Arabidopsis WALL-ASSOCIATED KINASES are not required for oligogalacturonide-induced signaling and immunity

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Carbohydrate-based cell wall signaling impacts plant growth, development, and stress responses; however, how cell wall signals are perceived and transduced remains poorly understood. Several cell wall breakdown products have been described as typical damage-associated molecular patterns (DAMPs) that activate plant immunity, including pectin-derived oligogalacturonides (OGs). Receptor kinases (RKs) of the WALL-ASSOCIATED KINASE (WAK) family have been shown to bind pectin and OGs, and were previously proposed as OG receptors. However, unambiguous genetic evidence for the role of WAKs in OG responses is lacking. Here, we investigated the role of Arabidopsis WAKs in OG perception using a novel deletion mutant of the clustered WAK family. Using a combination of immune assays for early and late pattern-triggered immunity (PTI), we show that WAKs are dispensable for OG-induced signaling and immunity, indicating that they are not bona fide OG receptors.
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Find this author on Google Scholar Find this author on PubMed Search for this author on this site Cyril Zipfel 1 Institute of Plant and Microbial Biology and Zürich-Basel Plant Science Center, University of Zürich , 8008 Zürich, Switzerland 4 The Sainsbury Laboratory, University of East Anglia, Norwich Research Park , NR4 7UH Norwich, United Kingdom Find this author on Google Scholar Find this author on PubMed Search for this author on this site ORCID record for Cyril Zipfel Abstract Full Text Info/History Metrics Preview PDF Abstract Carbohydrate-based cell wall signaling impacts plant growth, development, and stress responses; however, how cell wall signals are perceived and transduced remains poorly understood. Several cell wall breakdown products have been described as typical damage-associated molecular patterns (DAMPs) that activate plant immunity, including pectin-derived oligogalacturonides (OGs). Receptor kinases (RKs) of the WALL-ASSOCIATED KINASE (WAK) family have been shown to bind pectin and OGs, and were previously proposed as OG receptors. However, unambiguous genetic evidence for the role of WAKs in OG responses is lacking. Here, we investigated the role of Arabidopsis WAKs in OG perception using a novel deletion mutant of the clustered WAK family. Using a combination of immune assays for early and late pattern-triggered immunity (PTI), we show that WAKs are dispensable for OG-induced signaling and immunity, indicating that they are not bona fide OG receptors. Introduction Plants are exposed to myriad potential pests and pathogens, against which they have evolved sophisticated defense mechanisms. The plant cell wall acts as the initial physical barrier against invasion, and alterations in this structure intricately interact with the plant immune system ( Dora et al ., 2022 ; Wolf, 2022 ). The plant cell wall is composed of cellulose, hemicellulose, pectin, polyphenolic lignin and a series of structural and enzymatically active proteins ( Wolf, 2022 ; Cosgrove, 2023 ). Cell wall polysaccharides serve as extracellular sources for the generation of damage-associated molecular patterns (DAMPs) that are thought to be released upon mechanical damage or pathogen infection ( Pontiggia et al ., 2020 ). Several such carbohydrate DAMPs have been previously described, including cellulose-derived cellobiose and cellotriose, mixed linked glucans, and pectin-derived oligogalacturonides (OGs) ( Bacete et al ., 2018 ; Oelmüller et al ., 2023 ). OGs are generated from demethylesterified pectins and represent the best studied pectin-derived cell wall breakdown products. OGs with a degree of polymerization (DP) 10-15 (OG 10-15 ) have been shown to elicit canonical PTI signaling and confer plant protection against a range of pathogens ( Bishop et al ., 1981 ; Hahn et al ., 1981 ; Ridley et al ., 2001 ; De Lorenzo et al ., 2011 ). More recently, shorter OGs such as trimers (GalA 3 /OG 3 ) and tetramers have also been shown to trigger immune responses and defense ( Davidsson et al ., 2017 ; Liu et al ., 2023 ; Xiao et al ., 2024 ). In the model plant Arabidopsis thaliana (hereafter, Arabidopsis), demethylated pectin was shown to directly bind the extracellular domain (ECD) of several WALL-ASSOCIATED KINASES (WAKs) ( Decreux and Messiaen, 2005 ; Decreux et al ., 2006 ; Kohorn et al ., 2009 ; Liu et al ., 2023 ). WAKs belong to a large family of receptor kinases (RKs) comprising 5 WAKs and at least 21 WAK-likes (WAKLs) ( Verica and He, 2002 ) that are characterized by epidermal-growth factor (EGF)-like domains and a galacturonan-binding domain in their ECD ( He et al ., 1996 ; Verica and He, 2002 ; Kohorn et al ., 2012 ; Stephens et al ., 2022 ). WAK1 was the first identified RK physically linking the plasma membrane (PM) to the cell wall, as isolation from fractions of proteolytically digested cell walls indicated a strong interaction of WAK1 with the cell wall and native pectin in vivo ( He et al ., 1996 ; Anderson et al ., 2001 ; Wagner and Kohorn, 2001 ). Further experiments suggested WAKs and their association with cell wall pectin are involved in cell expansion ( Kohorn et al ., 2006 ), and, potentially the response to pathogens ( He et al ., 1998 ; Kohorn et al ., 2012 ). Later, WAK1 was also shown to bind pectin and OG 9-15 with a high affinity in vitro ( Decreux and Messiaen, 2005 ; Decreux et al ., 2006 ; Kohorn et al ., 2009 ), with the WAK1-ECD preferentially interacting with de-esterified pectin through a binding site formed by cationic amino acids ( Decreux and Messiaen, 2005 ; Decreux et al ., 2006 ). A chimeric approach using the ECD of WAK1 fused to the intracellular domain of the leucine-rich repeat RK ELONGATION FACTOR-TU RECEPTOR (EFR) served as evidence for a proposed role for WAK1 in OG perception ( Brutus et al ., 2010 ). Although OG treatment of WAK1-EFR chimera-expressing plants induced an EFR cytosolic domain-mediated defense response, critical genetic evidence that WAKs are bona fide OG receptors is still lacking. Direct genetics of WAKs was previously hindered by the genetic clustering of the WAK family in Arabidopsis, the assumption that wak1 null mutants were lethal, and expected functional redundancy among the five members of the WAK family ( He et al ., 1999 ; Brutus et al ., 2010 ; Kohorn and Kohorn, 2012 ). Recently, however, a CRISPR deletion mutant for most of the chromosomal cluster carrying the five Arabidopsis WAK genes, wakΔ , was generated. This mutant was shown to be less sensitive to the bacterial flagellin-derived epitope flg22, chitin and OGs in terms of reactive oxygen species (ROS) production ( Kohorn et al ., 2021 ); suggesting that WAKs may generally regulate immune receptor complexes, rather than function specifically as OG receptors ( Wang et al ., 2020 ; Zhang et al ., 2020 ). WAKs were also recently shown to be genetically required for GalA 3 -induced expression of the salicylic acid (SA) marker gene PATHOGENESIS-RELATED 1 (PR1) ( Liu et al ., 2023 ). In this work, we directly investigated the genetic involvement of WAKs in OG-induced signaling in Arabidopsis. We generated a novel deletion of the entire WAK1-5 region ( wakΔ2 ) and tested this mutant for OG-induced responses. Surprisingly, we found that wakΔ2 retained full responsiveness to OGs, as measured by both early and late outputs of immune signaling. In addition, wakΔ2 plants were not affected in OG-induced resistance against both bacterial and fungal pathogens. Furthermore, we tested the genetic involvement of WAKs in response to flg22 and could observe that flg22-induced responses are not affected in the wakΔ2 mutant. Together, our data indicate that WAKs are not genetically required for OG perception and ensuing immune signaling in Arabidopsis. Results Generation of the wakΔ2 mutant The Arabidopsis genome has five WAK genes located in cluster on chromosome 1 ( FIGURE 1 A ). Recently, a partial deletion mutant was published, wakΔ, which lacks most of the cluster; however, this mutant still potentially expresses a fusion protein of the N-terminal region of WAK4 and the C-terminal region of WAK2 ( FIGURE 1 A ) ( Kohorn et al ., 2021 ). While the wakΔ mutant showed partially impaired flg22, chitin and OG responsiveness, it suffered from the presence of this potential WAK4-WAK2 fusion protein. Therefore, to explore if WAKs are genetically required for OG-induced responses, we generated a novel mutant using CRISPR/Cas9 that has a 23-kb deletion ( wakΔ2 ), in which all WAK genes are absent ( Error! Reference source not found. A-D). Lack of WAK1-5 expression in wakΔ2 seedlings was confirmed using RT-qPCR ( FIGURE 1 D ). In agreement with the previously published WAK deletion mutants ( Kohorn et al ., 2021 ; Liu et al ., 2023 ), wakΔ2 displayed no obvious growth phenotype when grown on soil ( FIGURE 1 E ). Download figure Open in new tab FIGURE 1 wakΔ2 is a full WAK deletion mutant. A) Schematic representation of the genomic arrangement of WAK1-5 in Arabidopsis. Middle cartoon shows the genomic deletion in wakΔ and the consequent fusion of WAK4 and WAK2 . The lower cartoon shows the genomic region of the WAK cluster in wakΔ2 . Black arrows indicate primer pairs (P) used in B. B) Genotyping gel of Col-0, wakΔ and wakΔ2 . Ethidium bromide-stained PCR products for parts indicated in A on agarose gel. P1-P4 refer to the primer pairs shown in A. C) Sequencing results from the wakΔ2 aligned against the 5’UTR of WAK4 and part of the third exon of WAK2 of Col-0. D) Transcript levels of WAK1-5 in Col-0 and wakΔ2 determined by RT-qPCR. RNA was extracted from 14-day-old Arabidopsis seedlings grown in liquid culture. Transcripts were normalized to the house-keeping gene UBOX . Three biological replicates per experiment (Rep) were used. E) Representative images of four-week-old Arabidopsis plants grown on soil. These experiments were performed two times. OG-induced immune signaling does not require the WAK family Given that WAKs are proposed as receptors for OGs ( Brutus et al ., 2010 ), we investigated their genetic requirement for OG-induced immune responses using wakΔ2. Previous studies have extensively studied the immune responses in Arabidopsis triggered by exogenously applied OG 10-15 including extracellular ROS production, mitogen-activated protein kinase (MAPK) activation, marker gene expression, ethylene production, callose deposition, seedling growth inhibition (SGI), and resistance against pathogens ( Denoux et al ., 2008 ; Davidsson et al ., 2017 ; Gravino et al ., 2017 ; Bjornson et al ., 2021 ). Full loss-of-function mutants of a bona fide OG receptor should not be able to induce OG-induced responses, as shown for other ligand-perceiving receptors ( Gómez-Gómez and Boller, 2000 ; Chinchilla et al ., 2006 ; Zipfel et al ., 2006 ; Miya et al ., 2007 ; Yamaguchi et al ., 2010 ; Cao et al ., 2014 ; Ranf et al ., 2015 ; Rhodes et al ., 2021 ). To investigate if early immune signaling induced by OGs is dependent on WAKs, we measured extracellular ROS production in leaves of 3- to 4-week-old Arabidopsis plants. Surprisingly and in contrast to previous results ( Kohorn et al ., 2021 ), OG 10-15 -induced ROS production was unaltered in wakΔ2 in comparison to Col-0 grown in our conditions under short day ( FIGURE 2A,B ). In addition to ROS, OGs induce rapid and transient MAPK phosphorylation ( Gravino et al ., 2017 ). To determine if OG-induced MAPK activation is affected in the wakΔ2 , MAPK phosphorylation was determined in Arabidopsis seedlings 5 and 15 min after elicitor treatment by western blot analysis using a commercial phosphorylation site-specific antibody. As with ROS production, OG 10-15 -triggered MAPK phosphorylation was unaltered in wakΔ2 mutants ( FIGURE 2C ). In addition to OG 10-15 , OG 3 (GalA 3 ) was previously shown to trigger MAPK phosphorylation and WAKs have been shown to be required for OG 3 -induced PR1 expression ( Davidsson et al ., 2017 ; Liu et al ., 2023 ). We therefore additionally investigated if OG 3 -induced MAPK phosphorylation is dependent on WAKs. OG 3 -induced MAPK phosphorylation is comparatively weak but was still induced in wakΔ2 mutant plants ( FIGURE 2D ). OGs were also previously shown to induce synthesis of ethylene in Arabidopsis seedlings ( Ferrari et al ., 2008 ; Brutus et al ., 2010 ; Gravino et al ., 2015 ). In line with other early induced PTI pathways, OG 10-15 -induced ethylene production was not compromised in wakΔ2 mutants ( FIGURE 2E ). Together, these results indicate that WAK1-5 are not required for OG-induced early immune outputs and thus the signaling initiation of OG-induced responses. Download figure Open in new tab FIGURE 2 WAKs are not required for OG-induced early immune responses. A-B) ROS production in response to OG 10-15 in leaf discs of 3- to 4-week-old Arabidopsis plants (n = 12 leaf discs of 6 plants). 100 µg/mL – 1 mg/mL of OG 10-15 were used as concentration dependent of the experiment. Mean ± standard errors are plotted. RLU=relative luminescent units. A) Representative graph of the kinetics of one replicate. 1 mg/mL OG 10-15 was used as concentration. B) Values are means of total photon counts over 30 min. Data from three independent experiments (Rep) are shown. Shapes indicate different replicates. Outliers are included in statistical analysis. Statistical test: Kruskal-Wallis test (p < 2.62*10 -08 ), Dunn’s post-hoc test with Benjamin-Hochberg correction (p <= 0.05). Groups with like letter designations are not statistically different. C-D) MAPK activation assay with 2-week-old seedlings in response to 100 µg/mL OG 10-15 (C) or 100 µg/mL OG 3 (D). Samples were collected 0, 5 and 15 min after elicitation as indicated. Blot was probed with α-p44/42 and α-BAK1 was used as loading control. CBB=commassie brilliant blue was used as loading control as well. E) Ethylene accumulation after treatment with 100 µg/mL OG 10-15 or water as control in Arabidopsis seedlings. Box plots represent means ± SE of three replicates. Equal letters at the top of the panel indicate p > 0.05, two-way ANOVA and a post hoc Tukey test. These experiments were performed three times. Aside from rapid signaling, PTI additionally involves longer-term responses such as callose deposition ( Beffa et al ., 1996 ; Luna et al ., 2011 ; Wang et al ., 2021 ). To investigate the requirement of WAKs at later stages of OG-induced responses, OG 10-15 -induced callose deposition was measured in leaf discs of Col-0 and wakΔ2 twenty-four hours after infiltration of either water or 100 µg/mL OG 10-15 . OG 10-15 -induced callose deposition in both Col-0 and wakΔ2 ( FIGURE 3 3A,B ). As is true of many elicitors, both OG 3 and long OGs can inhibit plant growth ( Davidsson et al ., 2017 ). Arabidopsis seedlings grown in the presence of OG 10-15 showed a significant growth inhibition in comparison to mock-treated seedlings; however, no difference could be observed between Col-0 and wakΔ2 ( FIGURE 3 3C ). Another long-term measurement of plant immune signaling is the production of SA and ensuing signaling, which can be inferred through the accumulation of the PR1 marker protein by immunoblotting ( Tsuda et al ., 2009 ; Zhang and Li, 2019 ; Bender et al ., 2021 ). OG 10-15 and flg22 induced robust PR1 accumulation twenty-four hours after elicitor infiltration into leaves of Col-0 plants. Both flg22 and OG 10-15 -induced PR1 accumulation was not affected in wakΔ2 ( FIGURE 3 3D ). OG 3 induced very weak PR1 accumulation; however, no difference in PR1 accumulation could be detected between Col-0 and wakΔ2 ( FIGURE 3 3 D). Collectively, these results indicate that WAKs are not required for OG-induced immune signaling. Download figure Open in new tab FIGURE 3 3 WAKs are not required for OG-induced late immune responses. A-B) Callose deposition visualized by aniline blue staining in response to 100 µg/mL OG 10-15 or water 24 hours after infiltration into leaves of 3- to 4-week-old Arabidopsis plants. n=16-32 leaf discs from 4 different plants were taken per independent experiment. The experiment was performed two times with similar results. A) Representative images of OG-induced callose deposition in the presented genotypes stained with aniline blue. B) Callose deposits induced by OGs and water infiltration. C) Relative weight of seedlings grown in liquid media for 10 days in the presence of 200 µg/mL OG 10-15 or in the absence of neither (mock). Means ± SE are shown with individual values for each plant and experiment (n = 12-14 seedlings per experiment). Outliers are included in statistical analysis. Equal letters at the top of the panel indicate p > 0.05, one-way ANOVA and a post hoc Tukey test. Groups with like letter designations are not statistically different. The experiment was repeated three times with similar results. D) PR1 accumulation assessed by immunoblotting with PR1 antibodies. Leaves from 3-week-old Arabidopsis plants were infiltrated with water (m = mock), 1 µM flg22 (f) or 100 µg/mL OG 10-15 or 50 µg/mL OG 3 and harvested after 24 hours. The experiment was repeated three times with similar results. WAKs are not required for OG-induced immunity OGs have been shown to induce protection against the necrotrophic fungus Botrytis cinerea, the necrotrophic bacterium Pectobacterium carotovorum and the hemibiotrophic bacterium Pseudomonas syringae ( Davidsson et al ., 2017 ; Gravino et al ., 2017 ; Howlader et al ., 2020 ). To investigate if WAKs are required for OG-induced immunity, we drop-inoculated Arabidopsis Col-0 and wakΔ2 leaves with B. cinerea conidia 24 h after infiltration with water or 100 µg/mL OG 10-15 . Disease lesions on leaves were measured 48 h post inoculation. Plants pre-treated with water showed significantly larger lesions sizes in both Col-0 and wakΔ2 than plants that were pretreated with OG 10-15 ( FIGURE 4 4 A,B ). OG-induced protection against B. cinerea was not affected in wakΔ2 plants in comparison to wild-type plants. OG induced protection against P. syringae was similarly unaltered in wakΔ2 in comparison to Col-0 ( FIGURE 4 4 C ). Overall, these results indicate that WAKs are not required for OG-induced immunity against these necrotrophic or hemi-biotrophic pathogens. Download figure Open in new tab FIGURE 4 4 OG-induced immunity is not affected in wakΔ2 . A-B ) OG-induced resistance against B. cinerea . 4- to 5-week-old Col-0 or wakΔ2 plants were infiltrated with water or 100 µg/mL OG 10-15 24hours prior drop-inoculation with B. cinerea strain BMM spores (5 µL; 5×10 5 spores/mL). Lesion areas were measured 48 hours post inoculation. The experiment was performed four times. A) Quantification of lesion sizes. Results show mean ± SE (n = 18-24 per experiment). Equal letters at the top of the panel indicate p > 0.05, two-way ANOVA and a post hoc Tukey test. Groups with like letter designations are not statistically different. B) Representative images of OG-induced immunity in the different genotypes. Images were taken 48 hours post inoculation. C) OG-induced resistance against P. syringae pv tomato DC3000. Plants were pretreated with water or 100 µg/mL OG 10-15 for 24 hours before infiltration with P. syringae . 48 hours after P. syringae infiltration, bacteria were extracted and plated. Results show means ± SE and individual data points from the three pooled experiments (n = 6 per experiment). Equal letters at the top of the panel indicate p > 0.05, two-way ANOVA and a post hoc Tukey test. Groups with like letter designations are not statistically different. The experiment was performed three times. WAKs do not play a significant role in immune signaling triggered by other elicitors Aside from their role as potential OG receptors, WAKs were recently reported to function in immune signaling induced by bacterial flagellin in tomato and fungal chitin in cotton ( Wang et al ., 2020 ; Zhang et al ., 2020 ). While in tomato only some flagellin-induced responses involved WAKs, e.g. callose deposition and anti-bacterial immunity, Gh WAK7A was broadly required for full responsiveness to fungal chitin but not to OGs in cotton ( Wang et al ., 2020 ; Zhang et al ., 2020 ). In line with those observations, the Arabidopsis wakΔ mutant showed a reduction in ROS production induced by flg22, chitin and OGs ( Kohorn et al ., 2021 ). Intrigued by these findings, we also tested whether flg22-induced responses are affected by the full deletion of WAKs in Arabidopsis. In contrast to previous results, flg22-induced ROS production in leaves of 3- to 4-week-old Arabidopsis plants were not affected in wakΔ2 in comparison to Col-0 under our conditions ( FIGURE 5A,B ). As expected, flg22-induced ROS production was dependent on the receptor FLAGELLIN-SENSING 2 (FLS2) and its co-receptor BRASSINOSTEROID-INSENSITIVE 1 (BRI1)-ASSOCIATED KINASE 1 (BAK1). In line with this, flg22-induced MAPK activation, ethylene production and induced resistance against P. syringae were not reduced in wakΔ2 in comparison to Col-0 ( FIGURE 5C-E ). These results indicate that the deletion of WAKs does not affect flg22-induced responses under our growth conditions. Download figure Open in new tab FIGURE 5 flg22-induced immunity is not affected by the loss of WAK1-5. A-B) ROS production in leaf discs of 3- to 4-week-old plants using 100 nM flg22 in Col-0, bak1-5/bkk1-1 , fls2/efr/cerk1 ( fec ) and wakΔ2 . The experiment was repeated at least three times (A-B). Mean ± standard errors are plotted. RLU=relative luminescent units. A) Kinetics of three representative independent replicates over 40-60 minutes. B) Values are means of total photon counts over 60 minutes as stated in the graph. Individual data points show ROS production in individual plants (n = 6-8 plants with each two leaf discs). Outliers are included in statistical analysis. Kruskal-Wallis Test flg22 (p-value = 9.364.10 -15 ), Dunn’s post-hoc test with Benjamin-Hochberg correction (p <= 0.05). Groups with like letter designations are not statistically different. C) MAPK activation assay with 2-week-old seedlings in response to 1 µM flg22. Samples were collected 0, 5 and 15 min after elicitation as indicated. Blot was probed with α-p44/42. CBB = commassie brilliant blue was used as loading control as well. D) Ethylene accumulation after treatment with 1 µM flg22 or water as control in Arabidopsis seedlings. Box plots represent means ± SE of three replicates. Equal letters at the top of the panel indicate p > 0.05, two-way ANOVA and a post hoc Tukey. E) OG-induced resistance against P. syringae pv. tomato DC3000. Plants were pretreated with water or 1 µM flg22 for 24 hours before infiltration with P. syringae . 48 hours after P. syringae infiltration, bacteria were extracted and plated. Results show means ± SE and individual data points from the three pooled experiments (n = 6 per experiment). Equal letters at the top of the panel indicate p > 0.05, two-way ANOVA and a post hoc Tukey test. Groups with like letter designations are not statistically different. F) Primary root length of Col-0 and wakΔ2 seedlings. Plants were grown on ½ MS +1 % sucrose plates for 5 days and then transferred to liquid ½ MS +1 % sucrose without elicitor (mock), 10 nM pep1 or 100 nM flg22. Root-growth was determined after 4 days in liquid culture. 6 plants were measured per experiment. Values correspond to length of each root in cm. Equal letters at the top of the panel indicate p > 0.05, two-way ANOVA and a post hoc Tukey test. All experiments were performed three times with similar results, only primary root length was only measured twice. The wakΔ2 mutant had no obvious growth phenotype when grown on soil ( FIGURE 1E ). The only wak -related growth phenotype previously observed was reduced root length when seedlings were grown on MS medium lacking sucrose, most pronounced on 1/6 MS ( Kohorn et al ., 2006 , 2021 ). Therefore, to investigate if elicitor-induced root-growth inhibition is affected in the wakΔ2 mutant, both Col-0 and wakΔ2 plants were grown in the presence of 10 nM At pep1, 100 nM flg22 or without elicitor for 5 days. Elicitor-induced root-growth inhibition was similar in Col-0 and wakΔ2 in the same extent to Col-0 for both flg22 and At pep1 ( FIGURE 5F ). Discussion PTI is achieved by the recognition of diverse elicitor molecules as ligands for plasma membrane-resident pattern recognition receptors (PRRs) ( DeFalco & Zipfel, 2021 ). Cell walls are the first layer of defense against invading pathogens, many of which have evolved arsenals of enzymatic and mechanical means to degrade or penetrate the cell wall ( Bacete et al ., 2018 ; Dora et al ., 2022 ). Thus, the integrity of the cell wall needs to be carefully monitored by sensor proteins. Several RKs have been proposed as PRRs that perceive cell wall breakdown products, including WAKs based on their ability to interact with pectin and its breakdown products ( He et al ., 1996 ; Decreux and Messiaen, 2005 ; Decreux et al ., 2006 ; Kohorn et al ., 2009 ; Brutus et al ., 2010 ). Yet, genetic evidence that WAKs function as bona fide OG receptor(s) was missing. Here, we have used the wakΔ2 mutant, which lacks all five members of the WAK family, to demonstrate that none of the WAKs are required for responses to either short or long chain demethylated OGs in Arabidopsis. Previously, the galacturonan-binding domain of WAKs was shown to bind both pectins and demethylesterified OG 9-15 ( Decreux and Messiaen, 2005 ; Decreux et al ., 2006 ). Additionally, chimeric WAK-EFR receptors were able to induce EFR-like responses upon OG-treatment ( Brutus et al ., 2010 ). While our results indicate that WAKs are not genetically required for OG-induced responses, they do not contradict the ability of WAK ECDs to bind pectins or pectin breakdown products. Interestingly, the ECD of the malectin-like RK FERONIA was also recently reported to bind to pectin and pectin breakdown products (Feng et al. 2018; Tang et al. 2022; Lin et al. 2022), suggesting that this biochemical property might be true for several cell wall-anchored RKs without necessarily functioning as the true receptors for these carbohydrates. OG 10-15 were suggested to be produced during pathogen infection and to subsequently induce immune signaling ( Ferrari et al ., 2013 ; Xiao et al ., 2024 ). Although demethylesterified OG 10-15 are active as elicitors, recent evidence challenges their production in planta as most Ogs produced during infection with B. cinerea or Fusarium oxysporum were acetyl- and methylesterified ( Voxeur et al ., 2019 ; Gámez-Arjona et al ., 2022 ). While pectic fractions of various sizes and modifications show elicitor activity, the complexity of those in planta -produced Ogs as well as the profile of crude extracts produced in the lab complicates the attribution of individual OG species to the elicitor activity ( Liu et al ., 2023 ). Regardless of the exact nature of in planta OG species, WAKs have been previously proposed as the receptors for demethylesterified OG 10-15 based on in vitro binding studies and chimeric approaches, and we are here unable to confirm any corresponding genetic requirement for WAKs in OG 10-15 -induced signaling. Interestingly, electrostatic analysis of the WAK1 ECD predicted by Alphafold revealed a negatively charged galacturonan-binding domain at apoplastic pH, contradicting the suggested binding of polyanionic de-esterified pectins ( Lee and Santiago, 2023 ). While our data demonstrate that members of the WAK family are not required for OG-induced responses, it is possible that quantitative phenotype(s) are masked by persistent functional redundancy. WAKs are characterized by a galacturonan-binding domain and many WAKs contain one or more copies of EGF-like domains in their ECD ( Verica and He, 2002 ; Stephens et al ., 2022 ). In addition to 5 WAKs, there are at least 21 WAK-likes (WAKLs) in Arabidopsis. To date, clear evidence is missing that WAKLs are also able to bind cell wall fragments ( Kohorn, 2016 ), with the exception of WAKL22/RESISTANCE TO FUSARIUM OXYSPORUM 1 (RFO1) and WAKL14 ( Huerta et al ., 2023 ; Ma et al ., 2024 ). However, based on their phylogenetic relationship, WAKLs are obvious candidates to test for further genetic redundancy. Aside from a role in OG perception, WAKs were recently suggested to be involved in the regulation of other RK complexes during immunity, indicating that they might serve as accessory RKs of PRR complexes. In tomato and cotton, WAKs interact with and positively regulate PRR complexes and are required for full responsiveness to the corresponding elicitors ( Wang et al ., 2020 ; Zhang et al ., 2020 ). In Arabidopsis, the wakΔ mutant was less sensitive to multiple elicitors in terms of ROS production ( Kohorn et al ., 2021 ). In contrast with these previous results, no quantitative reduction in OG- or flg22-induced ROS production could be observed in the wakΔ2 mutant. Although this difference is striking, it might further underline the role of WAKs as accessory RKs under certain growth conditions rather than OG-perceiving receptors. While WAKs appear to interact with multiple elicitor-perceiving RKs, the exact mechanisms by which WAKs regulate immunity seem to differ between plant species or different WAKs. WAKs are found across land plants, with the WAK/WAKL family expanded in monocots ( de Oliveira et al ., 2014 ; Kanyuka and Rudd, 2019 ; Stephens et al ., 2022 ; Zhang et al ., 2023a ; Ngou et al ., 2024 ). Several WAKs or WAKLs have been identified as resistance genes and are required for basal resistance to pathogens in a variety of different crop plants ( Diener and Ausubel, 2005 ; Zuo et al ., 2015 ; Hurni et al ., 2015 ; Hu et al ., 2017 ; Saintenac et al ., 2018 ; Bot et al ., 2019 ; Larkan et al ., 2020 ; Li et al ., 2020 ; Stephens et al ., 2022 ; Zhang et al ., 2023b ; Dai et al ., 2024 ; Zhong et al ., 2024 ). While diverse roles and mechanisms for WAKs in plant immunity have been proposed, a clear possibility is that WAKs perceive pathogen-derived molecules. Indeed, Arabidopsis WAK3 was recently shown to be required for immune responses induced by bacterial harpins ( Held et al ., 2024 ) indicating that WAKs might indeed perceive microbial molecules. Additionally, three WAKs have also been demonstrated to exhibit a gene-for-gene interaction with specific pathogenic effectors in crops ( Stephens et al ., 2022 ). The WAK proteins Stb6 and Rlm9 provide resistance against Zymoseptoria tritici isolates expressing AvrSbt6 in wheat and Leptosphaeria maculans expressing AvrLm5-9 in oilseed rape, respectively ( Brading et al ., 2002 ; Larkan et al ., 2016 ; Larkan et al ., 2020 ). While no direct interaction could be detected between these fungal effectors and corresponding WAK resistance proteins ( Saintenac et al ., 2018 ; Larkan et al ., 2020 ), intriguingly, a direct interaction has been observed between the maize WAK protein Snn1 and the Phaeosphaeria nodorum effector protein Sn Tox1. Unlike most other WAKs studied thus far, Snn1 serves as susceptibility factor for P. nodorum leading to disease in Snn1-expressing plants ( Liu et al ., 2012 ; Stephens et al ., 2022 ; Shi et al ., 2023 ). Maize qRgls1 / WAKL Y was also recently shown to confer quantitative disease resistance against gray leaf spot caused by the fungi Cercospora zeae-maydis and C. zeina ( Zhong et al ., 2024 ). Notably, an aqueous extract of C. zeina hyphae and spores was sufficient to induce WAKL Y -dependent ROS production suggesting that WAKL Y perceives a fungal ligand. Altogether, there is emerging evidence that WAKs may perceive diverse molecules of microbial origin and orchestrate both broad-spectrum and race-specific resistance ( Kanyuka and Rudd, 2019 ), which is consistent with our evidence that they do not function as bona fide OG receptor(s) in Arabidopsis. However, the mechanisms by which WAKs contribute to immunity and their true ligand(s) remain to be definitively characterized. Material and methods Plant growth Arabidopsis seeds were surface-sterilized using ethanol, plated on 0.5 MS medium (1 % sucrose, pH 5.8, 0.9 % phytoagar), stratified for 48 hours in the dark at 4 °C, and grown at 22 °C under a 16-hour photoperiod (120 μmol * s -1 *m -2 illumination). For assays in adult plants, including ROS production, pathogen infection and callose deposition, seedlings were transferred to soil after 7-10 days growth on plates. Plants were grown in short-day cycles (10 h light/14 h dark, 60 % humidity, 20 °C) for an additional 2-3 weeks. For assays with seedlings, including MAPK activation, RNA extraction, seedling growth inhibition and root growth inhibition, these were transferred 5 days after exposure to light to liquid MS and grown there for 10 days. Mutants were generated in the A. thaliana Columbia (Col-0) ecotype and primers for genotyping are found in SUPPLEMENTAL TABLE 1 . CRISPR-Cas9 mutagenesis The WAK4 and WAK2 oligonucleotides used as templates for SgRNA-targeted sites (GCTGT TTCGTTATTGTTAAATGG) 432 bp 5’ to the WAK4 ATG start codon, and (GGGGAGATTGAACAC TTGCTCGG) 77 bp 5’ to the WAK2 stop codon were each cloned into pSkAtu26 ( Feng et al., 2013 ). These two expression Sg cassettes were then cloned into pCambia1302 that also had a pOLE1-RFP cassette inserted into the ASN718 site by PCR cloning ( Shimada et al., 2010 ). The T1, RFP + (expressing linked CAS9 and sgRNAs) were screened for a deletion by PCR using primers flanking the deletion, and then T2 RFP - plants were screened again by PCR to isolate a plant with a deletion but not expressing CAS9 or the sgRNAs. These isolates were self-crossed to generate a homozygous deletion. RNA extraction and real-time (RT) quantitative PCR analysis Total RNA was extracted from 2-week-old liquid-grown seedlings. Total RNA was extracted using TRI reagent (Sigma-Aldrich). To remove genomic DNA, samples were treated with TURBO DNA-free Kit (Thermo Fisher Scientific). cDNA synthesis was performed using 1 µg of DNA-free RNA sample with RevertAid First Strand cDNA Synthesis Kit (Thermo Fisher Scientific) according to the manufacturer’s protocol. RT-qPCR analysis was performed using diluted cDNA as template for PowerUp SYBR Green (Applied biosystems) with the primers provided in SUPPLEMENTAL TABLE 1 . MAPK activation MAPK activation was performed as previously described ( Mühlenbeck et al ., 2023 ). Five-day-old seedlings were transferred into 24-well plates containing 1 mL of liquid 0.5 MS (1 % sucrose). Two seedlings per well were grown there for another 10-12 days. Seedlings were treated with 100 µg/mL OG 10-15 (Elicityl, GAT114), 100 µg/mL OG 3 (GalA3, Megazyme) or 1 µM flg22, and harvested at each time point as indicated in figure captions. Total proteins were extracted using extraction buffer (50 mM Tris pH 7.5 (HCl), 150 mM NaCl, 10 % (v/v) glycerol, 2 mM EDTA, 1 mM homemade PPI (equivalent to Sigma-Aldrich Protease-inhibitor cocktail P9599), 1 mM NaF, 1 mM sodium-orthovanadate, 2 mM sodium-molybdate, 4 mM sodium-tartrate, 1 % (v/v) IGEPAL CA630, 5 mM DTT). Proteins were analyzed by SDS-PAGE and immunoblotting using p44/42 MAPK antibody (Cell Signaling Technology). Seedling growth inhibition Seedling growth inhibition assays was performed as previously described ( Abarca et al ., 2021 ). Briefly, 5-day-old Arabidopsis seedlings were transferred to 48-well plate with one seedling per well. Each well contained either 500 µL 0.5 liquid MS with or without 200 µg/mL OG 10-15 (Elicityl, GAT114). After 10 days of growth in the presence of the respective elicitor, individual seedling weight as assessed using an analytical balance. Root growth Inhibition Five-day-old seedlings were transferred from solid MS plates to 12-well plate with 6 seedling per well. Each well contained 4 mL of liquid MS supplemented with mock (sterile ddH 2 O), 10 nM At pep1 or 100 nM flg22. After 5 days of treatment, seedlings were transferred to MS plates and imaged. Root lengths were quantified with ImageJ. Ethylene production Four- to six-week-old Arabidopsis leaves were cut into 3-mm slices and floated on water overnight. For each sample, three leaf slices were transferred to a 6-mL glass tube containing 200 µL MES buffer (pH 5.7), followed by adding either water control or the elicitor to a final concentration of 1 µM. Vials were closed with a rubber septum and ethylene production in the free air space was measured by gas chromatography (Shimadzu, GC-14A) after 3 hours of incubation. ROS production Leaf-discs of 3- to 4-week-old plants were taken (4 mm Ø) and placed with the abaxial side down into a well of a white polystyrene 96-well plate containing 100 μL ddH 2 O and recovered overnight. The next day, the water was replaced by a solution containing 20 µg/mL horseradish peroxidase (HRP, sigma), luminol (17 µg/mL) and elicitor (100 nM for flg22, 100 µg/mL OG 10-15 (Elicityl, GAT114), as stated). Luminescence was immediately measured for 60 minutes using a charge-coupled device camera (Photek Ltd, East Sussex UK). Callose deposition Callose deposition assays were performed as described previously ( Mason et al ., 2020 ). Briefly, four leaves of 4- to 5-week-old plants were syringe-infiltrated with either mock (ddH 2 O), 1 µM flg22 or 100 µg/mL OG 10-15 (Elicityl, GAT114). Twenty-four hours after infiltration, leaf discs were taken and collected in 24-well plates filled with 1 mL 100 % EtOH until completely destained. Leaf discs were equilibrated in 1 mL 67 mM K 2 HPO 4 (pH 12) for 60 min. Afterwards, the tissue was stained using aniline blue (Acros Oganics) staining solution (0.01 % (w/v) aniline blue in 67 mM K 2 HPO 4 (pH 12) for 60 min and washed in 67 mM K 2 HPO 4 (pH=12) for 60 minutes. Stained tissue was mounted in mounting solution (80 % glycerol, 67 mM K 2 HPO 4 , pH 12) on microscope slides. Callose deposits were imaged using a Leica DM6000B and quantified in ImageJ. PR1 protein abundance PR1 accumulation was assayed as previously described ( Bender et al ., 2021 ). Briefly, three leaves of 3-week-old plants were infiltrated with mock (sterile ddH 2 O), 1 µM flg22, 100 µg/mL OG 10-15 (Elicityl, GAT114) or 100 µg/mL OG 3 (GalA3, Megazyme). Twenty-four hours after infiltration, leaves were harvested in 1.5-mL tubes and snap-frozen in liquid nitrogen and pulverized. Extraction buffer (50 mM Tris pH7.5 (HCl), 150 mM NaCl, 10 % (v/v) glycerol, 2 mM EDTA, 1x plant protease inhibitor cocktail) was added and protein concentration was adjusted by Bradford assay. Normalized protein extracts were analyzed by SDS-PAGE (15 %) and immunoblotting using PR1-antibodies (Agrisera). Induced resistance against Pseudomonas syringae Two leaves of 4- to 5-week-old plants were infiltrated with 1 µM flg22 or 100 µg/mL OG 10-15 (Elicityl, GAT114) or mock (sterile ddH 2 O). Freshly restreaked P. syringae pv tomato DC3000 was grown in liquid Kings B overnight and refreshed in a subculture the next morning for additional 1-2 hours. Bacteria were infiltrated into pretreated leaves with an OD 600 of 0.0002. Plants were covered for two days, after which 1 leaf disc was harvested per treated leaf (8 mm Ø) and pooled per plant. Leaf discs were ground in 10 mM MgCl 2 , thoroughly mixed and diluted in a 1:10 series until 1:10 -6 . Samples were plated on LB plates. After two days of growth at 28 °C, colony forming units were counted. Statistics were performed on log 10 (CFU/cm 2 ). Induced resistance against Botrytis cinerea Four leaves of 4- to 5-week-old plants were infiltrated with 1 µM flg22 or 100 µg/mL OG 10-15 (Elicityl, GAT114) or mock (sterile ddH 2 O) in the morning. The next day, spores of B. cinerea BMM were collected in sterile ddH 2 O and the spores were counted using a counting chamber. At least 1 hour prior infection, infection solutions were prepared with a final concentration 5×10 5 spores/mL in 0.5 Potato Dextrose Broth and incubated at RT. Five microliters of the Botrytis infection solution were dropped on the adaxial site next to the middle vein. Plant solid trays were filled with water, covered with a lid, and sealed with parafilm to produce high humidity. After 2 days after infection at dimmed light, leaves were detached, images were taken, and lesion size was measured using Image J. Author Contributions L.H. and C.H. performed the experiments and analyzed the data. B.K. generated the genetic material. T.N., T.A.D and C.Z designed and supervised the project. L.H. wrote the first draft of the manuscript. All authors contributed to the final version of the manuscript. Supplemental table View this table: View inline View popup Download powerpoint SUPPLEMENTAL TABLE 1 Primers used in this study. Acknowledgments We thank all the members of the Zipfel group for fruitful discussions during the project. We thank also Jiashu Chu, John Haidoulis and Jana Ordon for feedback on the manuscript. L.H. was funded by a Zurich-Basel Plant Science Center-Syngenta Fellowship. B.D.K. was supported by National Science Foundation grant IOS 1556057. T.N. was supported by DFG-TRR356 (B5). T.A.D. was supported by a Discovery Grant from the Natural Sciences and Engineering Council of Canada (NSERC RGPIN-2023-04222). 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