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Molecular and Functional Characterization of Medicago Truncatula Npf17 Gene
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Legumes are unique among plants for their ability to fix atmospheric nitrogen with the help of soil bacteria rhizobia. Medicago truncatula is used as a model legume to study different aspects of symbiotic nitrogen fixation. M. truncatula, in association with its symbiotic partner Sinorhizobium meliloti, fix atmospheric nitrogen into ammonia, which the plant uses for amino acid biosynthesis and the bacteria get reduced photosynthate in return. M. truncatula NPF1.7 previously called MtNIP/LATD is required for symbiotic nitrogen fixing root nodule development and for normal root architecture. Mutations in MtNPF1.7 have defects in these processes. MtNPF1.7 encodes a member of the NPF family of transporters. Experimental results showing that MtNPF1.7 functioning as a high-affinity nitrate transporter are its expression restoring chlorate susceptibility to the Arabidopsis chl1-5 mutant and high nitrate transport in Xenopus laevis oocyte system. However, the weakest Mtnip-3 mutant allele also displays high-affinity nitrate transport in X. laevis oocytes and chlorate susceptibility to the Atchl1-5 mutant, suggesting that MtNPF1.7 might have another biochemical function. Experimental evidence shows that MtNPF1.7 also functions in hormone signaling. Constitutive expression of MtNPF1.7 in several species including M. truncatula results in plants with a robust growth phenotype. Using a synthetic auxin reporter, the presence of higher auxin in both the Mtnip-1 mutant and in M. truncatula plants constitutively expressing MtNPF1.7 was observed. Previous experiments showed MtNPF1.7 expression is hormone regulated and the MtNPF1.7 promoter is active in root and nodule meristems and in the vasculature. Two potential binding sites for an auxin response factors (ARFs) were found in the MtNPF1.7 promoter. Chromatin immunoprecipitation-qRT-PCR confirmed MtARF1 binding these sites. Mutating the MtARF1 binding sites increases MtNPF1.7 expression, suggesting a mechanism for auxin repression of MtNPF1.7. Consistent with these results, constitutive expression of an ARF in wild-type plants partially phenocopies Mtnip-1 mutants’ phenotypes.
Title: Molecular and Functional Characterization of Medicago Truncatula Npf17 Gene
Description:
Legumes are unique among plants for their ability to fix atmospheric nitrogen with the help of soil bacteria rhizobia.
Medicago truncatula is used as a model legume to study different aspects of symbiotic nitrogen fixation.
M.
truncatula, in association with its symbiotic partner Sinorhizobium meliloti, fix atmospheric nitrogen into ammonia, which the plant uses for amino acid biosynthesis and the bacteria get reduced photosynthate in return.
M.
truncatula NPF1.
7 previously called MtNIP/LATD is required for symbiotic nitrogen fixing root nodule development and for normal root architecture.
Mutations in MtNPF1.
7 have defects in these processes.
MtNPF1.
7 encodes a member of the NPF family of transporters.
Experimental results showing that MtNPF1.
7 functioning as a high-affinity nitrate transporter are its expression restoring chlorate susceptibility to the Arabidopsis chl1-5 mutant and high nitrate transport in Xenopus laevis oocyte system.
However, the weakest Mtnip-3 mutant allele also displays high-affinity nitrate transport in X.
laevis oocytes and chlorate susceptibility to the Atchl1-5 mutant, suggesting that MtNPF1.
7 might have another biochemical function.
Experimental evidence shows that MtNPF1.
7 also functions in hormone signaling.
Constitutive expression of MtNPF1.
7 in several species including M.
truncatula results in plants with a robust growth phenotype.
Using a synthetic auxin reporter, the presence of higher auxin in both the Mtnip-1 mutant and in M.
truncatula plants constitutively expressing MtNPF1.
7 was observed.
Previous experiments showed MtNPF1.
7 expression is hormone regulated and the MtNPF1.
7 promoter is active in root and nodule meristems and in the vasculature.
Two potential binding sites for an auxin response factors (ARFs) were found in the MtNPF1.
7 promoter.
Chromatin immunoprecipitation-qRT-PCR confirmed MtARF1 binding these sites.
Mutating the MtARF1 binding sites increases MtNPF1.
7 expression, suggesting a mechanism for auxin repression of MtNPF1.
7.
Consistent with these results, constitutive expression of an ARF in wild-type plants partially phenocopies Mtnip-1 mutants’ phenotypes.
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