Epithelial polarization by the core planar cell polarity complex is exclusively non-autonomous

Devenport, Danelle 1 ; Posfai, Eszter 1 ; Basta, Lena 1 ; Joyce, Bradley 1

Published Mar 18, 2025 on Dryad. https://doi.org/10.5061/dryad.bvq83bkkb

Data files

Mar 18, 2025 version files 230.96 MB

Abstract

For cells to polarize collectively along a tissue plane, asymmetrically localized planar cell polarity (PCP) complexes must form intercellular contacts between neighboring cells. Yet, it is unknown whether asymmetric segregation of PCP complexes requires cell-cell contact, or if cell- autonomous, antagonistic interactions are sufficient for polarization. To test this, we generated mouse chimeras consisting of dual PCP-reporter cells mixed with unlabeled cells that cannot form PCP bridges. In the absence of intercellular interactions, PCP proteins failed to polarize cell autonomously. Rather, PCP-mediated contacts along single cell-cell interfaces were sufficient to sort PCP components to opposite sides of the junction, independent of junction orientation. Thus, intercellular binding of PCP complexes is the critical step that initiates sorting of opposing PCP complexes to generate asymmetry.

https://doi.org/10.5061/dryad.bvq83bkkb

Description of the data and file structure

This dataset contains all data crucial to the key findings of this study, including original raw images of chimeric embryonic skin (ads5704_RawImages.zip), data analysis (*ads5704_Data.xlsx), and scripts (ads5704_MATLAB scripts.zip). Using embryo aggregation, we generated mouse chimeras to test the hypothesis of whether planar cell polarity (PCP) can arise cell autonomously in the absence of intercelullar PCP interactions. The raw data is uploaded in original format allowing for replication of presented analyses and further analysis or interpretation.

Files and variables

File: ads5704_Data.xlsx

Description: Excel file containing all quantification of analyses presented in the publication. Each tab in the excel sheet corresponds with a figure as labeled by figure number. Each analyzed cell, cell pair or group of cells is labeled with a number that remains consistent across excel tabs of the same color.

Fig. 1G (tab 1): all data corresponding to Fig. 1G

Embryo: indicates biological replicate
Single cell number: cell identifier, corresponds to number of image in RawImages.zip
Anterior (A) or Posterior (P) cell border: indicates which border, A or P, is analyzed
Border mean intensity (Ij): mean fluorescence intensity of Fz6-3xGFP, tdTomato-Vangl2 and Celsr1 along individual cell borders
Cell mean intensity (Ic): mean fluorescence intensity of Fz6-3xGFP, tdTomato-Vangl2 and Celsr1 of the cell
Junction enrichment (Ij/Ic): ratio of border mean intensity/cell mean intensity

Fig. 1H (tab 2): all data corresponding to Fig. 1H

Embryo: indicates biological replicate
Single cell number: cell identifier, corresponds to number of image in RawImages.zip
Pearson’s coefficient: calculated pearson’s correlation coefficient between Fz6-3xGFP and tdtomato-Vangl2; Fz6-3xGFP and Celsr1; and tdtomato-Vangl2 and Celsr1 along cell border of single cell in Fz6-3xGFP; tdTomato-Vangl2 : WT chimeric skin

Fig. 2E (tab 3): all data corresponding to Fig. 2E

Embryo: indicates biological replicate
Single cell number: cell identifier, corresponds to number of image in RawImages.zip
Pearson’s coefficient: calculated pearson’s correlation coefficient between Fz6-3xGFP and tdtomato-Vangl2; Fz6-3xGFP and Celsr1; and tdtomato-Vangl2 and Celsr1 along cell border of single cell in Fz6-3xGFP; tdTomato-Vangl2 : Celsr1-/- chimeric skin

Fig. 3D (tab 4): all data corresponding to WT:WT junctions in Fig. 3D

Embryo: indicates biological replicate
Cell Pair Number: cell identifier, corresponds to number of image in RawImages.zip
Angle of junction: angle of analyzed junction relative to the AP axis
Border mean intensity (Ij): mean fluorescence intensity of Fz6-3xGFP, tdTomato-Vangl2 and Celsr1 along WT:WT cell junctions between dual-reporter cell pairs in in Fz6-3xGFP; tdTomato-Vangl2 : Celsr1-/- chimeric skin
Cell pair mean intensity (Ic): mean fluorescence intensity of Fz6-3xGFP, tdTomato-Vangl2 and Celsr1 of the cell pair
Junction enrichment (Ij/Ic): ratio of WT:WT border mean intensity/cell pair mean intensity

Fig. 3D (tab 5): all data corresponding to WT:mutant junctions in Fig. 3D

Embryo: indicates biological replicate
Cell Pair Number: cell identifier, corresponds to number of image in RawImages.zip
Angle of junction: angle of analyzed junction relative to the AP axis
Border mean intensity (Ij): mean fluorescence intensity of Fz6-3xGFP, tdTomato-Vangl2 and Celsr1 along WT:mutant cell junctions between dual-reporter cells and surrounding mutant cells in in Fz6-3xGFP; tdTomato-Vangl2 : Celsr1-/- chimeric skin
Cell pair mean intensity (Ic): mean fluorescence intensity of Fz6-3xGFP, tdTomato-Vangl2 and Celsr1 of the cell pair
Junction enrichment (Ij/Ic): ratio of WT:mutant border mean intensity/cell pair mean intensity

Fig. 3E (tab 6): all data corresponding to Fig. 3E

Embryo: indicates biological replicate
Cell Pair Number: cell identifier, corresponds to number of image in RawImages.zip
Junction: indicates analysis of either WT:WT junctions between cell pairs or WT:mutant junctions
Pearson’s coefficient: calculated pearson’s correlation coefficient between Fz6-3xGFP and tdtomato-Vangl2; Fz6-3xGFP and Celsr1; and tdtomato-Vangl2 and Celsr1 along WT:WT or WT:mutant cell borders in Fz6-3xGFP; tdTomato-Vangl2 : Celsr1-/- chimeric skin

Fig. 4D (tab 7): all data corresponding to Fig. 4D

Embryo: indicates biological replicate
WT:WT junction number: junction identifier, corresponds to number of image in RawImages.zip
Angle of junction: angle of analyzed junction relative to the AP axis, all junctions are “vertical” with angles between 45-90
Number of puncta pairs: counted number of puncta pairs in either F:V, V:F or ambiguous orientations per WT junction in large area of WT cells in Fz6-3xGFP; tdTomato-Vangl2 : Celsr1-/- chimeric skin
Percentage of puncta pair orientations: percentages calculated from the counted puncta pairs in the previous columns

Fig. 4M,N (tab 8): all data corresponding to Fig. 4D

Embryo: indicates biological replicate
WT:WT junction number: junction identifier, corresponds to number of image in RawImages.zip
Angle of junction: angle of analyzed junction relative to the AP axis. All junctions with angles between 45-90 are considered vertical, while all junctions with angles between 0-45 are considered horizontal.
Number of puncta pairs: counted number of puncta pairs in either F:V, V:F or ambiguous orientations per WT:WT junction between dual-reporter cell pairs in Fz6-3xGFP; tdTomato-Vangl2 : Celsr1-/- chimeric skin
Percentage of puncta pair orientations: percentages calculated from the counted puncta pairs in the previous columns

Fig. 5 (tab 9): all data corresponding to Fig. 5

Embryo: indicates biological replicate
Cell Group Number: analyzed cell identifier, corresponds to number of image in RawImages.zip, categorized based on orientation of the two WT:WT junctions (both vertical, both horizontal, or with one vertical and one horizontal junction)
Number of cells in group: the number of dual-reporter cells in the cluster of analyzed cells
Junction orientation: designates if the analyzed junction is vertical (between 45-90 degrees relative to the AP axis) or horizontal (between 0-45 degrees relative to the AP axis)
Number of puncta pairs: counted number of puncta pairs in either F:V, V:F or ambiguous orientations per WT:WT junction between dual-reporter cell groups in Fz6-3xGFP; tdTomato-Vangl2 : Celsr1-/- *chimeric skin
Percentage of puncta pair orientations: percentages calculated from the counted puncta pairs in the previous columns

File: ads5704_RawImages.zip

Description: All raw .tif images of analyzed cell, cell pairs or groups of cells are organized into folders corresponding with the figure where analyses are presented. STED super-resolution images uploaded are deconvolved using NIS elements software. All cells, cell pairs, or cell groups are labeled with numbers that correspond with the numbers in the uploaded excel sheet, as described above. Files can be opened and analyzed using ImageJ, Tissue Analyzer or MATLAB.

Code/software

File: ads5704_MATLAB scripts.zip

Description: MATLAB scripts required to analyze PCP protein puncta pair orientations along junctions acquired with STED super-resolution imaging. Data processing and analysis using scripts detailed in materials and methods of this study.