A Molecular Blueprint of Lignin Repression
TL;DR: This work provides a comprehensive overview of the molecular factors that negatively impact on the lignification process at both the transcriptional and post-transcriptional levels.
About: This article is published in Trends in Plant Science.The article was published on 2019-11-01 and is currently open access. It has received 20 citations till now. The article focuses on the topics: Lignocellulosic biomass.
Summary (3 min read)
Jump to: [Review] – [Transcriptional Repression of Lignin Biosynthesis] – [NAC TFs, the Two Sides of SCW Regulation] – [Key Figure] – [R2R3 MYBs, the Gatekeepers of SCW Formation and Lignification] – [KNOX, BELL, and Homeodomain: from Cell Division to Fiber SCW Thickening] – [Mediator, a Molecular Hub Coordinating Lignin Biosynthesis with Plant Growth] – [Post-Transcriptional Repression of Monolignol Biosynthesis and Lignin Polymerization] – [Non-Coding RNAs, Emerging Regulators for Genetic Control of Lignin Deposition] – [Protein Ubiquitination: the Signaling Wave to the Grave] – [Switching On/Off Enzymatic Activity with Phosphorylation] – [Concluding Remarks and Future Perspectives] and [Acknowledgments]
Review
- The Mediator complex adds another level of transcription regulation to the several transcription factors that are known to repress.
- The need to tailor the lignocellulosic biomass for more efficient biofuel production or for improved plant digestibility has fostered considerable advances in their understanding of the lignin biosynthetic pathway and its regulation.
- The authors provide a comprehensive overview of the molecular factors that negatively impact on the lignification process at both the transcriptional and post-transcriptional levels.
- Understanding the interactions between genes, non-coding RNAs, and proteins opens new avenues towards understanding secondary cell wall formation.
Transcriptional Repression of Lignin Biosynthesis
- Negative regulation of lignin biosynthesis is achieved through diverse mechanisms ranging from DNA accessibility to targeted proteolysis.
- The process, the timing, and the location of differentiation are under stringent genetic regulation.
- Usually TFs, also known as Heterodimer.
- An RNA that is not translated into protein, also known as Non-coding RNA.
NAC TFs, the Two Sides of SCW Regulation
- Members of the NAC family act as first- and second-level master switches in the regulation of a battery of downstream TFs and SCW biosynthetic genes [15–18].
- VND-INTERACTING 2 (VNI2) is a transcriptional repressor reported to regulate the timing and spatial regulation of xylem cell development [21].
- The SCW activator NST2 is negatively transcriptionally regulated by WRKY12 , which binds to the W-box cis-element in theNST2 promoter region (Table 1) [25].
- An intron-retained (IR) splice variant PtrVND6C1IR negatively regulates the expression of PtrMYB021 (a poplar ortholog of AtMYB46) by forming heterodimers with the full-size PtrVND6s, suppressing their positive transcriptional activity .
- In addition, PtrVND6-C1IR downregulates the expression of five full-size PtrVND6s.
Key Figure
- PtrhAT PtrMYB021 Transcriptional complex LAC AtVNDs AtVND7 AtVNI2 AtXND1 Active PtrAldOMT2 P Ser 123 Ser125 Inactive PtrAldOMT2 LTF1 Phosphorylated LTF1 U EgH1.3 TrendsinPlantScience.
- In this review the authors describe alternatively spliced proteins regulating the expression of closely related coding genes.
R2R3 MYBs, the Gatekeepers of SCW Formation and Lignification
- Some members of the R2R3-MYB TF family positively regulate gene expression of phenylpropanoid and lignin biosynthetic genes containing AC-rich cis-elements in their promoters [30], such as the 7 bp sequence ACC(A/T)A(A/C)(T/C), termed the secondary wall MYB-responsive element (SMRE) [31,32].
- The importance of MYBs as repressors of phenylpropanoid metabolism has been highlighted in a recent review [33].
- AtMYB4 belongs to subgroup 4 and, as the other proteins from this subgroup (AtMYB3, AtMYB7, and AtMYB32), contains an EARlike repression motif in its C-terminus [36].
- AtMYB4 is downregulated in thale cress ectopic lignification de-etiolated 3, pom-pom 1, and ectopic lignification 1 mutants [38], suggesting that it could negatively regulate lignin biosynthesis.
- Notably, PtrEPSP-TF harbors an additional N-terminal HTH DNA-binding motif that partially targets this protein to the nucleus, where it acts as a transcriptional repressor of its direct target PtrhAT, a hAT transposase family gene.
KNOX, BELL, and Homeodomain: from Cell Division to Fiber SCW Thickening
- Some members of the THREE AMINO ACID LOOP EXTENSION (TALE) family of homeodomain (HD) proteins may play a role in the repression of lignin biosynthesis .
- The cooperative heterodimer becomes completely contained in the nucleus, and the expression of the target genes is dramatically reduced relative to individual BELL or KNOX proteins [22,71].
- The heterodimer KNAT7–BLH6 negatively regulates the commitment to SCW formation in interfascicular fibers of thale cress through repression of REVOLUTA , which encodes a HD-leucine zipper TF binding to the sequence GTAATNATTAC [65,72].
- Indeed, the athb15 mutant showed increased xylan and lignin contents in the pith as well as higher expression of SCW genes [81].
- Of note, KNOX are also part of the transcriptional network regulating the formation of tension wood in poplar [85] that is characterized by the presence of a thick, weakly lignified, cellulose-rich gelatinous layer.
Mediator, a Molecular Hub Coordinating Lignin Biosynthesis with Plant Growth
- The ’mediator of RNA polymerase II transcription’, or Mediator complex (MED), is essential to transduce signals (both positively and negatively regulating gene expression) to the transcription machinery via direct interactions with specific TFs [86].
- Among the 27 MED subunits identified in thale cress [87], several negatively regulate the phenylpropanoid and monolignol biosynthetic pathways, contributing to the homeostasis of this family of secondary metabolites.
- The lignin monomeric composition is drastically modified in the triple mutant, consisting almost exclusively of H-lignin subunits (95% vs <2% in the wild type), suggesting that MED5a and MED5b are likely to have other functions [90].
- Dolan and colleagues [91] have also demonstrated that the MED5b phenotype requires functional MED2, MED16, and MED23, which probably physically and functionally interact with MED5, as do their homologs in humans [92].
Post-Transcriptional Repression of Monolignol Biosynthesis and Lignin Polymerization
- In addition to the numerous mechanisms of transcriptional regulation that land plants have established to repress monolignol biosynthesis and hence lignification in different tissues and developmental stages, additional post-transcriptional mechanisms have been observed.
- Post-transcriptional modifications typically affect a restricted number of transcripts/proteins, allowing precise control of the output of a metabolic pathway such as lignin biosynthesis.
Non-Coding RNAs, Emerging Regulators for Genetic Control of Lignin Deposition
- MicroRNAs are small non-coding RNAs that post-transcriptionally regulate many aspects of plant development.
- Their expression is developmentally regulated and/or under the control of external stimuli such as abiotic stress or nutrient availability [93,94].
- Overexpression of ptr-miR397a significantly reduces the expression of 17 of the 34 LAC found in poplar differentiating xylem, the global LAC activity of this tissue, and the lignin content of the whole plant [26].
- Similarly, 18 conserved miRNAs targeting 80 genes were found in hemp, where they may have similar functions to flax miRNAs [98].
- These lncRNAs may be directly functional or serve as precursors for miRNA sequences such asmiR397 [101], and provide a further level of complexity in the regulation of lignin biosynthesis.
Protein Ubiquitination: the Signaling Wave to the Grave
- PAL catalyzes the rate-limiting step of the phenylpropanoid pathway and thus constitutes an ideal target for regulating the flux of derived secondary metabolites.
- Thale cress KFB01, KFB20, KFB39, and KFB50 physically interact with the four PAL isozymes, thereby regulating the biosynthesis of phenylpropanoids during plant development and in response to environmental stimuli [27,103].
- The hemp ortholog of KFB39 is upregulated in mature bast fibers, suggesting a role for KFBs in the hypolignification of this cell type [83].
Switching On/Off Enzymatic Activity with Phosphorylation
- Phosphorylation is a widespread post-translational modification which may impact on the lignification process.
- Monophosphorylation of PtrAldOMT2 (that catalyzes the methylation of 5-hydroxyconiferaldehyde to sinapaldehyde) at either Ser123 or Ser125 inhibits its activity [105], in line with the observation that the pool of monolignol biosynthetic enzymes is usually not phosphorylated in vivo [106].
- The biological significance of this switch remains unknown.
- Alternatively, phosphorylation may also constitute a signal for protein degradation through proteasome activity.
- By screening TFs binding to the poplar 4CL promoter, Gui and colleagues identified a lignin biosynthesis-associated factor, LTF1, that represses several genes from this pathway (PAL2, C4H1, C3H2, 4CL1, CAld5H, COMT2, and CCoAOMT1) and decreases lignin content in overexpressing lines [107].
Concluding Remarks and Future Perspectives
- Further advances in synthetic and molecular biology combine with their growing knowledge about the molecular factors (mainly genes and proteins) driving SCW formation in various tissues and plant species to overcome the possible growth penalty of constitutive overexpression of genes repressing lignification (see Outstanding Questions).
- Similarly, the dwarf thale cress ccr1 mutant was rescued by driving the expression of CCR1 in metaxylem and protoxylem vessels through a proSNBE promoter transcriptionally activated by VND6 and VND7 [109].
- Targeted lignin biosynthesis repression may thus be achieved through temporal and/or spatial restriction of the activity of a selected gene using suitable promoters.
- Omics-based predictive analysis of variables determining wood quality following targeted gene downregulation [110] constitutes a valuable tool to optimize strategies.
- DNA methylation contributes to the regulation of cotton fiber development and can modulate the production of reactive oxygen species or the biosynthesis of lipids, flavonoids, and ascorbate [111].
Acknowledgments
- G. Guerriero acknowledges support from the Fonds National de la Recherche, Luxembourg (grant number C16/SR/ 11289002).
- J. Grima-Pettenati acknowledges support from the CNRS, the Université Paul Sabatier Toulouse III, and the Laboratoire d’Excellence TULIP (ANR-10-LABX-41; ANR-11- IDEX0002-02).
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Figures (3)
![Figure 2. PAL as a Case Study ofMultipleMechanisms Regulating Gene Expression and Protein Abundance. (A) PAL is directly repressed through binding of various TALE family transcription factors (TFs; e.g., BREVIPEDICELLUS) to the DNA knotted 1 (KN-1) motif, as well as by binding of subgroup 4 R2R3 MYBs (e.g., MYB4) to the AATAGTT motif. (B) PAL is indirectly regulated through BLH6–KNAT7-mediated repression of the HD-Zip III TF REVOLUTA. HB15 represses the expression of the master switches SND1 and NST2, which are activators of PAL expression. (C) Kelch F-box proteins ubiquitinate PAL to target it to the 26S proteasome for proteolysis. Other PAL regulatory pathways, including metabolic feedback repression (caffeic acid, cinnamic acid), environmental factors, and physical interactions with other phenylpropanoid enzymes (C4H) are beyond the scope of this figure but are reviewed in [44]. Abbreviations: BLH, BEL1-like homeodomain; HB, homeobox; KFB, kelch F-box; KNAT, knotted1-like TALE homeodomain; NST, NAC secondary wall thickening promoting factor; PAL, phenylalanine ammonia lyase; SND, secondary wall-associated NAC domain protein; Ub ubiquitin. This figure was created using BioRender (https://biorender.com/).](/figures/figure-2-pal-as-a-case-study-ofmultiplemechanisms-regulating-3c38lurv.png)
Figure 2. PAL as a Case Study ofMultipleMechanisms Regulating Gene Expression and Protein Abundance. (A) PAL is directly repressed through binding of various TALE family transcription factors (TFs; e.g., BREVIPEDICELLUS) to the DNA knotted 1 (KN-1) motif, as well as by binding of subgroup 4 R2R3 MYBs (e.g., MYB4) to the AATAGTT motif. (B) PAL is indirectly regulated through BLH6–KNAT7-mediated repression of the HD-Zip III TF REVOLUTA. HB15 represses the expression of the master switches SND1 and NST2, which are activators of PAL expression. (C) Kelch F-box proteins ubiquitinate PAL to target it to the 26S proteasome for proteolysis. Other PAL regulatory pathways, including metabolic feedback repression (caffeic acid, cinnamic acid), environmental factors, and physical interactions with other phenylpropanoid enzymes (C4H) are beyond the scope of this figure but are reviewed in [44]. Abbreviations: BLH, BEL1-like homeodomain; HB, homeobox; KFB, kelch F-box; KNAT, knotted1-like TALE homeodomain; NST, NAC secondary wall thickening promoting factor; PAL, phenylalanine ammonia lyase; SND, secondary wall-associated NAC domain protein; Ub ubiquitin. This figure was created using BioRender (https://biorender.com/). 
Table 1. Binding Sites of Proteins Involved in the Repression of Monolignol Biosynthesis 
Figure 1. The repressive activity of EgMYB1 increases when it is associated with EgH1.3. Some factors are devoted to specifically preventing monolignol biosynthesis (blue boxes), whereas others repress secondary cell wall (SCW) formation more widely (violet boxes). Proteins repressing SCW formation are essentially involved in the spatiotemporal regulation of specific tissue development, such as preventing SCW deposition in pith (AtWRKY12, AtHB15) or restricting the timing and localization of xylem cell development (AtVNI2). Abbreviations: 4CL, 4-coumarate-CoA ligase; AldOMT, 5-hydroxyconiferaldehyde O-methyltransferase; ARK, arborknox; BLH, BEL1-like homeodomain; BP, brevipedicellus; C4H, cinnamate-4-hydroxylase; DRIF, divaricata and radialis interacting factor; H1.3, linker histone variant; hAT, hobo activator Tam3 transposase; HB, homeobox; KFB Kelch F-box; KNAT, knotted1-like TALE homeodomain; LAC, laccase; LTF, lignin biosynthesisassociated transcription factor; MED, Mediator; NST, NAC secondary wall thickening promoting factor; OFP, ovate family protein; P, phosphorylation; PAL, phenylalanine ammonia lyase; PCN, popcorona; SND, secondary wall-associated NAC domain protein; U, ubiquitin; VND vascular-related NAC domain; VNI, VND interacting; XND, xylem NAC domain. This figure was created using BioRender (https://biorender.com/).
![Figure 2. PAL as a Case Study ofMultipleMechanisms Regulating Gene Expression and Protein Abundance. (A) PAL is directly repressed through binding of various TALE family transcription factors (TFs; e.g., BREVIPEDICELLUS) to the DNA knotted 1 (KN-1) motif, as well as by binding of subgroup 4 R2R3 MYBs (e.g., MYB4) to the AATAGTT motif. (B) PAL is indirectly regulated through BLH6–KNAT7-mediated repression of the HD-Zip III TF REVOLUTA. HB15 represses the expression of the master switches SND1 and NST2, which are activators of PAL expression. (C) Kelch F-box proteins ubiquitinate PAL to target it to the 26S proteasome for proteolysis. Other PAL regulatory pathways, including metabolic feedback repression (caffeic acid, cinnamic acid), environmental factors, and physical interactions with other phenylpropanoid enzymes (C4H) are beyond the scope of this figure but are reviewed in [44]. Abbreviations: BLH, BEL1-like homeodomain; HB, homeobox; KFB, kelch F-box; KNAT, knotted1-like TALE homeodomain; NST, NAC secondary wall thickening promoting factor; PAL, phenylalanine ammonia lyase; SND, secondary wall-associated NAC domain protein; Ub ubiquitin. This figure was created using BioRender (https://biorender.com/).](/figures/figure-2-pal-as-a-case-study-ofmultiplemechanisms-regulating-3c38lurv.webp)
Citations
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References
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TL;DR: It is shown that a laccase gene, LAC4, regulated by a microRNA, miR397b, controls both lignin biosynthesis and seed yield in Arabidopsis.
Abstract: Plant laccase (LAC) enzymes belong to the blue copper oxidase family and polymerize monolignols into lignin. Recent studies have established the involvement of microRNAs in this process; however, physiological functions and regulation of plant laccases remain poorly understood. Here, we show that a laccase gene, LAC4, regulated by a microRNA, miR397b, controls both lignin biosynthesis and seed yield in Arabidopsis. In transgenic plants, overexpression of miR397b (OXmiR397b) reduced lignin deposition. The secondary wall thickness of vessels and the fibres was reduced in the OXmiR397b line, and both syringyl and guaiacyl subunits are decreased, leading to weakening of vascular tissues. In contrast, overexpression of miR397b-resistant laccase mRNA results in an opposite phenotype. Plants overexpressing miR397b develop more than two inflorescence shoots and have an increased silique number and silique length, resulting in higher seed numbers. In addition, enlarged seeds and more seeds are formed in these miR397b overexpression plants. The study suggests that miR397-mediated development via regulating laccase genes might be a common mechanism in flowering plants and that the modulation of laccase by miR397 may be potential for engineering plant biomass production with less lignin.
159 citations
"A Molecular Blueprint of Lignin Rep..." refers background in this paper
...been described in thale cress, wheremiRNA857 andmiRNA397bmodulate the abundance ofAtLAC7 and AtLAC4 transcripts, respectively [94,99]....
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01 Jan 2012
TL;DR: This work has shown that cell wall-related NAC and MYB transcription factors have been intensively investigated in different species and shown to be master switches of secondary cell wall biosynthesis, and negative regulators, which function upstream of NAC master switches, have also been identified in different plant tissues.
Abstract: 第二等的房间墙向植物提供刚硬和力量支持他们的身体重量并且保证水和滋养的运输。他们也为人的使用提供纺织品,木材,和潜在地第二代的 biofuels。为不同房间的合成负责的基因围部件,也就是纤维素, hemicelluloses,和木质素,并列地被表示并且在 transcriptional 下面规定。在过去的几年里,房间墙相关的 NAC 和 MYB 抄写因素强烈地在不同种类被调查了并且出现是第二等的房间墙生合成的主人开关。积极、否定的管理者, NAC 主人在上游的功能交换,也在不同植物纸巾被识别了。房间墙合成的规章的机制的进一步的说明将便于对 biofuel 生产合适的植物化工物品的工程。
159 citations
TL;DR: It is reported that the Arabidopsis thaliana mutant sensitive to ABA and drought2 (sad2), which harbors a T-DNA insertion in an importin β-like gene, is more tolerant to UV-B radiation than the wild type.
Abstract: We report that the Arabidopsis thaliana mutant sensitive to ABA and drought2 (sad2), which harbors a T-DNA insertion in an importin β-like gene, is more tolerant to UV-B radiation than the wild type. Analysis of cyclobutane pyrimidine dimer accumulation revealed that less DNA damage occurred in sad2 than in the wild type during UV-B treatment. No significant growth difference was observed between sad2 and the wild type when treated with the genotoxic drug methyl methanesulfonate, suggesting that SAD2 functions in UV-B protection rather than in DNA damage repair. Whereas the R2R3-type transcription repressor MYB4 has previously been shown to negatively regulate the transcription of cinnamate 4-hydroxylase (C4H) and thus to regulate the synthesis of sinapate esters, expression of both MYB4 and C4H and accumulation of UV-absorbing compounds were significantly higher in sad2 than in the wild type. MYB4 did not localize to the nucleus in the sad2 mutant, suggesting that SAD2 is required for MYB4 nuclear trafficking. SAD2 and MYB4 coimmunoprecipitated, indicating that these proteins localize in the same complex in vivo. MYB4 protein specifically bound to its own promoter in gel shift assays and repressed its own expression, demonstrating that MYB4 protein and mRNA are part of a negative autoregulatory loop. This feedback loop is altered in the sad2 mutant due to the absence of MYB4 protein in the nucleus, leading to the constitutive expression of MYB4 and C4H and resulting in accumulation of UV-absorbing pigments that shield the plant from UV-B radiation.
157 citations
TL;DR: It is proposed that KNAT7 forms a functional complex with OFP proteins to regulate aspects of secondary cell wall formation and both OFP1 and OFP4 enhance KNat7's transcriptional repression activity.
Abstract: The homeodomain transcription factor KNAT7 has been reported to be involved in the regulation of secondary cell wall biosynthesis. Previous work suggested that KNAT7 can interact with members of the Ovate Family Protein (OFP) transcription co-regulators. However, it remains unknown whether such an OFP-KNAT7 complex could be involved in the regulation of secondary cell wall biosynthesis in Arabidopsis. We re-tested OFP1 and OFP4 for their abilities to intact with KNAT7 using yeast two-hybrid assays, and verified KNAT7-OFP4 interaction but found only weak interaction between KNAT7 and OFP1. Further, the interaction of KNAT7 with OFP4 appears to be mediated by the KNAT7 homeodomain. We used bimolecular fluorescence complementation to confirm interactions and found that OFP1 and OFP4 both interact with KNAT7 in planta. Using a protoplast transient expression system we showed that KNAT7 as well as OFP1 and OFP4 act as transcriptional repressors. Furthermore, in planta interactions between KNAT7 and both OFP1 and OFP4 enhance KNAT7's transcriptional repression activity. An ofp4 mutant exhibited similar irx and fiber cell wall phenotypes as knat7, and the phenotype of a double ofp4 knat7mutant was similar to those of the single mutants, consistent with the view that KNAT7 and OFP function in a common pathway or complex. Furthermore, the pleiotropic OFP1 and OFP4 overexpression phenotype was suppressed in a knat7 mutant background, suggesting that OFP1 and OFP4 functions depend at least partially on KNAT7 function. We propose that KNAT7 forms a functional complex with OFP proteins to regulate aspects of secondary cell wall formation.
149 citations
"A Molecular Blueprint of Lignin Rep..." refers background in this paper
...The transcriptional repression by KNAT7 and BLH6 is enhanced by their interaction with other TFs, including OVATE FAMILY PROTEIN (OFP) 1 and 4, during SCW biosynthesis [74,75]....
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TL;DR: It is shown that initiation and maintenance of the Arabidopsis SAM, including that of floral meristems, requires the combinatorial action of three members of the BELL-family of TALE homeodomain proteins, ARABIDOPSIS THALIANA HOMEOBOX 1 (ATH1), PENNYWISE (PNY) and POUND-FOOLISH (PNF).
Abstract: In plants, most of the above-ground body is formed post-embryonically by the continuous organogenic potential of the shoot apical meristem (SAM). Proper function of the SAM requires maintenance of a delicate balance between the depletion of stem cell daughters into developing primordia and proliferation of the central stem cell population. Here we show that initiation and maintenance of the Arabidopsis SAM, including that of floral meristems, requires the combinatorial action of three members of the BELL-family of TALE homeodomain proteins, ARABIDOPSIS THALIANA HOMEOBOX 1 (ATH1), PENNYWISE (PNY) and POUND-FOOLISH (PNF). All three proteins interact with the KNOX TALE homeodomain protein STM, and combined lesions in ATH1, PNY and PNF result in a phenocopy of stm mutations. Therefore, we propose that ath1 pny pnf meristem defects result from loss of combinatorial BELL-STM control. Further, we demonstrate that heterodimerization-controlled cellular localization of BELL and KNOX proteins involves a CRM1/exportin-1-mediated nuclear exclusion mechanism that is probably generic to control the activity of BELL and KNOX combinations. We conclude that in animals and plants corresponding mechanisms regulate the activity of TALE homeodomain proteins through controlled nuclear-cytosolic distribution of these proteins.
146 citations
"A Molecular Blueprint of Lignin Rep..." refers background in this paper
...The cooperative heterodimer becomes completely contained in the nucleus, and the expression of the target genes is dramatically reduced relative to individual BELL or KNOX proteins [22,71]....
[...]