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. 2023 Feb 3;19(2):e1010621. doi: 10.1371/journal.pgen.1010621

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© 2023 Li 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 credited.

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Fig 6 — (A-B) GFP-RPG (green) and TGN/EE marker SYP61-mCherry (magenta) were co-expressed in N. benthamiana leaf cells (A) or L. japonicus root protoplasts (B). (C) Co-expressed RPG-CERBERUS BiFC construct (yellow) and NLS-DsRed (magenta) in N. benthamiana leaf cells. Plots (A‴-C‴) show fluorescence intensities of the regions of interest (indicated by white line in [A″-C″]). (D) Confocal images of SPPR1-GFP in L. japonicus WT, rpg-1 and cerberus-12 transgenic roots inoculated with M. loti R7A/lacZ 2 days after Brefeldin-A induced BFA body formation. E, Quantification of BFA bodies size in WT, rpg-1 and cerberus-12 expressing SPPR1-GFP after 2 h BFA treatment. Asterisks indicate significant differences (Students t-test), between mutants and WT (error bars represent SE). Scale bars: 25 μm (A, C); 20 μm (B); 200 μm (D).