Figures and data in Perception of a conserved family of plant signalling peptides by the receptor kinase HSL3

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4 figures, 1 table and 21 additional files

Figures

Figure 1 with 2 supplements

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CTNIPs are a novel family of plant signalling peptide.

(a) Heat map showing log₂(FC) expression levels of CTNIP1–4 in response to a range of elicitors (data obtained from Bjornson et al., 2021). CTNIP5 was excluded as it is unannotated in the TAIR10 annotation, which was used to map the RNA sequencing reads. (b) Sequence probability logo from *Arabidopsis* CTNIP1–4 generated using WebLogo3. Signal peptide (as predicted by SignalP5.0) and CTNIP motif are indicated, and conserved cysteine residues are highlighted in yellow. Amino acids are coloured based on their biochemical properties: red = acidic; blue = basic; black = hydrophobic, and green = polar. (**c–d**) Cytoplasmic calcium influx measured in *p35S::AEQUORIN* seedlings after treatment with 1 μM CTNIP relative to pre-treated levels (n = 8 seedlings). (c) Points represent mean; error bars represent SEM. (d) Represents mean relative Ca²⁺ influx between 5 and 15 min. A line represents mean; error bars represent SD. p-Values indicate significance relative to the wild-type (WT) control in a Dunnett’s multiple comparison test following one-way ANOVA. (e) Western blot using α-p42/p44-ERK recognising phosphorylated MAP kinases in seedlings treated with 100 nM CTNIPs or mock for 15 min. The membrane was stained with CBB, as a loading control. (**f–g**) ROS production in leaf disks collected from 4-week-old *Arabidopsis* plants induced by 1 μM CTNIP4 application (n ≥8). (f) Points represent mean; error bars represent SEM. (g) Integrated ROS production over 40 min. Line represents mean; error bars represent SD. p-Values indicate significance relative to the WT control in a two-tailed t-test. All experiments were repeated and analysed three times with similar results. ROS, reactive oxygen species; CBB, Coomassie brilliant blue.

Figure 1—source data 1 CTNIPs are a novel family of plant signalling peptide.: https://cdn.elifesciences.org/articles/74687/elife-74687-fig1-data1-v2.xlsx
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Figure 1—source data 2 CTNIP-induced MAPK phosphorylation.: https://cdn.elifesciences.org/articles/74687/elife-74687-fig1-data2-v2.pdf
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Figure 1—figure supplement 1

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Alignment and phylogeny of *Arabidopsis* CTNIPs.

(a) Expression heat map showing log₂(FC) expression levels of *CTNIP1*, *CTNIP2*, *CTNIP3,* and *CTNIP5* taken from ArrayExpress which mapped to the Araport11 annotation (Athar et al., 2019; Bjornson et al., 2021). *CTNIP4* overlaps with the adjacent transcript *AT2G31340* in the Araport11 annotation. Thus, no reads mapped uniquely to *CTNIP4* and consequently no differential expression data could be obtained. (b) Phylogeny of *Arabidopsis* CTNIPs. Full-length protein sequences were aligned using MUSCLE and a phylogeny was inferred using the maximum-likelihood method and JTT matrix-based model conducted in MEGAX. 1000 bootstraps were performed and values shown in blue. Branch lengths are shown in black. (c) Alignment used to generate (b). CTNIP motif is highlighted in red.

Figure 1—figure supplement 1—source data 1 Expression levels of CTNIP1, CTNIP2, CTNIP3, and CTNIP5.: https://cdn.elifesciences.org/articles/74687/elife-74687-fig1-figsupp1-data1-v2.xlsx
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Figure 1—figure supplement 2

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Characterisation of CTNIP synthetic peptides.

(a) Alignment of CTNIP4 peptide sequences used in this manuscript. (b) Western blot using α-p42/p44-ERK recognising phosphorylated MAP kinases in seedlings treated with 100 nM CTNIP4 fragments or mock for 15 min. The membrane was stained with Coomassie brilliant blue (CBB), as a loading control. (c) Mean relative Ca²⁺ influx induced by 1 μM CTNIP in *p35S::AEQUORIN* seedlings between 5 and 15 min, relative to pre-treatment (n = 8 seedlings). A line represents mean; error bars represent SD. p-Values indicate significance relative to the wild-type (WT) control in a Dunnett’s multiple comparison test following one-way ANOVA.

Figure 1—figure supplement 2—source data 1 CTNIP-induced calcium influx.: https://cdn.elifesciences.org/articles/74687/elife-74687-fig1-figsupp2-data1-v2.xlsx
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Figure 1—figure supplement 2—source data 2 CTNIP-induced MAPK phosophorylation.: https://cdn.elifesciences.org/articles/74687/elife-74687-fig1-figsupp2-data2-v2.pdf
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Figure 2 with 3 supplements

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HAESA-LIKE 3 (HSL3) forms a CTNIP-induced receptor complex with BAK1.

(a) Schematic representation of BAK1-GFP immunoprecipitation in the (1) absence or (2) presence of CTNIP4 treatment to identify protein associations induced by CTNIP. Figure generated using Biorender. (b) HSL3-specific spectral counts identified in four independent biological replicates where BAK1-GFP was pulled down in the presence or absence of 1 μM CTNIP4 treatment. Circle diameter is proportional to the number of replicates. Red lines indicate the mean spectral counts for each treatment. p-Values indicate significance relative to the untreated control in a two-tailed t-test. (c) Affinity purification of BAK1 with HSL3-GFP from HSL3-GFP seedlings treated with 1 μM CTNIP4^48-70 or water for 10 min. Western blots were probed with antibodies α-GFP and α-BAK1. This experiment was repeated three times with similar results. (d) Isothermal titration calorimetry (ITC) summary table of HSL3 vs. CTNP4^48-70, CTNP4^C58S/C68S and INFLORESCENCE DEFICIENT IN ABSCISSION (IDA) peptides, and contribution of the BAK1 co-receptor to the ternary complex formation. *K_d*, (dissociation constant) indicates the binding affinity between the two molecules considered (nM). The N indicates the reaction stoichiometry (N=1 for a 1:1 interaction). The values indicated in the table are the mean ± SEM of two independent experiments. (e) ITC experiments of HSL3 vs. CTNIP4 and CTNIP4^C58S/C68S, in the absence and presence of the co-receptor BAK1. GFP, green fluorescent protein.

Figure 2—source data 1 HSL3-specific spectral counts.: https://cdn.elifesciences.org/articles/74687/elife-74687-fig2-data1-v2.xlsx
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Figure 2—source data 2 Westernblots showing affinity purification of BAK1 with HSL3-GFP.: https://cdn.elifesciences.org/articles/74687/elife-74687-fig2-data2-v2.pdf
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Figure 2—figure supplement 1

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Phylogeny of *Arabidopsis* leucine-rich repeat receptor kinase (LRR-RK) subfamily XI.

Phylogeny of full-length protein sequences of the *Arabidopsis* LRR-RK subfamily XI. Sequences were aligned using MUSCLE and a phylogeny was inferred using the maximum-likelihood method and JTT matrix-based model conducted in MEGAX. 1000 bootstraps were performed and are indicated based on the size of the blue circles. Expression of these receptors in response to 1 μM flg22 treatment was extracted from Bjornson et al., 2021, and is represented in a heat map. Known ligands for LRR-RK subfamily XI are highlighted to the right (Butenko et al., 2003; Cho et al., 2008; Crook et al., 2020; Doblas et al., 2017; Doll et al., 2020; Hou et al., 2014; Krol et al., 2010; Morita et al., 2016; Mou et al., 2017; Nakayama et al., 2017; Ogawa et al., 2008; Okuda et al., 2020; Ou et al., 2016; Qian et al., 2018; Rojo et al., 2002; Roman et al., 2022; Santiago et al., 2016; Shinohara et al., 2016; Song et al., 2016; Tabata et al., 2014; Yamaguchi et al., 2010; Yamaguchi et al., 2006; Zhang et al., 2016).

Figure 2—figure supplement 1—source data 1 Flg22-induced expression data of LRR-RK subfamily XI.: https://cdn.elifesciences.org/articles/74687/elife-74687-fig2-figsupp1-data1-v2.xlsx
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Figure 2—figure supplement 2

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Isothermal titration calorimetry (ITC) independent experiments and purification of HAESA-LIKE 3 (HSL3) and BAK1 used in the binding experiments.

(a) Analytical size exclusion chromatography (SEC) of the ectodomains of HSL3 and BAK1. An SDS-PAGE of the two proteins is shown alongside. (b) ITC raw thermograms of experiments shown in the ITC table summary in Figure 2d.

Figure 2—figure supplement 3

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Structural comparison of the binding pockets between the receptors HAESA and HAESA-LIKE 3 (HSL3).

(a) The hydroxyproline pocket required for anchoring the INFLORESCENCE DEFICIENT IN ABSCISSION (IDA) peptide to the HAESA receptor is missing in HSL3. Close view of the binding pocket of the structural superimposition of the HAESA-IDA complex (PDB:5IXQ) and a homology model of HSL3 (AlphaFold: https://alphafold.ebi.ac.uk/). The HAESA receptor is depicted in surface representation in teal blue, IDA in yellow sticks, and HSL3 in magenta cartoon. In HSL3, the hydroxyproline pocket is replaced by the bulky residue Phe286, colliding with the potential anchoring of the IDA peptide to the receptor. (b) The conserved RxR motif necessary for the coordination of the COO^- group the last Asn in IDA is not present in the HSL3 receptor. Zoom in of the C-terminal region of the peptide-binding surface of HAESA (teal blue) (left panel) and HSL3 (magenta) (right panel). In HAESA the motif RxR closes the binding pocket allowing for the coordination of the C-terminal of IDA. In HSL3 this structural motif is substituted by the residues Thr406 and Gln408, leaving the binding surface open to potentially accommodate a longer peptide ligand. Figures were done using the PyMOL Molecular Graphics System, Version 2.0 Schrödinger, LLC.

Figure 3 with 5 supplements

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HAESA-LIKE 3 (HSL3) is strictly required for CTNIP perception and growth regulation.

(a) Western blot using α-p42/p44-ERK recognising phosphorylated MAP kinases in seedlings treated with 100 nM CTNIPs or mock for 15 min. The membrane was stained with Coomassie brilliant blue (CBB), as a loading control. (b) Heat map showing all significantly differentially expressed genes (p<0.05, |log₂(FC)|>1) in *Arabidopsis* wild-type (WT) or *hsl3-1* seedlings treated with or without 100 nM CTNIP4^48-70 for 30 min relative to a mock control. (c) Mean relative cytoplasmic Ca²⁺ influx in leaf disks of *Nicotiana benthamiana* transiently expressing the defined constructs induced by 1 μM CTNIP or mock application (n = 8 leaf disks). A line represents mean; error bars represent SD. p-Values indicate significance relative to the GUS-transformed control in a Dunnett’s multiple comparison test following one-way ANOVA. (d) Fresh weight of 14-day-old seedlings grown in the presence of 500 nM CTNIP4^48-70 for 10 days relative to mock (n = 8 seedlings). A line represents mean; error bars represent SD. p-Values indicate significance relative to the WT control in a two-tailed t-test. (e) Representative images of (d). (**f,i**) Nine-day-old vertically grown *Arabidopsis* seedlings on 1/2 Murashige and Skoog (MS) agar medium with 1% sucrose. Pictures were taken from the front of the plate. (**g–h,j–k**) Root parameters were quantified from the base of the hypocotyl to the root tip using ImageJ. (g) Root angle is shown relative to mock. Negative values indicate leftward root skewing. (j) Absolute root angle with 90° representing the gravity vector. Angles < 90° represent skewing to the left. A line represents mean; error bars represent SD. p-Values indicate significance relative to the WT control in a Dunnett’s multiple comparison test following one-way ANOVA. All experiments were repeated and analysed three times with similar results.

Figure 3—source data 1 HSL3 is strictly required for CTNIP perception and growth regulation.: https://cdn.elifesciences.org/articles/74687/elife-74687-fig3-data1-v2.xlsx
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Figure 3—source data 2 HSL3-dependency of CTNIP-induced MAPK phosphorylation.: https://cdn.elifesciences.org/articles/74687/elife-74687-fig3-data2-v2.pdf
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Figure 3—figure supplement 1

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Genetic characterisation of *hsl3* mutants.

(a) Gene model showing the location of T-DNA inserts. (b) PCR confirming T-DNA insertion and mutant homozygosity.

Figure 3—figure supplement 1—source data 1 Genetic characterisation of hsl3 mutants.: https://cdn.elifesciences.org/articles/74687/elife-74687-fig3-figsupp1-data1-v2.pdf
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Figure 3—figure supplement 2

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CTNIP-induced seedling growth inhibition.

(**a–b**) Fresh weight of 14-day-old seedlings grown in the presence of 500 nM CTNIPs for 10 days relative to mock (n = 8 seedlings). A line represents mean; error bars represent SD. p-Values indicate significance relative to the wild-type (WT) control in a Dunnett’s multiple comparison test following one-way ANOVA.

Figure 3—figure supplement 2—source data 1 CTNIP-induced seedling growth inhibition.: https://cdn.elifesciences.org/articles/74687/elife-74687-fig3-figsupp2-data1-v2.xlsx
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Figure 3—figure supplement 3

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Correlation of CTNIP4-induced transcriptomic response with that of elicitors at 30min.

CTINP4-induced gene expression is well correlated with elicitor-induced gene expression from Bjornson et al., 2021. Circle colour and size are proportional to the Spearman correlation coefficient (R-squared value) of each pairwise comparison of log₂(fold changes).

Figure 3—figure supplement 3—source data 1 Correlation of CTNIP4-induced transcriptomic response with that of elicitors at 30min.: https://cdn.elifesciences.org/articles/74687/elife-74687-fig3-figsupp3-data1-v2.csv
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Figure 3—figure supplement 4

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Characterisation of CTNIP and chimeric receptor lines.

(a) Western blot using α-FLAG recognising BIR3_ecto-HSL3_cyto-FLAG in seedlings to confirm expression. The membrane was stained with Coomassie brilliant blue (CBB), as a loading control. (b) Ten-day-old vertically grown *Arabidopsis* seedlings on 1/2 Murashige and Skoog (MS) agar medium with 1% sucrose. Pictures were taken from the front of the plate. All seedlings are T1 transgenics and were initially selected upon plates containing glufosinate-ammonium and carbenicillin plates for 5 days before being transferred to fresh plates and grown for a further 5 days. (c) Documentation of the Cas9-induced mutations observed within the *ctnip1-4* polymutant and their predicted effects on protein products. (d) qRT-PCR documenting the overexpression of CTNIP lines. Expression of *CTNIP4* is shown relative to *U-Box* (*At5g15400*). Points represent independent biological replicates each comprising two technical replicates. Lines represent the mean of biological replicates.

Figure 3—figure supplement 4—source data 1 Characterisation of CTNIP and chimeric receptor lines.: https://cdn.elifesciences.org/articles/74687/elife-74687-fig3-figsupp4-data1-v2.pdf
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Figure 3—figure supplement 5

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*HSL3-CTNIP* mutants do not show altered resistance to *Pseudomonas syringae* pv tomato DC3000 *ΔAvrPto/ΔAvrPtoB.*

Four-week-old plants were spray inoculated with *P. syringae* pv tomato DC3000 *ΔAvrPto/ΔAvrPtoB* (OD₆₀₀=0.2). Data points represent individual plants (n=8). Red bars represent medians. Dashed lines represent the Col-0 median (black) and 95% confidence intervals of the median (grey). p-Values indicate significance relative to the wild-type (WT) control in a Dunnett’s multiple comparison test following one-way ANOVA.

Figure 3—figure supplement 5—source data 1 HSL3-CTNIP mutants do not show altered resistance to Pseudomonas syringae pv tomato DC3000 ΔAvrPto/ΔAvrPtoB.: https://cdn.elifesciences.org/articles/74687/elife-74687-fig3-figsupp5-data1-v2.xlsx
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Figure 4 with 1 supplement

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The HSL3-CTNIP signalling module predates extant angiosperms.

(a) Phylogeny of the full-length amino acid sequences of HAE/HSL/CEPR/RLK7/IKU2 clade of receptor kinases. Eudicot sequences are indicated in blue, monocot sequences in green, and *Amborella* sequences in red. Clades are named based upon the *Arabidopsis* genes. Alignment shown in Supplementary file 14. Further details of species, sequence identification, alignment, and phylogeny generation are described in the Materials and methods. (b) Species tree with number of CTNIP and HSL3 orthologs identified. Annotated CTNIPs are shown in grey whilst unannotated CTNIPs are shown in black. Sequences are shown in Supplementary files 10 and 16. (c) Phylogeny of the full-length amino acid sequences of CTNIPs. Eudicot sequences are indicated in blue, monocot sequences in green, and *Amborella* sequences in red. Sequences shown in Supplementary file 10. Further details of species, sequence identification, alignment, and phylogeny generation are described in the Materials and methods. (d) Sequence logo generated from CTNIP alignment from (c) using the R-package ggseqlogo. Amino acids are coloured based on their biochemical properties: red = acidic; blue = basic; black = hydrophobic; purple = neutral, and green = polar. (e) Cytoplasmic calcium influx measured after treatment with 1 μM CTNIP in *p35S::AEQUORIN Nicotiana benthamiana* leaf disks transiently expressing the defined construct, relative to pre-treatment (n = 8 leaf disks). Points represent mean; error bars represent SEM. Experiments were repeated and analysed three times with similar results. HSL3, HAESA-LIKE 3.

Figure 4—source data 1 The HSL3-CTNIP signalling module predates extant angiosperms.: https://cdn.elifesciences.org/articles/74687/elife-74687-fig4-data1-v2.xlsx
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Figure 4—figure supplement 1

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HAE/HSL/CEPR/RLK7/IKU2 clade phylogenies.

Phylogenies of HAE/HSL/CEPR/RLK7/IKU2 clade LRR domains and kinase domains. Eudicot sequences are indicated in blue, monocot sequences in green, and *Amborella* sequences in red. Corresponding alignments and Newick files can be found in Supplementary file 16,Supplementary file 17, Supplementary file 18, Supplementary file 19, Supplementary file 20.

Tables

Key resources table

Reagent type (species) or resource	Designation	Source or reference	Identifiers	Additional information
Gene (Arabidopsis thaliana)	HSL3	ARAPORT11	AT5G25930, Q9XGZ2_ARATH
Gene (Arabidopsis thaliana)	CTNIP1	ARAPORT11	AT1G06135, Q8LCX3_ARATH
Gene (Arabidopsis thaliana)	CTNIP2	ARAPORT11	AT1G06137, F4IBZ9_ARATH
Gene (Arabidopsis thaliana)	CTNIP3	ARAPORT11	AT2G31335, Q1G3B9_ARATH
Gene (Arabidopsis thaliana)	CTNIP4	ARAPORT11	AT2G31345, Q8L9Z1_ARATH
Gene (Arabidopsis thaliana)	CTNIP5	ARAPORT11	AT2G23123, A0A1I9LM80_ARATH
Gene (Medicago truncatula)	MtHSL3	Mt4.0	G7J3I8_MEDTR, MTR_3g110450, MtrunA17_Chr3g0140551
Gene (Medicago truncatula)	MtCTNIP	Mt4.0	G7I613_MEDTR, MTR_1g044470, MtrunA17_Chr1g0168241
Genetic reagent (Arabidopsis thaliana)	hsl3-1	euNASC	salk_207895
Genetic reagent (Arabidopsis thaliana)	hsl3-2	euNASC	wiscdslox450b04
Genetic reagent (Arabidopsis thaliana)	bak1-4/pBAK1::BAK1-GFP	https://doi.org/10.1105/tpc.111.090779	bak1-4/pBAK1::BAK1-GFP
Genetic reagent (Arabidopsis thaliana)	bak1-5	https://doi.org/10.1371/journal.pgen.1002046	bak1-5
Genetic reagent (Arabidopsis thaliana)	p35S::AEQUORIN	https://doi.org/10.1038/352524a0
Genetic reagent (Nicotiana benthamiana)	p35S::AEQUORIN	https://doi.org/10.1104/pp.110.171249
Genetic reagent (Arabidopsis thaliana)	35S::HSL3-GFP	This paper		Figure 3 and Materials and methods
Genetic reagent (Arabidopsis thaliana)	pHSL3::BIR3-HSL3-FLAG	This paper		Chimera created using the method from https://doi.org/10.1105/tpc.20.00138
Cell line (Trichoplusia ni)	Tnao38	https://doi.org/10.1186/1472-6750-12-12		Cell line maintained in J Santiago lab
Antibody	Anti-BAK1 (rabbit polyclonal)	https://doi.org/10.1105/tpc.111.084301		WB (1:2000)
Antibody	Anti-GFP (HRP-conjugated mouse monoclonal)	Santa Cruz	sc-9996	WB (1:5000)
Antibody	Anti-pMAPK (rabbit polyclonal)	Cell Signaling	p44/42 MAPK (Erk1/2) antibody #9,102	WB (1:4000)
Recombinant DNA reagent	35S::HSL3-GFP (plasmid)	This paper		Figure 3
Recombinant DNA reagent	pHSL3::BIR3-HSL3-FLAG (plasmid)	This paper		Used to generate transgenic plants in Figure 3
Recombinant DNA reagent	pHSL3::LTI6B-Citrine (plasmid)	This paper		Used to generate transgenic plants in Figure 3—figure supplement 4
Recombinant DNA reagent	pHSL3::BIR3^F146A,R170A -HSL3-Citrine (plasmid)	This paper		Used to generate transgenic plants in Figure 3—figure supplement 4
Recombinant DNA reagent	pHSL3::BIR3-HSL3-CITRINE (plasmid)	This paper		Used to generate transgenic plants in Figure 3—figure supplement 4
Commercial assay or kit	GFP-Trap	Chromotek	Cat. #: gta-20
Software, algorithm	GraphPad	GraphPad software