single carpel is located within the staminal tube.
  • Figure 1M shows accumulation of PA in carpels.
  • PAs or their monomers were detected only in multicellular trichomes of aerial vegetative organs of white clover, including peduncles, stolons, stipules, petioles and leaves (Figure 1 N-P). Trichomes staining heavily with DMACA were seen in leaves at stage 0.2 (Thomas, 1987, Figure 10). Accumulation of PAs in peduncles was similarly restricted to trichomes ( Figure 1P). ANTs accumulated in both epidermal and sub-epidermal cells of aerial vegetative organs with no detectable accumulation in trichomes.
  • ANTs were virtually undetectable in inner floral whorls including carpels and stamens under normal conditions, but could be synthesized in these whorls under stress conditions of low temperature and high light intensity.
  • leaves ANT mainly accumulate in epidermal cells located on adaxial side (Figure 1V, W), but could be found also on abaxial side under stress conditions of low temperature and high light intensity.
  • the epidermal cells of petals are the main location where PAs and ANTs are likely to be spatially co-localized.
  • PAs were extracted in butanol-HCI, bound to PVPP and heated to release colored anthocyanidins as degradation products of PAs. This method showed that a very low level of PAs accumulated in leaves, reflecting their presence only in trichomes (Figure 2B). A higher level of PA was detected at flower stages 2 and 3, peaking at stage 4. Analysis of the free 2,3-flavan-3-ol level and composition in inflorescences using LC-MS revealed the presence of only gallocatechin (GC) and epigallocatechin (EGC) monomeric units (Figure 2C). The accumulation of EGC and GC was found to be developmentally regulated in flowers with detectable levels of free monomers at the stage 2 and the highest levels recorded at stage 3. A higher level of GC than EGC was seen at all six stages of flower development.
  • GC gallocatechin
  • ECC epigallocatechin
  • Figure 3 shows graphical views of the normalized expression data with the expression value of each gene plotted on a log scale against the six developmental stages. All of these profiles passed the significance filter at p ⁇ 0.05. A total of 2398 genes showed expression differences when at least two of the six developmental stages were compared. The expression profiles for significantly differentially expressed genes across the 6 development stages were clustered using a self organising map. This map had 7 X 8 output nodes and organised genes into 56 clusters of similar gene expression (Figure 3C).
  • TrCHS chalcone synthase
  • TrCHH and TrCHI2 chalcone isomerase-like genes
  • TrCHH and TrCHI2 chalcone isomerase-like genes
  • TrCytB5-1 a homolog of a flower-specific cytochrome b5 gene, which is known to regulate F3'5'H activity and the accumulation of 5'-substituted anthocyanins (de Vetten et al., 1999), showed an expression profile very similar to that of TrF3'5'H ⁇ 1.
  • TrCytB5- 2 a second cytochrome h5 gene, (TrCytB5- 2) showed a broader expression profile, peaking at stages 2, 3 and 4.
  • Two dihydroflavonol 4-reductase-like genes, TrDFRL.1 and TrDFRL2 showed expression that peaked between stages 1 and 3 and sharply declined at later stages.
  • TrANSL.1 and TrANSL2 Two anthocyanidin synthase-like genes, (TrANSL.1 and TrANSL2), was also up- regulated during early stages of flower development, with the highest level at stage 3.
  • the expression of ANR was higher than that of LAR at all stages of flower development.
  • LBGs most of which encode enzymes involved in the modification of flavonoids, including flavonol 3-O-glucosyltransferases, UDP-glucose glucosyltransferases, O-methyltransferases, anthocyanidin rhamnosyl-transferases and UDP-glucose 4-epimerases, were well represented in profile A.
  • Three genes homologous to an Arabidopsis laccase o-diphenol and para(p)-diphenol:dioxygen oxidoreductase, 7770) involved in the oxidative polymerization of flavonoids (Pourcel et al., 2005), were also detected in the profile A group.
  • Two of these genes, (TrLACI and TrLAC2) displayed a sharp expression peak at stage 3 and expression of a third laccase-like gene (TrLAC3) peaked at stages 1-2.
  • TrMYBI R2R3 MYB transcription factors
  • TrMYCI MYC factor
  • TrWDR1-3 WDR proteins
  • Transporters were represented by 16 candidate genes potentially involved in the compartmentalization of flavonoids into the vacuole. These included ABC transporters, a glutathione S-transferase and a vacuolar sorting protein. Most showed an expression peak at stage 3.
  • TrCHS9 and TrCHS11 CHS-like genes
  • TrCHS8 and TrCHSW two CHS-like genes
  • TrF3H2 and TrF3H3 Two F3H candidates, TrF3H2 and TrF3H3, showed distinct expression profiles.
  • Expression of TrF3H2 was almost the same between stages 4-6 and that of TrF3H3 peaked at stage 6.
  • TrDFRL3 and TrDFRL4 showed sharp up-regulation at stage 5.
  • An F3'H homolog TrF3 !
  • Some profile B genes potentially encoded transporters involved in vacuolar sequestration of flavonoids including a multidrug resistance-associated protein, a H+- transporting ATPase, ATP-binding cassette (ABC) transporters, a glutathione S- transferase and a vacuolar sorting protein.
  • a number of auxin-regulated genes and genes involved in auxin transport were up-regulated at stages 4-6 but not at earlier developmental stages.
  • Real-time RT-PCR was used to validate the microarray data, with an emphasis on the expression of molecular markers of PA biosynthesis (TrANR and TrLAR), ANT biosynthesis (ANT 5' aromatic acetylase and UDP-glucosyltransferase), as well as CHS and ANS-like genes, representing EBGs and LBGs.
  • Profile A genes included: TrANR, TrLAR, TrCHS7, TrCHS6, TrCHS2, TrANSLI and TrMYBL
  • Profile B genes included: TrANAT3, TrUFGT4, TrCHSW, TrANSL3, TrMYB8 and TrMYB5. In all cases, there was a good correlation between real-time RT-PCR and microarray results (Figure 4).
  • TrCHSW was found to be sepal-enhanced and TrCHS6 showed an intermediate expression profile, with most expression within the inner whorls, but relatively high expression in sepals.
  • TrANAT3 and TrUFGT were found to be expressed specifically in the inner whorls.
  • TrANS3 and TrMYB8 were expressed in both inner whorls and sepals.
  • TrANR The translation product of a 1 ,014-bp TrANR cDNA (338 amino acids) shared 92.4% sequence similarity (88.2% identity) with a functionally characterized ANR from M. truncatula and 84% similarity (75.4% identity) with the BANYULS protein of A. thaliana (Xie et al., 2003).
  • the position of TrANR in a phylogenetic tree of the superfamily of reductase-epimerase-dehydrogenase (RED) proteins is shown in Figure 10.
  • the ANR family is most closely related to DFRs, forming a separate branch in the RED family and sharing a core 315- to 320-amino acid region.
  • ANRs differ from DFRs by having 6-8 extra amino acids at the N-terminus and longer carboxy-terminal regions.
  • Three putative LAR genes were identified among white clover expressed sequence tags (EST) sequences on the basis of similarity to the D. uncinatum LAR sequence (AJ550154; Tanner et al., 2003). All three have ORFs of 1 ,071 bp that are predicted to encode proteins of 356 amino acids in length.
  • the TrLARa and TrLARb ORFs are distinguished by a single nucleotide difference and encode proteins with 99.7% amino acid identity.
  • the TrLARa ORF also contains a frameshift, most likely caused by the loss of G418 during cDNA synthesis.
  • TrLARb and TrLARc are distinguished by 9 nucleotide differences, encoding proteins with 98.9% amino acid identity.
  • the four amino acids that discriminate TrLARb from TrLARc are not located within conserved motifs previously described (Tanner et al., 2003; Bogs et al., 2005). Since white clover is an allotetraploid species, these sequence variants may represent homeologs or allelic variation. Consequently, TrLARb was selected for further analysis and will henceforth be referred to as TrLAR.
  • the deduced amino acid sequence of TrLAR is similar to LAR proteins from M. truncatula (86.5% amino acid identity), L.
  • TrLAR corniculatus LAR2-1 (71.6%) and Phaseolus coccineus (71.7%) (Bogs et al., 2005; Pang et al., 2007; Paolocci et al., 2007). TrLAR also shares 64.6% amino acid identity with L. corniculatus LAR1-1 and 62% identity with D. uncinatum LAR. Four motifs conserved in LAR sequences but absent from closely related isoflavone reductases (IFR) were identified in TrLAR.
  • IFR isoflavone reductases
  • KRFLPSEFGHD (residues 116-126), ICCNSIA(g/a/s)WPY (residues 160-170), and THDIFI(n/k)GCQ (residues 276-285)
  • DIGKFT A fourth shorter motif, is located between residues 203-208.
  • Figure 10 shows the relationship between the sequences of TrLAR and other enzymes in the reductase-epimerase-dehydrogenase (RED) superfamily (Paolocci et al., 2007).
  • RED reductase-epimerase-dehydrogenase
  • Transgenic white clover plants ectopically expressing dsRNAi silencing constructs containing 3' end sequences of the TrANR (18 plants) and TrLAR (10 plants) cDNA sequences, and a fusion between the TrANR and TrLAR fragments, (9 plants) under control of the 35S RNA promoter from CaMV were generated to elucidate the function of TrANR and TrLAR in white clover flowers.
  • the presence of transgenes in the To generation of transformed plants was verified by real-time PCR.
  • TrANR dsRNAi lines displayed three main colour phenotypes, white/light pink, resembling wild-type flowers (lines 6-9B, 6-1 OA, 6-1 F), pink (lines, 6-8A, 6-9C1 and 6-10C) and dark red (lines 6-10B, 6-14D, 6-11A, 6-9B1 , 6- 4B, 15-2B) ( Figure 6A-C, respectively).
  • the strongest level of ANT accumulation in the red flowered lines was observed at flower stages 3 and 4.
  • TrANR-TrLAR dsRNAi plants showed flower phenotypes similar to those of TrANR dsRNAi lines. However, no red flower phenotype was seen among the TrLAR dsRNAi lines. The inflorescences of these lines resembled those of wild-type plants at all stages of development.
  • TrANR gene Transcript levels of the TrANR gene were measured in 50% open inflorescences (stages 3 and 4) of transgenic dsRNAi and wild-type plants using real-time RT-PCR.
  • a red-flowered phenotype correlated with reduction in the level of TrANR expression in TrANR dsRNAi lines ( Figure 7A, lines 6-10B, 6-14D, 6-11A, 6-4B, 15-2B).
  • TrLAR dsRNAi lines showed a reduced level of TrLAR expression in comparison to the wild-type and two lines, 11-10A and 11-4C, showed almost a 10- fold reduction in expression. (Figure 7B).
  • TrANR-TrLAR dsRNAi lines with red-flowered phenotypes were found to have reduced levels of both TrANR and TrLAR transcripts (Figure 7C).
  • TrLAR dsRNAi lines showed lower levels of GCs than wild-type plants.
  • TrLAR dsRNAi lines 11-1 OA and 11 -4C
  • TrLAR dsRNAi lines showed dramatically higher levels of EGC in comparison to control plants.
  • TrANR-TrLAR dsRNAi lines with red petals (22-2A, 22-4A, 22-1 B.14-2B) that showed strong down-regulation of TrANR and TrLAR expression also had reduced GC levels, relative to control plants.
  • a pink flowered line (14- 1A) with a higher level of TrANR and TrLAR expression did not have significantly reduced levels of EGC and GC in comparison to control plants.
  • the level and relative abundance of four major flavonol glycosides was modified in flowers from some TrANR dsRNAi lines, in comparison to those of wild-type plants ( Figure 8C).
  • the level of myricetin glycoside (F1 , m/z 479), was up to 3-fold higher in red-flowered transgenic TrANR dsRNAi and TrANR-TrLAR dsRNAi lines than in the wild-type.
  • An intermediate level of myricetin glycoside accumulation was detected in transgenic lines with a pink-flowered phenotype.
  • Production of kaempferol glycoside F3, m/z 477) was slightly lower in the red-flowered transgenic lines than in transgenic lines with pink and white flowers and wild-type plants.
  • There was no significant correlation between the accumulation of two quercetin glycosides (F2, m/z 463 and F4, m/z 505), ANT and flavan-3-ols in white clover flowers.
  • TrANR dsRNAi lines were up-regulated and 123 were down-regulated in the TrANR dsRNAi lines relative to wild-type plants. These comprised gene classes encoding putative flavonoid enzymes, transcription factors, transporters, cell signaling proteins, proteins involved in protein-protein interactions or protein stability, mediators of auxin biosynthesis and signal transduction, proteins involved in transcription and translation and enzymes of other metabolic pathways (see Tables 3 and 4).
  • TrANR dsRNAi lines Twenty eight flavonoid pathway genes were up-regulated in red flowered TrANR dsRNAi lines, relative to wild-type clover plants (see Table 3). Most of the genes encoded enzymes involved in modification of ANTs. Two genes involved in the late steps of ANT biosynthesis, flavonoid 3-O-glucosyltransferase and UDP- glucuronosyl/UDP-glucosyltransferase, showed the highest rates of induction, 8.2- and 7.5-fold, respectively in TrANR dsRNAi lines.
  • TrANR dsRNAi lines include those encoding four glucosyltransferases, two glutathione S-transferases, two o-methyltransferases, anthocyanidin rhamnosyl-transferase and anthocyanin 5-aromatic acyltransferase.
  • TrANR dsRNAi lines were also up-regulated in inflorescences of TrANR dsRNAi lines, relative to wild-type plants. These genes included three dihydroflavonol-4-reductase homologs (TrDFRL5, TrDFRL2, TrDFRL3), seven chalcone synthase homologs (TrCHS9, TrCHS11, TrCHS5, TrCHS2, TrCHS6, TrCHSIO), an anthocyanidin synthase-like gene (TrANSL.1), a flavanone 3-hydroxylase homolog (TrF3H2) and a chalcone isomerase homolog (TrCHI2).
  • TrDFRL5 dihydroflavonol-4-reductase homologs
  • TrCHS9, TrCHS11, TrCHS5, TrCHS2, TrCHS6, TrCHSIO seven chalcone synthase homologs
  • TrANSL.1 an anthocyanidin synthase-like
  • TrANR dsRNAi plants were up-regulated in inflorescences of red- flowered TrANR dsRNAi plants, relative to wild-type plants.
  • TrMYC3 and TrbHLH2 were up-regulated 1.5- and 1.4-fold, respectively, in red-flowered TrANR dsRNAi plants.
  • Genes encoding homologs of the circadian clock-associated genes, CCA1 ⁇ TrMYBW) and LHY (TrMYBH) were up-regulated 2.9- and 2.4-fold respectively, in the transgenic lines.
  • TrANR dsRNAi lines Thirty genes encoding proteins involved in protein-protein interactions and protein stability, 22 genes involved in cell signaling and 13 transporters were expressed at higher levels in red-flowered TrANR dsRNAi lines, relative to wild-type plants. Lipid transfer proteins, vesicle-associated membrane proteins and vacuolar sorting proteins involved in intracellular compartmentalization of the flavonoid enzymes and/or their products were strongly represented among genes highly expressed in inflorescences of red-flowered TrANR dsRNAi lines. Approximately 500 genes were down-regulated in the inflorescences of TrANR dsRNAi lines, relative to wild-type plants (see Table 4). Approximately 300 of these genes showed no BLAST hits or matched only hypothetical proteins.
  • TrANR Ten genes down- regulated in TrANR dsRNAi plants encoded flavonoid-related enzymes. As expected, the expression of TrANR was much lower in these lines.
  • TrIFRI NADPH:isoflavone reductase
  • TrIFOMTI isoflavone-7-O-methytransferase
  • TrANR dsRNAi plants were suppressed in TrANR dsRNAi plants, among them members of the MYB/bHLH/WDR module, namely TrWDR7 (x3.5) and TrMYB12 (x1.37). These genes had not been differentially expressed during the development of white clover flowers.
  • these genes (14) are flavonoid-related, including six chalcone synthase homologs (TrCHS2, profile A, TrCHS6, profile A, TrCHS5, profile A; TrCHS9, profile B; TrCHSIO, profile B; TrCHS11, profile B), two out of three dihydroflavonol-4-reductase homologs (TrDFRL2, profile A; TrDFRL3, profile B), one chalcone isomerase homolog (TrCHI2, profile A), one flavonoid 3-hydroxylase homolog (TrF3H2, profile B), one anthocyanidin synthase homolog (TrANSI, profile A), and one cytochrome b5 DIF homolog (TrCytB5-1, profile A).
  • TrUFGT4 profile B
  • TrOMT5 profile B
  • TrARTI anthocyanidin rhamnosyl-transferase
  • TrANR dsRNAi lines Six transcription factors up-regulated in TrANR dsRNAi lines were differentially expressed during the development of wild-type flowers, including the R2R3 MYB-related genes TrMYB2 (profile A), TrMYB3 (profile B) and TrMYB6 (profile B). Other transcription factors up-regulated in TrANR dsRNAi lines and differentially expressed during flower development included TrMYC2 (profile B), a CONSTANS-like zinc finger protein (profile B) and a SQUAMOSA promoter-binding protein (profile A).
  • TrANR dsRNAi lines Six out of 8 of the genes encoding flavonoid pathway enzymes that were down- regulated in TrANR dsRNAi lines showed differential expression between at least two flower stages. The remaining two were candidate anthocyanin 5-aromatic acyltransferase (TrANATS) and UDP-glucose glucosyltransferase (TrUFGTG) genes.
  • TrANATS anthocyanin 5-aromatic acyltransferase
  • TrUFGTG UDP-glucose glucosyltransferase
  • Example 11 Distinct Representatives of Flavonoid-Related Multigene Families Contribute to Spatio-Temporal Profiles of ANT and PA Accumulation in Floral Organs
  • PAs and ANTs are produced by two related but distinct branches of the flavonoid pathway. Both branches involve the conversion of 4-coumaroyl CoA and malonyl CoA to flavan-3,4-diol and 3-OH-anthocyanidin molecules.
  • Activation of both pathways requires the recruitment of R2R3-MYB, WDR and bHLH transcription factors for the transcriptional activation of early and late flavonoid biosynthesis genes.
  • Molecular studies in a range of plant species have revealed that almost all of the flavonoid enzymes are encoded by members of multigene families.
  • the ANT and PA pathways in white clover flowers may recruit exactly the same enzymes or distinct isoforms of enzymes encoded by different members of multigene families, for shared steps in flavonoid production.
  • ANS represents a branch point between the PA and ANT pathways converting flavan- 3,4-diols to 3-OH-anthocyanidins, potential substrates for both pathways.
  • the ANT pathway modifies 3-OH-anthocyanidins by a chain of glycosylation and esterification reactions and the PA pathway involves the reduction of 3-OH-anthocyanidins to 2,3-c/s- flavan-3-ols by ANR.
  • Three ANS-like proteins from white clover, TrANSI, TrANS2 and TrANS3 show 94.4%, 94.4%, and 70% deduced amino acid sequence identity to . truncatula ANS, respectively.
  • TrANSI contains the DHQ1-, DHQ2- and MES/ascorbate-binding domains specific to ANS enzymes, but not other 2- oxoglutarate iron-dependent oxygenases, including flavanone 3-D -hydroxylases (F3H) and flavonol synthases (FLS).
  • TrANS2 and TrANS3 share a low level of amino acid identity with Arabidopsis FLS (41.9% and 35%, respectively) and F3H (31.1% and 26.5%, respectively).
  • the TrANS2 and TrANS3 genes showed distinct profile A and profile B-specific expression, respectively, whilst TrANSI expression peaked at stage 3, but remained relatively high during stages 4 and 5.
  • R2R3-MYB, bHLH and WDR transcription factors have redundant functions in plant development.
  • the Arabidopsis representatives of these families (TT2, TT8 and TTG1) are involved in PA, ANT and mucilage biosynthesis, root-hair patterning and trichome development.
  • Six candidate genes encoding white clover MYB factors were closely related to R2R3-MYB proteins identified in other plant species.
  • the R2R3 repeat region of white clover MYBs is highly conserved and contains the motif [D/E]Lx2[R/K]x3Lx6Lx3R for interaction with bHLH proteins, whereas the C-terminal regions show a low level of similarity to other MYB factors.
  • TrMYB3 (profile B) is closely related to the Arabidopsis subgroup 10 MYBs and clustered with other R2R3-MYB gene products involved in anthocyanin biosynthesis, including PAP1 , PAP2, PhAN2, LeANTI , WMYBA2 and VvMYBAI .
  • the deduced amino acid sequence of TrMYB6 (profile A) clustered with MIXTA and PhMYBI, sharing 89% amino acid sequence similarity in the R2R3 DNA-binding domain. Representatives of the bHLH, WDR, MADS box and WRKY box gene families were also found in both expression profiles.
  • Both bHLH and WDR factors are components of the R2R3-MYB/bHLH/WDR transcription factor complex that regulates enzymes in both the PA and ANT pathways in different plants.
  • Arabidopsis TTG2 a WRKY box factor, regulates at least three separate morphogenetic processes in L1 -derived cells: trichome development and the production of mucilage and condensed tannin in seed coats.
  • BANYULS promoter activity is not affected in ttg2 mutants and both TTG2 and TT1 , a zinc finger protein, may be involved in post- transcriptional regulation of BANYULS expression. Therefore, the white clover TTG2 homolog could potentially regulate TrANR expression in trichomes and epidermal cells.
  • the Arabidopsis MADS-box factor TT16/ABS is known to be expressed in the ovule, mediating BANYULS expression and PA accumulation in the endothelium of seed coats.
  • One of the white clover MADS box factors up-regulated early in flower development might similarly control PA production by transcriptionally activating the TrANR gene.
  • the PA and ANT pathways are localized within different groups of epidermal cells in sepals: a low level of PA accumulates in trichomes and a high level of ANT is present in a subset of epidermal cells at stages 1-6 ( Figure 1).
  • the fact that some of the selected flavonoid genes, including molecular markers of the PA (TrANR and TrLAR) and ANT (ANT acetylase, UFGT) pathways, early (CHS) and late (/WS-like) flavonoid biosynthetic genes as well as R2R3-MYB transcription factors, displayed organ-specific expression profiles (Figure 5) suggests that the PA and ANT pathways in sepals and petals recruit (at least partially) different flavonoid-specific members of multigene families.
  • the data suggest that spatio-temporal patterns of ANT and PA accumulation in floral organs reflect developmentally-regulated and organ-specific expression profiles of distinct isoforms of flavonoid-related enzymes encoded by multigene families.
  • ANR and LAR participate in two separate branches of the PA pathway in most PA-producing species.
  • LAR functions downstream of DFR, catalyzing the conversion of 2,3-flavan-3,4-diols to 2,3-frans-flavan-3-ols.
  • ANR acts immediately downstream of ANS catalyzing the conversion 3-OH-anthocyanidins to 2,3-c/s-flavan-3-ols.
  • Expression of both genes has been found to be developmental ⁇ regulated in PA-accumulating tissues of different species.
  • VvANR and VvLARI are up-regulated at early stages of berry development, 7 weeks before veraison, which correlates well with accumulation of the corresponding flavan-3-ols and PA.
  • MdLARI and MdANR were also shown to be highest during early development of apple (Malus x domestica Borkh. cv. 'Cripps Red') fruit. Furthermore, transcript levels of both the ANR and LAR genes are higher in immature leaves than in mature leaves of L. comiculatus, correlating well with increased accumulation of PAs at early stages of leaf development.
  • the spatio-temporal expression patterns of the TrANR and TrLAR genes in white clover flowers also correlate with the pattern of c/s- and irans-flavan-3-ol accumulation. Interestingly, a higher level of TrANR than TrLAR expression correlates with higher levels of GC than EGC monomers at all tested stages of flower development.
  • prodelphinidin polymers in T. repens flowers consist of terminal and extender units with nearly equal proportions of the two epimers.
  • a higher expression level of ANR, relative to LAR, has also been seen in L. comiculatus herbage and in the skin of red apples.
  • a higher level of VvANR expression than WLAR7 and VvLAR2 expression in grape flowers was found to correlate with a higher level of catechins than epicatechins.
  • the expression of VvANR correlates with a high level of flavan-3-ols and extension subunits with 2,3-c/s- stereochemistry only in grape leaves, where VvLARI is not expressed and WLAR2 is only expressed late in development.
  • most grape tissues accumulate significant levels of epicatechin-based PAs.
  • TrLAR Gene Activity is Necessary but Insufficient for 2,3-trans-flavan-3-ol
  • ANR and LAR genes are coordinately regulated by the same family of transcription factors in grape berries and L. corniculatus tissues.
  • the absence of LAR genes in plants producing only 2,3-c/s- flavan-3-ols, such as Arabidopsis may suggest that LAR genes are involved in the biosynthesis of 2,3-frans-flavan-3-ols.
  • MtLAR expression contrasted with the virtual absence of 2,3-frans-flavan-3-ol subunits in PA from M. truncatula plants.
  • the ectopic expression of LAR genes from M. truncatula and D. uncinatum in tobacco and white clover did not increase levels of irar?s-flavan-3-ols in leaves or flowers.
  • the PA level was actually lower in transgenic tobacco lines than in control plants.
  • Alternative or multiple functions of the LAR gene have been suggested.
  • the LAR gene is encoded by multigene families in some PA-producing species, including grape and L corniculatus. Only one of the L corniculatus LAR genes showed in vitro activity in E. coli.
  • TrLAR is most similar to LAR proteins from M. truncatula and P. coccineus, species which, like white clover, lack appreciable PA biosynthesis in leaf, stem and root tissues.
  • LcLAR2 did not show specific LAR activity when expressed in E. coli.
  • the spatio-temporal profile of white clover LAR expression correlates well with accumulation of GC in PA-producing organs.
  • TrLAR dsRNAi and TrANR-TrLAR dsRNAi lines significantly decreased the level of TrLAR transcripts and correspondingly, the GC level in white clover flowers.
  • the much more pronounced reduction in GC level, compared to the TrLAR transcript level in some TrLAR dsRNAi lines (11-15A, 10-12A and 11-8A) suggests that expression of another TrLAR gene(s) could be affected in TrLAR dsRNAi lines.
  • Our phenotypic, molecular and biochemical data suggest that LAR activity is necessary for GC biosynthesis in white clover flowers.
  • ectopic expression of LAR genes in tobacco and white clover plants resulted in no changes in GC production suggests that LAR activity alone is not sufficient for the biosynthesis of 2,3-frans-flavan-3-ols.
  • TrANR Gene Activity is Necessary and Sufficient for 2,3-cis-flavan-3-ol
  • Loss of ANR function in the Arabidopsis banyuls mutant results in a transparent testa phenotype with a decreased level of 2,3-c/ ' s-flavan-3-ols and accumulation of anthocyanin in the seed coat.
  • expression of recombinant MtANR protein converts cyanidin, delphinidin and pelargonidin molecules into epicatechines, epigallocatechin and epiafzelechin, respectively, suggests that ANR activity is necessary and sufficient for the production of 2,3-c/s-flavan-3-ols.
  • TrANR As in the banyuls mutant, down-regulation of TrANR reduced the level of ANR transcripts and EGC molecules and increased the level of ANT in PA producing cells of white clover.
  • the levels of TrLAR transcripts were twice as high in TrANR-TrLAR dsRNAi lines 22-1B and 14-2B as in TrLAR dsRNAi lines 11-10A and 11-4C, but GC levels were lower in the TrANR-TrLAR dsRNAi lines.
  • TrANR-TrLAR dsRNAi lines GC was virtually undetectable in the 22-2A and 22-4A TrANR-TrLAR dsRNAi lines, suggesting that the effect of silencing the TrANR and TrLAR genes on 2,3-fraA7s-flavan-3-ol production was additive.
  • a reduced level of GC in TrANR dsRNAi and TrANR-TrLAR dsRNAi lines might be explained by ANR having an additional direct or indirect role in the biosynthesis of 2,3- frans-flavan-3-ols.
  • the ANT and PA pathways share dihydroflavonols as precursor molecules.
  • afzelechins R3 -H, R5 -H
  • Glycosylated forms of three flavonols representing all three B-ring hydroxylated variants of dihydroflavonols, were found in white clover flowers with an abundance of myricetin glycosides (F1 , m/z 479, R3 -OH, R5 -OH) at stages 1-2 and an increased level of quercetin glycosides (F2, m/z 463 and F4, m/z 505, R3 -OH, R5 -H) at later developmental stages (3-6).
  • ANT composition at all these stages showed the predominance of delphinidin-based ANTs and a much lower level of cyanidin-based ANTs.
  • TrANR Down-regulation of TrANR led to a decrease in the level of epigallocatechin and an increase in the level of products of the flavonol and anthocyanin pathways with hydroxylation of the B-ring at the 3' and 5' positions (Figure 9).
  • Enhanced accumulation of delphinidin-based ANTs could be explained by diversion of intermediates, such as delphinidins, from 2,3-flavan-3-ol to ANT production.
  • TrANR dsRNAi lines Enhanced expression of genes encoding potential glucosyltransferases, UDP- glucuronosyl/UDP-glucosyltransferases, glutathione transferases, methyltransferases and anthocyanidin rhamnosyl-transferases functioning downstream of ANS in TrANR dsRNAi lines suggests that their transcriptional regulation was triggered by a reduced level of the TrANR transcript and/or an excess of unused metabolic intermediates. Of these genes, TrUFGT4 and TrGT12 showed the highest levels of up-regulation in red- flowered TrANR dsRNAi lines (8.2- and 7.5-fold, respectively).
  • TrANR Down-regulation of TrANR led to a 3 fold increase in the level of myricetin glycosides produced by the flavonol pathway, which branches from the PA and ANT pathways up- stream of ANR. It is difficult to explain these changes simply by metabolic spillover or diversion of delphinidin intermediates. Moreover, changes in the expression levels of most EBG, LBG and genes encoding transcription factors in TrANR dsRNAi lines, in comparison to wild-type plants, suggest that re-programming of the whole flavonoid pathway had occurred.
  • Ectopic expression of one R2-R3 MYB transcription factor, PAP1 , in Arabidopsis resulted in an elevated level of cyanidin-type ANTs and quercetin type flavonols as well as the up-regulation of almost all genes encoding ANT biosynthetic enzymes.
  • Down-regulation of a single gene encoding a metabolic enzyme, TrANR also led to dramatic changes in the levels of flavonoids and changes in the expression of almost all the genes encoding enzymes known to be involved in ANT and PA biosynthesis in white clover (Figure 9).
  • TrANR dsRNAi lines included representatives of genes functioning upstream of TrANR in the general flavonoid pathway or in another branch, such as isoflavone biosynthesis, namely TrCHS, TrCHI, TrF3H2, TrF3'H1, TrDFRL, TrANS, TrCHR, TrlF3'H, TrIFOMT and TrVR candidate genes.
  • TrCHS TrCHI
  • TrF3H2 TrF3'H1
  • TrDFRL TrANS
  • TrCHR TrlF3'H
  • TrIFOMT TrVR candidate genes.
  • TrF3'H gene Although down-regulation of a TrF3'H gene correlated with an increase in the level of delphinidin-3-sambudioside, this was not accompanied by increased expression of TrF3'5'H, suggesting that the level of this transcript does not limit flux in the pathway producing delphinidin-based ANTs.
  • TrANR dsRNAi lines Some transcription factors were also up-regulated in TrANR dsRNAi lines, providing further support for the metabolic re-programming model.
  • Six MYB genes, two MYC or bHLH genes and three WDR genes were up-regulated in flowers of TrANR dsRNAi lines in comparison to wild-type plants.
  • TrWDR5, TrWDR6, TrMYBW TrMYB11, TrMYB9 and TrbHLH3 were up-regulated in red flowered TrANR dsRNAi lines.
  • TrMYB12 and I WDRJ were down-regulated in these transgenic lines.
  • TrANR TrANR dsRNAi lines.
  • TrDFRU profile A
  • TrDFRL2 profile A
  • TrDFRL3 profile B
  • TrDFRL5 neither profile
  • TrDFR4 profile B
  • TrANR dsRNAi lines Only one member of each of the white clover F3H and ANS gene families was up-regulated in TrANR dsRNAi lines.
  • Differential expression was also detected among members of the white clover OMT, GT and WAT gene families.
  • Two representatives of the TrIFOMTgene showed contrasting expression patterns: TrIFOMTI was down-regulated and TrlFOMT2 was up-regulated in TrANR dsRNAi lines, relative to wild-type plants.
  • Flavonoids have been implicated in direct and indirect interactions with transcription/translation machinery, trafficking, anion channels, mediators of cell signaling and cell-to-cell communication. Flavonoids are involved in polar auxin transport, responses to wounding and pathogens, interactions between plants or between plants and animals, embryonic development and seed germination. Loss of ANS/TT18/TDS4 (TANNIN DEFICIENT SEED 4) function in A.
  • thaliana resulted in the appearance of multiple small vacuoles, suggesting that PA or intermediate accumulation is a signal for vacuolar maturation.
  • the molecular targets of flavonoids include transcription factors, kinases, ABC transporters, hydrolases, peptidases, tyrosine phosphatases and serine/threonine kinases. Some of these proteins are transcriptionally up-regulated by a R2-R3-MYB/bHLH/WDR transcription factor complex in other species. Hence, it is interesting that candidate MYB, bHLH and WDR genes showed enhanced expression in TrANR dsRNAi lines. A number of metabolism-related transcription factors (MTFs) have been recently described.
  • MTFs are metabolic enzymes or their homologs that use NAD, FAD and CoA as cofactors and directly link metabolism with gene regulation binding directly to DNA, or regulating gene expression by interacting with other transcription factors.
  • Both ANR and LAR proteins require NADPH/NADH cofactors for their activities.
  • Nuclear localization is a key requirement for regulation of transcription.
  • Transient expression of the Z5S:.MtANR in tobacco and 35S::TrANR in Arabidopsis leaf epidermal cells demonstrated cytosolic localization.
  • both ANR and LAR proteins lack the known nuclear localization signals and domains involved in protein-protein interaction. Subcellular localization of these proteins in PA-producing cells could provide crucial information about their potential function as MTFs.
  • Example 16 Metabolic Channeling
  • the metabolic channeling model suggests that sequential enzymes in a metabolic pathway are organised into macromolecular complexes. The movement of intermediates directly between enzymes within these structures increases catalytic efficiency by limiting their diffusion and interaction with other cell components.
  • the channeling model also allows the possibility of combinatorial regulation, resulting in a variety of enzyme complexes producing related but distinct metabolites.
  • the spatial and temporal profiles of PA and ANT biosynthesis in white clover epidermal cells suggests two possible channeling models: (i) the existence of independent channels producing PA and ANT; and (ii) the existence of a single core channel branching at the ANS point allowing production of PA and ANT pathways potentially competing for the anthocyanidin substrate.
  • the second model could function when ANT and PA channels are located in the same spatial vicinity. In this case, modification of one of the metabolic channels would re-direct the flow of intermediate molecules, resulting in quantitative changes in the final products.
  • Results from both white clover and Arabidopsis lines lacking functional ANR provide evidence for the second model by showing that down-regulation of the ANR gene leads to enhanced ANT accumulation in tissues that normally produce PA ( Figure 6).
  • a reduced level of ANT in tobacco petals ectopically expressing ANR genes suggests a flexible mechanism(s) of flux diversion at the branch- point between the ANT and PA pathways, with competition between ANR and anthocyanidin glucosyltransferase enzymes for the anthocyanidin substrate.

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Abstract

The present invention relates to a method of identifying a gene encoding a polypeptide or polypeptide isoform which is substantially more active in either a proanthocyanidin (PA) or anthocyanin (ANT) pathway of a plant, said method including providing material from said plant; and an oligonucleotide probe capable of hybridizing with RNA from a gene encoding a polypeptide which is active in a flavonoid biosynthetic pathway; extracting RNA from said plant material; hybridizing the oligonucleotide probe with the RNA to generate an expression profile; measuring PA and/or ANT levels in said plant material to generate a metabolic profile; comparing said expression profile with said metabolite profile to identify said gene encoding a polypeptide or polypeptide isoform which is substantially active in either a PA or ANT pathway.

Description

Manipulation of flavonoid biosynthetic pathway
Field of the invention
The present invention relates to methods for manipulating or identifying genes involved in the flavonoid biosynthetic pathway in plants, and to related constructs, plants, plant cells, plant seeds and other plant parts.
Background of the invention
Flavonoids constitute a relatively diverse family of aromatic molecules that are derived from phenyalanine and malonyl-coenzyme A (CoA, via the fatty acid pathway). These compounds include six major subgroups that are found in most higher plants: the chalcones, flavones, flavonols, flavandiols, anthocyanins and proanthocyanidins (or condensed tannins). A seventh group, the aurones, is widespread, but not ubiquitous.
Some plant species also synthesize specialised forms of flavonoids, such as the isoflavonoids that are found in legumes and a small number of non-legume plants. Similarly, sorghum, maize and gloxinia are among the few species known to synthesize 3-deoxyanthocyanins (or phlobaphenes in the polymerised form). The stilbenes, which are closely related to flavonoids, are synthesised by another group of unrelated species that includes grape, peanut and pine.
Besides providing pigmentation to flowers, fruits, seeds, and leaves, flavonoids also have key roles in signalling between plants and microbes, in male fertility of some plant species, in defense as antimicrobial agents and feeding deterrants, and in UV protection.
Flavonoids also have significant activities when ingested by animals, and there is great interest in their potential health benefits, particularly for compounds such as isoflavonoids, which have been linked to anticancer benefits, and stilbenes that are believed to contribute to reduced heart disease.
Flavonoid biosynthesis is one of the most intensively studied secondary metabolism pathways in plants. It is regulated by a complex network of signals triggered by internal metabolic cues and external signals, including visible light, ultraviolet (UV) radiation, pathogen attack, nitrogen, phosphorus and iron deficiencies, low temperature and wounding. Regulation of the flavonoid branch pathway producing the flavan-3-ols, the building blocks of proanthocyanidins (PAs) has been studied in species including Arabidopsis thaliana, legumes (Medicago sativa, M. truncatula, Desmodium uncinatum, Lotus corniculatus ), grape, apple and tobacco.
Much of our recent understanding of flavan-3-ol and PA biosynthesis has arisen from genetic and biochemical analyses of mutants in the model plant A. thaliana. These mutant lines have a 'transparent testa' phenotype because they fail to accumulate or oxidize PAs, which normally give seed coats their brown pigmentation. Sixteen out of nineteen TRANSPARENT TESTA (TT) genes have been identified and characterized at the molecular level. Eight are structural genes, encoding the biosynthetic enzymes chalcone synthase (CHS), chalcone isomerase (CHI), flavonoid 3 - hydroxylase (F3H), flavonoid 3'- hydroxylase (F3'H), flavonoid 3'-5'- hydroxylase (F3'5'H), dihydroflavonol- 4-reductase (DFR), anthocyanidin synthase (ANS) and anthocyanidin reductase (ANR, BANYULS gene). Four TT genes (TT1, TT2, TT8, TT16), two TRANSPARENT TESTA GLABRA genes {TTG1, TTG2) and PURPLE ANTHOCYANIN PIGMENTATION 1 (PAP1) encode regulatory proteins. Mutations of TT1, encoding a zinc finger protein, and TT16/ABS, encoding a MADS-box factor, affect the spatial pattern of BANYULS expression. TT16/ABS mediates the expression of BANYULS and PA accumulation in the endothelium of seed coats except for the chalazal-micropylar area. TTG2, a WRKY-box transcription factor, is involved in regulating late steps of PA biosynthesis after the leucoanthocyanidin branch point. Cooperative action of two transcription factors, TT2, an R2R3-MYB factor, and TT8, an R/B-like bHLH factor, directly regulate expression of the late biosynthesis genes (LBG) involved in PA production.
Two TT genes (TT12, TT19) and Arabidopsis H+-ATPase 10 are involved in the compartmentalization of flavonoids. The TT10 gene, encoding a laccase-like enzyme thought to be involved in oxidation and condensation of PA subunits, has also been characterized. Recent studies have identified key genes and enzymes of the PA branch of the flavonoid pathway controlling the biosynthesis of the 2,3-fraA7S-flavan-3-ols (afzelechin, catechin, and gallocatechin) and 2,3-c/'s-fIavan-3-ols (epiafzelechin, epicatechin, and epigallocatechin) from flavan-3,4-diols (leucoanthocyanidins). The first pathway involves direct reduction of 2,3-flavan-3,4-diols to 2,3-irans-flavan-3-ols by leucoanthocyanidin reductase (LAR, EC 1.17.1.3). The corresponding gene was initially isolated from D. uncinatum and was later characterized in other legumes, camellia, grape and apple.
The second pathway involves the sequential conversion of 2,3-flavan-3,4-diols to anthocyanidin molecules by anthocyanidin synthase (ANS, EC 1.14.11.19) and the reduction of anthocyanidins to 2,3-c/s-flavan-3-ols by anthocyanidin reductase (ANR, EC 1.3.1.77). The BANYULS gene, encoding ANR, has been isolated and characterised in A. thaliana, M. truncatula, apple, Lotus corniculatus and grape.
Legumes offer many opportunities for studying PAs and include species that accumulate a range of PA levels and compositions in different tissues. Extensive genetic and functional genomic resources make M. truncatula an ideal model legume for studying PA biosynthesis M. sativa and M. truncatula plants accumulate a low level of PAs in flowers, stems, roots and leaves.
White clover {Trifolium repens L.) is a major component of temperate improved pastures, worldwide, and is a key forage plant in countries with intensive livestock production systems. A low level of proanthocyanidins (3% of dry weight) in forages is beneficial in preventing pasture bloat and increasing nutrient uptake in ruminant livestock. Although white clover plants accumulate a high level of PAs in flowers and seed coats, there is a very low level in vegetative tissues, where PAs, and/or their flavan-3-ol monomers, are restricted to trichome cells.
In spite of the characterization of PA-related genes and biochemical studies of corresponding proteins and metabolites in different species, some steps of PA biosynthesis are still poorly understood. For example, it is not clear whether the role of ANR is restricted only to the biosynthesis of cs-flavan-3-ols or if its activity is required for the production of both the cis and trans 2,3-flavan-3-ol epimers. Six years after isolation and characterization of the first LAR gene from D. uncinatum molecular aspects of 2,3-fraA7s-flavari-3-ol biosynthesis and the contribution of the R gene to PA biosynthesis are still unclear and based only on in vitro activity of recombinant LAR enzymes and expression profiles of LAR genes in PA-accumulating tissues. Transgenic approaches are limited to ectopic expression studies in tobacco and white clover plants. Loss-of-function approaches are not suitable in Arabidopsis and M. truncatula, where trans 2,3-flavan-3-ols are absent or produced at a low level.
While nucleic acid sequences encoding some flavonoid biosynthetic enzymes have been isolated for certain species of plants, there remains a need for materials useful in modifying flavonoid biosynthesis; in modifying protein binding, metal chelation, anti- oxidation, and UV-light absorption; in modifying plant pigment production; in modifying plant defense to biotic stresses such as viruses, micro-organisms, insects or fungal pathogens; in modifying forage quality, for example by disrupting protein foam and/or reducing rumen pasture bloat, particularly in forage legumes and grasses, including alfalfa, medics, clovers, ryegrasses and fescues, and for methods for their use.
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.
Summary of the invention
Applicants have used an extensive transcriptomics approach, in combination with biochemical analysis of selected flavonoids, for molecular dissection of the PA and ANT pathways, co-localized in epidermal cells of floral organs. Spatio-temporal profiles of flavonoid gene expression and accumulation of the corresponding metabolites suggests that components of the ANT and PA pathways may be encoded by distinct members of multigene families. Applicants' gene-to-metabolite approach, integrating transcriptomic and biochemical data from transgenic white clover plants in which the TrANR and TrLAR genes were down-regulated, suggests that cross-talk occurs between the ANT and PA pathways and that both the ANR- and LAR-specific branches of the PA biosynthetic pathway are active in white clover flowers. Applicants provide the first genetic evidence that LAR activity is required for 2,3-fra ?s-flavan-3-ol biosynthesis in white clover flowers.
Applicants propose that metabolic re-programming of the flavonoid pathway to increase the PA level in leaves is an attractive strategy for enhancing bloat safety. Floral PAs in T. repens consist of nearly equal proportions of epigallocatechins and gallocatechins. This and the relatively high genetic transformation efficiency of white clover make it a good system for functional analysis of genes involved in biosynthesis of both 2,3-trans- flavan-3-ols and 2,3-c/s-flavan-3-ols. Co-localization of the ANT and PA pathways in floral tissues is another advantage of this system, allowing the possibility of metabolic crosstalk to be investigated. In one aspect, the present invention provides a method of identifying a gene encoding a polypeptide or polypeptide isoform which is substantially more active in either a proanthocyanidin (PA) or anthocyanin (ANT) pathway of a plant, said method including providing
material from said plant; and
an oligonucleotide probe capable of hybridizing with RNA from a gene encoding a polypeptide which is active in a flavonoid biosynthetic pathway;
extracting RNA from said plant material;
hybridizing the oligonucleotide probe with the RNA to generate an expression profile;
measuring PA and/or ANT levels in said plant material to generate a metabolic profile;
comparing said expression profile with said metabolite profile to identify said gene encoding a polypeptide or polypeptide isoform which is substantially active in either a PA or ANT pathway. In a preferred embodiment, the method may be performed using an electronic device, such as a computer.
By a 'polypeptide' is meant a polymer of linked amino acids, which may be an enzyme, regulatory protein or transporter protein. The enzyme may be a biosynthetic enzyme such as CHS, CHI, F3H, F3'H, F3'5'H, DFR, LAR, ANS, ANR, GST, G3T, UFGT, OlvlT, ART, ANAT or AAT. The regulatory protein may be a transcription factor such as TT1, TT2, TT8, TT16, TTG1 , TTG2, MYB, bHLH, MYC, WDR or PAP1. The transporter protein may be a polypeptide involved in the compartmentalisation of flavonoids, such as TT12, TT19 or H+-ATPase 10. By a 'polypeptide isoform' is meant one of two or more different forms of a polypeptide, which may be produced from related genes, or may arise from the same gene by alternative splicing. The isoforms may be produced by single nucleotide polymorphisms (SNPs), small genetic differences between alleles of the same gene.
By 'substantially more active in either a PA or ANT pathway' is meant that the polypeptide or polypeptide isoform has higher activity in either the branch of the flavonoid biosynthetic pathway that produces PAs or the branch of the flavonoid biosynthetic pathway that produces ANTs, when compared with its activity in the other pathway.
In a preferred embodiment the polypeptide or polypeptide isoform has activity at least approximately 15% higher, more preferably at least approximately 25% higher, more preferably at least approximately 35% higher, more preferably at least approximately 50% higher in one pathway relative to the other pathway.
For example, activity may be between approximately 15% and 100% higher, more preferably between approximately 25% and 200% higher, more preferably between approximately 35% and 300% higher, more preferably between approximately 50% and 500% higher in one pathway relative to the other pathway.
In a particularly preferred embodiment, the polypeptide or polypeptide isoform may be active in one pathway, and have no detectable activity in the other pathway.
In a preferred embodiment the polypeptide or polypeptide isoform may be substantially more active in a PA pathway relative to an ANT pathway.ln a particularly preferred embodiment, the polypeptide or polypeptide isoform may be active in the PA pathway and have no detectable activity in the ANT pathway. In a preferred embodiment, the polypeptide or polypeptide isoform may be an enzyme which is active late in the ANT pathway.
By an "enzyme which is active late in the ANT pathway" or a "late ANT pathway enzyme" is meant an enzyme which catalyses one of the final reactions in the synthesis of anthocyganins, after the leucoanthocyanidin branch point.
For example, the late ANT-pathway enzyme may be selected from the group consisting of GST, G3T, UFGT, OMT, ART, ANAT and AAT.
In an alternate preferred embodiment, the polypeptide or polypeptide isoform may be a transcription factor. For example, the transcription factor may be selected from the group consisting of MYB, bHLH, MYC and WDR.
The material from said plant is preferably material from said plant at two or more developmental stages. In preferred embodiments, the plant material may be a plant organ or tissue, such as a flower or inflorescence, or part thereof such as a floret, petal, sepal or stamen, or other floral tissue, or a vegetative organ or part thereof such as a leaf or other plant tissue.
Preferably, the material from said plant is floral material. Preferably, the floral material is at two or more developmental stages, for example immature, partially open (eg. approximately 5 to 35% open, approximately 35 to 65% open, and approximately 65- 95% open) and mature stages of development.
By an Oligonucleotide probe' is meant a short nucleic acid polymer, preferably having between approximately 5 and 200 bases, more preferably between approximately 10 and 100 bases, more preferably between approximately 20 and 50 bases.
By 'nucleic acid' is meant a chain of nucleotides capable of carrying genetic information. The term generally refers to genes or functionally active fragments or variants thereof and or other sequences in the genome of the organism that influence its phenotype. The term 'nucleic acid' includes DNA (such as cDNA or genomic DNA) and RNA (such as mRNA or microRNA) that is single- or double-stranded, optionally containing synthetic, non-natural or altered nucleotide bases, synthetic nucleic acids and combinations thereof. It will be understood by those of skill in the art that the term Oligonucleotide probe' applies to one or more oligonucleotide molecules, either identical or non-idential, which are designed, selected, and/or otherwise able to specifically hybridize to a target RNA. Additionally, an oligonucleotide probe as defined herein may comprise a collection of different oligonucleotide molecules targeted to one or more target regions of the same RNA. Thus, the term Oligonucleotide probe' as used herein may mean either the singular or the plural, such meaning being made clear by the context of usage in the present specification. Preferably a pair of oligonucleotide probes is used.
In a particularly preferred embodiment, the pair of oligonucleotide probes is selected from the pairs shown in Table 5 hereto and functionally active fragments and variants thereof.
By 'functionally active fragment or variant' in relation to an oligonucleotide probe is meant that the fragment or variant (such as an analogue, derivative or mutant) is capable of hybridizing with RNA from the gene encoding a polypeptide active in a flavonoid biosynthetic pathway. Additions, deletions, substitutions and derivatizations of one or more of the nucleotides are contemplated so long as the modifications do not result in loss of functional activity of the fragment or variant. Preferably the functionally active fragment or variant has at least approximately 80% identity to the relevant part of the above mentioned sequence to which the fragment or variant corresponds, more preferably at least approximately 90% identity, even more preferably at least approximately 95% identity, even more preferably at least approximately 98% identity even more preferably at least approximately 99% identity. Preferably the fragment has a size of between approximately 5 and 200 bases, more preferably between approximately 10 and 100 bases, more preferably between approximately 20 and 50 bases. Preferred fragments and variants include those having a single addition or deletion, or substitution of a single nucleic acid, when compared with an oligonucleotide probe shown in Table 5 hereto.
By 'capable of hybridizing with' is meant that the oligonucleotide probe has a nucleotide sequence sufficiently complementary to a target RNA sequence to permit said oligonucleotide to hybridize therewith under hybridization conditions.
The term 'hybridization' is understood to mean the process during which, under suitable conditions, two nucleotide fragments having sufficiently complementary sequences are capable of forming a double strand with stable and specific hydrogen bonds. A nucleotide fragment 'capable of hybridizing' with a polynucleotide is a fragment which can hybridize with said polynucleotide under hybridization conditions which are determined in a known manner in each case. The hybridization conditions are determined by means of the stringency, ie. the severity of the operating conditions. The higher the stringency at which the hybridization is carried out, the more specific the hybridization is. The stringency is defined in particular according to the base composition of a probe/target duplex, and also by means of the degree of mismatching between two nucleic acids.
The 'stringency' can also depend on the parameters of the reaction, such as the concentration and the type of ion species present in the hybridization solution, the nature and the concentration of denaturing agents and/or the hybridization temperature. The stringency of the conditions under which a hybridization reaction should be carried out will depend mainly on the target probes used. All these data are well known and the appropriate conditions can be determined by those skilled in the art.
Preferably, high stringency conditions may be used. By 'high stringency conditions' is meant the hybridization takes place at a temperature between approximately 35°C and 65°C and at a salt concentration of between approximately 0.5 to 1m, more preferably at a temperature between 50°C and 65°C and at a salt concentration of between approximately 0.8 to 1M. By 'RNA from a gene encoding a polypeptide which is active in a flavonoid biosynthetic pathway' is generally meant mRNA transcribed or otherwise generated from the gene.
The gene encoding a polypeptide which is active in a flavonoid biosynthetic pathway may encode any polypeptide which catalyses a reaction or is otherwise involved in flavonoid biosynthesis in a plant, for example an enzyme, regulatory protein or transporter protein, as hereinbefore described. Preferably the polypeptide which is active in a flavonoid biosynthetic pathway is selected from the polypeptides listed in Tables 1-4 hereto.
RNA may be extracted from the plant material by methods known to the person skilled in the art. For example, a CTAB-based extraction method may be employed. Further purification of the extracted RNA may be carried out, again by methods known to those skilled in the art.
The step of hybridizing the oligonucleotide probe with the RNA may also be carried out by methods known to those skilled in the art. Preferably a microarray is used to generate an expression profile.
By an 'expression profile' is meant that the activity or level of RNA expression of the gene is measured for the material from the plant, preferably at two or more developmental stages.
The step of measuring PA and/or ANT levels in the plant material may be carried out qualitatively and/or quantitatively.
A qualitative measurement may be carried out by visualising PA and/or ANT in untreated or stained plant material.
In a preferred embodiment, plant material may be stained for the presence of PA, for example using DMACA, and then PA visualised. In a preferred embodiment, ANT may be visualised in untreated plant tissues. A semi-quantitative measurement of PA may be carried out using a PVPP assay.
PA and/or ANT levels in the plant materials may also be measured quantitatively by measuring metabolites using liquid chromatography mass spectroscopy (LCMS).
The step of comparing said expression profile with said metabolic profile may be carried out by methods known to those skilled in the art. Preferably, the profiles are compared to identity genes that are up- or down-regulated, the up- or down-regulation correlating with PA or ANT accumulation. The step of comparing the expression profile with the metabolic profile is preferably performed using an electronic device, such as a computer. In a further aspect, the present invention provides a method of manipulating the flavonoid biosynthetic pathway in a plant, said method including identifying a gene encoding a polypeptide or polypeptide isoform which is substantially more active in either a PA or ANT pathway of said plant and up- or down-regulating expression of said gene to increase or decrease the level of PA or ANT in said plant. In a preferred embodiment, said method includes identifying a gene encoding a polypeptide or polypeptide isoform which is substantially more active in the PA pathway and up-regulating expression of said gene.
In an alternate preferred embodiment, said method includes identifying a gene encoding a polypeptide or polypeptide isoform which is substantially more active in the PA pathway and down-regulating expression of said gene.
In an alternate preferred embodiment, said method includes identifying a gene encoding a polypeptide or polypeptide isoform which is substantially more active in the ANT pathway and up-regulating expression of said gene.
In an alternate preferred embodiment, said method includes identifying a gene encoding a polypeptide or polypeptide isoform which is substantially more active in the ANT pathway and down-regulating expression of said gene. In a preferred embodiment, said method may include down-regulating expression of a gene encoding a polypeptide or polypeptide isoform which is active late in the ANT pathway.
For example, for targeted modification of the anthocyanin pathway in a red leaf white clover mutant expressing TrANR (anthocyanidin reductase) gene, the modification may include down-regulation of late anthocyanin-specific genes.
Particularly preferred genes include those encoding GST, G3T, UFGT, OMT, ART, ANAT and AAT.
In an alternate preferred embodiment, said method may include up- and/or down- regulating expression of one or more genes encoding a transcription factor.
For example, for targeted modification of the anthocyanin pathway in a red leaf white clover mutant expressing TrANR (anthocyanidin reductase) gene, the modification may include up- and/or down-regulation of genes encoding transcription factors.
Particularly preferred genes include those encoding MYB, bHLH, MYC and WDR. By 'manipulating the flavonoid biosynthetic pathway' is meant modifying flavonoid biosynthesis in a plant relative to a control plant. Preferably, flavonoid biosynthesis may be modified to increase PA biosynthesis relative to ANT biosynthesis. However, for some applications it may be desirable to increase ANT biosynthesis relative to PA biosynthesis. Preferably, the step of identifying a gene encoding a polypeptide or polypeptide isoform which is substantially more active in a PA or ANT pathway is carried out by a method as hereinbefore described. Alternatively, in certain circumstances the gene may already be indentified and the method may omit the identification step.
By 'up-regulating' expression of said gene is meant increasing expression of said gene and, as a result, the protein encoded by the gene, in a plant relative to a control plant. By 'down-regulating' expression of said gene is meant decreasing expression of said gene and, as a result, the protein encoded by the gene, in a plant relative to a control plant.
The up-regulation or down-regulation may be carried out by methods known to those skilled in the art. For example, a gene may be up-regulated by incorporating additional copies of a sense copy of the gene. A gene may be down-regulated, for example, by incorporating an antisense nucleic acid, a frame-shifted or otherwise modified sense copy of the gene, or a nucleic acid encoding interfering RNA (RNAi).
The up- or down-regulation may be carried out by introducing into said plant an effective amount of a genetic construct including the gene or a modified form thereof, such as an antisense nucleic acid, a frame shifted copy of the gene or a nucleic acid encoding RNAi.
Techniques for incorporating the genetic constructs of the present invention into plant cells (for example by transduction, transfection or transformation) are known to those skilled in the art. Such techniques include Agrobacterium mediated introduction, electroporation to tissues, cells and protoplasts, protoplast fusion, injection into reproductive organs, injection into immature embryos and high velocity projectile introduction to cells, tissues, calli, immature and mature embryos. The choice of technique will depend largely on the type of plant to be transformed. Cells incorporating the genetic constructs of the present invention may be selected, as described above, and then cultured in an appropriate medium to regenerate transformed plants, using techniques well known in the art. The culture conditions, such as temperature, pH and the like, will be apparent to the person skilled in the art. The resulting plants may be reproduced, either sexually or asexually, using methods well known in the art, to produce successive generations of transformed plants.
By 'an effective amount' is meant an amount sufficient to result in an identifiable phenotypic trait in said plant, or in a plant, plant seed or other plant part derived therefrom. Such amounts can be readily determined by an appropriately skilled person, taking into account the type of plant, the route of administration and other relevant factors. Such a person will readily be able to determine a suitable amount and method of administration. See, for example, Maniatis et al, Molecular Cloning: A Laboratory Manual, Cold Spring Harbor Laboratory, Cold Spring Harbor, the entire disclosure of which is incorporated herein by reference.
In a still further aspect, the present invention provides a method of enhancing bloat safety of a plant, said method including
identifying a gene encoding a polypeptide or polypeptide isoform which is substantially more active in a PA pathway and up-regulating or down-regulating expression of said gene to increase the level of PA in said plant; or
identifying a gene encoding a polypeptide or polypeptide isoform which is substantially more active in an ANT pathway and up-regulating or down-regulating expression of said gene to increase the level of PA in said plant.
In a preferred embodiment, said method may include down-regulating expression of a gene encoding a polypeptide or polypeptide isoform which is active late in the ANT pathway.
For example, for targeted modification of the anthocyanin pathway in a red leaf white clover mutant expressing TrANR (anthocyanidin reductase) gene, the modification may include down-regulation of late anthocyanin-specific genes. Particularly preferred genes include those encoding GST, G3T, UFGT, OMT, ART, ANAT and AAT.
In an alternate preferred embodiment, said method may include up- and/or down- regulating expression of one or more genes encoding a transcription factor.
For example, for targeted modification of the anthocyanin pathway in a red leaf white clover mutant expressing TrANR (anthocyanidin reductase) gene, the modification may include up- and/or down-regulation of genes encoding transcription factors.
Particularly preferred genes include those encoding MYB, bHLH, MYC and WDR. By 'enhancing bloat safety' of a plant is meant reducing the tendency of the plant to cause bloating in an animal which eats the plant.
Preferably, the step of identifying a gene encoding a polypeptide or polypeptide isoform which is substantially more active in a PA or ANT pathway is carried out by a method as hereinbefore described. Alternatively, in certain circumstances the gene may already be indentified and the method may omit the identification step.
In a still further aspect of the present invention, there is provided a genetic construct capable of manipulating the flavonoid biosynthetic pathway in a plant, said genetic construct including a gene encoding a polypeptide or polypeptide isoform which is substantially more active in either a PA or ANT pathway of said plant, or a modified form of said gene.
In a preferred embodiment, the genetic construct according to the present invention may be a vector.
By a 'genetic construct' is meant a recombinant nucleic acid molecule. By a 'vector' is meant a genetic construct used to transfer genetic material to a target cell.
The vector may be of any suitable type and may be viral or non-viral. The vector may be an expression vector. Such vectors include chromosomal, non-chromosomal and synthetic nucleic acid sequences, eg. derivatives of plant viruses; bacterial plasmids; derivatives of the Ti plasmid from Agrobacterium tumefaciens; derivatives of the Ri plasmid from Agrobacterium rhizogenes; phage DNA; yeast artificial chromosomes; bacterial artificial chromosomes; binary bacterial artificial chromosomes; vectors derived from combinations of plasmids and phage DNA. However, any other vector may be used as long as it is replicable or integrative or viable in the plant cell. In a preferred embodiment of this aspect of the invention, the genetic construct may further include a regulatory element and a terminator; said regulatory element, gene and terminator being operably linked. The regulatory element, gene and terminator may be of any suitable type and may be endogenous to the target plant cell or may be exogenous, provided that they are functional in the target plant cell.
By Operatively linked' is meant that said regulatory element is capable of causing expression of said gene or modified form thereof in a plant cell and said terminator is capable of terminating expression of gene or modified form thereof in a plant cell. Preferably, said regulatory element is upstream of said gene or modified form thereof and said terminator is downstream of said gene or modified form thereof.
By 'capable of causing expression of said gene' is meant that the gene or modified form thereof and the regulatory element, such as a promoter, are linked in such a way as to permit expression of said gene under appropriate conditions, for example when appropriate molecules such as transcriptional activator proteins are bound to the regulatory sequence.
By 'upstream' is meant in the 3'->5' direction along the nucleic acid. Preferably the regulatory element is a promoter. A variety of promoters which may be employed in the vectors of the present invention are well known to those skilled in the art. Factors influencing the choice of promoter include the desired tissue specificity of the vector, and whether constitutive or inducible expression is desired and the nature of the plant cell to be transformed (eg. monocotyledon or dicotyledon). Particularly suitable constitutive promoters include the Cauliflower Mosaic Virus 35S (CaMV 35S) promoter.
A variety of terminators which may be employed in the vectors of the present invention are also well known to those skilled in the art. The terminator may be from the same gene as the promoter sequence or a different gene. Particularly suitable terminators are polyadenylation signals, such as the CaMV 35S polyA and other terminators from the nopaline synthase (nos) and the octopine synthase (ocs) genes.
The genetic construct, in addition to the regulatory element, the gene or modified form thereof and the terminator, may include further elements necessary for expression of the gene or modified form thereof, in different combinations, for example vector backbone, origin of replication (ori), multiple cloning sites, spacer sequences, enhancers, introns (such as the maize Ubiquitin Ubi intron), antibiotic resistance genes and other selectable marker genes [such as the neomycin phosphotransferase (npt2) gene, the hygromycin phosphotransferase (hph) gene, the phosphinothricin acetyltransferase (bar or pat) gene], and reporter genes (such as beta-glucuronidase (GUS) gene (gusA)]. The genetic construct may also contain a ribosome binding site for translation initiation. The genetic construct may also include appropriate sequences for amplifying expression.
As an alternative to use of a selectable marker gene to provide a phenotypic trait for selection of transformed host cells, the presence of the genetic construct in transformed cells may be determined by other techniques well known in the art, such as PGR (polymerase chain reaction), Southern blot hybridisation analysis, histochemical assays (e.g. GUS assays), thin layer chromatography (TLC), northern and western blot hybridisation analyses. Those skilled in the art will appreciate that the various components of the genetic construct are operatively linked, so as to result in expression of said gene or modified form thereof. Techniques for operatively linking the components of the genetic construct of the present invention are well known to those skilled in the art. Such techniques include the use of linkers, such as synthetic linkers, for example including one or more restriction enzyme sites.
Preferably, the genetic construct is substantially purified or isolated.
By 'substantially purified' is meant that the genetic construct is free of the genes, which, in the naturally-occurring genome of the organism from which the nucleic acid or promoter is derived, flank the nucleic acid or promoter. The term therefore includes, for example, a genetic construct which is incorporated into a vector; into an autonomously replicating plasmid or virus; or into the genomic DNA of a prokaryote or eukaryote; or which exists as a separate molecule (eg. a cDNA or a genomic or cDNA fragment produced by PCR or restriction endonuclease digestion) independent of other sequences. It also includes a genetic construct which is part of a hybrid gene encoding additional polypeptide sequence.
Preferably, the substantially purified genetic construct is at least approximately 90% pure, more preferably at least approximately 95% pure, even more preferably at least approximately 98% pure. The term "isolated" means that the material is removed from its original environment (eg. the natural environment if it is naturally occurring). For example, a naturally occurring nucleic acid present in a living plant is not isolated, but the same nucleic acid separated from some or all of the coexisting materials in the natural system, is isolated. Such nucleic acids could be part of a vector and/or such nucleic acids could be part of a composition, and still be isolated in that such a vector or composition is not part of its natural environment.
Preferably, the gene included in the genetic construct of the present invention is identified by a method as hereinbefore described.
In a preferred embodiment, the gene may encode a polypeptide or polypeptide isoform which is active late in the ANT pathway. For example, the late ANT-pathway enzyme may be selected from the group consisting of GST, G3T, UFGT, OMT, ART, ANAT and AAT.
In an alternate preferred embodiment, the gene may encode a transcription factor. For example, the transcription factor may be selected from the group consisting of MYB, bHLH, MYC and WDR.
In a further aspect of the present invention there is provided a transgenic plant cell, plant, plant seed or other plant part with modified flavonoid biosynthetic characteristics relative to an untransformed control plant; said plant cell, plant, plant seed or other plant part including a genetic construct or vector according to the present invention. By 'modified flavonoid biosynthetic characteristics' is meant that the transformed plant exhibits increased flavonoid biosynthesis and/or contains increased levels of soluble carbohydrate relative to an untransformed control plant. Preferably, said transformed plant exhibits increased PA biosynthesis and/or contains increased levels of PA relative to an untransformed control plant.
In a preferred embodiment, the transgenic plant cell, plant, plant seed or other plant part with modified flavonoid biosynthetic characteristics has an increase in soluble carbohydrate, preferably an increase in PA, of least approximately 15%, more preferably at least approximately 25%, more preferably at least approximately 35%, more preferably at least approximately 50% relative to an untransformed control plant.
For example, soluble carbohydrate, preferably PA, may be increased by between approximately 15% and 500%, more preferably between approximately 25% and 300%, more preferably between approximately 35% and 200%, more preferably between approximately 50% and 100% relative to an untransformed control plant.
Preferably the transgenic plant cell, plant, plant seed or other plant part is produced by a method according to the present invention.
The present invention also provides a transgenic plant, plant seed or other plant part derived from a plant cell of the present invention and including a genetic construct or vector of the present invention.
The present invention also provides a transgenic plant, plant seed or other plant part derived from a plant of the present invention and including a genetic construct or vector of the present invention. The plant cell, plant, plant seed or other plant part may be from any suitable species, including dicotyledons, moncotyledons and gymnosperms. In a preferred embodiment the plant cell, plant, plant seed or other plant part may be from a dicotyledon, preferably forage legume species such as clovers (Trifolium species) and medics (Medicago species), more preferably white clover (Trifolium repens), red clover (Trifolium pratense), subterranean clover (Trifolium subterraneum) and alfalfa (Medicago sativa).
Preferably, the transgenic plant cell, plant, plant seed or other plant part is a clover species, more preferably white clover, or an alfalfa species. For example, the present invention enables the production of clover plants with increased PA in leaf blades, for improved nutrition for grazing animals.
By 'plant cell' is meant any self-propagating cell bounded by a semi-permeable membrane and containing a plastid. Such a cell also requires a cell wall if further propagation is desired. Plant cell, as used herein includes, without limitation, algae, cyanobacteria, seeds suspension cultures, embryos, meristematic regions, callus tissue, leaves, roots, shoots, gametophytes, sporophytes, pollen and microspores.
By 'transgenic' is meant any cell which includes a DNA sequence which is inserted by artifice into a cell and becomes part of the genome of the organism which develops from that cell. As used herein, the transgenic organisms are generally transgenic plants and the DNA (transgene) is inserted by artifice into either the nuclear or plastidic genome.
The methods of the present invention may be applied to a variety of plants, including monocotyledons [such as grasses (e.g. forage and bioenergy grasses including perennial ryegrass, tall fescue, Italian ryegrass, red fescue, reed canarygrass, big bluestem, cordgrass, napiergrass, wildrye, wild sugarcane, Miscanthus, switchgrass), corn or maize, rice, wheat, barley, sorghum, sugarcane, rye, oat) and energy crops (e.g. energy cane, energy sorghum)], dicotyledons [such as Arabidopsis, tobacco, soybean, canola, alfalfa, potato, cassava, clovers (e.g. white clover, red clover, subterranean clover), vegetable brassicas, lettuce, spinach] and gymnosperms. Preferably, the methods are applied to alfalfa and clover, more preferably white clover.
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 exclude further additives, components, integers or steps.
As used herein, except where the context requires otherwise, the term "include" and variations of the term, such as "including", "includes" and "included", may have the same meaning as the term "comprise" and variations of the term. 21
Detailed description of the embodiments
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.
Brief description of the drawings / figures
In the figures:
Figure 1. Accumulation of Proanthocyanidins and Anthocyanins in White Clover Organs and Tissues at Different Stages of Development. (A) to ( ) 4- Dimethylaminocinnemaldehyde staining of PA in inflorescences and flowers. (N) to (P) Staining of PA in vegetative organs. (Q) to (W) Visualisation of anthocyanins in florets and leaves, ab-abaxial; ad-adaxial; c-carpels; s-sepals, st-stamens; 1 -standard petal; 2- lateral wing petals; 3-keel petals.
Figure 2. Analysis of Flavonoid Levels in White Clover Inflorescences. (A) Appearance of white clover inflorescences and flowers at six stages of development. (B) Proanthocyanidin level. (C) Level and composition of free 2,3-flavan-3-ols. Black bars- GC, open bars-EGC. (D) Level and composition of anthocyanins. Open bars-A1, black bars- A2. (E) Level and composition of flavonol glycosides. Open bars-F1 , black bars-F2, grey bars-F3, cross-hatched bars-F4. GC-gallocatechin, EGC- epigallocatechin. A1-delphinidin-3-sambudioside, A2-cyanidin-3-sambudioside; F1- myricetin glycoside, m/z 479; F2-quercetin glycoside, m/z 463; F3-kaempferol glycoside, m/z 477; F4-quercetin quercetin acetyl-glycoside, m/z 505.
Figure 3. Normalized Expression Data from Genes Differentially-Expressed (p> 0.05). (A) Line plot showing gene expression patterns across 6 developmental stages of white clover flowers. The black lines represent genes up-regulated at stages 1-3 and down- regulated at stages 4-6. The medium grey lines represent genes down-regulated at stages 1-3 and up-regulated at stages 4-6. The light grey lines represent genes constitutively expressed. (B) Heat map derived from hierarchical clustering of genes showing similar expression patterns across the six developmental stages. For each of the stages represented the darker to grey colour depicted the higher the observed gene expression. (C) A self organising map with 7 X 8 output nodes organising genes into 56 clusters of similar gene expression. Figure 4. Transcript Levels of Selected Genes at Six Stages of White Clover Flower Development. Normalized relative transcript levels of indicated genes determined by real-time RT-PCR are shown as bars (scale on the left) and microarray results (scale on the right), as lines. Numbers on the x-axes represent developmental stages.
Figure 5. Organ-Specific Expression of Selected Genes at Developmental Stages 3, 4, 5 and 6 of White Clover Flower Development. Normalized relative transcript levels of indicated genes were determined by real-time RT-PCR. Black bars represent expression in inner whorls (petals, carpel and stamens). Grey bars represent expression in sepals. Numbers on the x-axes represent developmental stages.
Figure 6. Phenotypes of Flowers from White Clover Lines Containing a dsRNAi Construct Targeting TrANR. (A) to (C) 50% open inflorescences and flowers of TrANR dsRNAi lines showing white (6-1 OA), pink (6-8A) and red (6-14D) flower phenotypes, respectively. (D) Inflorescence of the 6-14D line at stages 5 and 6. (E) Individual flowers of the 6-14D line at different developmental stages. (F) Immature inflorescences at stage 3 of the wild-type (left) and 6-14D line (right). (G) Standard petals of wild-type (upper image) and line 6-14D (lower image) at stage 3. (H) Wing (right) and keel (left) petals at stage 3. (I) Petal epidermal cells under x X magnification. (J) Protoplasts isolated from petals of transgenic and wild-type plants (bottom left). (K) Cross-section of a line 6-14D flower at stage 3. (L-M) Anther filaments of wild-type plants stained with DMACA (stage 3) under X3.2 and X16 magnification, respectively. (N-O) Anther filaments of line 6-14D (stage 3) under X3.2 and X16 magnification, respectively. (P) Carpels of wild-type plants stained with DMACA (stage 3). (Q-R) Carpel of line 6-14D under X1.5 and X16 magnification, respectively. (S-T) Cross-section of a carpel from a wild-type plant stained with DMACA and an unstained carpel from line 6-14D (stage 4) under x40 magnification. Figure 7. Analysis of TrANR and TrLAR Transcript Levels in White Clover Lines Containing dsRNAi Constructs Targeting TrANR and TrLAR.
(A) Transcript levels of the TrANR gene in TrANR dsRNAi lines.
(B) Transcript levels of the TrLAR gene in TrLAR dsRNAi lines. (C) Transcript levels of the TrLAR and TrANR genes in TrANR-TrLAR dsRNAi lines. Normalized relative transcript levels were determined in 50% open inflorescences of the indicated lines by real-time RT-PCR. Black bars: TrANR, open bars: TrLAR. WT-wild- type.
Figure 8. Analysis of Flavonoid Levels in White Clover Lines Containing dsRNAi Constructs Targeting TrANR and TrLAR.
(A) to (C) Level and composition of flavonoid pathway products in 50% open inflorescences of wild-type lines and transgenic lines in which TrANR, TrLAR or both genes were targeted by dsRNAi constructs. (A) Free flavan-3-ols. (B) Anthocyanins.
(C) Flavonol glycosides. GC-gallocatechin, EGC-epigallocatechin. A1-delphinidin-3- sambudioside, A2-cyanidin-3-sambudioside; F1- myricetin glycoside, m/z 479; F2- quercetin glycoside, m/z 463; F3-kaempferol glycoside, m/z 477; F4-quercetin glycoside, m/z 505. Lines 6 and15- TrANR dsRNAi; lineslO and -TrLAR dsRNAi; lines 14 and 22- TrANR- TrLAR dsRNAi; wt-wild-type cv 'Mink'.
Figure 9. A Model for Flavonoid Biosynthesis in White Clover Flowers Based on Biochemical and Transcriptomic Data.
Specific compounds are listed in the lower case. Classes of compounds are listed in bold type. Enzymes are shown as open boxes, with preferred late-anthocyanin-specific genes highlighted in the heavy box and preferred transcription factors highlighted in the dotted box. Compounds and genes marked with an asterisk (*) were up-regulated in TrANR dsRNAi lines. Those marked with a hash (#) were down-regulated in TrANR dsRNAi lines. Figure 10. Phylogenetic tree of several classes of reductase-epimerase- dehydrogenase (RED) proteins: flavonol synthases (FLS), isoflavone reductases (IFR) and isoflavone reductase-like proteins (IFRL), phenylcoumaran benzylic ether reductases (PBER), (+)-pinoresinol/(+)-lariciresinol reductase protein (PLR), flavanone 3-hydroxylases (F3H), leucoanthocyanidin reductases (LAR), anthocyanidin reductases (ANR) and anthocyanidin reductase-like proteins (ANRL) involved in flavonoid biosynthesis. The phylogenetic tree was constructed from a ClustalW alignment using the neighbor-joining method in the MEGA4.0.2 package. VITV-V/'f/'s vinifera, PINTA- Pinus taeda, LOTCO-Lotus corniculatus, TR\RE-Trifolium repens, MEDTR-Medicago truncatula, PHACO-Phaseolus coccineus, ORYSA-Oryza sativa, ORVU-Hordeum vulgare, GOSAR-Gossypium arboretum, GOSRA-Gossypium raimondii, VITSH-V/i/s shuttleworthii , MALDO-Malus x domestica, ARAY -Arabidopsis thaliana, DESUN- Desmodium uncinatum, ZEAMA-Zea mays, CAMSI-Came///a sinensis FORI -Forsythia x intermedia, CICAR-C/cer arietinum. The accession numbers are as follows. Swissprot: Q84V83.1 , Q00016.1. P5 110.1. Genbank: CAI56335.1 , CAI56334.1, CAI56333.1 , CAI56332.1 , CAI56330.1, CAI56331.1 , AAC49608.1, AAF64174.1 , CAD91910.1, CAI56323.1 , CAI56324.1 , CAI56319.1 , CAI56325.1 , CAI56320.1 , AAN77735.1 , CAI56327.1 , CAI56328.1 , FJ842544, FJ842546, CAD91909.1, CAI56322.1, CAI56321.1 , CAD91911.1 , CAI56326.1 , CAI26310.1 , CAI26308.1 , CAA28734.1, AAZ79363.1 , AAZ79364.1, AAZ79365.1 , BAB92999.1 , AAT68773.1 , ABC71337.1 , AAV71171.1 , ABC71324.1 , ABC71328.1, AAV71171.1. RefSeq: NP_199094.1, NP_176365.1.
Figure 11. Normalised gene expression data from genes showing a significantly different expression (p> 0.05) in flowers of 3 TrANR dsRNAi lines in comparison to 3 wild-type white clover plants. Grey dots represent genes up-regulated in TrANR dsRNAi lines compared to wild-type plants. Black dots represent genes down-regulated in TrANR dsRNAi lines compared to wild-type plants.
Figure 12. Transcript Levels of Selected Genes in TrANR dsRNAi Lines in Comparison to Wild-Type Plants. Normalized relative transcript levels of indicated genes, as determined by real-time RT-PCR, are shown as bars (scale on the left) and microarray results (scale on the right) as lines. Table 1. Transcripts Induced at Stages 1-3 of Flower Development in White Clover
Table 2. Transcripts Induced at Stages 4-6 of Flower Development in White Clover
Table 3. Transcripts Up-Regulated in Flowers of TrANR dsRNAi Lines, Relative to Wild- Type Plants. Genes marked with an asterisk (*) were up-regulated at flower stages 1-3 in wild-type plants. Genes marked with a hash (#) were up-regulated at stages 4-6 in wild-type plants.
Table 4. Transcripts Down-regulated in in Flowers of TrANR dsRNAi Lines, Relative to Wild-Type Plants. Genes marked with an asterisk (*) were up-regulated at flower stages 1-3 in wild-type plants. Genes marked with a hash (#) were up-regulated at stages 4-6 in wild-type plants.
Table 5. List of Primers Used for Real Time RT-PCR Analysis
It will be understood that the invention disclosed and defined in this specification extends to all alternative combinations of two or more of the individual features mentioned or evident from the text or drawings. All of these different combinations constitute various alternative aspects of the invention.
Example 1 - Methods Plant Growth Conditions
Wild type and transgenic white clover lines were vernalised in a controlled growth room for 6 weeks at 5°C with an 8 h photoperiod and a light intensity of 41+/-5 μηηοΙ-ιτι"1-3"1 at canopy height. Flowering was then induced in a controlled growth cabinet (Enconair) by growing plants for 4 weeks at 22°C with a 16 hour photoperiod and a light intensity of 240+/-30 μηηοΙ-ηη"1-8"1 at canopy height.
Generation of Transgenic Plants
Transgenic white clover plants (Trifolium repens L. cv Mink) were generated by Agrobacterium-medlated transformation using cotyledonary explants and selection with 50 mg/L kanamycin sulfate as previously described (Ding et al., 2003). DNA was extracted from leaf tissue of putative transgenic lines using the Wizard DNA purification kit (Promega) and screened by real-time PCR for the presence of the npt2 selectable marker gene using the primers 5'-GGCTATGACTGGGCACAACA-3' and 5'- ACCGGACAGGTCGGTCTTG-3'. PCR mixtures were set up in a laminar flow hood with aerosol-free pipette tips using SYBR Green PCR Master Mix (cat# 4309155, Applied Biosystems), according to the manufacturers instructions, using at least 2 technical replicates and a 25 μΙ reaction volume. Thermal cycling was performed with a MX3000P thermal cycler (Stratagene) using the following cycling conditions for the detection of the npt2 gene: 10 mins at 95°C; 40 cycles of 30 sec at 95°C, 30 sec at 60°C and 30 sec at 72°C; 1 min at 95°C, 30 sec at 55°C and 30 sec at 95°C.
Visualisation of Proanthocyanidins and Anthocyanins
Plant material was stained for the presence of proanthocyanidins and monomeric flavan-3-ols using 0.01% (w/v) 4-dimethylaminocinnemaldehyde (DMACA) in absolute ethanol containing 1% (w/v) concentrated hydrochloric acid (McMurrough and McDowell, 1978). Anthocyanins were visualized in untreated white clover tissues. Images were captured using a Leica MZFLIII light microscope (Leica Microsystems) fitted with a CCD camera.
Biochemical Analysis of Flavonoids
A semi-quantitative PVPP-butanol-HCI assay was used to measure total proanthocyanidin levels in 5 -10 mg samples of freeze-dried, finely ground white clover material (Ray et al., 2003). Samples were analyzed using a spectrophotometer (Nanodrop) and final values were normalized against the mass of individual samples. Three biological replicates were performed. Flavonol glycosides, flavan-3-ols and anthocyanins were identified and quantified by LC-MS analysis. Three technical replicates of freeze dried, finely ground plant material (approximately 5 mg) were extracted three times in 0.5 ml aliquots of 80% methanol in water. The combined extracts were dried with gentle warming under a stream of nitrogen and reconstituted in 200 μL· of 80% methanol/water. An Agilent 1100 series HPLC system (Waldbronn) equipped with a quaternary gradient pump, column heater, autosampler with sample cooler (maintained at 4°C), and diode array detector (data acquired over 190-800 nm), coupled to a Thermo Electron LTQ ion trap mass spectrometer was used for LC-MS analysis. 5 μΙ aliquots of each sample were injected onto a 150 x 2.1 mm id., 3μ, Thermo BDS Hypersil C18 column maintained at 40°C. The mobile phase consisted of two components: A (water with 0.1% formic acid) and B (acetonitrile with 0.1% formic acid); and followed the gradients at a flow rate of 0.2 ml/min: Gradient 1: 0-5 min, 98% A; 5-25 min, 62% A; 26-35 min, (0.3ml/min) 98% A.
For identification of metabolites, LC-MS was run in polarity switching mode with MS" data acquired in both negative and positive modes. Analysis of the ESI negative mode MS and MS" data allowed the identification of four flavonol glycosides, and analysis of the ESI positive mode MS and MSn data along with the PDA data allowed the identification of two anthocyanins. For enhanced sensitivity needed to quantify metabolites, LC-MS data was acquired in ESI negative mode with a mass range limited to 200 to 1000 amu. Prior to data acquisition the system was tuned using a 20 μg/ml standard of epicatechin (EC). Standard curves for EC and epigallocatechin (EGC) were prepared by serial dilution of stock solutions and analysed in conjunction with the samples. The results were linear over the range examined (8-285 ng for EGC, 5-81 ng for GC). Standards for the flavonol glycosides and anthocyanins were not obtained and absolute quantitation was not possible. Results were based on relative levels of the metabolites in each sample, based on the area of the peak for the [M-H]" ion for the flavonols and for the UV-Vis absorption (500-550 nm) peak area for the anthocyanins.
Characterisation of the White Clover ANR and LAR Genes
cDNA clones containing the white clover ANR and LAR genes were identified using the sequences of the Arabidopsis thaliana BANYULS gene and the Desmodium unicinatum LAR gene as input data for BLAST searches of a white clover EST database (Altschul et al., 1997; Sawbridge et al. 2003). The deduced protein sequences of the white clover ANR and LAR genes were compared to sequences of related genes in the reductase- epimerase-dehydrogenase (RED) superfamily by constructing a phylogenetic tree with bootstrapping from a ClustalW alignment using the neighbor-joining method in the MEGA4.0.2 package (Tamura et al., 2007; Kumar et al., 2008). Preparation of Constructs for Plant Transformation
cDNA clones in pGEM-T Easy (Promega, Madison, USA) encoding the white clover ANR and LAR genes were previously generated as part of an EST discovery project (Sawbridge et al., 2003). The characterized TrANR and TrLAR cDNA clones were used as templates for PCR reactions. A 331 bp fragment from the 3' end of TrANR was amplified using the primers 5'-attB1-ATGCAGTTTCTGTCGGGTTC-3' and 5'-attB2- ATCAAAATCTAATTCTTC AGTGC-3' . A 386 bp fragment from the 3' end of TrLAR was amplified using the primers 5'-attB1 -TGAATGAGCTTGCTTCTTTGTG-3' and 5'-attB2- TAGATCCACCTCAGGTGAACC-3'. These PCR products were inserted into pDONR221 and fully sequenced clones were introduced into a GATEWAY®-enabled plant expression vector containing TrANR and TrLAR in hairpin constructs under the control of an enhanced CaMV 35S promoter and the 35S terminator and named TrANR dsRNAi and TrLAR dsRNAi, respectively. A 335 bp PCR fragment amplified from TrANR using the primers 5'-ATGCAGTTTCTGTCGGGTTC-3' and 5'- AGCAAGCTCATTCAATCAAAATCTAATTCTTCAGTGC-3' and a 371 bp PCR fragment amplified from TrLAR using the primers 5'-
GAATTAGATTTTGATTGAATGAGCTTGCTTCTTTGTG-3' and 5'-
TGAACCTTTTCAACAGGAAGC-3' were used as a template for a secondary PCR reaction using the GATEWAY primers 5'-attB1 -ATGCAGTTTCTGTCGGGTTC-3' and 5'-attB2-TAGATCCACCTCAGGTGAACC-3'. The 706 bp product, containing sequences from TrANR and TrLAR, was inserted into pDONR221 and a fully- sequenced clone was introduced into the GATEWAY®-enabled plant expression vector to produce TrANR-TrLAR dsRNAi.
Analysis of Gene Expression in White Clover
Proprietary Combimatrix CustomArray software was used to design single oligonucleotide probes of 35 to 40 bases in length for each white clover unigene. The resulting probe set was then assigned to a Combimatrix Custom 12k array.
To analyse differential expression of the genes at six developmental stages, samples were taken from the upper and lower halves of immature, 50% open and mature inflorescences in wild-type white clover, cv Mink. In order to test the effect of down- regulating TrANR on global gene expression, the 50% open inflorescences were harvested from wild-type white clover and red-flowered TrANR dsRNAi lines. Both microarray experiments involved three biological replicates, represented by different genotypes or transformation events, and two technical replicates. RNAs were extracted using the CTAB-based method of Chang et al. (1993) and were further purified using an RNeasy® Mini kit following the manufacturer's protocol (QIAGEN). The RNA samples were amplified and labelling was performed using the MessageAmp™ll aRNA Amplification Kit (Ambion) and Biotin-ULS aRNA Fluorescent Labelling Kit (Kreatech), according to the manufacturers' instructions. Each sample was hybridized to a separate array following the protocol recommended by the manufacturer (CombiMatrix). Slides were labeled, post-hybridisation, with streptavidin-cy5 according to the manufacturer's protocols (http://www.combimatrix.com). Slides were re-used up to 4 times and were stripped between uses with the Combimatrix stripping reagent as per http://www.combimatrix.com. The hybridized arrays were scanned with an Axon GenePix4000B instrument. Data was extracted using Combimatrix Microarray Imager software (http://webapps.combimatrix.com/customarrav/customarravHome.isp).
Background subtraction was performed by computing the mean signal intensity from the faintest 5% of all probes plus two standard deviation units, and deducting this value from all spots on the array. A minimum floor value was then set at 20 to eliminate any zero or negative spot values. The data on each array was then normalized using global median normalization (Draghici 2003) prior to being LOG2 transformed. Significant differences in gene expression levels between treatments were identified using analysis of variance (ANOVA) using the MAANOVA Bioconductor package (http://cran.r- proiect.org/src/contrib/Descriptions/maanova.html) (Wu et al. 2003). Genes that showed a difference with a significance of P>0.05 were identified as showing markedly different gene expression between the treatments. Genes showing similar expression profiles across the 6 phenological ranges of flower development in the first experiment were identified using self organizing maps in the SOM package from the R statistical programming environment (http://www. r-proiect.org/) and hierarchical clustering from the Bioconductor package (http://www.bioconductor.org). Thirteen white clover flavonoid genes representing different expression profiles and four internal control genes were selected for validation of microarray data. The housekeeping gene, elongation factor 1 -alpha (Ef1- ), was also included. A standard curve method for absolute quantitation was used with DNA standards of known concentration for each gene. Reverse transcription of 1 μg of RNA was performed using Transcriptor First Strand cDNA Synthesis kit (Roche) according to the manufacturer's recommendations. A list of the primers is shown in Table S5. The thermal profile: 95°C 10 min, [95.0°C 30 sec, 60.0°C 30 sec]x 40, melting curve protocol began immediately after amplification and consisted of 95°C 1 min, 60°C 1 min, 20 min ramp time from 60°C to 95°C followed by 95°C for 30 sec. Duplicate controls included RT-PCR reactions lacking reverse transcriptase or no template. Expression values were normalised by geometric averaging of four internal control genes encoding glyceraldehyde-3P-dehydrogenase (GAPDH), elongation factor 1 -alpha (EF1 ), histone H4 {HH4) and S-adenosylmethionine (SAMS), using geNorm software (PrimerDesign Ltd).
Accession Numbers
Sequence data can be found in the GenBank/EMBL database under the following accession numbers: TrANR, FJ842544 and TrLAR, FJ842546, the entire disclosures of which are incorporated herein by reference. Example 2
Proanthocyanidins and Anthocyanins are Co-Localized in Floral Epidermal Cells
PAs and their monomers were histochemically stained in white clover organs and tissues using DMACA (Figure 1). Floral organs stained strongly indicating that a high level of PA and 2,3-flavan-3-ol monomers were present. Accumulation of PAs in inflorescences at immature, partially (50%) open and mature stages of development is shown in Figure 1 (A-G). The accumulation of PAs appeared to be developmental^ regulated within all three developmental stages as indicated by intense staining of the oldest florets located at the base of each inflorescence (Figure 1B, D,E,G). White clover flowers have a calyx that consists of 5 fused sepals in which PAs or their monomers were detected only in multicellular trichomes (Figure 1H). The white or pale pink asymmetrical corolla contains 5 petals: a single large standard petal and two lateral wing petals, which enclose two interior keel petals (Figure 11). At early stages of flower development, PA accumulation was most clearly seen in the standard petal (Figure 1J- K), followed by the inner, wing and keel petals. PA accumulation appeared to start in epidermal cells located on the abaxial side of the petal and proceed to epidermal cells on the adaxial side during development (Figure 1J-K). The bases of all five petals are fused to a tube of 10 stamens. A mosaic pattern of PA accumulation was detected on the abaxial side of stamen filaments (Figure 1 L). A single carpel is located within the staminal tube. Figure 1M shows accumulation of PA in carpels. PAs or their monomers were detected only in multicellular trichomes of aerial vegetative organs of white clover, including peduncles, stolons, stipules, petioles and leaves (Figure 1 N-P). Trichomes staining heavily with DMACA were seen in leaves at stage 0.2 (Thomas, 1987, Figure 10). Accumulation of PAs in peduncles was similarly restricted to trichomes (Figure 1P). ANTs accumulated in both epidermal and sub-epidermal cells of aerial vegetative organs with no detectable accumulation in trichomes. The accumulation of ANTs in floral organs was restricted to epidermal cells, mainly in a small group of cells on the sepals (Figure 1Q-E) and in petals (Figure 1 R, U). ANTs were virtually undetectable in inner floral whorls including carpels and stamens under normal conditions, but could be synthesized in these whorls under stress conditions of low temperature and high light intensity. In leaves ANT mainly accumulate in epidermal cells located on adaxial side (Figure 1V, W), but could be found also on abaxial side under stress conditions of low temperature and high light intensity. Thus, the epidermal cells of petals are the main location where PAs and ANTs are likely to be spatially co-localized. Example 3
Flavonoid Levels and Composition Change During Floral Development in White Clover
We divided the inflorescences transversely at three selected developmental stages, namely, immature inflorescences, 50% open and mature inflorescences, for quantitative analyses of flavonols, PA, flavan-3-ols and ANT during flower development. This allowed the less developed flowers (upper part of inflorescence) and more developed flowers (lower part of inflorescence) within each inflorescence to be analysed separately (Figure 2A). As a result, flower development was represented by six stages, the youngest being the upper part of immature inflorescences (stage 1) and the most developed being the lower part of mature inflorescences (stage 6) (Figure 2A).
PAs were extracted in butanol-HCI, bound to PVPP and heated to release colored anthocyanidins as degradation products of PAs. This method showed that a very low level of PAs accumulated in leaves, reflecting their presence only in trichomes (Figure 2B). A higher level of PA was detected at flower stages 2 and 3, peaking at stage 4. Analysis of the free 2,3-flavan-3-ol level and composition in inflorescences using LC-MS revealed the presence of only gallocatechin (GC) and epigallocatechin (EGC) monomeric units (Figure 2C). The accumulation of EGC and GC was found to be developmentally regulated in flowers with detectable levels of free monomers at the stage 2 and the highest levels recorded at stage 3. A higher level of GC than EGC was seen at all six stages of flower development.
Analysis of anthocyanins in developing flowers revealed two major molecules, delphinidin-3-sambudioside (A1) and cyanidin-3-sambudioside (A2), the level of A1 being approximately two- to three-fold that of A2 (Figure 2D). Both ANTs showed the highest level of accumulation at stage 3, reflecting ANTs visible in sepals and emerging parts of the petals (Figure 1). Analysis of the level and composition of flavonols revealed 4 main flavonol glycoside species with myricetin (F1, m/z 479), quercetin (F2, m/z 463, F4, m/z 505) and kaempferol (F3, m/z 477) backbones (Figure 2E). The stereochemistry of the sugar unit and the position of the acetate moiety in these molecules was not established. Levels of the four flavonol glycosides increased during flower development, showing the highest level in mature flowers. The myricetin glycosides (F1 , m/z 479, R3 -OH, R5 -OH) were predominant in immature inflorescences (stages 1-2), almost equal levels of myricetin and quercetin glycosides (F2, m/z 463 and F4, m/z 505, R3'=OH, R5'=H) were found at flower stage 3, and quercetin glycosides were most abundant at later developmental stages. Example 4
Flavonoid Gene Expression is Developmental^ Regulated in White Clover
Flowers
We monitored the transcript accumulation patterns of 12,000 T. repens genes at the six stages of flower development. Figure 3 (A and B) shows graphical views of the normalized expression data with the expression value of each gene plotted on a log scale against the six developmental stages. All of these profiles passed the significance filter at p≤ 0.05. A total of 2398 genes showed expression differences when at least two of the six developmental stages were compared. The expression profiles for significantly differentially expressed genes across the 6 development stages were clustered using a self organising map. This map had 7 X 8 output nodes and organised genes into 56 clusters of similar gene expression (Figure 3C). We were interested in identifying groups of genes with expression profiles that temporally coincided with patterns of PA accumulation (stages 1-3) or ANT production in epidermal cells of developing white clover flowers (stages 4-6). Eleven clusters (654 genes) showed higher expression at stages 1-3 (dark & light blue) (Figure 3C). 21 clusters (928 genes) showed higher expression at stages 4-6 (red and brown) (Figure 3C). There were no clear differences in expression of the remaining genes between stages 1-3 and 4-6. Lists of genes with expression peaks between stages 1 and 3 (expression profile A), and those with expression peaks between stages 4 and 6 (expression profile B), are shown in Tables 1 and 2. We grouped the genes in terms of seven classes of potential functions, namely, flavonoid enzymes, transcription factors, mediators of protein-protein interactions and protein stability, transporters, mediators of auxin biosynthesis and signal transduction, proteins involved in cell signalling and metabolic enzymes not involved in flavonoid biosynthesis.
Example 5
Genes Expressed Between Stages 1 and 3 of Flower Development
Most members of the early and late flavonoid biosynthesis gene (EBG and LBG) families showed expression profile A (see Table 1 , online). Seven chalcone synthase (CHS) homologs showed expression profile A. The deduced amino acid sequences of these homologs, apart from TrCHSI, contain amino acids required for correct substrate binding, based on the crystal structure of Medicago sativa CHS (Jez et al., 2000). Five of these CHS-like genes, TrCHSI, TrCHS2, TrCHS3, TrCHS4, TrCHS6 and TrCHS7, showed expression profiles that peaked sharply at stages 2 and 3. TrCHS5 showed equally high levels of expression at stages 2, 3 and 4. The expression profiles of two chalcone isomerase (CHI)-like genes, TrCHH and TrCHI2, peaked sharply at stage 3 and showed equally high expression levels at stages 2 and 4, respectively. The expression of white clover homologs of flavonoid-3-hydroxylase (TrF3H1) and flavonoid- 3',5'-hydroxylase (TrF3'5'H1) genes peaked at stage 3 and declined at later developmental stages. TrCytB5-1, a homolog of a flower-specific cytochrome b5 gene, which is known to regulate F3'5'H activity and the accumulation of 5'-substituted anthocyanins (de Vetten et al., 1999), showed an expression profile very similar to that of TrF3'5'H~1. Interestingly the expression of a second cytochrome h5 gene, (TrCytB5- 2) showed a broader expression profile, peaking at stages 2, 3 and 4. Two dihydroflavonol 4-reductase-like genes, TrDFRL.1 and TrDFRL2, showed expression that peaked between stages 1 and 3 and sharply declined at later stages. Expression of two anthocyanidin synthase-like genes, (TrANSL.1 and TrANSL2), was also up- regulated during early stages of flower development, with the highest level at stage 3. Two genes homologous to anthocyanidin reductase (TrANR) and leucoanthocyanidin reductase (TrLAR), showed developmental^ regulated expression profiles with the highest levels of gene expression at stage 3, correlating well with accumulation of the corresponding flavan-3-ols. The expression of ANR was higher than that of LAR at all stages of flower development. LBGs, most of which encode enzymes involved in the modification of flavonoids, including flavonol 3-O-glucosyltransferases, UDP-glucose glucosyltransferases, O-methyltransferases, anthocyanidin rhamnosyl-transferases and UDP-glucose 4-epimerases, were well represented in profile A. Three genes homologous to an Arabidopsis laccase (o-diphenol and para(p)-diphenol:dioxygen oxidoreductase, 7770) involved in the oxidative polymerization of flavonoids (Pourcel et al., 2005), were also detected in the profile A group. Two of these genes, (TrLACI and TrLAC2) displayed a sharp expression peak at stage 3 and expression of a third laccase-like gene (TrLAC3) peaked at stages 1-2.
We found 19 transcription factors in the list of profile A genes. Among them were members of the R2R3-MYB/bHLH/WDR module involved in regulation of flavonoid genes. These included two R2R3 MYB transcription factors, (TrMYBI), one MYC factor (TrMYCI) and three WDR proteins (TrWDR1-3). Genes similar to those encoding other regulatory proteins involved in flavonoid biosynthesis (GLABRA2, TT1 , MADS-box, WRKY and GRAS), were also found to be expressed at early stages of white clover flower development. The expression of TrMYB2, TrWDR1-3 and TrTT1 peaked very early during flower development (stage 1).
Transporters were represented by 16 candidate genes potentially involved in the compartmentalization of flavonoids into the vacuole. These included ABC transporters, a glutathione S-transferase and a vacuolar sorting protein. Most showed an expression peak at stage 3.
Example 6
Genes Expressed Between Stages 4-6 of Flower Development
Members of some gene families with representatives up-regulated at stages 1-3 were found to be induced at later stages of flower development (see Table 2). For example, two CHS-like genes (TrCHS9 and TrCHS11), showed a sharp peak at stage 4 and two others, (TrCHS8 and TrCHSW), showed broad expression peaks at stages 3-5. Two F3H candidates, TrF3H2 and TrF3H3, showed distinct expression profiles. Expression of TrF3H2 was almost the same between stages 4-6 and that of TrF3H3 peaked at stage 6. Two DFR-like genes, TrDFRL3 and TrDFRL4, showed sharp up-regulation at stage 5. An F3'H homolog (TrF3!H1) and an ANS-like gene (TrANSLS) had expression peaks at stage 4. Genes encoding anthocyanin 5-aromatic acyltransferase, isoflavone- 7-O-methytransferase, methyltransferase, glucosyltransferase, UDP-glucuronosyl/UDP- glucosyltransferase and UTP-glucose glucosyltransferase enzymes conformed to expression profile B. Two isoflavone-7-O-methytransferase genes and two NADPH:isoflavone reductase candidate genes were identified among profile B genes. Some profile B genes potentially encoded transporters involved in vacuolar sequestration of flavonoids including a multidrug resistance-associated protein, a H+- transporting ATPase, ATP-binding cassette (ABC) transporters, a glutathione S- transferase and a vacuolar sorting protein. Interestingly a number of auxin-regulated genes and genes involved in auxin transport were up-regulated at stages 4-6 but not at earlier developmental stages.
White clover homologs of genes encoding components of the MYBR2R3- MYB/bHLH/WDR module, which potentially regulates flavonoid production, were also well represented within the profile B genes. These include six R2R3-MYB candidates (TrMYB3-6,8) four MYC/bHLH candidates (TrMYC2-3, TrbHLH1-2) and one WDR factor (TrWDR4). Genes encoding proteins similar to the YABBY, MADS-box, WRKY and GAI/GRAS classes of transcription factors, potentially involved in flavonoid biosynthesis, were also found to be expressed at late stages of white clover flower development. Real-time RT-PCR was used to validate the microarray data, with an emphasis on the expression of molecular markers of PA biosynthesis (TrANR and TrLAR), ANT biosynthesis (ANT 5' aromatic acetylase and UDP-glucosyltransferase), as well as CHS and ANS-like genes, representing EBGs and LBGs. Profile A genes included: TrANR, TrLAR, TrCHS7, TrCHS6, TrCHS2, TrANSLI and TrMYBL Profile B genes included: TrANAT3, TrUFGT4, TrCHSW, TrANSL3, TrMYB8 and TrMYB5. In all cases, there was a good correlation between real-time RT-PCR and microarray results (Figure 4).
To test both the spatial and temporal expression patterns of profile A and B genes we separated the sepals, which accumulate a high level of ANT and a low level of PA, from the inner floral whorls, which accumulate a high level of PA and a low level of ANT, sampling flowers at stages 3, 4, 5 and 6. Expression of the PA pathway-specific genes, TrANR and TrLAR, was highest within the inner whorls, correlating well with histochemical DMACA staining for PA accumulation in flowers (Figure 5 and Figure 1). TrANSLI and TrMYBI showed a similar expression profile. The four selected CHS genes showed a range of spatial expression profiles within the flowers. TrCHS7 and TrCHS2 were expressed mainly in inner whorls. Among the selected profile B genes, expression of TrCHSW was found to be sepal-enhanced and TrCHS6 showed an intermediate expression profile, with most expression within the inner whorls, but relatively high expression in sepals. TrANAT3 and TrUFGTwere found to be expressed specifically in the inner whorls. TrANS3 and TrMYB8 were expressed in both inner whorls and sepals. Example 7
Characterization of the White Clover ANR and LAR Genes
The translation product of a 1 ,014-bp TrANR cDNA (338 amino acids) shared 92.4% sequence similarity (88.2% identity) with a functionally characterized ANR from M. truncatula and 84% similarity (75.4% identity) with the BANYULS protein of A. thaliana (Xie et al., 2003). The position of TrANR in a phylogenetic tree of the superfamily of reductase-epimerase-dehydrogenase (RED) proteins is shown in Figure 10. The ANR family is most closely related to DFRs, forming a separate branch in the RED family and sharing a core 315- to 320-amino acid region. ANRs differ from DFRs by having 6-8 extra amino acids at the N-terminus and longer carboxy-terminal regions. Three putative LAR genes were identified among white clover expressed sequence tags (EST) sequences on the basis of similarity to the D. uncinatum LAR sequence (AJ550154; Tanner et al., 2003). All three have ORFs of 1 ,071 bp that are predicted to encode proteins of 356 amino acids in length. The TrLARa and TrLARb ORFs are distinguished by a single nucleotide difference and encode proteins with 99.7% amino acid identity. The TrLARa ORF also contains a frameshift, most likely caused by the loss of G418 during cDNA synthesis. The ORFs of TrLARb and TrLARc are distinguished by 9 nucleotide differences, encoding proteins with 98.9% amino acid identity. The four amino acids that discriminate TrLARb from TrLARc are not located within conserved motifs previously described (Tanner et al., 2003; Bogs et al., 2005). Since white clover is an allotetraploid species, these sequence variants may represent homeologs or allelic variation. Consequently, TrLARb was selected for further analysis and will henceforth be referred to as TrLAR. The deduced amino acid sequence of TrLAR is similar to LAR proteins from M. truncatula (86.5% amino acid identity), L. corniculatus LAR2-1 (71.6%) and Phaseolus coccineus (71.7%) (Bogs et al., 2005; Pang et al., 2007; Paolocci et al., 2007). TrLAR also shares 64.6% amino acid identity with L. corniculatus LAR1-1 and 62% identity with D. uncinatum LAR. Four motifs conserved in LAR sequences but absent from closely related isoflavone reductases (IFR) were identified in TrLAR. Three of these motifs, KRFLPSEFGHD (residues 116-126), ICCNSIA(g/a/s)WPY (residues 160-170), and THDIFI(n/k)GCQ (residues 276-285), are present in functionally active LAR enzymes. A fourth shorter motif, DIGKFT, is located between residues 203-208. Figure 10 shows the relationship between the sequences of TrLAR and other enzymes in the reductase-epimerase-dehydrogenase (RED) superfamily (Paolocci et al., 2007). Example 8
Down-Regulation of TrANR Correlates with the Accumulation of ANT in Floral Organs
Transgenic white clover plants ectopically expressing dsRNAi silencing constructs containing 3' end sequences of the TrANR (18 plants) and TrLAR (10 plants) cDNA sequences, and a fusion between the TrANR and TrLAR fragments, (9 plants) under control of the 35S RNA promoter from CaMV were generated to elucidate the function of TrANR and TrLAR in white clover flowers. The presence of transgenes in the To generation of transformed plants was verified by real-time PCR.
No significant phenotypic differences were found between the transgenic and wild-type plants in vegetative organs and sepals sampled at different stages of development. The main differences were seen in petals, carpels and stamens of flowers from stages 2 and 3 of development. The petals of TrANR dsRNAi lines displayed three main colour phenotypes, white/light pink, resembling wild-type flowers (lines 6-9B, 6-1 OA, 6-1 F), pink (lines, 6-8A, 6-9C1 and 6-10C) and dark red (lines 6-10B, 6-14D, 6-11A, 6-9B1 , 6- 4B, 15-2B) (Figure 6A-C, respectively). The strongest level of ANT accumulation in the red flowered lines was observed at flower stages 3 and 4. The colour of the petals was paler at later developmental stages (Figure 6D-E). In contrast to wild-type plants, the uppermost flowers of inflorescences in the red-flowered TrANR dsRNAi lines did not fully develop at stage 6 (Figure 1 F and Figure 6C). No significant differences were seen between sepals of the wild-type and transgenic lines at any developmental stages (Figure 6E-F). Light microscopy revealed a high level of ANT accumulation in the epidermal cells of petals, carpels, stamens and protoplasts of TrANR dsRNAi lines from early stages (2-3) of flower development (Figure 6G-K) in red-flowered lines. No ANT was detected in these organs in wild-type plants at corresponding stages. A mosaic pattern of ANT accumulation in epidermal cells of stamen filaments and carpels in TrANR dsRNAi lines correlated with the distribution of PA-producing cells in wild-type plants, as shown in Figure 6L-T. Transgenic TrANR-TrLAR dsRNAi plants showed flower phenotypes similar to those of TrANR dsRNAi lines. However, no red flower phenotype was seen among the TrLAR dsRNAi lines. The inflorescences of these lines resembled those of wild-type plants at all stages of development.
Transcript levels of the TrANR gene were measured in 50% open inflorescences (stages 3 and 4) of transgenic dsRNAi and wild-type plants using real-time RT-PCR. A red-flowered phenotype correlated with reduction in the level of TrANR expression in TrANR dsRNAi lines (Figure 7A, lines 6-10B, 6-14D, 6-11A, 6-4B, 15-2B). Pink- flowered TrANR dsRNAi lines (Figure 7A, lines 6-9B1 , 6-8A, 6-9C1, 6-10C) showed an intermediate level of TrANR expression that was higher than that of red-flowered transgenics, but lower than that of most transgenic lines with white or light pink flowers (lines 6-9B, 6-1 OA, 6-1 F) and the wild-type (Figure 7A).
Four of the six tested TrLAR dsRNAi lines showed a reduced level of TrLAR expression in comparison to the wild-type and two lines, 11-10A and 11-4C, showed almost a 10- fold reduction in expression. (Figure 7B).
Four of the five tested TrANR-TrLAR dsRNAi lines with red-flowered phenotypes (lines 22-2A, 22-4A, 22-1 B, 14-2B) were found to have reduced levels of both TrANR and TrLAR transcripts (Figure 7C). A higher level of both of these genes was found in TrANR-TrLAR dsRNAi lines with white/light pink flowers (14-1 A, 22-9A, 14-3A), but this level was still significantly lower than that of control plants.
Example 9 Down-Regulation of TrANR and TrLAR Correlates with Changed Levels of
Flavonoids in White Clover Flowers
Biochemical analysis of flavan-3-ols in 50% open inflorescences (stages 3 and 4) showed a reduction in the level of EGC in 4 out of seven tested TrANR dsRNAi lines (6- 10B, 6-9. B.1 , 6-4B and 15-2B) with red-flowered phenotypes and a reduced level of TrANR transcript, in comparison to wild-type plants (Figure 8A). Four tested TrANR dsRNAi lines (6-4B, 15-2B, 6-1 A and 15-8A) showed a decreased level of GC in comparison to control plants. The 6-4B and 15-2B lines showed a reduced level of both EGC and GC, when compared to control plants. Line 6-11 A did not show a reduced level of EGC, relative to control plants, but the level of GC was significantly reduced.
Interestingly, all tested TrLAR dsRNAi lines showed lower levels of GCs than wild-type plants. Two out of five analyzed TrLAR dsRNAi lines (11-1 OA and 11 -4C) that down- regulated TrLAR expression also showed a significantly reduced GC level than those of control plants. All TrLAR dsRNAi lines showed dramatically higher levels of EGC in comparison to control plants.
All tested TrANR-TrLAR dsRNAi lines with red petals (22-2A, 22-4A, 22-1 B.14-2B) that showed strong down-regulation of TrANR and TrLAR expression also had reduced GC levels, relative to control plants. Two lines, (22-2A and 22-4A) also had reduced EGC levels. GC was virtually absent in these two lines. Conversely, a pink flowered line (14- 1A) with a higher level of TrANR and TrLAR expression did not have significantly reduced levels of EGC and GC in comparison to control plants.
There was a positive correlation between ANT levels in 50% open inflorescences of transgenic plants and the intensity of petal coloration (Figure 8B). All lines with red- flowered phenotypes had higher levels of both delphinidin-3-sambudioside (A1) and cyanidin-3-sambudioside (A2), relative to wild-type plants, with a much higher level of A1 than A2. No significant differences were observed in A1 and A2 levels between white/light pink-flowered transgenic lines and wild-type plants.
The level and relative abundance of four major flavonol glycosides was modified in flowers from some TrANR dsRNAi lines, in comparison to those of wild-type plants (Figure 8C). The level of myricetin glycoside (F1 , m/z 479), was up to 3-fold higher in red-flowered transgenic TrANR dsRNAi and TrANR-TrLAR dsRNAi lines than in the wild-type. An intermediate level of myricetin glycoside accumulation was detected in transgenic lines with a pink-flowered phenotype. Production of kaempferol glycoside (F3, m/z 477) was slightly lower in the red-flowered transgenic lines than in transgenic lines with pink and white flowers and wild-type plants. There was no significant correlation between the accumulation of two quercetin glycosides (F2, m/z 463 and F4, m/z 505), ANT and flavan-3-ols in white clover flowers. Example 10
Down-regulation of TrANR Correlates with Global Changes in the Expression of Flavonoid-Related Genes
We compared the transcript accumulation patterns of 12,000 T. repens genes in 50% open inflorescences of three red-flowered TrANR dsRNAi lines and three wild-type lines using CombiMatrix™ custom oligonucleotide arrays. Only expression profiles that passed the significance filter at p < 0.05 were analyzed (see Tables 3 and 4). Approximately 900 genes were up-regulated and 600 genes were down-regulated in the red flowered TrANR dsRNAi lines, relative to wild-type plants (see Figure 11). A large proportion of these genes (approx 400) showed no BLAST hits or matched only hypothetical proteins. Of the annotated genes potentially involved in metabolic pathways, 150 were up-regulated and 123 were down-regulated in the TrANR dsRNAi lines relative to wild-type plants. These comprised gene classes encoding putative flavonoid enzymes, transcription factors, transporters, cell signaling proteins, proteins involved in protein-protein interactions or protein stability, mediators of auxin biosynthesis and signal transduction, proteins involved in transcription and translation and enzymes of other metabolic pathways (see Tables 3 and 4).
Twenty eight flavonoid pathway genes were up-regulated in red flowered TrANR dsRNAi lines, relative to wild-type clover plants (see Table 3). Most of the genes encoded enzymes involved in modification of ANTs. Two genes involved in the late steps of ANT biosynthesis, flavonoid 3-O-glucosyltransferase and UDP- glucuronosyl/UDP-glucosyltransferase, showed the highest rates of induction, 8.2- and 7.5-fold, respectively in TrANR dsRNAi lines. Other ANT-related genes up-regulated in TrANR dsRNAi lines included those encoding four glucosyltransferases, two glutathione S-transferases, two o-methyltransferases, anthocyanidin rhamnosyl-transferase and anthocyanin 5-aromatic acyltransferase.
Genes encoding eleven flavonoid enzymes, representing both EBG and LBG and functioning upstream of the TrANR gene, were also up-regulated in inflorescences of TrANR dsRNAi lines, relative to wild-type plants. These genes included three dihydroflavonol-4-reductase homologs (TrDFRL5, TrDFRL2, TrDFRL3), seven chalcone synthase homologs (TrCHS9, TrCHS11, TrCHS5, TrCHS2, TrCHS6, TrCHSIO), an anthocyanidin synthase-like gene (TrANSL.1), a flavanone 3-hydroxylase homolog (TrF3H2) and a chalcone isomerase homolog (TrCHI2). Genes encoding two homologs of cytochrome b5 DIF were also up-regulated 1.8- and 1.5-fold. Interestingly, homologs of genes encoding some enzymes of the isoflavonoid pathway, namely isoflavone 3'- hydroxylase, vestitone reductase, NADPH: isoflavone reductase, chalcone reductase, and isoflavone-7-O-methytransferase were also up-regulated in the red-flowered TrANR dsRNAi lines, relative to wild-type plants.
Genes encoding 19 transcription factors were up-regulated in inflorescences of red- flowered TrANR dsRNAi plants, relative to wild-type plants. Representatives of two components of the R2R3-MYB/bHLH/WDR module, namely TrWDR5, TrWDR6, TrMYB2, TrMYB6 and TrMYB3, showed the highest levels of up-regulation (X5, X1 ,2, X4.5, X1.7 and X1.4, respectively). Genes encoding representatives of the bHLH and MYC families of transcription factors, TrMYC3 and TrbHLH2, were up-regulated 1.5- and 1.4-fold, respectively, in red-flowered TrANR dsRNAi plants. Genes encoding homologs of the circadian clock-associated genes, CCA1 {TrMYBW) and LHY (TrMYBH) were up-regulated 2.9- and 2.4-fold respectively, in the transgenic lines.
Thirty genes encoding proteins involved in protein-protein interactions and protein stability, 22 genes involved in cell signaling and 13 transporters were expressed at higher levels in red-flowered TrANR dsRNAi lines, relative to wild-type plants. Lipid transfer proteins, vesicle-associated membrane proteins and vacuolar sorting proteins involved in intracellular compartmentalization of the flavonoid enzymes and/or their products were strongly represented among genes highly expressed in inflorescences of red-flowered TrANR dsRNAi lines. Approximately 500 genes were down-regulated in the inflorescences of TrANR dsRNAi lines, relative to wild-type plants (see Table 4). Approximately 300 of these genes showed no BLAST hits or matched only hypothetical proteins. Ten genes down- regulated in TrANR dsRNAi plants encoded flavonoid-related enzymes. As expected, the expression of TrANR was much lower in these lines. Surprisingly, two genes involved in isoflavonoid biosynthesis, NADPH:isoflavone reductase (TrIFRI, X24) and isoflavone-7-O-methytransferase (TrIFOMTI , X3.7) were strongly down-regulated. Homologs of flavonoid 3 -hydroxylase (TrF3'H1, X2.4), dihydroflavonol 4-reductase (TrDFR4, X1.7), UDP-glucose 6-dehydrogenase (X2.3), anthocyanin 5-aromatic acyltransferase (X3.3), UDP glucuronosyl/UDP glucosyltransferase (X2.9), flavonoid 3- O-glucosyltransferase (X1.88), and methyltransferase (X1.5), genes were also down- regulated in TrANR dsRNAi lines.
Expression of 18 transcription factors was suppressed in TrANR dsRNAi plants, among them members of the MYB/bHLH/WDR module, namely TrWDR7 (x3.5) and TrMYB12 (x1.37). These genes had not been differentially expressed during the development of white clover flowers.
Real-time RT-PCR was used to validate data from the second microarray experiment. A sample of genes up-regulated or down-regulated in TrANR dsRNAi lines relative to wild- type plants was selected, namely, TrANSI, TrCHSIO, TrCHS2, TrCHS6, and TrANR (see Figure 12). The expression profiles of these genes correlated well with the results of the microarray experiment (see Tables 3 and 4).
A comparison of the two microarray data sets revealed that 22% (33 out of 150) of the genes up-regulated in inflorescences of red-flowered TrANR dsRNAi lines showed differential expression during flower development in wild-type plants. Genes in this subset corresponding to expression profiles A and B are highlighted in blue and yellow, respectively, in Tables 3 and 4. It is interesting that the highest proportion of these genes (14) are flavonoid-related, including six chalcone synthase homologs (TrCHS2, profile A, TrCHS6, profile A, TrCHS5, profile A; TrCHS9, profile B; TrCHSIO, profile B; TrCHS11, profile B), two out of three dihydroflavonol-4-reductase homologs (TrDFRL2, profile A; TrDFRL3, profile B), one chalcone isomerase homolog (TrCHI2, profile A), one flavonoid 3-hydroxylase homolog (TrF3H2, profile B), one anthocyanidin synthase homolog (TrANSI, profile A), and one cytochrome b5 DIF homolog (TrCytB5-1, profile A). Of the 12 homologs of transferases involved in ANT modification and up-regulated in TrANR dsRNAi lines, just three showed differential expression during wild-type flower development. These were a UDP-glucuronosyl/UDP-glucosyltransferase homolog, TrUFGT4 (profile B), a methyltransferase, TrOMT5 (profile B) and anthocyanidin rhamnosyl-transferase, TrARTI (profile A).
Six transcription factors up-regulated in TrANR dsRNAi lines were differentially expressed during the development of wild-type flowers, including the R2R3 MYB-related genes TrMYB2 (profile A), TrMYB3 (profile B) and TrMYB6 (profile B). Other transcription factors up-regulated in TrANR dsRNAi lines and differentially expressed during flower development included TrMYC2 (profile B), a CONSTANS-like zinc finger protein (profile B) and a SQUAMOSA promoter-binding protein (profile A).
Six out of 8 of the genes encoding flavonoid pathway enzymes that were down- regulated in TrANR dsRNAi lines showed differential expression between at least two flower stages. The remaining two were candidate anthocyanin 5-aromatic acyltransferase (TrANATS) and UDP-glucose glucosyltransferase (TrUFGTG) genes. The transcription factors TrWDRl and TrMYB12, which were down-regulated in TrANR dsRNAi plants, did not show differential expression during flower development.
Example 11 Distinct Representatives of Flavonoid-Related Multigene Families Contribute to Spatio-Temporal Profiles of ANT and PA Accumulation in Floral Organs
The developmentally-regulated anthocyanin and proanthocyanidin pathways were found to be spatially co-localized in epidermal cells of white clover flower petals. Accumulation of 2,3-flavan-3-ol monomers and PA started in immature inflorescences and peaked at stages 3 and 4, respectively. ANT accumulation began in epidermal cells of petals when they emerged from the sepals and were exposed to light (stages 3-6, Figure 2A, D). The onset of light-induced pigmentation coincided with declining levels of 2,3-flavan-3-ols and TrANR and TrLAR transcripts (Figure 2C and Figure 4). This suggests that the activities of the PA and ANT pathways are separated temporally, with the PA pathway active at stages 1-3 and the accumulation of ANT occurring in the same cells at later stages of floral development. The activities of the two pathways appear to overlap at stage 3. This raises questions about the molecular organization of these pathways and their potential cross-talk in epidermal cells. PAs and ANTs are produced by two related but distinct branches of the flavonoid pathway. Both branches involve the conversion of 4-coumaroyl CoA and malonyl CoA to flavan-3,4-diol and 3-OH-anthocyanidin molecules. Activation of both pathways requires the recruitment of R2R3-MYB, WDR and bHLH transcription factors for the transcriptional activation of early and late flavonoid biosynthesis genes. Molecular studies in a range of plant species have revealed that almost all of the flavonoid enzymes are encoded by members of multigene families. The ANT and PA pathways in white clover flowers may recruit exactly the same enzymes or distinct isoforms of enzymes encoded by different members of multigene families, for shared steps in flavonoid production.
The expression of homologues of PA pathway-specific genes, including TrANR, TrLAR, TrTT1 and TrTTIO, showed strict profile A expression, peaking during flower" stages 1-3 and declining at later developmental stages. This correlated well with the production of 2,3-flavan-3-ol monomers in the inner floral whorls. Homologs of ANT pathway-specific genes involved in conversion of 3-OH-anthocyanidin molecules to anthocyanins were found in both profiles, correlating with ANT production in sepals at all stages of development and the increase in ANT biosynthesis in inner floral whorls at stage 3 (Figure 2C-D). Representatives of multigene families encoding CHS, DFR, ANS and F3H enzymes, MYB, bHLH and WDR transcription factors and transporters were also found in both expression profiles. Representatives of some of the genes shared by both the PA and ANT biosynthesis pathways, such as CHI (profile A), F3'H (profile B) and F3'5'H (profile A) were found only in one profile, although expression of these genes was detectable at both early and late stages of flower development. For example, expression of the single F3'5'H candidate gene peaked at stages 2 and 3 but remained high through stages 4 and 5. This correlated well with expression of homologs of the flower-specific cytochrome b5 gene, which regulates F3'5'H activity, and with the main increase in production of 5'-hydroxylated flavan-3-ols throughout flower development (Figure 2C).
ANS represents a branch point between the PA and ANT pathways converting flavan- 3,4-diols to 3-OH-anthocyanidins, potential substrates for both pathways. The ANT pathway modifies 3-OH-anthocyanidins by a chain of glycosylation and esterification reactions and the PA pathway involves the reduction of 3-OH-anthocyanidins to 2,3-c/s- flavan-3-ols by ANR. Three ANS-like proteins from white clover, TrANSI, TrANS2 and TrANS3, show 94.4%, 94.4%, and 70% deduced amino acid sequence identity to . truncatula ANS, respectively. Multiple sequence alignment confirmed the presence of three conserved residues (His-232, His-288, and Asp-234) required to coordinate ferrous iron at the catalytic center of iron-containing soluble oxygenases, and Arg-298, Y-217 and S-300, which are assumed to contribute to the specific binding of 2- oxoglutarate in the TrANS proteins. However, only TrANSI contains the DHQ1-, DHQ2- and MES/ascorbate-binding domains specific to ANS enzymes, but not other 2- oxoglutarate iron-dependent oxygenases, including flavanone 3-D -hydroxylases (F3H) and flavonol synthases (FLS). TrANS2 and TrANS3 share a low level of amino acid identity with Arabidopsis FLS (41.9% and 35%, respectively) and F3H (31.1% and 26.5%, respectively). The TrANS2 and TrANS3 genes showed distinct profile A and profile B-specific expression, respectively, whilst TrANSI expression peaked at stage 3, but remained relatively high during stages 4 and 5.
R2R3-MYB, bHLH and WDR transcription factors have redundant functions in plant development. The Arabidopsis representatives of these families (TT2, TT8 and TTG1) are involved in PA, ANT and mucilage biosynthesis, root-hair patterning and trichome development. Six candidate genes encoding white clover MYB factors were closely related to R2R3-MYB proteins identified in other plant species. The R2R3 repeat region of white clover MYBs is highly conserved and contains the motif [D/E]Lx2[R/K]x3Lx6Lx3R for interaction with bHLH proteins, whereas the C-terminal regions show a low level of similarity to other MYB factors. TrMYB3 (profile B) is closely related to the Arabidopsis subgroup 10 MYBs and clustered with other R2R3-MYB gene products involved in anthocyanin biosynthesis, including PAP1 , PAP2, PhAN2, LeANTI , WMYBA2 and VvMYBAI . The deduced amino acid sequence of TrMYB6 (profile A) clustered with MIXTA and PhMYBI, sharing 89% amino acid sequence similarity in the R2R3 DNA-binding domain. Representatives of the bHLH, WDR, MADS box and WRKY box gene families were also found in both expression profiles. Both bHLH and WDR factors are components of the R2R3-MYB/bHLH/WDR transcription factor complex that regulates enzymes in both the PA and ANT pathways in different plants. Arabidopsis TTG2, a WRKY box factor, regulates at least three separate morphogenetic processes in L1 -derived cells: trichome development and the production of mucilage and condensed tannin in seed coats. BANYULS promoter activity is not affected in ttg2 mutants and both TTG2 and TT1 , a zinc finger protein, may be involved in post- transcriptional regulation of BANYULS expression. Therefore, the white clover TTG2 homolog could potentially regulate TrANR expression in trichomes and epidermal cells. The Arabidopsis MADS-box factor TT16/ABS is known to be expressed in the ovule, mediating BANYULS expression and PA accumulation in the endothelium of seed coats. One of the white clover MADS box factors up-regulated early in flower development might similarly control PA production by transcriptionally activating the TrANR gene.
The PA and ANT pathways are localized within different groups of epidermal cells in sepals: a low level of PA accumulates in trichomes and a high level of ANT is present in a subset of epidermal cells at stages 1-6 (Figure 1). The fact that some of the selected flavonoid genes, including molecular markers of the PA (TrANR and TrLAR) and ANT (ANT acetylase, UFGT) pathways, early (CHS) and late (/WS-like) flavonoid biosynthetic genes as well as R2R3-MYB transcription factors, displayed organ-specific expression profiles (Figure 5) suggests that the PA and ANT pathways in sepals and petals recruit (at least partially) different flavonoid-specific members of multigene families. Taken together, the data suggest that spatio-temporal patterns of ANT and PA accumulation in floral organs reflect developmentally-regulated and organ-specific expression profiles of distinct isoforms of flavonoid-related enzymes encoded by multigene families.
Example 12
Roles of the White Clover ANR and LAR Genes in PA Biosynthesis
According to the most recent models, ANR and LAR participate in two separate branches of the PA pathway in most PA-producing species. LAR functions downstream of DFR, catalyzing the conversion of 2,3-flavan-3,4-diols to 2,3-frans-flavan-3-ols. ANR acts immediately downstream of ANS catalyzing the conversion 3-OH-anthocyanidins to 2,3-c/s-flavan-3-ols. Expression of both genes has been found to be developmental^ regulated in PA-accumulating tissues of different species. In grapes, VvANR and VvLARI are up-regulated at early stages of berry development, 7 weeks before veraison, which correlates well with accumulation of the corresponding flavan-3-ols and PA. The expression of MdLARI and MdANR was also shown to be highest during early development of apple (Malus x domestica Borkh. cv. 'Cripps Red') fruit. Furthermore, transcript levels of both the ANR and LAR genes are higher in immature leaves than in mature leaves of L. comiculatus, correlating well with increased accumulation of PAs at early stages of leaf development. The spatio-temporal expression patterns of the TrANR and TrLAR genes in white clover flowers also correlate with the pattern of c/s- and irans-flavan-3-ol accumulation. Interestingly, a higher level of TrANR than TrLAR expression correlates with higher levels of GC than EGC monomers at all tested stages of flower development. Despite the higher level of GC we observed in comparison to EGC, prodelphinidin polymers in T. repens flowers consist of terminal and extender units with nearly equal proportions of the two epimers. A higher expression level of ANR, relative to LAR, has also been seen in L. comiculatus herbage and in the skin of red apples. A higher level of VvANR expression than WLAR7 and VvLAR2 expression in grape flowers was found to correlate with a higher level of catechins than epicatechins. The expression of VvANR correlates with a high level of flavan-3-ols and extension subunits with 2,3-c/s- stereochemistry only in grape leaves, where VvLARI is not expressed and WLAR2 is only expressed late in development. Interestingly, in spite of the high level of catechin monomers, most grape tissues accumulate significant levels of epicatechin-based PAs.
Example 13
TrLAR Gene Activity is Necessary but Insufficient for 2,3-trans-flavan-3-ol
Production in White Clover Flowers
Although the role of the ANR gene in biosynthesis of the 2,3-c/s-flavan-3-ols has been clearly demonstrated using molecular, genetic and biochemical approaches, the contribution of the LAR gene to PA biosynthesis is still unclear, mainly due to the lack of genetic studies. Most functional information is based on the in vitro activity of recombinant LAR proteins, ectopic expression of LAR genes in tobacco and white clover and the expression profiles of LAR and ANR genes in PA-accumulating tissues. LAR and ANR genes have been found to be co-expressed in tissues producing PA, namely L. corniculatus leaves, apple fruit, grape berries, seed coats of M. truncatula and white clover flowers (this study). The expression of ANR and LAR genes is coordinately regulated by the same family of transcription factors in grape berries and L. corniculatus tissues. The absence of LAR genes in plants producing only 2,3-c/s- flavan-3-ols, such as Arabidopsis may suggest that LAR genes are involved in the biosynthesis of 2,3-frans-flavan-3-ols.
On the other hand, a relatively high level of MtLAR expression contrasted with the virtual absence of 2,3-frans-flavan-3-ol subunits in PA from M. truncatula plants. The ectopic expression of LAR genes from M. truncatula and D. uncinatum in tobacco and white clover did not increase levels of irar?s-flavan-3-ols in leaves or flowers. The PA level was actually lower in transgenic tobacco lines than in control plants. Alternative or multiple functions of the LAR gene have been suggested. The LAR gene is encoded by multigene families in some PA-producing species, including grape and L corniculatus. Only one of the L corniculatus LAR genes showed in vitro activity in E. coli. Transgenic approaches aiming to characterize the function of LAR genes have not been successful. Gain-of-function experiments failed to show increased levels of 2,3-trans- flavan-3-ol subunits in transgenic tobacco and white clover lines ectopically expressing LAR genes. The function of LAR genes has not been successfully characterized by loss-of-function approaches in the model plants, A. thaliana and M. truncatula, which have PA that lacks, or contains virtually no £ra/7s-flavan-3-ol monomers. Floral PAs and free flavan-3-ols in T. repens contain both epigallocatechins and gallocatechins. This feature and the high genetic transformation efficiency of T. repens make it an attractive system for the functional analysis of PA-related genes, including ANR and LAR. Phylogenetic analysis showed that TrLAR is most similar to LAR proteins from M. truncatula and P. coccineus, species which, like white clover, lack appreciable PA biosynthesis in leaf, stem and root tissues. When compared to Lotus corniculatus LAR proteins, the amino acid sequence of TrLAR is more similar to LcLAR2 than to LcLARl It is interesting that LcLAR2 did not show specific LAR activity when expressed in E. coli. The spatio-temporal profile of white clover LAR expression correlates well with accumulation of GC in PA-producing organs. Down-regulation of the TrLAR gene in TrLAR dsRNAi and TrANR-TrLAR dsRNAi lines significantly decreased the level of TrLAR transcripts and correspondingly, the GC level in white clover flowers. The much more pronounced reduction in GC level, compared to the TrLAR transcript level in some TrLAR dsRNAi lines (11-15A, 10-12A and 11-8A) suggests that expression of another TrLAR gene(s) could be affected in TrLAR dsRNAi lines. Our phenotypic, molecular and biochemical data suggest that LAR activity is necessary for GC biosynthesis in white clover flowers. However, the fact that ectopic expression of LAR genes in tobacco and white clover plants resulted in no changes in GC production suggests that LAR activity alone is not sufficient for the biosynthesis of 2,3-frans-flavan-3-ols.
Down-regulation of the TrLAR gene leads to a dramatic increase in the level of EGC in TrLAR dsRNAi lines. However, there were no significant changes in the levels of the two main anthocyanins in the petals. This suggests that the pool of intermediate 3-OH- anthocyanidin molecules appeared to be diverted towards 2,3-c/s-flavan-3-ol rather than anthocyanin production when TrLAR was down-regulated, in contrast to the down- regulation of TrANR in white clover plants. Example 14
TrANR Gene Activity is Necessary and Sufficient for 2,3-cis-flavan-3-ol
Production in White Clover Flowers
Loss of ANR function in the Arabidopsis banyuls mutant results in a transparent testa phenotype with a decreased level of 2,3-c/'s-flavan-3-ols and accumulation of anthocyanin in the seed coat. Combined with the finding that expression of recombinant MtANR protein converts cyanidin, delphinidin and pelargonidin molecules into epicatechines, epigallocatechin and epiafzelechin, respectively, suggests that ANR activity is necessary and sufficient for the production of 2,3-c/s-flavan-3-ols. As in the banyuls mutant, down-regulation of TrANR reduced the level of ANR transcripts and EGC molecules and increased the level of ANT in PA producing cells of white clover. An intriguing finding was that down-regulation of the TrANR gene correlated with reduced levels of both EGC and GC in TrANR dsRNAi and TrANR-TrLAR dsRNAi lines. Interestingly, the levels of TrLAR transcripts were twice as high in TrANR-TrLAR dsRNAi lines 22-1B and 14-2B as in TrLAR dsRNAi lines 11-10A and 11-4C, but GC levels were lower in the TrANR-TrLAR dsRNAi lines. GC was virtually undetectable in the 22-2A and 22-4A TrANR-TrLAR dsRNAi lines, suggesting that the effect of silencing the TrANR and TrLAR genes on 2,3-fraA7s-flavan-3-ol production was additive. A reduced level of GC in TrANR dsRNAi and TrANR-TrLAR dsRNAi lines might be explained by ANR having an additional direct or indirect role in the biosynthesis of 2,3- frans-flavan-3-ols. Interestingly, the trans (enf) epimers of catechin, gallocatechin and afzelechin were detected as minor products after incubation of recombinant MtANR protein with cyanidin, delphinidin and pelargonidin molecules, respectively. This finding was explained as an artifact caused by epimerization of the thermodynamically less stable 2,3-c/s diastereoisomers into more stable 2,3-trans- (ent) forms. Further experiments are needed to clarify whether this reaction occurs naturally in wild-type plants or is triggered only by an artificially high level of pathway intermediates.
Example 15
Cross-Talk within the Flavonoid Pathway
The ANT and PA pathways share dihydroflavonols as precursor molecules. Three classes of these molecules, differing only in the extent of B-ring hydroxylation, have been identified in legumes. Modification of dihydrokaempferols (R3 -H, R5 -H), dihydroquercetins (R3'=0H, R5'=H), and dihydromyricetins (R3'=0H, R5'=0H) by DFR, ANS and a range of anthocyanidin-modifiying enzymes leads to the biosynthesis of ANTs with pelargonidin (R3'=H, R5'=H), cyanidin (R3'=0H, R5'=H) and delphinidin (R3 -0H, R5 -0H) backbones, respectively. Alternatively dihydroflavonols can be converted to cis and trans epimeric forms of afzelechins (R3 -H, R5 -H), catechins (R3'=0H, R5'=H) and gallocatechins (R3'=0H, R5'=0H) by DFR, LAR, ANS and ANR enzymes in the PA pathway. Glycosylated forms of three flavonols, representing all three B-ring hydroxylated variants of dihydroflavonols, were found in white clover flowers with an abundance of myricetin glycosides (F1 , m/z 479, R3 -OH, R5 -OH) at stages 1-2 and an increased level of quercetin glycosides (F2, m/z 463 and F4, m/z 505, R3 -OH, R5 -H) at later developmental stages (3-6). ANT composition at all these stages showed the predominance of delphinidin-based ANTs and a much lower level of cyanidin-based ANTs. A low level of kaempferol-based ANTs (F3, m/z 477, R3 -H, R5 -H) and virtually no pelargonidin-based ANTs were found at ail developmental stages. Analysis of 2,3-flavan-3-ols detected only gallocatechins and epigallocatechins at all developmental stages, with a higher level of gallocatechins.
Down-regulation of TrANR led to a decrease in the level of epigallocatechin and an increase in the level of products of the flavonol and anthocyanin pathways with hydroxylation of the B-ring at the 3' and 5' positions (Figure 9). The level of myricetin glycosides and delphinidin-3-sambudioside was enhanced up to 3 and 5-7 fold, respectively, in red-flowered transgenic TrANR dsRNAi and TrANR-TrLAR dsRNAi lines. Enhanced accumulation of delphinidin-based ANTs could be explained by diversion of intermediates, such as delphinidins, from 2,3-flavan-3-ol to ANT production. The finding that ANT accumulation was clearly enhanced in epidermal cells of the inner whorls of immature flowers, which normally produce only PA (Figure 6K), supports a metabolic diversion model. Light-induced up-regulation of ANT biosynthesis in carpels and stamens at stages 2 and 3, when they were covered by petals and sepals, is very unlikely to have occurred. The finding that an increased level of ANT in red-flowered TrANR dsRNAi and TrANR-TrLAR dsRNAi lines is developmental^ regulated, showing the most intense coloration at stage 3 and fading later (Figure 6D,E), suggests that a temporary excess of intermediate molecules at stages 1-3, due to down-regulation of the TrANR gene, may trigger this metabolic change.
Enhanced expression of genes encoding potential glucosyltransferases, UDP- glucuronosyl/UDP-glucosyltransferases, glutathione transferases, methyltransferases and anthocyanidin rhamnosyl-transferases functioning downstream of ANS in TrANR dsRNAi lines suggests that their transcriptional regulation was triggered by a reduced level of the TrANR transcript and/or an excess of unused metabolic intermediates. Of these genes, TrUFGT4 and TrGT12 showed the highest levels of up-regulation in red- flowered TrANR dsRNAi lines (8.2- and 7.5-fold, respectively). The expression of some of these genes was not detected or not shown to vary significantly between the six developmental stages of wild-type flowers studied in the first microarray experiment (Figure 9). This subset of genes included TrGST5, TrGST6, TrGT11, TrGT12, TrGT13, TrGT , TrUFGT6, TrOMT6, TrANAT4 and TrAATL
Down-regulation of TrANR led to a 3 fold increase in the level of myricetin glycosides produced by the flavonol pathway, which branches from the PA and ANT pathways up- stream of ANR. It is difficult to explain these changes simply by metabolic spillover or diversion of delphinidin intermediates. Moreover, changes in the expression levels of most EBG, LBG and genes encoding transcription factors in TrANR dsRNAi lines, in comparison to wild-type plants, suggest that re-programming of the whole flavonoid pathway had occurred. Ectopic expression of one R2-R3 MYB transcription factor, PAP1 , in Arabidopsis resulted in an elevated level of cyanidin-type ANTs and quercetin type flavonols as well as the up-regulation of almost all genes encoding ANT biosynthetic enzymes. Down-regulation of a single gene encoding a metabolic enzyme, TrANR, also led to dramatic changes in the levels of flavonoids and changes in the expression of almost all the genes encoding enzymes known to be involved in ANT and PA biosynthesis in white clover (Figure 9). Genes up-regulated in TrANR dsRNAi lines included representatives of genes functioning upstream of TrANR in the general flavonoid pathway or in another branch, such as isoflavone biosynthesis, namely TrCHS, TrCHI, TrF3H2, TrF3'H1, TrDFRL, TrANS, TrCHR, TrlF3'H, TrIFOMT and TrVR candidate genes. However, not all of these changes in gene expression were accompanied by changes in the levels of flavonoid products. Although down-regulation of a TrF3'H gene correlated with an increase in the level of delphinidin-3-sambudioside, this was not accompanied by increased expression of TrF3'5'H, suggesting that the level of this transcript does not limit flux in the pathway producing delphinidin-based ANTs.
Some transcription factors were also up-regulated in TrANR dsRNAi lines, providing further support for the metabolic re-programming model. Six MYB genes, two MYC or bHLH genes and three WDR genes were up-regulated in flowers of TrANR dsRNAi lines in comparison to wild-type plants. TrWDR5, TrWDR6, TrMYBW TrMYB11, TrMYB9 and TrbHLH3 were up-regulated in red flowered TrANR dsRNAi lines. TrMYB12 and I WDRJ were down-regulated in these transgenic lines.
Another interesting outcome of down-regulating the TrANR gene was the differential expression of members of the same gene family. Among DFR-like genes, expression of TrDFRU (profile A) did not change, expression of TrDFRL2 (profile A), TrDFRL3 (profile B) and TrDFRL5 (neither profile) was up-regulated, and expression of TrDFR4 (profile B) was down-regulated in TrANR dsRNAi lines. Only one member of each of the white clover F3H and ANS gene families was up-regulated in TrANR dsRNAi lines. Differential expression was also detected among members of the white clover OMT, GT and WAT gene families. Two representatives of the TrIFOMTgene showed contrasting expression patterns: TrIFOMTI was down-regulated and TrlFOMT2 was up-regulated in TrANR dsRNAi lines, relative to wild-type plants.
A possible mechanism for the re-programming of the flavonoid pathway in TrANR dsRNAi lines involves changes in gene expression in response to the accumulation of intermediate molecules, such as 2,3-flavan-3,4-diols and 3-OH-anthocyanidins. Flavonoids have been implicated in direct and indirect interactions with transcription/translation machinery, trafficking, anion channels, mediators of cell signaling and cell-to-cell communication. Flavonoids are involved in polar auxin transport, responses to wounding and pathogens, interactions between plants or between plants and animals, embryonic development and seed germination. Loss of ANS/TT18/TDS4 (TANNIN DEFICIENT SEED 4) function in A. thaliana resulted in the appearance of multiple small vacuoles, suggesting that PA or intermediate accumulation is a signal for vacuolar maturation. The molecular targets of flavonoids include transcription factors, kinases, ABC transporters, hydrolases, peptidases, tyrosine phosphatases and serine/threonine kinases. Some of these proteins are transcriptionally up-regulated by a R2-R3-MYB/bHLH/WDR transcription factor complex in other species. Hence, it is interesting that candidate MYB, bHLH and WDR genes showed enhanced expression in TrANR dsRNAi lines. A number of metabolism-related transcription factors (MTFs) have been recently described. MTFs are metabolic enzymes or their homologs that use NAD, FAD and CoA as cofactors and directly link metabolism with gene regulation binding directly to DNA, or regulating gene expression by interacting with other transcription factors. Both ANR and LAR proteins require NADPH/NADH cofactors for their activities. Nuclear localization is a key requirement for regulation of transcription. Transient expression of the Z5S:.MtANR in tobacco and 35S::TrANR in Arabidopsis leaf epidermal cells demonstrated cytosolic localization. Moreover, both ANR and LAR proteins lack the known nuclear localization signals and domains involved in protein-protein interaction. Subcellular localization of these proteins in PA-producing cells could provide crucial information about their potential function as MTFs. Example 16 Metabolic Channeling
The metabolic channeling model suggests that sequential enzymes in a metabolic pathway are organised into macromolecular complexes. The movement of intermediates directly between enzymes within these structures increases catalytic efficiency by limiting their diffusion and interaction with other cell components. The channeling model also allows the possibility of combinatorial regulation, resulting in a variety of enzyme complexes producing related but distinct metabolites. The spatial and temporal profiles of PA and ANT biosynthesis in white clover epidermal cells suggests two possible channeling models: (i) the existence of independent channels producing PA and ANT; and (ii) the existence of a single core channel branching at the ANS point allowing production of PA and ANT pathways potentially competing for the anthocyanidin substrate. Spatio-temporal expression profiles of flavonoid-related genes suggest that the first model may be valid in white clover flowers. In support of this model, different representatives of the CHS, DFR, ANS, F3H, R2R3-MYB, bHLH and WDR and transporter gene families were identified in both expression profiles. In support of the second model, only one likely ANS homolog has been found in Medicago and white clover. Single homologs of the F3'H, CHI and F3'5'H genes may be also shared between the ANT and PA biosynthetic pathways. The first model suggests that the ANT and PA channels may be spatially and temporally separated. Modification of the one of the metabolic channels in this case may not necessarily affect the other pathway. The second model could function when ANT and PA channels are located in the same spatial vicinity. In this case, modification of one of the metabolic channels would re-direct the flow of intermediate molecules, resulting in quantitative changes in the final products. Results from both white clover and Arabidopsis lines lacking functional ANR provide evidence for the second model by showing that down-regulation of the ANR gene leads to enhanced ANT accumulation in tissues that normally produce PA (Figure 6). Furthermore, a reduced level of ANT in tobacco petals ectopically expressing ANR genes suggests a flexible mechanism(s) of flux diversion at the branch- point between the ANT and PA pathways, with competition between ANR and anthocyanidin glucosyltransferase enzymes for the anthocyanidin substrate. In summary, we present experimental data correlating spatio-temporal patterns of ANT and PA biosynthesis with differential expression patterns of fiavonoid-related genes in developing white clover flowers. Our findings support a model where the ANT and PA pathways are spatially co-localized within epidermal cells of petals, temporally overlap at stages 2-4 and recruit distinct isoforms of fiavonoid-related enzymes encoded by multigene families. Altered levels of flavonoid pathway products and changes in the expression of many fiavonoid-related genes provide evidence for metabolic re- programming in TrANR dsRNAi lines and the possibility of cross-talk between metabolic channels producing PAs, ANTs and flavonol glycosides. We also present the first in vivo genetic evidence that a plant LAR protein is required for the biosynthesis of 2,3- frans-flavan-3-ols. Our findings support the idea of a role for the ANR enzyme in the biosynthesis of 2,3-fraA7s-flavan-3-ols, in addition to its known function in the reduction of anthocyanidins to 2,3-c/s-flavan-3-ols. Our work will facilitate genetic modification of the flavonoid pathway to increase PA levels in herbage for enhancing bloat safety in key forage legumes, such as alfalfa and white clover.
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Claims

The claims defining the invention are as follows:
1. A method of identifying a gene encoding a polypeptide or polypeptide isoform which is substantially more active in either a proanthocyanidin (PA) or anthocyanin (ANT) pathway of a plant, said method including
providing
material from said plant; and
an oligonucleotide probe capable of hybridizing with RNA from a gene encoding a polypeptide which is active in a flavonoid biosynthetic pathway;
extracting RNA from said plant material;
hybridizing the oligonucleotide probe with the RNA to generate an expression profile;
measuring PA and/or ANT levels in said plant material to generate a metabolic profile;
comparing said expression profile with said metabolite profile to identify said gene encoding a polypeptide or polypeptide isoform which is substantially active in either a PA or ANT pathway.
2. A method according to claim 1 wherein the polypeptide or polypeptide isoform is active late in the ANT pathway.
3. A method according to claim 2 wherein said polypeptide or polypeptide isoform is selected from the group consisting of GST, G3T, UFGT, OMT, ART, ANAT and AAT.
4. A method according to claim 1 wherein the polypeptide or polypeptide isoform is a transcription factor.
5. A method according to claim 4, wherein said polypeptide or polypeptide isoform is selected from the group consisting of MYB, bHLH, MYC and WDR.
6. A method of manipulating the flavonoid biosynthetic pathway in a plant, said method including identifying a gene encoding a polypeptide or polypeptide isoform which is substantially more active in either a PA or ANT pathway of said plant and up- or down-regulating expression of said gene to increase or decrease the level of PA or ANT in said plant.
7. A method according to claim 6 wherein said method includes down-regulating expression of a gene encoding a polypeptide or polypeptide isoform which is active late in the ANT pathway.
8. A method according to claim 6 wherein said method includes up- and/or down- regulating expression of one or more genes encoding a transcription factor.
9. A method of enhancing bloat safety of a plant, said method including
identifying a gene encoding a polypeptide or polypeptide isoform which is substantially more active in a PA pathway and up-regulating or down-regulating expression of said gene to increase the level of PA in said plant; or
identifying a gene encoding a polypeptide or polypeptide isoform which is substantially more active in an ANT pathway and up-regulating or down-regulating expression of said gene to increase the level of PA in said plant.
10. A method according to claim 9 wherein said method includes down-regulating expression of a gene encoding a polypeptide or polypeptide isoform which is active late in the ANT pathway.
11. A method according to claim 9 wherein said method includes up- and/or down- regulating expression of one or more genes encoding a transcription factor.
12. A genetic construct capable of manipulating the flavonoid biosynthetic pathway in a plant, said genetic construct including a gene encoding a polypeptide or polypeptide isoform which is substantially more active in either a PA or ANT pathway of said plant, or a modified form of said gene.
13. A genetic construct according to claim 12 wherein said gene encodes a polypeptide or polypeptide isoform which is active late in the ANT pathway.
14. A genetic construct according to claim 12, wherein said gene encodes a transcription factor.
15. A transgenic plant cell, plant, plant seed or other plant part with modified flavonoid biosynthetic characteristics relative to an untransformed control plant; said plant cell, plant, plant seed or other plant part including a genetic construct according to claim 12.
16. A transgenic plant, plant seed or other plant part derived from a plant cell according to claim 15 and including a genetic construct according to claim 12.
17. A transgenic plant, plant seed or other plant part derived from a plant according to claim 15 and including a genetic construct according to claim 12.
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KR101680570B1 (en) 2015-02-27 2016-11-29 충남대학교산학협력단 Single nucleotide polymorphism marker for discerning purple cabbage cultivar and uses thereof
CN107201378A (en) * 2016-03-17 2017-09-26 刘海亮 Cotton fiber Color Related Gene and its application in regulating cotton color
WO2018035115A1 (en) * 2016-08-16 2018-02-22 University Of North Texas Methods for regulating extractable proanthocyanidins (pas) in plants by affecting leucoanthocyanidin reductase (lar)
KR20190048451A (en) * 2017-10-31 2019-05-09 주식회사 씨더스 농업회사법인 Molecular marker for discriminating purple color of Perilla leaf and uses thereof
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CN113512553A (en) * 2021-03-19 2021-10-19 河南科技大学 Potato TF72354 gene and application thereof in anthocyanin synthesis regulation
CN113512553B (en) * 2021-03-19 2022-09-20 河南科技大学 Potato TF72354 gene and application thereof in anthocyanin synthesis regulation

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EP2488010B1 (en) 2017-12-06
CA2777249A1 (en) 2011-04-21
AU2010306410A1 (en) 2012-05-03
US20120204289A1 (en) 2012-08-09
EP2488010A4 (en) 2014-01-29
DK2488010T3 (en) 2018-03-05
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CA2777249C (en) 2021-03-09
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