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. 2015 Jan 30;10(1):e0116385. doi: 10.1371/journal.pone.0116385

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© 2015 Xu et al

This is an open-access article distributed under the terms of the Creative Commons Attribution License, which permits unrestricted use, distribution, and reproduction in any medium, provided the original author and source are properly credited.

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(A) Interaction tests using yeast two-hybrid assays between AGB1 and AtMPK6. Yeast cells with AGB1 (AD-AGB1) and AtMPK6 (BD-MPK6) were placed in different liquid concentrations on control medium SD/-Trp/-Leu (SD/LT) and selection medium SD/-Trp/-Leu/-His/-Ade (SD/LTHA). For negative controls, pGBKT7 without insert (BD alone), pGADT7 without insert (AD alone), and the empty vectors AD and BD were used. Experiments were performed three times and a representative result is shown. (B) AGB1 interacted with AtMPK6 by BiFC assays in Arabidopsis protoplast. The recombinant constructs AGB1-YFP^N (YFP N-terminal) and MPK6-YFP^C (YFP C-terminal) were co-transformed into protoplast cells of Arabidopsis WT (Col-0). For negative controls, pSPYNE without insert AGB1 (YFP^N) (iii) and pSPYCE without insert MPK6 (YFP^C) (ii) were used. The combination of bZIP63-YFP^N and bZIP63-YFP^C was used as a positive control (iiii), Fluorescence was recorded 20 h after transformation. Experiments were performed 10 times and a representative result is shown. Bars = 40 μm in (i), (iii) and (iiii), and 20 μm in (ii). (C) Interaction assay using pull-down analysis. AGB1 and AtMPK6 fused with GST and His tags, respectively were mixed and passed through a glutathione column (binding GST tag). After elution with pull-down binding buffer, samples were separated by SDS-PAGE, and His-MPK6 was detected by immunoblotting with anti-His antibody. GST alone was used as the negative control. Experiments were performed three times and a representative result is shown. (D) Co-IP assay of AGB1 with AtMPK6. AGB1-Flag and MPK6-Myc or AGB1-Flag and empty pCAMBIA1300 vector (contained Myc-tags) were transiently co-transformed into Arabidopsis protoplast. After 16 h, the total Arabidopsis cell lysates were prepared for Co-IP with anti-Myc agarose. Then, anti-Myc immunoprecipitates were subjected to Western blot analysis with anti-Flag antibody (top). Meanwhile, the total cell lysates were also subjected to Western blot analysis with anti-Flag (middle), and anti-Myc (bottom, for MPK6-Myc expression) antibodies. Experiments were performed three times and a representative result is shown.