Crystal structure of the plant dual-affinity nitrate transporter NRT1.1

被引:0
|
作者
Ji Sun
John R. Bankston
Jian Payandeh
Thomas R. Hinds
William N. Zagotta
Ning Zheng
机构
[1] Box 357280,Department of Pharmacology
[2] University of Washington,Department of Physiology and Biophysics
[3] Box 357290,undefined
[4] University of Washington,undefined
[5] Howard Hughes Medical Institute,undefined
[6] Box 357280,undefined
[7] University of Washington,undefined
[8] Present address: Department of Structural Biology,undefined
[9] Genentech Inc.,undefined
[10] South San Francisco,undefined
[11] California 94080,undefined
[12] USA.,undefined
来源
Nature | 2014年 / 507卷
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摘要
Nitrate is a primary nutrient for plant growth, but its levels in soil can fluctuate by several orders of magnitude. Previous studies have identified Arabidopsis NRT1.1 as a dual-affinity nitrate transporter that can take up nitrate over a wide range of concentrations. The mode of action of NRT1.1 is controlled by phosphorylation of a key residue, Thr 101; however, how this post-translational modification switches the transporter between two affinity states remains unclear. Here we report the crystal structure of unphosphorylated NRT1.1, which reveals an unexpected homodimer in the inward-facing conformation. In this low-affinity state, the Thr 101 phosphorylation site is embedded in a pocket immediately adjacent to the dimer interface, linking the phosphorylation status of the transporter to its oligomeric state. Using a cell-based fluorescence resonance energy transfer assay, we show that functional NRT1.1 dimerizes in the cell membrane and that the phosphomimetic mutation of Thr 101 converts the protein into a monophasic high-affinity transporter by structurally decoupling the dimer. Together with analyses of the substrate transport tunnel, our results establish a phosphorylation-controlled dimerization switch that allows NRT1.1 to uptake nitrate with two distinct affinity modes.
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页码:73 / 77
页数:4
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