1Cell-autonomous immunity is widespread in plant-fungus interactions and terminates fungal pathogenesis either at the cell surface or after pathogen entry. Although post-invasive resistance responses typically coincide with a self-contained cell death of plant cells undergoing attack by parasites, these cells survive pre-invasive defence. Mutational analysis in Arabidopsis identified PEN1 syntaxin as one component of two pre-invasive resistance pathways against ascomycete powdery mildew fungi 1-3 . Here we show that plasma-membrane-resident PEN1 promiscuously forms SDS-resistant soluble N-ethylmaleimide sensitive factor attachment protein receptor (SNARE) complexes together with the SNAP33 adaptor and a subset of vesicle-associated membrane proteins (VAMPs). PEN1-dependent disease resistance acts in vivo mainly through two functionally redundant VAMP72 subfamily members, VAMP721 and VAMP722. Unexpectedly, the same two VAMP proteins also operate redundantly in a default secretory pathway, suggesting dual functions in separate biological processes owing to evolutionary co-option of the default pathway for plant immunity. The disease resistance function of the secretory PEN1-SNAP33-VAMP721/722 complex and the pathogen-induced subcellular dynamics of its components are mechanistically reminiscent of immunological synapse formation in vertebrates, enabling execution of immune responses through focal secretion.Arabidopsis is immune to non-adapted powdery mildew fungi such as Blumeria graminis and Erysiphe pisi, which in nature colonize grass and pea species, respectively. This non-host resistance requires both pre-and post-invasive immune responses, which are under separate genetic control 2 . The former response engages PEN1 syntaxin, peroxisomal PEN2 b-glycosyl hydrolase and the plasmamembrane-resident PEN3 ABC transporter 1-3 . PEN2 and PEN3 act in the same pathway and are implicated in the cytoplasmic synthesis and transport of small antimicrobial compounds across the plasma membrane at attempted fungal entry sites, respectively 2,3 . PEN1 syntaxin acts in a second pathway and could, by analogy to known syntaxin functions in yeast and animals, either participate in vesicle fusion processes 4 or modulate ion-channel activity through interactions with plasma-membrane-resident ion channels 5 . Genetic studies defy mechanistic interpretations but suggest direct or indirect PEN1 repressor activity in defence responses that are dependent on salicylic acid, as well as an overlapping function with the closely related syntaxin of plant 122 (SYP122) 6 . Compared with largely resistant PEN1 wild type and severely defence-compromised pen1-1 null mutants, plants containing the pen1-3 allele allow intermediate B. graminis entry rates, indicating residual PEN1-3 resistance activity ( Supplementary Fig. 1a). In the deduced PEN1-3 protein, a glycine residue is substituted by a glutamate in the SNARE domain 1 (Supplementary Fig. 1b). Because this mutation affects a hydrophobic residue that is thought to stabilize interactions with ...
In yeast and animal cells, members of the superfamily of Nethylmaleimide-sensitive factor adaptor protein receptor (SNARE)-domain-containing proteins are key players in vesicle-associated membrane fusion events during transport processes between individual compartments of the endomembrane system, including exocytosis and endocytosis. Compared with genomes of other eukaryotes, genomes of monocotyledonous and dicotyledonous plants encode a surprisingly high number of SNARE proteins, suggesting vital roles for this protein class in higher plant species. Although to date it remains elusive whether plant SNARE proteins function like their yeast and animal counterparts, genetic screens have recently begun to unravel the variety of biological tasks in which plant SNAREs are involved. These duties involve fundamental processes such as cytokinesis, shoot gravitropism, pathogen defense, symbiosis, and abiotic stress responses, suggesting that SNAREs contribute essentially to many facets of plant biology.
Root hairs are fast-growing tubular protrusions on root epidermal cells that play important roles in water and nutrient uptake in plants. The tip-focused polarized growth of root hairs is accomplished by the secretion of newly synthesized materials to the tip via the polarized membrane trafficking mechanism. Here, we report the function of two different types of plasma membrane (PM) Qa-SNAREs (soluble N-ethylmaleimide-sensitive factor attachment protein receptors), SYP123 and SYP132, in the growth of root hair in Arabidopsis. We found that SYP123, but not SYP132, localizes in the tip region of root hairs by recycling between the brefeldin A (BFA)-sensitive endosomes and the PM of the expanding tip in an F-actin-dependent manner. The vesicle-associated membrane proteins VAMP721/722/724 also exhibited tip-focused localization in root hairs and formed ternary SNARE complexes with both SYP123 and SYP132. These results demonstrate that SYP123 and SYP132 act in a coordinated fashion to mediate tip-focused membrane trafficking for root hair tip growth.
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