A Two-Hybrid-Receptor Assay Demonstrates Heteromer Formation as Switch-On for Plant Immune Receptors

Receptor kinases sense extracellular signals and trigger intracellular signaling and physiological responses. However, how does signal binding to the extracellular domain activate the cytoplasmic kinase domain? Activation of the plant immunoreceptor Flagellin sensing2 (FLS2) by its bacterial ligand flagellin or the peptide-epitope flg22 coincides with rapid complex formation with a second receptor kinase termed brassinosteroid receptor1 associated kinase1 (BAK1). Here, we show that the receptor pair of FLS2 and BAK1 is also functional when the roles of the complex partners are reversed by swapping their cytosolic domains. This reciprocal constellation prevents interference by redundant partners that can partially substitute for BAK1 and demonstrates that formation of the heteromeric complex is the molecular switch for transmembrane signaling. A similar approach with swaps between the Elongation factor-Tu receptor and BAK1 also resulted in a functional receptor/coreceptor pair, suggesting that a “two-hybrid-receptor assay” is of more general use for studying heteromeric receptor complexes.Cell surface receptors are chemical sensors, often with an exquisite specificity and sensitivity, which detect extracellular signals and initiate corresponding intracellular response programs. Many of these receptors are transmembrane proteins with an extracellular ligand-binding domain and an intracellular protein kinase domain. Higher plants, such as Arabidopsis (Arabidopsis thaliana), have several hundred genes encoding receptor like kinases (Shiu and Bleecker, 2001; Shiu and Li, 2004). How are these receptor like kinases activated by their ligands, and how do they initiate a subsequent intracellular signaling cascade? In our work, we used the leucine-rich repeat receptor kinase (LRR-RK) Flagellin sensing2 (FLS2), which specifically detects bacterial flagellin or its peptide epitope flg22 at subnanomolar concentrations (Gomez-Gomez and Boller, 2000; Gómez-Gómez et al., 2001; Chinchilla et al., 2006). FLS2 undergoes heteromeric complex formation with brassinosteroid receptor1 associated kinase1 (BAK1) within seconds after application of the flagellin-derived peptide ligand flg22 (Chinchilla et al., 2007; Heese et al., 2007; Schulze et al., 2010). Thus, BAK1 might act as a coreceptor of FLS2. However, as previously observed (Chinchilla et al., 2007; Roux et al., 2011), FLS2 is still functional in the absence of BAK1, although with a reduced efficiency. This raises the question whether the ligand-induced heteromeric complex has merely an enhancing effect or whether association with BAK1 or a functional substitute acts as the essential switch-on for transmembrane signaling of FLS2. BAK1 is one of the five members that form the somatic embryogenesis receptor kinase (SERK) family (Albrecht et al., 2008), and other members of this family might partially substitute for BAK1 (Roux et al., 2011). However, a rigorous genetic approach to delineate the role of these potential substitutes is not feasible because triple mutants (serk1 serk3 serk4) and quadruple mutants (serk1 serk2 serk3 serk4) exhibit severe general phenotypes of dwarfing or even lethality at the early embryo stage (He et al., 2007; Gou et al., 2012) that might be due to the important role of SERKs in plant developmental processes (Li et al., 2002; Nam and Li, 2002).To address the role of the heteromeric complex with BAK1 in the absence of other interfering SERKs, we took a two-hybrid-receptor approach based on the premise that the apoplastic and cytoplasmic domains of FLS2 and BAK1 function in a modular manner. A heteromeric complex might thus also form and function when the roles of FLS2 and BAK1 are reversed by reciprocal swapping of their cytoplasmic protein kinase domains (Fig. 1A, schematic view).Open in a separate windowFigure 1.Heteromeric complex formation of FLS with BAK1 switches on flagellin-dependent transmembrane signaling. A, Model for the flg22-dependent heteromeric receptor complex. Schematic representation of FLS2 (blue), BAK1 (red), and the chimeric receptor constructs Ftm-B and Btm-F. Ftm-B comprises the extracellular and the transmembrane domains of FLS2 (blue) and the cytoplasmic domain of BAK1 (red). The receptor chimera Btm-F represents the reciprocal construct with the cytoplasmic part of BAK1 replaced by that of FLS2. The cytoplasmic domain of FLS2 was C-terminally tagged with a GFP. B and C, Functional comparison of native FLS2 and BAK1 (B) with the two hybrid receptors Ftm-B and Btm-F (C). The experiments show luciferase activity in Arabidopsis fls2 bak1-4 double mutant protoplasts cotransformed with pFRK1::Luciferase as a reporter and the receptor constructs indicated. At 0 h (dashed line) protoplasts were treated with 100 nm of flg22 (black diamonds) or 100 nm of the inactive analog flg22^Atum (white circles). Light emission of the protoplasts was measured with a luminometer. Values represent averages and sds of three replicates. Data shown are representative for at least three independent repetitions of the experiments with all constructs. D and E, Dose-response relationship for flg22-dependent induction of pFRK1::Luciferase in protoplasts expressing the receptor constructs indicated. Values represent increase in luciferase activity after 5 h of treatment as percentage of the increase observed with FLS2 plus BAK1 treated with saturating doses of greater than or equal to 10 nm flg22. Comparison of (half-maximal stimulation values in D and E shows that cells coexpressing Ftm-B plus Btm-F responded at least as sensitive to flg22 as cells coexpressing FLS2 plus BAK1. A combination of Ftm-B with the kinase dead version Btm-F_KD was not functional, even when treated with 1,000 nm flg22. LU, Light units.