cDNA cloning and characterization of chalcone isomerase-fold proteins from snapdragon (Antirrhinum majus L.) flowers

Fujino, Naoto; Yamazaki, Tatsuya; Li, Yanbing; Kera, Kota; Furuhashi, Erika; Yamashita, Satoshi; Morita, Yasumasa; Nakayama, Masayoshi; Takahashi, Shigetoshi; Nakayama, Tôru

doi:10.5511/plantbiotechnology.14.0109c

Cited by 10 publications

(9 citation statements)

References 26 publications

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“…Thus, a split‐ubiquitin (SU) system (Iyer et al ., ) was used to screen for interactions between these P450 proteins and other soluble flavonoid enzymes in snapdragon [i.e. CHS (AmCHS1 or Nivea) (Hatayama et al ., ); CHI (AmCHI1) (Fujino et al ., ); F3H (AmF3H or Incolorata); DFR (AmDFR or Pallida); and C4′GT (AmC4′GT) (Ono et al ., ); Figures and S1]. Because the coding sequence of the snapdragon anthocyanidin synthase gene ( ANS ) was not available in databases, ANS was not included in these interaction assays.…”

Section: Resultsmentioning

confidence: 99%

“…Binary interactions among torenia flavonoid enzymes [i.e. CHS, two isozymes of type‐1 CHI (CHI1_1 and CHI1_2; Fujino et al ., ), FNSII (Akashi et al ., ; Ueyama et al ., ), F3H, DFR, ANS, F3′H (Ueyama et al ., ) and F3′5′H] were comprehensively analyzed using the SU and Y2H systems (Figures and S6). The analyses of yeast growth and β‐galactosidase activity in the SU system (Figure ) revealed FNSII interacted with CHI1_1, CHI1_2, F3H and DFR (Figure a).…”

Section: Resultsmentioning

confidence: 99%

“…The complete open reading frames encoding the following flavonoid enzymes (DDBJ/ENA/GenBank accession numbers in parentheses) were cloned into the pGEM‐T Easy vector (Promega, Madison, WI, USA), and the nucleotide sequence of the inserted DNA was confirmed by sequencing: AmCHS1 (X03710) (Hatayama et al ., ), AmCHI1 (AB861648) (Fujino et al ., ), AmFNSII (AB028151) (Akashi et al ., ), AmF3H (LC194907), AmDFR (P14721) (Beld et al ., ), AmC4′GT (AB198665) (Ono et al ., ), AmAS1 (AB044884) (Nakayama et al ., ), AmF3 ′ H (DQ272592) (Schwinn et al ., ), ThCHS1 (AB106522) (Fukusaki et al ., ), ThCHI1_1 (LC194908), ThCHI1_2 (LC194909), ThFNSII (AB028152) (Akashi et al ., ), ThF3H (AB211958), ThDFR (AB012924) (Suzuki et al ., ), ThANS (identical to Torenia fournieri ANS; AB044091) (Nakamura et al ., ), THF3 ′ H (AB057672) (Ueyama et al ., ) and ThF3′5′H (AB012925) (Suzuki et al ., ). The AmF3H and AmDFR cDNAs were kindly provided by Dr Yuji Kishima, Hokkaido University.…”

Section: Methodsmentioning

confidence: 99%

“…To obtain anti‐AmCHS1 and anti‐AmCHI1 antibodies, electrophoretically homogeneous preparations of the non‐denatured forms of recombinant AmCHS1 (Hatayama et al ., ) and AmCHI1 (Fujino et al ., ) were used to immunize female Japanese white rabbits by an intradermal injection at multiple sites according to standard protocols (Vaitukaitis, ). To obtain anti‐AmFNSII and anti‐DFR antibodies, the peptides corresponding to amino acid residues 469–487 of AmFNS and residues 334–352 of AmDFR, which were predicted to serve as epitopes, were used to immunize female Japanese white rabbits.…”

Section: Methodsmentioning

confidence: 99%

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Physical interactions among flavonoid enzymes in snapdragon and torenia reveal the diversity in the flavonoid metabolon organization of different plant species

et al. 2018

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Flavonoid metabolons (weakly-bound multi-enzyme complexes of flavonoid enzymes) are believed to occur in diverse plant species. However, how flavonoid enzymes are organized to form a metabolon is unknown for most plant species. We analyzed the physical interaction partnerships of the flavonoid enzymes from two lamiales plants (snapdragon and torenia) that produce flavones and anthocyanins. In snapdragon, protein-protein interaction assays using yeast and plant systems revealed the following binary interactions: flavone synthase II (FNSII)/chalcone synthase (CHS); FNSII/chalcone isomerase (CHI); FNSII/dihydroflavonol 4-reductase (DFR); CHS/CHI; CHI/DFR; and flavonoid 3'-hydroxylase/CHI. These results along with the subcellular localizations and membrane associations of snapdragon flavonoid enzymes suggested that FNSII serves as a component of the flavonoid metabolon tethered to the endoplasmic reticulum (ER). The observed interaction partnerships and temporal gene expression patterns of flavonoid enzymes in red snapdragon petal cells suggested the flower stage-dependent formation of the flavonoid metabolon, which accounted for the sequential flavone and anthocyanin accumulation patterns therein. We also identified interactions between FNSII and other flavonoid enzymes in torenia, in which the co-suppression of FNSII expression was previously reported to diminish petal anthocyanin contents. The observed physical interactions among flavonoid enzymes of these plant species provided further evidence supporting the long-suspected organization of flavonoid metabolons as enzyme complexes tethered to the ER via cytochrome P450, and illustrated how flavonoid metabolons mediate flower coloration. Moreover, the observed interaction partnerships were distinct from those previously identified in other plant species (Arabidopsis thaliana and soybean), suggesting that the organization of flavonoid metabolons may differ among plant species.

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Section: Resultsmentioning

confidence: 99%

Section: Resultsmentioning

confidence: 99%

Section: Methodsmentioning

confidence: 99%

Section: Methodsmentioning

confidence: 99%

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Physical interactions among flavonoid enzymes in snapdragon and torenia reveal the diversity in the flavonoid metabolon organization of different plant species

et al. 2018

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“…As the authors suggested, it could be related to the role of flavonoids in nodule development, as signal molecules during interactions with rhizobia. Recently, it was concluded that CHILs are enhancers of flavonoid production and flower pigmentation, and their function is conserved among diverse land plant species (Fujino et al, 2014 ; Morita et al, 2014 ).…”

Section: Discussionmentioning

confidence: 99%

Structure, expression profile and phylogenetic inference of chalcone isomerase-like genes from the narrow-leafed lupin (Lupinus angustifolius L.) genome

et al. 2015

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Lupins, like other legumes, have a unique biosynthesis scheme of 5-deoxy-type flavonoids and isoflavonoids. A key enzyme in this pathway is chalcone isomerase (CHI), a member of CHI-fold protein family, encompassing subfamilies of CHI1, CHI2, CHI-like (CHIL), and fatty acid-binding (FAP) proteins. Here, two Lupinus angustifolius (narrow-leafed lupin) CHILs, LangCHIL1 and LangCHIL2, were identified and characterized using DNA fingerprinting, cytogenetic and linkage mapping, sequencing and expression profiling. Clones carrying CHIL sequences were assembled into two contigs. Full gene sequences were obtained from these contigs, and mapped in two L. angustifolius linkage groups by gene-specific markers. Bacterial artificial chromosome fluorescence in situ hybridization approach confirmed the localization of two LangCHIL genes in distinct chromosomes. The expression profiles of both LangCHIL isoforms were very similar. The highest level of transcription was in the roots of the third week of plant growth; thereafter, expression declined. The expression of both LangCHIL genes in leaves and stems was similar and low. Comparative mapping to reference legume genome sequences revealed strong syntenic links; however, LangCHIL2 contig had a much more conserved structure than LangCHIL1. LangCHIL2 is assumed to be an ancestor gene, whereas LangCHIL1 probably appeared as a result of duplication. As both copies are transcriptionally active, questions arise concerning their hypothetical functional divergence. Screening of the narrow-leafed lupin genome and transcriptome with CHI-fold protein sequences, followed by Bayesian inference of phylogeny and cross-genera synteny survey, identified representatives of all but one (CHI1) main subfamilies. They are as follows: two copies of CHI2, FAPa2 and CHIL, and single copies of FAPb and FAPa1. Duplicated genes are remnants of whole genome duplication which is assumed to have occurred after the divergence of Lupinus, Arachis, and Glycine.

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Managing enzyme promiscuity in plant specialized metabolism: A lesson from flavonoid biosynthesis

2020

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Specificities of enzymes involved in plant specialized metabolism, including flavonoid biosynthesis, are generally promiscuous. This enzyme promiscuity has served as an evolutionary basis for new enzyme functions and metabolic pathways in land plants adapting to environmental challenges. This phenomenon may lead, however, to inefficiency in specialized metabolism and adversely affect metabolite‐mediated plant survival. How plants manage enzyme promiscuity for efficient specialized metabolism is, thus, an open question. Recent studies of flavonoid biosynthesis addressing this issue have revealed a conserved strategy, namely, a homolog of chalcone isomerase with no catalytic activity binds to chalcone synthase, a key flavonoid pathway enzyme, to narrow (or rectify) the enzyme's highly promiscuous product specificity. Reducing promiscuity via specific protein–protein interactions among metabolic enzymes and proteins may be a solution adopted by land plants to achieve efficient operation of specialized metabolism, while the intrinsic promiscuity of enzymes has likely been retained incidentally.

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cDNA cloning and characterization of chalcone isomerase-fold proteins from snapdragon (Antirrhinum majus L.) flowers

Cited by 10 publications

References 26 publications

Physical interactions among flavonoid enzymes in snapdragon and torenia reveal the diversity in the flavonoid metabolon organization of different plant species

Physical interactions among flavonoid enzymes in snapdragon and torenia reveal the diversity in the flavonoid metabolon organization of different plant species

Structure, expression profile and phylogenetic inference of chalcone isomerase-like genes from the narrow-leafed lupin (Lupinus angustifolius L.) genome

Managing enzyme promiscuity in plant specialized metabolism: A lesson from flavonoid biosynthesis

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