Developmental Biology

SMAD4 promotes somatic-germline contact during murine oocyte growth

Sofia Granados-Aparici author has email address
Qin Yang
Hugh Clarke author has email address

Research Institute, McGill University Health Centre, 1001 Boul. Décarie, Montréal, QC, Canada H4A 3J1
Cancer CIBER (CIBERONC), Madrid
Pathology Department, Medical School, University of Valencia-INCLIVA, Valencia
Departments of Obstetrics and Gynecology and Biology, Division of Experimental Medicine, McGill University

https://doi.org/10.7554/eLife.91798.2

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Figures and data

SMAD4 is efficiently depleted in granulosa cells of GOCs in vitro using tamoxifen-induced Cre recombinase
A. Immunoblot of primordial follicles, growing follicles, and granulosa cells and oocytes isolated from antral follicles, probed using anti-SMAD4 and anti-SMAD2/3.
B. Breeding scheme to delete Smad4 in the granulosa cells using Amhr2-Cre. The mTmG cassette enables Cre recombinase activity to be verified through expression of EGFP.
C. Left: Confocal images of histological sections of paraffin-embedded 12-d ovary (i, ii) and an isolated follicle (iii) stained using an anti-GFP antibody and DAPI to counterstain DNA. Relatively few granulosa cells are GFP-positive (arrow in iii). Scale bars: 50 µm, 20 µm, 10 µm. Right: Histogram and chart showing the percentage of FACS-sorted GFP+ and GFP-granulosa cells from growing follicles. Granulosa cells expressing both td tomato and GFP and GFP alone were scored as GFP+.
D. Breeding scheme to delete Smad4 in vitro using generate tamoxifen-inducible ER-Cre. The mTmG cassette enables Cre recombinase activity to be verified through expression of EGFP.
E. Left: Schematic illustrating time-line of GOC exposure to tamoxifen and subsequent incubation. Center: Bright-field image of GOCs following incubation and confocal image of a representative GOC stained using anti-GFP antibody and DAPI to counterstain DNA. Scale bar = 10µm and 100µm, respectively. Right: Bar chart showing the percentage of FACS-sorted GFP+ and GFP-granulosa cells from GOCs. Granulosa cells expressing td tomato and GFP and GFP alone are counted as GFP+.
F. Left: Confocal image of representative GOCs stained with single-molecule RNA FISH probe for Smad4 exon 8 and DAPI to counterstain DNA. Right: Mean and SEM of the average number of Smad4 mRNA foci per cell (left) and relative mRNA amounts of Smad4 quantified using qRT-PCR (right) in granulosa cells five days after tamoxifen treatment.
G. Immunoblot and plot of mean and SEM of SMAD4 protein content in granulosa cells from GOCs five days after tamoxifen treatment.
Statistical analysis using t-test (F, left) and one-sample t-test (F, right and G), ***P< 0.001; ****P < 0.0001.

Depletion of SMAD4 reduces TZP-number but does not affect granulosa cell communication with the oocyte or proliferation.
A. Confocal images of GOCs five days after tamoxifen treatment stained with anti-GFP, phalloidin to visualize F-actin and DAPI to counterstain DNA. Arrow shows GFP-labelled TZPs. Scale bar = 20 µm.
B. Mean and SEM of oocyte diameter and TZP number five days after tamoxifen treatment. TZP number in each GOC is normalized to the oocyte diameter.
C. Confocal image of a denuded GOC five days after tamoxifen treatment and removal of the granulosa cells, stained with anti-GFP, phalloidin to visualize F-actin and DAPI to counterstain DNA. Arrow shows phalloidin-labelled TZPs that remain embedded in the zona pellucida. Scale bar = 20µm.
D. Mean and SEM of oocyte diameter and TZP number five days after tamoxifen treatment in denuded GOCs. TZP number for each specimen is normalized to the oocyte diameter.
E. Left: Time course of fluorescence recovery in oocyte of GOCs following bleaching. Each line represents an individual GOC. Right: Mean and SEM of the ratio of the final to pre-bleach fluorescence in each GOC.
F. Left: Confocal image of a GOC after tamoxifen treatment followed by treatment with EdU and visualization. DNA stained using DAPI. Scale bar = 20 µm. Right: Mean and SEM of the ratio of Edu-labelled cells to the total number of cells.
Statistical analysis using t-test, *P< 0.05; ****P < 0.0001; ns, not significant.

Depletion of SMAD4 in GOCs reduces the number of TZPs per granulosa cell and alters their morphometric parameters.
A. Schematic illustrating the experimental protocol. GFP+ granulosa cells in clusters were used for calculations in C and individual GFP+ granulosa cells were used for calculations in D.
B. Three-dimensional reconstruction of a GOC, showing granulosa cell bodies, TZPs and oocyte cortex. Serial optical confocal sections were processed using Imaris software. GOCs were stained using anti-GFP (green), phalloidin (red) and DAPI (blue). Scale bar = 10 µm (upper, middle), 3 µm (lower).
C. Mean and SEM of volumes and sphericities of individual granulosa cells from a cluster and those selected for TZP analyses.
D. Mean and SEM of volumes of individual granulosa cells selected for TZP analysis, number of TZPs per cell, TZP length and width.
Statistical analysis using t-test, ****P < 0.0001; ns, non-significant.

Depletion of SMAD4 in reaggregates reduces the number of newly generated TZPs and alters their morphometric parameters.
A. Schematic illustrating the reaggregation procedure.
B. Three-dimensional reconstruction of a reaggregate, showing granulosa cell bodies, TZPs and oocyte cortex. Serial optical confocal sections were processed using Imaris software. GOCs were stained using anti-GFP (green), phalloidin (red) and DAPI (blue). Scale bar =10 µm (upper), 3 µm (lower).
C. Mean and SEM of volumes and sphericities of individual granulosa cells.
D, E Mean and SEM of volumes of individual granulosa cells, number of TZPs per cell, TZP length and TZP width.
F. Upper: Schematic illustrating how the distance from the origin and the tip, respectively, of TZPs (blue) and non-TZP projections (red) to the oocyte surface was determined. Lower: TZP trajectories of 3D-reconstructed TZPs, representing the distance from origin relative to the position on the TZP axis.
G. Left: Mean and SEM of the difference between the distance from the origin and the tip of individual TZPs to the oocyte surface. Blue symbols (>0) represent TZPs oriented towards the oocyte; red symbols (<0) represent non-TZPs oriented away from the oocyte. Right: Mean and SEM of the proportion of TZPs in individual cells that were oriented away from the oocyte.
Statistical analysis using t-test, *P < 0.05; **P < 0.01; ****P < 0.0001; ns, non-significant.

Expression of transmembrane N-cadherin and Notch proteins is reduced in SMAD4-depleted granulosa cells.
A. Immunoblot and graph showing mean and SEM of SMAD4 and N-cadherin in granulosa cells. Protein quantities are normalized to amounts in ER-Cre^- cells.
B. As in A, showing Notch2.
C. Mean and SEM of relative mRNA amounts of Smad4, Cdh2 (encoding N-cadherin), and Notch2 in granulosa cells purified from GOCs five days after tamoxifen treatment. mRNA quantities are normalized to amounts in ER-Cre^- cells.
D. As in C, showing Smad4, Myo10, Fscn1 and Daam1.
Statistical analysis using one-sample t-test, ***P < 0.001; ****P < 0.0001; ns non-significant.

Model for regulation of the size of the TZP population.
Upper: Dynamics of an individual TZP. When growing TZP contacts the surface of the oocyte, it becomes stably attached if there is sufficient N-cadherin, as in wild-type cells. In SMAD4-depleted cells, there is insufficient N-cadherin to stabilize the attachment. The TZP may continue to elongate but eventually becomes retracted. Lower: Dynamics of the population of TZPs. Owing to increased stability of attachment of individual TZPs to the oocyte surface, the total number of TZPs becomes larger in wild-type cells than in SMAD4-depleted cells.

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