research papers\(\def\hfill{\hskip 5em}\def\hfil{\hskip 3em}\def\eqno#1{\hfil {#1}}\)

Journal logoSTRUCTURAL
BIOLOGY
ISSN: 2059-7983

Structure of the Arabidopsis receptor kinase SRF6 ectodomain determined from crystals obtained using the LRR crystallization screen

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aStructural Plant Biology Laboratory, Department of Plant Science, University of Geneva, 1211 Geneva, Switzerland
*Correspondence e-mail: [email protected]

Edited by B. Kobe, University of Queensland, Australia (Received 26 March 2026; accepted 25 May 2026; online 12 June 2026)

Plant-specific membrane receptor kinases with structurally diverse extracellular domains regulate key processes in plant growth, development, immunity and symbiosis. Structural studies of these glycoproteins are often hampered by the limited quantities in which they can be obtained. Here, we describe the leucine-rich repeat (LRR) crystallization screen, which has enabled the successful crystallization and structure determination of multiple receptor kinase ecto­domains, including ligand- and co-receptor-bound complexes. As an example, we report the 1.5 Å resolution crystal structure of the LRR domain of STRUBBELIG-RECEPTOR FAMILY 6 (SRF6) from Arabidopsis thaliana. The SRF6 ectodomain contains seven LRRs and a disulfide-bond-stabilized N-terminal capping domain but lacks the canonical C-terminal cap and the N-glycosylation pattern typically found in other family members. Previously reported protein–protein interactions between the SRF6 and SRF7 ectodomains and the receptor kinases BRI1, BRL1, BRL3, SERK3 and BIR1–BIR3 could not be confirmed by quantitative isothermal titration calorimetry and grating-coupled interferometry assays, suggesting that these structurally conserved LRR receptor kinases may have signalling functions outside the brassinosteroid pathway.

1. Introduction

Plant genomes harbour a large family of unique membrane receptor kinases (RKs) with extracellular leucine-rich repeat (LRR) extracellular domains (Shiu & Bleecker, 2001View full citation; Zhang et al., 2026View full citation). Members of this family include receptor kinases that bind small-molecule, peptide or protein ligands (Hohmann et al., 2017View full citation; Zhang et al., 2017View full citation; Moussu & Santiago, 2019View full citation), co-receptor kinases required for receptor activation (Brandt & Hothorn, 2016View full citation) and receptor pseudo-kinases that regulate the formation of active signalling complexes (Ma et al., 2017View full citation; Hohmann, Nicolet et al., 2018View full citation). The extracellular LRR domains of plant RKs are often stabilized by disulfide bridges and are extensively N-glycosylated (Di Matteo et al., 2003View full citation; Hothorn et al., 2011View full citation; She et al., 2011View full citation; Jia et al., 2024View full citation). Consequently, crystallographic studies on plant LRR-RKs largely rely on ectodomains obtained by secreted expression in baculovirus-infected insect cells (Hothorn et al., 2011View full citation; She et al., 2011View full citation). The resulting low protein yields, often further reduced by enzymatic deglycosylation prior to crystallization (Okuda et al., 2020View full citation), can severely limit the amount of sample available for high-throughput crystallization screening.

Testing a large number of variables that may influence sample crystallization (McPherson, 2004View full citation) often relies on commercial crystallization screens covering conditions previously associated with crystallization success (Berry et al., 2006View full citation) or derived from systematic approaches (Gorrec, 2015View full citation; Gorrec & Bellini, 2022View full citation). Here, we report the LRR crystallization screen, which has so far yielded a dozen different plant LRR-RK ectodomain structures with minimal sample requirements (as low as 50 µl of concentrated protein sample per project). As an example, we describe the crystallization and structure solution of the LRR-RK STRUBBELIG-RECEPTOR FAMILY 6 (SRF6).

SRF6 is part of a small protein family of plant receptor kinases. Its founding member STRUBBELIG (SUB/SRF9) was originally described in a genetic screen for mutants defective in ovule development (Schneitz et al., 1997View full citation) and is involved in plant organ development and cell-wall signalling (Chevalier et al., 2005View full citation; Kwak & Schiefelbein, 2007View full citation; Kwak et al., 2005View full citation; Eyüboglu et al., 2007View full citation; Chaudhary et al., 2020View full citation, 2021View full citation). The kinase activity of SUB appears to be dispensable for signalling (Chevalier et al., 2005View full citation). The interaction of SUB with other membrane-integral proteins has been reported (Fulton et al., 2009View full citation; Vaddepalli et al., 2014View full citation; Chen et al., 2023View full citation), but a validated ligand or interaction partner for its extracellular LRR domain remains to be identified.

Mutations in the STRUBBELIG-RECEPTOR FAMILY members SRF3 result in altered immune responses (Alcázar et al., 2010View full citation, 2014View full citation; Atanasov et al., 2018View full citation; Duan et al., 2024View full citation) and iron homeostasis (Platre et al., 2022View full citation). For SRF6, functions in brassinosteroid (BR) signalling (Eyüboglu et al., 2007View full citation; Smakowska-Luzan et al., 2018View full citation) and in the perception of the cell-wall breakdown product trigalacturonic acid (Bhasin et al., 2025View full citation) have been proposed. Here, we report the crystal structure of the SRF6 ectodomain refined at 1.5 Å resolution, and biochemically characterize whether the SRF6 or SRF7 extracellular domains can interact with selected BR signalling components (Nolan et al., 2020View full citation). At the molecular level, BR signalling is mediated by the steroid receptor LRR-RKs BRI1, BRL1 and BRL3 (Li & Chory, 1997View full citation; Caño-Delgado et al., 2004View full citation; Caregnato et al., 2025View full citation), which upon sensing a BR ligand interact with the LRR co-receptor kinases SERK1–SERK4 (Li et al., 2002View full citation; Nam & Li, 2002View full citation; Gou et al., 2012View full citation; Hohmann, Santiago et al., 2018View full citation). The SERK co-receptors may be kept from interacting with BR receptors by constitutively interacting with the LRR receptor pseudokinases BIR1–BIR4 (Imkampe et al., 2017View full citation; Hohmann, Nicolet et al., 2018View full citation).

2. Materials and methods

2.1. Protein expression and purification

The coding sequence of the AtSRF6 LRR ectodomain (residues 26–287, UniProt ID A8MQH3; https://uniprot.org) was obtained as a synthetic gene codon-optimized for expression in Spodoptera frugiperda (Twist Bioscience) and was introduced by Gibson-assembly cloning (Gibson et al., 2009View full citation) into a modified pFastBac vector (Geneva Biotech), which provides a Drosophila melanogaster Bip signal peptide (MKLCILLAVVAFVGLSLD; Soejima et al., 2013View full citation) and a Tobacco etch virus protease (TEV)-cleavable C-terminal StrepII-9×His-tag. For protein expression, Trichoplusia ni (strain Tnao38; Hashimoto et al., 2010View full citation) cells were infected with 10 ml of virus in 250 ml of cells at a density of 2.0 × 106 cells ml−1, incubated for 24 h at 28°C and 110 rev min−1 and then for a further 48 h at 22°C and 110 rev min−1. The secreted SRF6 ectodomain was purified from the supernatant by sequential Ni2+ (HisTrap Excel; GE Healthcare; equilibrated in 25 mM potassium phosphate pH 7.8, 500 mM NaCl) and StrepII (Strep-Tactin XT; IBA; equilibrated in 25 mM Tris pH 8.0, 250 mM NaCl, 1 mM EDTA) affinity chromatography, followed by size-exclusion chromatography on a HiLoad 16/600 Superdex 200 pg column (GE Healthcare) equilibrated in 10 mM sodium citrate pH 5.0, 250 mM NaCl. About 5 mg of purified SRF6 could be obtained from 1 l of insect-cell culture. The monomeric peak fraction was concentrated to 14 mg ml−1 using an Amicon Ultra concentrator (molecular-weight cutoff 10 000; Millipore) and directly used for protein crystallization.

The protein samples used to assess the LRR screen were obtained as described: SERK1 (12 mg ml−1 in 25 mM citric acid pH 5.0, 100 mM NaCl; Santiago et al., 2013View full citation), BRI1–BLD–SERK1 (10 mg ml−1 in 25 mM citric acid pH 5.0, 100 mM NaCl; Santiago et al., 2013View full citation), HAESA–IDA (5 mg ml−1 in 20 mM citric acid pH 5.0, 100 mM NaCl; Santiago et al., 2016View full citation), HAESA–IDA–SERK1 (12 mg ml−1 in 20 mM citric acid pH 5.0, 100 mM NaCl; Santiago et al., 2016View full citation), BIR2 (9 mg ml−1 in 20 mM sodium citrate pH 5.0, 150 mM NaCl; Hohmann, Nicolet et al., 2018View full citation), BIR3–SERK1 (14 mg ml−1 in 20 mM sodium citrate pH 5.0, 150 mM NaCl; Hohmann, Nicolet et al., 2018View full citation), PDLP5 (70 mg ml−1 in 20 mM sodium citrate pH 5.0, 150 mM NaCl; Vaattovaara et al., 2019View full citation), SOBIR1 (20 mg ml−1 in 20 mM sodium citrate pH 5.0, 150 mM NaCl; Hohmann & Hothorn, 2019View full citation), GSO1–CIF2 (1 mg ml−1 in 20 mM sodium citrate pH 5.0, 150 mM NaCl; Okuda et al., 2020View full citation), BRI1–A1JME (6 mg ml−1 in 20 mM citric acid pH 5.0, 250 mM NaCl; Caregnato et al., 2025View full citation), BRL3–A1JMF (7 mg ml−1 in 20 mM citric acid pH 5.0, 250 mM NaCl; Caregnato et al., 2025View full citation) and BRL2 (6 mg ml−1 in 20 mM citric acid pH 5.0, 250 mM NaCl; Caregnato et al., 2025View full citation).

For isothermal titration calorimetry (ITC) and grating-coupled interferometry (GCI) assays AtSRF7 (residues 26–287, UniProt ID B5X583) was cloned, expressed and purified as described for SRF6. BRI1, BRL1, BRL3 and SERK3 were expressed and purified as described previously (Hohmann, Santiago et al., 2018View full citation; Caregnato et al., 2025View full citation), as was the expression and purification of BIR1–BIR4 (Hohmann, Nicolet et al., 2018View full citation). For ITC assays, the C-terminal affinity tags in BRL1 and SRF7 were removed by TEV cleavage overnight at 4°C, followed by size-exclusion chromatography into ITC buffer (25 mM sodium citrate pH 5.0, 150 mM NaCl). BRI1, BRL1 and BRL3 biotinylation for grating-coupled interfero­metry was achieved by incubating the respective Avi-tagged receptor with His-tagged BirA (Fairhead & Howarth, 2015View full citation). The receptor at a final concentration of 20 µM was incubated for 1 h at 30°C with BirA, biotin, ATP and MgCl2 at final concentrations of 85 µM, 150 µM, 2 mM and 5 mM, respectively. The BirA enzyme was subsequently removed by Ni2+ affinity chromatography and the biotinylated receptor was concentrated and loaded onto a HiLoad Superdex 200 16/200 pg column (Cytiva) equilibrated in 20 mM sodium citrate pH 5.0, 150 mM NaCl. The C-terminal affinity tags from SRF6, SRF7, SERK3 and BIR1–BIR4 were removed for these assays as described above.

2.2. LRR protein crystallization screening

The LRR crystallization screen was prepared in 96 50 ml Falcon tubes from stock solutions. Precipitants: PEG 1000 [Sigma #81188, 50%(w/v) stock solution], PEG 3350 [Sigma #88276, 50%(w/v) stock solution], PEG 8000 [Sigma #89510, 40%(w/v) stock solution], sodium malonate (3.4 M stock solution, pH 4.0–8.0, Hampton Research), ammonium sulfate (Sigma #A4418, 4 M stock solution). Salts: ammonium sulfate (Sigma #A4418, 2 M stock solution), lithium sulfate (Sigma #13029, 0.5 M stock solution), sodium chloride (Sigma #S9888, 2 M stock solution), sodium citrate [0.5 M stock solution from 0.5 M citric acid (#Sigma 251275) with 1.5 M sodium hydroxide], ammonium acetate (Sigma #09688, 0.5 M stock solution), magnesium chloride (Sigma #M2393, 0.5 M stock solution), lithium chloride (Sigma #L9650, 2 M stock solution). Buffers: citric acid/NaOH pH 4.0 (Sigma #251275, 1 M stock solution), sodium acetate/acetic acid pH 5.5 (Sigma #S8750, 1 M stock solution), bis-Tris–HCl pH 7.0 (Sigma B7535, 1 M stock solution), Tris base/HCl pH 8.5 (Sigma #T4661, 1 M stock solution). Crystallization experiments were performed at room temperature in 96-well MRC 2-well sitting-drop plates (SWISSCI #MRC96T-UVP). Drops were composed of 0.2 µl protein solution and 0.2 µl crystallization buffer suspended over 100 µl of the latter as reservoir solution. The second drop was set up with the protein diluted 1:3 in protein storage buffer. Plates were inspected after 24 h, 3 d and two months on a CX31 microscope (Olympus). In the case of AtSRF6, diffraction-quality crystals appeared after 3 d in LRR screen conditions C5 [25%(w/v) PEG 3350, 0.2 M sodium chloride, 0.1 M citric acid pH 4.0] and F9 [20%(w/v) PEG 8000, 0.2 M magnesium chloride, 0.1 M citric acid pH 4.0]. A needle-shaped crystal (∼300 × 50 × 50 µm) from condition F9 was transferred to reservoir solution supplemented with 15%(v/v) glycerol and flash-cooled in liquid N2.

2.3. Crystallographic data collection, structure solution and refinement

Redundant sulfur single-wavelength anomalous dispersion (SAD) data (λ = 2.079 Å, five 360° wedges at 0.1° oscillation, with χ set to −20°, −10°, 0°, 10°, 20°) were collected to 2.3 Å resolution on beamline X06DA of the Swiss Light Source (SLS), Villigen, Switzerland equipped with a PILATUS 2M-F detector (Dectris) and a multi-axis goniometer. Next, the needle-shaped crystal was translated and an additional high-resolution native dataset (λ = 0.978 Å, one 360° wedge at 0.1° oscillation) was collected to 1.5 Å resolution. Data were processed and scaled with XDS and XSCALE, respectively (Kabsch, 1993View full citation). Analysis with phenix.xtriage (Zwart et al., 2005View full citation) indicated that the anomalous signal of the scaled SAD dataset extended only to ∼4.5 Å. Therefore, the native dataset was input into the MORDA automatic molecular-replacement (MR) pipeline (https://www.ccp4.ac.uk/morda-automatic-molecular-replacement-pipeline/), which returned a marginal solution in space group P43212 (translation function Z-score 8.4, Rwork = 0.486, Rfree = 0.495) using a single molecule of the previously reported Arabidopsis POLLEN RECEPTOR-LIKE KINASE 6 (PRK6) ectodomain structure in the asymmetric unit (PDB entry 5y9w; Zhang et al., 2017View full citation). The MORDA solution was input into Phaser for MR-SAD phasing against the SAD dataset at 2.3 Å [the starting figure of merit (FOM) was 0.309 at 2.3 Å resolution], yielding four putative sulfur sites by log-likelihood-gradient completion (the final FOM was 0.475). After merging with the high-resolution native dataset, these starting phases were used for automatic model building in ARP/wARP (Langer et al., 2008View full citation). The resulting structure was completed in iterative cycles of manual model correction in Coot (Emsley & Cowtan, 2004View full citation) and restrained refinement in REFMAC5 (Murshudov et al., 1997View full citation). The final model had excellent stereochemistry as assessed with phenix.molprobity (Davis et al., 2007View full citation). Structural diagrams were prepared with PyMOL (https://pymol.org) and ChimeraX (Meng et al., 2023View full citation). Phased anomalous difference maps were generated with phenix.find_peaks_holes and were displayed in ChimeraX.

2.4. Analytical size-exclusion chromatography

Analytical size-exclusion chromatography (SEC) experiments were performed on a Superdex 200 Increase 10/300 GL column (GE Healthcare) pre-equilibrated in 20 mM sodium citrate pH 5.0, 250 mM NaCl. 500 µg of a mixture containing the BRL1 and SRF6 ectodomains in a 1:1 molar ratio was injected in a volume of 100 µl onto the column and elution at 0.75 ml min−1 was monitored by ultraviolet absorbance at λ = 280 nm. Peak fractions were analysed by SDS–PAGE.

2.5. Isothermal titration calorimetry

The ITC experiment was performed at 25°C using a Nano ITC (TA Instruments) with a 1.0 ml standard cell and a 250 µl titration syringe. SRF6 and BRL1 samples were prepared by gel filtration into ITC buffer (25 mM sodium citrate pH 5.0, 150 mM NaCl). 10 µl SRF7 aliquots (∼220 µM) were injected into ∼23 µM BRL1 in the cell at 150 s intervals in the absence of a BR. ITC data were corrected for the heat of dilution by subtracting the mixing enthalpies for titrant solution injections into protein-free ITC buffer. Data were analysed using the NanoAnalyze program (version 3.5) as provided by the manufacturer.

2.6. SRF-family phylogeny

A multiple sequence alignment of the SRF1 (TAIR ID AT2G20850; https://www.arabidopsis.org/), SRF2 (AT5G06820), SRF3 (AT4G03390), SRF5 (AT1G78980), SRF6 (AT1G53730), SRF7 (AT3G14350), SRF8 (AT4G22130) and SRF9/SUB (AT1G11130) protein sequences was generated with Prob­align (Roshan & Livesay, 2006View full citation). The phylogenetic tree was generated with IQ-TREE 2 (Minh et al., 2020View full citation) and displayed in FigTree (https://tree.bio.ed.ac.uk/software/figtree/).

2.7. Grating-coupled interferometry

GCI assays were performed on a Creoptix WAVE system (Malvern Panalytical). Binding of the isolated SRF6, SRF7 and SERK3 (positive control) was measured by amine-coupling the BRI1, BRL1, BRL3, BIR1, BIR2, BIR3 or SERK3 ectodomains (ligand) onto 2PCP WAVEchips (quasi-planar polycarboxylate surface; Creoptix AG, Switzerland). Chips were conditioned using borate buffer (100 mM sodium borate pH 9.0, 1 M NaCl; Xantec, Germany) and the respective ligand was immobilized on the chip surface via a standard amine-coupling protocol, which consisted of 7 min activation with a 1:1 mixture of 400 mM N-(3-dimethylaminopropyl)-N′-ethylcarbodiimide hydrochloride and 100 mM N-hydroxysuccinimide (both from Xantec, Germany), followed by injection of the ligand (1–50 µg ml−1) in 10 mM sodium acetate pH 5.0 (Sigma, Germany) until the desired density was reached, and quenching with 1 M ethanolamine pH 8.0 for 7 min (Xantec, Germany). BSA (0.5% in 10 mM sodium acetate pH 5.0; BSA from Roche, Switzerland) was used to passivate the surface between ligand injection and ethanol­amine quenching. The isolated SRF6, SRF7 or SERK3 ectodomains were used as analytes. Kinetic analyses were performed at 25°C with a 1:2 dilution series from 2 µM in 20 mM sodium citrate pH 5.0, 250 mM NaCl, 100 nM brassinolide, with blank injections for double referencing and DMSO calibration for bulk correction. Data correction and analysis was performed with the Creoptix WAVEcontrol software (corrections applied: X and Y offset, DMSO calibration and double referencing). Data were fitted to either one-to-one binding models or mass-transport-limited models using bulk correction.

3. Results

3.1. A high-throughput crystallization screen for extracellular LRR proteins

The recombinant expression and purification of the first plant LRR-RK ectodomain in baculovirus-infected insect cells yielded only 50–200 µg of purified BRI1 per litre of cell culture (Hothorn et al., 2011View full citation). For the subsequent crystallization of the BRI1–BLD–SERK1 complex (Santiago et al., 2013View full citation), a tailored crystallization screen was therefore developed. The screen simply combined the crystallization conditions reported for the few LRR domain structures that had been previously reported for different animal and plant extracellular proteins (Table 1[link]; Uff et al., 2002View full citation; He et al., 2003View full citation; Di Matteo et al., 2003View full citation; Kim et al., 2005View full citation; Choe et al., 2005View full citation; Bell et al., 2005View full citation; Liu et al., 2008View full citation; Han et al., 2008View full citation; Hothorn et al., 2011View full citation; She et al., 2011View full citation). The conditions were replicated using a buffer system covering a pH range of 4.0–8.5 (the mean pH of the screen is 5.4; Table 2[link]). This was based on the idea that extracellular proteins usually reside in an acidic environment (the pH range of the plant apoplast is 4.5–6.5; Almeida & Huber, 1999View full citation) and that the mean pH of many commercially available, high-throughput crystallization screens is close to neutral (Crystal Screen HT, pH 6.6; Index HT, mean pH 6.8; PEG Ion, pH 6.8; Hampton Research).

Table 1
LRR ectodomain crystallization conditions reported between 2002 and 2011

Protein Precipitant Salt Buffer Reference
GPIbα 2 M ammonium sulfate   0.1 M Tris–HCl pH 6.5 Uff et al. (2002View full citation)
NgR 35% PEG 4000 0.25 M sodium chloride 0.1 M sodium acetate pH 6.5 He et al. (2003View full citation)
PGIP 20–30% PEG 4000 0.2 M ammonium acetate 0.1 M sodium acetate pH 4.6 Di Matteo et al. (2003View full citation)
CD14 1.9 M lithium sulfate 0.005 M nickel chloride 0.1 M HEPES pH 7.5 Kim et al. (2005View full citation)
TLR3 23% PEG 2000 0.4 M ammonium sulfate   Choe et al. (2005View full citation)
TL3 25% PEG 4000 0.2 M lithium sulfate 0.1 M sodium acetate pH 4.6 Bell et al. (2005View full citation)
mTL3 15% PEG 6000, 5% Dextran 5000 1 M lithium chloride 0.1 M citric acid pH 4.0 Liu et al. (2008View full citation)
mTLR3–dsRNA 13% PEG 3350, 5% Dextran 5000 0.2 M ammonium citrate pH 5.5   Liu et al. (2008View full citation)
VLR–RBC36 2 M ammonium sulfate 0.2 M sodium/potassium tartrate 0.1 M sodium citrate pH 5.6 Han et al. (2008View full citation)
BRI1–BLD 14% PEG 4000 0.2 M ammonium sulfate 0.1 M citric acid pH 4.0 Hothorn et al. (2011View full citation)
BRI1–BLD 20% PEG 3350 0.2 M ammonium sulfate   She et al. (2011View full citation)

Table 2
LRR screen formulation

Well Precipitant Salt Buffer
A1 30% PEG 1000 0.2 M ammonium sulfate 0.1 M citric acid pH 4.0
A2 30% PEG 1000 0.2 M ammonium sulfate 0.1 M sodium acetate pH 5.5
A3 30% PEG 1000 0.2 M ammonium sulfate 0.1 M bis-Tris pH 7.0
A4 30% PEG 1000 0.2 M ammonium sulfate 0.1 M Tris pH 8.5
A5 25% PEG 3350 0.2 M ammonium sulfate 0.1 M citric acid pH 4.0
A6 25% PEG 3350 0.2 M ammonium sulfate 0.1 M sodium acetate pH 5.5
A7 25% PEG 3350 0.2 M ammonium sulfate 0.1 M bis-Tris pH 7.0
A8 25% PEG 3350 0.2 M ammonium sulfate 0.1 M Tris pH 8.5
A9 20% PEG 8000 0.2 M ammonium sulfate 0.1 M citric acid pH 4.0
A10 20% PEG 8000 0.2 M ammonium sulfate 0.1 M sodium acetate pH 5.5
A11 20% PEG 8000 0.2 M ammonium sulfate 0.1 M bis-Tris pH 7.0
A12 20% PEG 8000 0.2 M ammonium sulfate 0.1 M Tris pH 8.5
B1 30% PEG 1000 0.2 M lithium sulfate 0.1 M citric acid pH 4.0
B2 30% PEG 1000 0.2 M lithium sulfate 0.1 M sodium acetate pH 5.5
B3 30% PEG 1000 0.2 M lithium sulfate 0.1 M bis-Tris pH 7.0
B4 30% PEG 1000 0.2 M lithium sulfate 0.1 M Tris pH 8.5
B5 25% PEG 3350 0.2 M lithium sulfate 0.1 M citric acid pH 4.0
B6 25% PEG 3350 0.2 M lithium sulfate 0.1 M sodium acetate pH 5.5
B7 25% PEG 3350 0.2 M lithium sulfate 0.1 M bis-Tris pH 7.0
B8 25% PEG 3350 0.2 M lithium sulfate 0.1 M Tris pH 8.5
B9 20% PEG 8000 0.2 M lithium sulfate 0.1 M citric acid pH 4.0
B10 20% PEG 8000 0.2 M lithium sulfate 0.1 M sodium acetate pH 5.5
B11 20% PEG 8000 0.2 M lithium sulfate 0.1 M bis-Tris pH 7.0
B12 20% PEG 8000 0.2 M lithium sulfate 0.1 M Tris pH 8.5
C1 30% PEG 1000 0.2 M sodium chloride 0.1 M citric acid pH 4.0
C2 30% PEG 1000 0.2 M sodium chloride 0.1 M sodium acetate pH 5.5
C3 30% PEG 1000 0.2 M sodium chloride 0.1 M Bis-Tris pH 7.0
C4 30% PEG 1000 0.2 M sodium chloride 0.1 M Tris pH 8.5
C5 25% PEG 3350 0.2 M sodium chloride 0.1 M citric acid pH 4.0
C6 25% PEG 3350 0.2 M sodium chloride 0.1 M sodium acetate pH 5.5
C7 25% PEG 3350 0.2 M sodium chloride 0.1 M bis-Tris pH 7.0
C8 25% PEG 3350 0.2 M sodium chloride 0.1 M Tris pH 8.5
C9 20% PEG 8000 0.2 M sodium chloride 0.1 M citric acid pH 4.0
C10 20% PEG 8000 0.2 M sodium chloride 0.1 M sodium acetate pH 5.5
C11 20% PEG 8000 0.2 M sodium chloride 0.1 M bis-Tris pH 7.0
C12 20% PEG 8000 0.2 M sodium chloride 0.1 M Tris pH 8.5
D1 30% PEG 1000 0.2 M sodium citrate 0.1 M citric acid pH 4.0
D2 30% PEG 1000 0.2 M sodium citrate 0.1 M sodium acetate pH 5.5
D3 30% PEG 1000 0.2 M sodium citrate 0.1 M bis-Tris pH 7.0
D4 30% PEG 1000 0.2 M sodium citrate 0.1 M Tris pH 8.5
D5 25% PEG 3350 0.2 M sodium citrate 0.1 M citric acid pH 4.0
D6 25% PEG 3350 0.2 M sodium citrate 0.1 M sodium acetate pH 5.5
D7 25% PEG 3350 0.2 M sodium citrate 0.1 M bis-Tris pH 7.0
D8 25% PEG 3350 0.2 M sodium citrate 0.1 M Tris pH 8.5
D9 20% PEG 8000 0.2 M sodium citrate 0.1 M citric acid pH 4.0
D10 20% PEG 8000 0.2 M sodium citrate 0.1 M sodium acetate pH 5.5
D11 20% PEG 8000 0.2 M sodium citrate 0.1 M bis-Tris pH 7.0
D12 20% PEG 8000 0.2 M sodium citrate 0.1 M Tris pH 8.5
E1 30% PEG 1000 0.2 M ammonium acetate 0.1 M citric acid pH 4.0
E2 30% PEG 1000 0.2 M ammonium acetate 0.1 M sodium acetate pH 5.5
E3 30% PEG 1000 0.2 M ammonium acetate 0.1 M bis-Tris pH 7.0
E4 30% PEG 1000 0.2 M ammonium acetate 0.1 M Tris pH 8.5
E5 25% PEG 3350 0.2 M ammonium acetate 0.1 M citric acid pH 4.0
E6 25% PEG 3350 0.2 M ammonium acetate 0.1 M sodium acetate pH 5.5
E7 25% PEG 3350 0.2 M ammonium acetate 0.1 M bis-Tris pH 7.0
E8 25% PEG 3350 0.2 M ammonium acetate 0.1 M Tris pH 8.5
E9 20% PEG 8000 0.2 M ammonium acetate 0.1 M citric acid pH 4.0
E10 20% PEG 8000 0.2 M ammonium acetate 0.1 M sodium acetate pH 5.5
E11 20% PEG 8000 0.2 M ammonium acetate 0.1 M bis-Tris pH 7.0
E12 20% PEG 8000 0.2 M ammonium acetate 0.1 M Tris pH 8.5
F1 30% PEG 1000 0.2 M magnesium chloride 0.1 M citric acid pH 4.0
F2 30% PEG 1000 0.2 M magnesium chloride 0.1 M sodium acetate pH 5.5
F3 30% PEG 1000 0.2 M magnesium chloride 0.1 M bis-Tris pH 7.0
F4 30% PEG 1000 0.2 M magnesium chloride 0.1 M Tris pH 8.5
F5 25% PEG 3350 0.2 M magnesium chloride 0.1 M citric acid pH 4.0
F6 25% PEG 3350 0.2 M magnesium chloride 0.1 M sodium acetate pH 5.5
F7 25% PEG 3350 0.2 M magnesium chloride 0.1 M bis-Tris pH 7.0
F8 25% PEG 3350 0.2 M magnesium chloride 0.1 M Tris pH 8.5
F9 20% PEG 8000 0.2 M magnesium chloride 0.1 M citric acid pH 4.0
F10 20% PEG 8000 0.2 M magnesium chloride 0.1 M sodium acetate pH 5.5
F11 20% PEG 8000 0.2 M magnesium chloride 0.1 M bis-Tris pH 7.0
F12 20% PEG 8000 0.2 M magnesium chloride 0.1 M Tris pH 8.5
G1 3.4 M sodium malonate pH 4.0    
G2 3.4 M sodium malonate pH 5.0    
G3 3.4 M sodium malonate pH 6.0    
G4 3.4 M sodium malonate pH 8.0    
G5 2.5 M sodium malonate pH 4.0    
G6 2.5 M sodium malonate pH 5.0    
G7 2.5 M sodium malonate pH 6.0    
G8 2.5 M sodium malonate pH 8.0    
G9 1.8 M sodium malonate pH 4.0    
G10 1.8 M sodium malonate pH 5.0    
G11 1.8 M sodium malonate pH 6.0    
G12 1.8 M sodium malonate pH 8.0    
H1 3.5 M ammonium sulfate   0.1 M citric acid pH 4.0
H2 3.5 M ammonium sulfate   0.1 M sodium acetate pH 5.5
H3 3.5 M ammonium sulfate   0.1 M bis-Tris pH 7.0
H4 3.5 M ammonium sulfate   0.1 M Tris pH 8.5
H5 3.5 M ammonium sulfate   0.1 M citric acid pH 4.0
H6 3.5 M ammonium sulfate   0.1 M sodium acetate pH 5.5
H7 3.5 M ammonium sulfate   0.1 M bis-Tris pH 7.0
H8 3.5 M ammonium sulfate   0.1 M Tris pH 8.5
H9 20% PEG 3350 1.0 M lithium chloride 0.1 M citric acid pH 4.0
H10 20% PEG 3350 1.0 M lithium chloride 0.1 M sodium acetate pH 5.5
H11 20% PEG 3350 1.0 M lithium chloride 0.1 M bis-Tris pH 7.0
H12 20% PEG 3350 1.0 M lithium chloride 0.1 M Tris pH 8.5

Despite its rather simple design principle, the LRR crystallization screen enabled the crystallization and structural analysis of the steroid receptor kinase BRI1sud1, the isolated ectodomain of the co-receptor kinase SERK1 and the BRI1sud1–BLD–SERK1 complex (Santiago et al., 2013View full citation; Fig. 1[link]). Over the years, our laboratory has used the LRR screen to determine the structures of several additional plant receptor kinase domains, including isolated LRR ectodomains (Hohmann, Nicolet et al., 2018View full citation; Hohmann, Santiago et al., 2018View full citation; Hohmann & Hothorn, 2019View full citation), receptor–small molecule and receptor–peptide ligand complexes (Santiago et al., 2016View full citation; Okuda et al., 2020View full citation; Caregnato et al., 2025View full citation), as well as receptor–co-receptor or regulatory complexes (Santiago et al., 2016View full citation; Hohmann, Nicolet et al., 2018View full citation; Fig. 1[link]). Outside our laboratory, the screen has been used to crystallize the ectodomains of the cell-wall protein LRX4 in complex with its peptide ligand RALF4 (conditions E6 and E7; Moussu et al., 2020View full citation), the LRR-RK HSL1 (condition A1; Roman et al., 2022View full citation) and the related HSL3 (condition E5; Jiménez-Sandoval et al., 2025View full citation). Finally, the LRR screen was used to crystallize the plant receptor-like protein PDLP5, which has a non-LRR tandem-malectin ectodomain (Vaattovaara et al., 2019View full citation; Fig. 1[link]).

[Figure 1]
Figure 1
Initial crystallization hits for ten different plant receptor kinases obtained using the LRR crystallization screen. Shown are schematic representations of a 96-well high-throughput crystallization screen plate with positive hits highlighted in cyan, observed after two months of incubation at room temperature. A ribbon diagram of the respective structure is shown alongside, with isolated ectodomain structures coloured from red (N-terminus) to green (C-terminus). Receptor–ligand complexes are shown in blue (ribbon diagram) and yellow (bond representation), respectively. Co-receptor kinases are depicted in orange.

3.2. Structure solution of SRF6 crystallized with the LRR screen

Next, we used the LRR screen to determine the structure of the isolated LRR ectodomain of the Arabidopsis thaliana receptor kinase SRF6 (see Fig. 2[link]a). SRF6 crystallized readily in various conditions in the screen, forming diffraction-quality, needle-shaped crystals in conditions E9 and F6 after three days of incubation at room temperature (see Section 2[link]; Fig. 2[link]b). Redundant SAD and a high-resolution native dataset data were collected from a single crystal. The structure of SRF6 was solved by the MR-SAD method implemented in Phaser (McCoy et al., 2007View full citation). The solution contains a single monomer in the asymmetric unit and four sulfur sites corresponding to a disulfide bridge involving Cys59 and Cys88 to Met42 in the N-terminal capping domain and to Met91 in the LRR core (Fig. 2[link]c). The final model was refined against the high-resolution native dataset at 1.50 Å resolution (Table 3[link], Fig. 2[link]d). An example region of the final (2FoFc) map is shown in Fig. 2[link](e). Overall, SRF6 shares the overall ecto­domain structure with other plant LRR receptor and co-receptor kinases (Hohmann et al., 2017View full citation). The SRF6 LRR domain comprises seven LRRs, rather than six as previously suggested for the related SRF9/SUB (Vaddepalli et al., 2011View full citationl; Fig. 2[link]d). Several genetic missense alleles identified for SRF9/SUB map to the N-terminal capping domain of SRF6, supporting the function of the N-cap in the folding of LRR domains (Truhlar & Komives, 2008View full citation; shown in magenta in Fig. 2[link]d). One of the alleles in SRF9/SUB results in the mutation of Cys57 to tyrosine, and the corresponding cysteine residue in SRF6 is involved in a disulfide bond (Fig. 2[link]d). Functionally, this specific mutation in SRF9/SUB is to the bri1-5 allele (Cys69-Tyr) in the BR receptor BRI1. It causes BRI1 to be misfolded and retained in the endoplasmic reticulum, triggering the plant's endoplasmic reticulum-associated degradation (ERAD) pathway (Hong et al., 2009View full citation). In contrast to many other LRR-RK ectodomain structures, SRF6 lacks any visible N-glycans, and its C-terminal capping domain is devoid of a stabilizing disulfide bridge, as previously seen, for example, in the co-receptor kinase SERK1 (Santiago et al., 2013View full citation; Fig. 2[link]f). Instead, the C-terminal cap of SRF6 is structurally reminiscent of the situation described for the immune receptor kinase SOBIR1 (Hohmann & Hothorn, 2019View full citation; Fig. 2[link]f).

Table 3
SRF6 crystallographic data-collection, phasing and refinement statistics

Values in parentheses are for the highest resolution shell.

  Sulfur MR-SAD High resolution
Data collection    
 Wavelength (Å) 2.0785 0.9779
 Space group P43212 P43212
a, b, c (Å) 76.76, 76.76, 86.51 76.72, 76.72, 86.43
α, β, γ (°) 90, 90, 90 90, 90, 90
 Resolution (Å) 45.98–2.30 (2.36–2.30) 45.95–1.50 (1.59–1.50)
Rmeas 0.152 (0.872) 0.174 (2.58)
 CC1/2 (%) 100 (92.5) 100 (50.8)
 〈I/σ(I)〉 35.0 (4.2) 13.9 (1.1)
 Completeness (%) 99.7 (96.6) 99.9 (99.3)
 Multiplicity 61.8 (25.8) 13.6 (12.9)
 Wilson B factor2) 22.5 16.7
Phasing
 Resolution (Å) 45.98–2.30  
 No. of sites 4  
 FOM 0.475  
Refinement
 Resolution (Å)   45.95–1.50 (1.54–1.50)
 No. of reflections   39715 (2853)
Rwork/Rfree§   0.162/0.195 (0.319/0.329)
 No. of atoms
  Protein   1756
  Buffer   15
  Water   237
 Residue B factors§2)
  Protein   19.9
  Buffer   30.36
  Water   31.45
 R.m.s deviations
  Bond lengths (Å)   1.82
  Bond angles (°)   0.012
MolProbity results
  Ramachandran outliers (%)   0
  Ramachandran favoured (%)   91.52
  MolProbity score   1.54
 PDB code   28wb
†As defined in XDS.
‡Final figure of merit of the MR-SAD experiment as defined in Phaser.
§As defined in REFMAC5.
¶As defined in phenix.molprobity.
[Figure 2]
Figure 2
Crystallographic analysis of the LRR ectodomain of the Arabidopsis receptor kinase SRF6. (a) Schematic representation of SRF6 (SP, signal peptide; N-cap, N-terminal capping domain; C-cap, C-terminal capping domain; TM, transmembrane helix; JM, juxta-membrane motif). The crystallized fragment is indicated by a red line. (b) Schematic representation of a 96-well high-throughput crystallization-screen plate; conditions containing SRF6 crystals after 3 d of incubation at room temperature are shown in cyan. (c) Ribbon diagram of the SRF6 N-terminal capping domain, with Met42, Cys59, Cys68 and Met91 shown in bond representation and including a phased anomalous difference map contoured at 9σ (green mesh). (d) Overall structure of the SRF6 ectodomain. A ribbon diagram is shown; the secondary structure was assigned using DSSP (Kabsch & Sander, 1983View full citation). The N- and C-terminal capping domains are shown in yellow and the LRR core in blue. A disulfide bond in the N-terminal capping domain is shown in bond representation; genetic alleles previously characterized for SRF9/SUB are highlighted in magenta. (e) Example region of the SRF6 structure covering residues 50–53 and 62–64 (yellow ball-and-stick representation) and including the final (2FoFc) electron-density map contoured at 1.5σ (blue mesh). (f) Structural comparison of the C-terminal capping domains in the Arabidopsis receptor kinases SERK1 (PDB entry 4lsc), SRF6 and SOBIR1 (PDB entry 6r1h). The LRR ectodomain (blue) structures of SERK1 (r.m.s.d. of ∼1.5 Å comparing 163 corresponding Cα atoms) and SOBIR1 (r.m.s.d. of ∼3.4 Å comparing 133 corresponding Cα atoms) were superimposed on the SRF6 LRR domain and presented side-by-side in ChimeraX. The C-terminal capping domains are highlighted in yellow.

3.3. Assessing the interaction between the SRF6 and SRF7 ectodomains and BR signalling components

Next, we sought to characterize the potential roles of SRF RKs in BR signalling. Previous studies have reported that SRF6 gene expression is upregulated following BR treatment (Eyüboglu et al., 2007View full citation). In addition, high-throughput inter­action assays revealed that the ectodomains of SRF4, SRF6, SRF7 and SRF9 interacted with the LRR ectodomains of the BR receptors BRI1 and BRL1 in the absence of the steroid ligand (Smakowska-Luzan et al., 2018View full citation). In the same screen, different SRF ectodomains additionally interacted with SERK co-receptor kinases and BIR1–BIR4 receptor pseudokinases (Smakowska-Luzan et al., 2018View full citation). Furthermore, the potato SRF receptor StLRPK1 was reported to constitutively interact with the co-receptor kinase SERK3 in co-immunoprecipitation assays (Wang et al., 2018View full citation).

We purified the LRR ectodomains of SRF6 and SRF7 (see Section 2[link]) and examined their interactions with components of the BR signalling pathway. When mixed in equimolar ratios in the absence of BRs, the BRL1 and SRF7 ectodomains did not co-migrate in analytical size-exclusion chromatography assays (Fig. 3[link]a). Consistently, no interaction was detected by isothermal titration calorimetry in the absence of the steroid ligand brassinolide (Fig. 3[link]b).

[Figure 3]
Figure 3
The ectodomains of the SRF6 and SRF7 proteins do not display high-affinity binding to the Arabidopsis BR receptors BRI1, BRL1 and BRL3. (a) Analytical size-exclusion chromatography of an equimolar mixture of BRL1 and SRF6. The absorbance trace at λ = 280 nm is shown in blue. Indicated are the void volume (v0) and the elution volumes for molecular-mass standards (Al, aldolase, 158 kDa; Ov, ovalbumin, 43 kDa; CA, carbonic anhydrase, 29 kDa). A Coomassie-stained SDS–PAGE of the peak fractions is shown alongside. (b) Isothermal titration calorimetry of SRF6 (in the syringe) versus BRL1 (in the cell). Shown are integrated heat peaks (upper panel) versus time and binding isotherms versus molar ratio of SRF6 ligand (lower panel). (c) Phylogenetic tree of the nine SRF family members annotated in the Arabidopsis genome. (d) Grating-coupled interferometry (GCI) binding kinetics of BRI1, BRL1 and BRL3 versus SRF6 and SRF7 in the presence of 100 nM brassinolide. The known BR co-receptor kinase SERK3 served as a positive control. Sensorgrams are shown with raw data in red and their respective fits in black. Binding kinetics were analysed by a 1:1 binding model. Tabular summaries of kinetic parameters are shown alongside (ka, association rate constant; kd, dissociation rate constant; KD, dissociation constant; n.d., no detectable binding).

As an alternative approach, we analysed the binding of SRF6 and its close homologue SRF7 (Fig. 2[link]c; ∼70% amino-acid sequence identity) by grating-coupled interferometry (GCI). The LRR ectodomains of the BR receptor kinases BRI1, BRL1 and BRL3 bound the co-receptor kinase SERK3 in the presence of brassinolide, consistent with previous reports (Fig. 2[link]d; Hohmann, Santiago et al., 2018View full citation; Caregnato et al., 2025View full citation). In contrast, no binding was detected when either the SRF6 or SRF7 ectodomain was used as the analyte and in the presence of brassinolide (Fig. 3[link]d).

BIR receptor pseudo-kinases have been identified as negative regulators of BR signalling (Imkampe et al., 2017View full citation), a function that depends on their LRR domains constitutively interacting with the ectodomains of SERK co-receptor kinases (Ma et al., 2017View full citation; Hohmann, Nicolet et al., 2018View full citation). The LRR domains of BIR1–BIR3, immobilized on the GCI chip (see Section 2[link]), all interacted with the SERK3 ectodomain, as previously reported (Hohmann, Santiago et al., 2018View full citation; Fig. 4[link]a). In contrast, no interaction was detected for SRF6 or SRF7 (Fig. 4[link]). Similarly, no binding was observed when testing interactions between SRF6 or SRF7 and SERK3 coupled to the chip (Fig. 4[link]a).

[Figure 4]
Figure 4
The ectodomains of SRF6 and SRF7 do not display high-affinity binding to Arabidopsis BIR receptor pseudokinases or to SERK3. (a) Grating-coupled interferometry (GCI) binding kinetics of BIR1, BIR2, BIR3 and SERK3 versus SRF6 and SRF7. The known, ligand-independent interaction between BIRs and SERK3 served as a positive control. Sensorgrams are shown with raw data in red and their respective fits in black. Binding kinetics were analysed by a 1:1 binding model. Tabular summaries of kinetic parameters are shown alongside (ka, association rate constant; kd, dissociation rate constant; KD, dissociation constant; n.d., no detectable binding). (b) Key residues required for BR hormone binding and BRI1 receptor association in SERK3 are not conserved in SRF6. A structural superposition of the SRF6 (blue ribbon diagram) and SERK3 (orange, PDB entry 8wec) ectodomains is shown (r.m.s.d. of ∼0.95 Å comparing 175 corresponding Cα atoms). Phe60 and His61 in SERK3, which are part of the steroid hormone binding site in the BRI1–SERK complex, correspond to Arg64 and Gly65 in SRF6, respectively. Tyr100 and Tyr124 in SERK3 involved in the binding of the BRI1 LRR domain correspond to Ser104 and Ala126 in SRF6. (c) Residues in BIR receptor pseudokinases involved in the interaction with SERK proteins are not conserved in SRF6. A structural superposition of SRF6 and BIR2 (purple, PDB entry 6fg7, r.m.s.d. of ∼0.92 Å comparing 113 corresponding Cα atoms) reveals that the distal SERK binding surface in BIR2 involving Trp73, Phe152 and Arg176 is not conserved in SRF6.

Together, our experiments did not reveal direct, high-affinity interactions between the LRR domains of SRF6 or SRF7 and early components of the BR signalling pathway.

4. Discussion

Structural biology has provided important insights into the ligand-recognition and receptor-activation mechanisms of plant membrane receptor kinases (Hohmann et al., 2017View full citation; Song et al., 2017View full citation; Moussu & Santiago, 2019View full citation). However, the recombinant expression of these proteins and the production of diffraction-quality crystals remain significant challenges. The LRR crystallization screen described here enabled the successful crystallization and structure determination of several plant RK ectodomains and ectodomain complexes (Fig. 1[link]). We speculate that the relatively low pH of the screen conditions is a key factor promoting the crystallization of extracellular proteins in otherwise standard PEG- or salt-based crystallization buffers. The individual conditions can be readily prepared from common crystallization stock solutions and stored in sterile-filtered 50 ml Falcon tubes, facilitating the long-term preservation and routine use of this in-house screen.

The SRF6 ectodomain crystallized readily in several LRR screen conditions and its structure could be determined at high resolution by MR-SAD. The resulting model reveals a compact LRR ectodomain architecture that overall resembles other plant LRR receptor kinases and co-receptor kinases, supporting the notion that SRF proteins belong to the structurally conserved LRR-RK superfamily (Fig. 2[link]).

Motivated by previous reports linking SRF proteins to BR responses, we have examined whether the SRF6 and SRF7 ectodomains interact directly with key components of the BR signalling pathway. However, using multiple complementary biochemical approaches, including analytical size-exclusion chromatography, isothermal titration calorimetry and grating-coupled interferometry, we were unable to detect direct interactions between the ectodomains of SRF6 or SRF7 and BR receptors, co-receptor kinases and receptor pseudo-kinases (Figs. 3[link] and 4[link]). These biochemical observations are consistent with the absence in SRF6 of key residues previously shown to be essential for BR ligand binding (corresponding to Phe60 and His6 in SERK31) and for BR receptor–co-receptor interactions (corresponding to Tyr100 and Tyr124 in SERK3) (Fig. 4[link]b; Santiago et al., 2013View full citation; Hohmann, Santiago et al., 2018View full citation). Likewise, the SERK-binding interface previously identified in the LRR domains of BIR receptor pseudokinases is not conserved in SRF6, providing a structural explanation for the lack of detectable interaction between SRF6 and BIR1–BIR4 (Figs. 4[link]a and 4[link]c; Ma et al., 2017View full citation; Hohmann, Nicolet et al., 2018View full citation).

Taken together, these results suggest that the SRF6 and SRF7 ectodomains do not form stable, high-affinity complexes with early components of the BR receptor complex under the conditions tested. This observation contrasts with previous high-throughput interaction screens (Smakowska-Luzan et al., 2018View full citation) and in planta biochemical assays (Wang et al., 2018View full citation). One possible explanation is that such interactions may be transient, indirect or mediated by additional factors present in the cellular context but absent from the in vitro binding assays used here. Alternatively, SRF receptors may participate in signalling pathways that intersect with BR responses downstream of receptor activation rather than through direct receptor–receptor interactions at the plasma membrane. Future studies will be required to elucidate the physiological functions of SRF receptors in plant organ development and in cell-wall sensing. The extracellular SRF LRR domain may also function as a ligand-binding module for a cell-wall-derived signalling molecule (Bhasin et al., 2025View full citation), an intriguing possibility that warrants further investigation.

Supporting information


Footnotes

Present address: Institute of Molecular Biology, 55128 Mainz, Germany.

Acknowledgements

We thank Y. Belkhadir for discussions and the staff of beamline X06DA (PXIII) at the Swiss Light Source (SLS) Villigen, Switzerland for technical help during data collection.

Data availability

Raw diffraction images and XDS processing files have been deposited at https://doi.org/10.5281/zenodo.18745496.

Funding information

This work was supported by Swiss National Science Foundation grant No. 310030_205201. Open access publishing facilitated by Université de Geneve, as part of the Wiley – Université de Geneve agreement via the Consortium Of Swiss Academic Libraries.

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