The roots of most higher plants form arbuscular mycorrhiza, an ancient, phosphate-acquiring symbiosis with fungi, whereas only four related plant orders are able to engage in the evolutionary younger nitrogen-fixing root-nodule symbiosis with bacteria. Plant symbioses with bacteria and fungi require a set of common signal transduction components that redirect root cell development. Here we present two highly homologous genes from Lotus japonicus, CASTOR and POLLUX, that are indispensable for microbial admission into plant cells and act upstream of intracellular calcium spiking, one of the earliest plant responses to symbiotic stimulation. Surprisingly, both twin proteins are localized in the plastids of root cells, indicating a previously unrecognized role of this ancient endosymbiont in controlling intracellular symbioses that evolved more recently.
The mechanism underlying perinuclear calcium spiking induced during legume root endosymbioses is largely unknown. Lotus japonicus symbiosis-defective castor and pollux mutants are impaired in perinuclear calcium spiking. Homology modeling suggested that the related proteins CASTOR and POLLUX might be ion channels. Here, we show that CASTOR and POLLUX form two independent homocomplexes in planta. CASTOR reconstituted in planar lipid bilayers exhibited ion channel activity, and the channel characteristics were altered in a symbiosis-defective mutant carrying an amino acid replacement close to the selectivity filter. Permeability ratio determination and competition experiments reveled a weak preference of CASTOR for cations such as potassium over anions. POLLUX has an identical selectivity filter region and complemented a potassium transport-deficient yeast mutant, suggesting that POLLUX is also a potassium-permeable channel. Immunogold labeling localized the endogenous CASTOR protein to the nuclear envelope of Lotus root cells. Our data are consistent with a role of CASTOR and POLLUX in modulating the nuclear envelope membrane potential. They could either trigger the opening of calcium release channels or compensate the charge release during the calcium efflux as counter ion channels.
SUMMARYIntracellular invasion of root cells is required for the establishment of successful endosymbioses in legumes of both arbuscular mycorrhizal (AM) fungi and rhizobial bacteria. In both interactions a requirement for successful entry is the activation of a common signalling pathway that includes five genes required to generate calcium oscillations and two genes required for the perception of the calcium response. Recently, it has been discovered that in Medicago truncatula, the Vapyrin (VPY) gene is essential for the establishment of the arbuscular mycorrhizal symbiosis. Here, we show by analyses of mutants that the same gene is also required for rhizobial colonization and nodulation. VPY encodes a protein featuring a Major Sperm Protein domain, typically featured on proteins involved in membrane trafficking and biogenesis, and a series of ankyrin repeats. Plants mutated in this gene have abnormal rhizobial infection threads and fewer nodules, and in the case of interactions with AM fungi, epidermal penetration defects and aborted arbuscule formation. Calcium spiking in root hairs in response to supplied Nod factors is intact in the vpy-1 mutant. This, and the elevation of VPY transcripts upon application of Nod factors which we show to be dependent on NFP, DMI1, and DMI3, indicates that VPY acts downstream of the common signalling pathway.
Nuclear-associated Ca(2+) oscillations mediate plant responses to beneficial microbial partners--namely, nitrogen-fixing rhizobial bacteria that colonize roots of legumes and arbuscular mycorrhizal fungi that colonize roots of the majority of plant species. A potassium-permeable channel is known to be required for symbiotic Ca(2+) oscillations, but the calcium channels themselves have been unknown until now. We show that three cyclic nucleotide-gated channels in Medicago truncatula are required for nuclear Ca(2+) oscillations and subsequent symbiotic responses. These cyclic nucleotide-gated channels are located at the nuclear envelope and are permeable to Ca(2+) We demonstrate that the cyclic nucleotide-gated channels form a complex with the postassium-permeable channel, which modulates nuclear Ca(2+) release. These channels, like their counterparts in animal cells, might regulate multiple nuclear Ca(2+) responses to developmental and environmental conditions.
Legumes overcome nitrogen shortage by developing root nodules in which symbiotic bacteria fix atmospheric nitrogen in exchange for host-derived carbohydrates and mineral nutrients. Nodule development involves the distinct processes of nodule organogenesis, bacterial infection, and the onset of nitrogen fixation. These entail profound, dynamic gene expression changes, notably contributed to by microRNAs (miRNAs). Here, we used deep-sequencing, candidate-based expression studies and a selection of Lotus japonicus mutants uncoupling different symbiosis stages to identify miRNAs involved in symbiotic nitrogen fixation. Induction of a noncanonical miR171 isoform, which targets the key nodulation transcription factor Nodulation Signaling Pathway2, correlates with bacterial infection in nodules. A second candidate, miR397, is systemically induced in the presence of active, nitrogen-fixing nodules but not in that of noninfected or inactive nodule organs. It is involved in nitrogen fixation-related copper homeostasis and targets a member of the laccase copper protein family. These findings thus identify two miRNAs specifically responding to symbiotic infection and nodule function in legumes.
We have established tools for forward and reverse genetic analysis of the legume Lotus (Lotus japonicus). A structured population of M2 progeny of 4,904 ethyl methanesulfonate-mutagenized M1 embryos is available for single nucleotide polymorphism mutation detection, using a TILLING (for Targeting Induced Local Lesions IN Genomes) protocol. Scanning subsets of this population, we identified a mutation load of one per 502 kb of amplified fragment. Moreover, we observed a 1:10 ratio between homozygous and heterozygous mutations in the M2 progeny. This reveals a clear difference in germline genetics between Lotus and Arabidopsis (Arabidopsis thaliana). In addition, we assembled M2 siblings with obvious phenotypes in overall development, starch accumulation, or nitrogen-fixing root nodule symbiosis in three thematic subpopulations. By screening the nodulation-defective population of M2 individuals for mutations in a set of 12 genes known to be essential for nodule development, we identified large allelic series for each gene, generating a unique data set that combines genotypic and phenotypic information facilitating structure-function studies. This analysis revealed a significant bias for replacements of glycine (Gly) residues in functionally defective alleles, which may be explained by the exceptional structural features of Gly. Gly allows the peptide chain to adopt conformations that are no longer possible after amino acid replacement. This previously unrecognized vulnerability of proteins at Gly residues could be used for the improvement of algorithms that are designed to predict the deleterious nature of single nucleotide polymorphism mutations. Our results demonstrate the power, as well as the limitations, of ethyl methanesulfonate mutagenesis for forward and reverse genetic studies. (Original mutant phenotypes can be accessed at http://data.jic.bbsrc.ac.uk/cgi-bin/lotusjaponicus. Access to the Lotus TILLING facility can be obtained through
Sandal et al. MPMI 4 INTRODUCTIONGenetic analysis and application of genetic approaches in the model legume Lotus japonicus (Handberg and Stougaard 1992) has progressed rapidly. Several key genes important for symbiosis with mycorrhizal fungi, root nodule development and other developmental processes have been identified using molecular genetics. The developmental regulators Nin (Schauser et al. 1999) and Pfo (Zhang et al. 2002) were isolated by transposon tagging while map-based cloning led to the molecular characterisation of Har1, SymRK, Nfr1, Nfr5, Castor and Pollux involved in autoregulation, Nod-factor signal perception or signal transduction (Schauser et al. 1999, Krusell et al. 2002 Nishimura et al. 2002a;Stracke et al. 2002;Radutoiu et al. 2003;Madsen et al. 2003; Imaizumi-Anraku et al. 2005). Genetic loci required for the early stages of endosymbiosis have attracted particular interest. Diallelic crosses together with phenotypical studies defined seven loci, SymRK, Nup133, Castor, Pollux, Sym6, Sym15,Sym24, in the common pathway required for both rhizobial and mycorrhizal symbiosis (Kistner et al. unpublished data) and map-based cloning of these loci has been accomplished or is advancing rapidly. A similar interest and effort is now emerging for genetic dissection of nodule organogenesis and function using the Fix -mutants arrested at various stages of nodule development or impaired in nodule function. Cloning of the Sst1 sulfate transporter required in functional root nodules is a first example (Krusell et al. 2005).Continuous isolation of new plant mutant lines is important for completing the genetic dissection of symbiosis and so far six independent mutant populations have been obtained by chemical (EMS) mutagenesis (Perry et al. 2003;Szczyglowski et al. 1998; Webb et al. unpublished data; Gresshoff et al. unpublished data), four populations after T-DNA or transposon insertion mutagenesis (Thykjaer et al. 1995;Schauser et al. 1998;Webb et al. 2000; Gresshoff et al. unpublished data), one population made with fast neutrons (Gresshoff et al. unpublished Umehara and Kouchi (unpublished data). All in all more than 400 symbiotic Lotus mutant lines were identified by screening in these populations and more are likely to follow. Assignment to complementation groups is next logical step in order to determine the number of loci involved, identify all alleles that contribute to phenotypic characterisation of mutants and genotyping of loci. However, diallelic crossing is a relatively slow process where progress is determined by generation time and slowed by a continuously increasing number of individual crosses necessary to keep up with mutant isolation programs. Given the number of symbiotic mutant lines already available and considering the time used to define seven complementation groups with a total of 26 alleles constituting the common pathway (Kistner et al. unpublished data), this approach is unlikely to encompass all alleles in near future. Detection of alleles in already cloned genes ...
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