Fig 2: Lack of fetus-derived IGF2 reduces the expansion of feto-placental microvasculature in late gestation(A) Functions enriched in DEGs at E19.(B) qRT-PCR analysis of angiopoietin-Tie2/TEK signaling components in Lz (n = 6–8 per group).(C) TUNEL (terminal deoxynucleotidyl transferase dUTP nick end labeling) staining in E16 Lz (arrows point to apoptotic cells) and data quantification (n = 6 samples per group); scale bars, 50 µm.(D) Left: representative double immunostaining for TUNEL (red) and laminin (green, marker of feto-placental capillaries) in the Lz of an E16 Igf2EpiKO mutant placenta (DAPI, blue marks the nuclei; white and red arrows indicate TUNEL+ FPECs and LT, respectively; scale bars, 25 µm). Right: quantification of TUNEL+ cells that are positive or negative for laminin (n = 6 Igf2EpiKO mutant placentae).(E) Feto-placental endothelial cell (FPEC) proliferation measured by flow cytometry (left—representative histograms at E16; right—data quantification; n = 4–11 per group).(F) qRT-PCR analysis of Adgre1 in Lz.(G) Representative F4/80 immunostainings in E16 Lz (arrows indicate macrophages). Scale bars, 100 µm. Right: percentage of macrophages/Lz at E16 (n = 6–8 samples per group).(H) Representative CD31 immunostaining in Lz (scale bars, 100 µm).(I) qRT-PCR analysis for SynT-II (syncytiotrophoblast layer II) marker genes. For all graphs, data are presented as averages or individual values; error bars are SD; *p < 0.05, **p < 0.01, ***p < 0.001 by two-way ANOVA plus Sidak’s multiple comparisons tests in (B), (C), (E), (F), and (I) or Mann-Whitney tests in (G). See also Figure S4 and Table S2.

Fig 3: Lz expansion is associated with increasing levels of circulating and endothelial IGF2(A) Weights of micro-dissected Lz.(B) Linear correlation analyses between fetal and Lz weights: p = 0.002 (E14), p < 0.0001 (E16), and p < 0.0001 (E19) (n = 46–189 placentae from n > 10 L per group in [A] and [B]).(C) Levels of IGF2 (ng/mL) in plasma of wild-type fetuses.(D) Linear correlation analyses between fetal weights and circulating IGF2: p < 0.0001 (E16 and E19) (n = 70–79 per group in [C] and [D]).(E) Igf2 mRNA in situ hybridization (blue) in E14 wild-type Lz (red arrows—FPEC, feto-placental endothelial cells; AS, antisense probe; inset with S, sense probe; scale bars, 20 µm).(F) Relative Igf2 mRNA expression levels measured by qRT-PCR in FPEC from wild-type Lz (n = 6–7 per group).(G) Imprinted genes that rank within top 100 expressed genes in E16 wild-type FPEC (FPKM, fragments per kilobase million; n = 4).(H) Double immunostaining for IGF2 and CD31 in E19 wild-type placenta. Endothelial cells are very thin and hard to detect except where the cytoplasm is more voluminous around the nucleus, with intense IGF2 stain (white arrows). Transmembrane glycoprotein CD31 immunostaining is in the membrane and largely marks endothelial intercellular junctions (scale bars, 20 µm).(I) Semi-quantitative measurement of IGF2 protein in FPEC versus trophoblast cells (E19 wild-type Lz, n = 60 cells per group from two placentae). White arrows—endothelial cells; scale bars, 50 µm. For (E), (H), and (I): FC, fetal capillaries; MBS, maternal blood spaces; LT, labyrinthine trophoblast cells; S-TGC, sinusoidal trophoblast giant cells. Data in (A), (C), (F), (G), and (I) are presented as averages ± standard deviation (SD); ***p < 0.001 calculated by one-way ANOVA plus Tukey’s multiple comparisons test in (A) and (F) or by unpaired t test with Welch’s correction in (C) and (I). See also Table S1.

Fig 4: Deletion of Igf2 in the epiblast or endothelium impairs Lz expansion(A) Left: schematic of Igf2 expression in conceptuses with conditional deletion driven by Meox2Cre. Right: immunostaining for YFP (green) in a representative fetus and placenta paraffin section at E12 of gestation, double transgenic for Meox2Cre and Rosa26flSTOPflYFP10 reporter. YFP expression in the placenta is localized to the Lz and Cp (high magnification, inset). Blue—DAPI stain for nuclei; scale bars: 1 mm (low magnification) and 100 µm (high magnification).(B) Fetal and placental growth kinetics, measured as average wet-weights for each genotype per litter (E12: n = 10 L [n = 41 controls {C} and n = 32 Igf2EpiKO]; E14: n = 25 L [n = 114 C and n = 88 Igf2EpiKO]; E16: n = 37 L [n = 154 C and n = 127 Igf2EpiKO]; E19: n = 37 L [n = 164 C and n = 121 Igf2EpiKO]).(C) Absolute volumes of the placental layers (Db, decidua basalis; Jz, junctional zone; Lz, labyrinthine zone; Cp, chorionic plate), measured by stereology (n = 6 per group).(D) Absolute volumes of Lz components, measured by stereology (LT, labyrinthine trophoblast; MBSs, maternal blood spaces; FCs, fetal capillaries) (n = 6 per group).(E) Left: schematic representation of Igf2 expression in conceptuses with conditional deletion driven by TekCre. Right: representative confocal microscopy of frozen sections from a fetus and its corresponding placenta, double transgenic for TeKCre and Ai9(RCL-tdT) reporter at E16 of gestation. Scale bars: 2 mm (fetus) and 1 mm (placenta).(F) Fetal and placental growth kinetics (E12: n = 5 L [n = 17 C and n = 16 Igf2ECKO]; E14: n = 8 L [n = 26 C and n = 34 Igf2ECKO]; E16: n = 13 L [n = 60 C and n = 46 Igf2ECKO]; E19: n = 7 L [n = 31 C and n = 27 Igf2ECKO]).(G) Absolute volumes of the placental layers measured by stereology (n = 5–7 per group).(H) Absolute volumes of Lz components, measured by stereology (n = 5–7 per group).(I) Double immunostaining for EPCAM (epithelial cell adhesion molecule) (red) and MCT1 (monocarboxylate transporter 1) (green) in a representative frozen placental section at E12 of gestation. EPCAM expression is observed as clusters of positive cells within the Lz placenta. Blue—DAPI (4',6-diamidino-2-phenylindole) stain for nuclei; scale bars: 500 µm (left panel) and 20 µm (right panel).(J) Analysis of EPCAMhigh-positive cells by flow cytometry. Left panel: example of gating used to identify EPCAMhigh-positive cells (the viability dye 7-aminoactinomycin D [7-AAD] was used to exclude dead cells). Right: quantification of placental EPCAMhigh-positive cells at E12 in conceptuses with conditional Igf2 deletion driven by Meox2Cre (n = 10 C and n = 9 Igf2EpiKO from 2 L) or TekCre (n = 8 C and n = 8 Igf2ECKO from 2 L). For all graphs data are shown as averages; error bars represent SD in (C), (D), (G), (H), and (J) or 95% confidence intervals (95% CI) in (B) and (F); N.S.—statistically not significant; *p < 0.05; **p < 0.01; ***p < 0.001 calculated by a mixed effects model in (B) and (F) (see STAR Methods), two-way ANOVA plus Sidak’s multiple comparisons tests in (D) and (H) or unpaired t tests in (C), (G), and (J). See also Figures S1–S3.

Fig 5: Heterogeneity and Distinct Injury Response of Immune Cells(A) UMAP representation of different myeloid cell populations analyzed.(B) Heatmap showing expression of top enriched genes for each myeloid cell sub-population.(C–G) UMAP plots showing expression of Cd86, an M1-macrophage marker gene (C); Arg1, an M2-macrophage marker gene (D); Plac8, a monocyte-enriched gene (E); Ly6c2, an M1 monocyte-enriched gene (F); and Naaa, a DC-like cell enriched gene (G).(H) Percentage of each immune cell population over total nonmyocytes within each sample.(I) UMAP plot showing expression of Clcf1 among different cell types present in the P1+1 dpi and dps scRNA-seq data.(J) Representative images showing EdU incorporation (magenta) and cardiac troponin T (cTnT) immunofluorescent staining (green) of NRVM cells treated with 200 ng/mL BSA (negative control), 20 ng/mL recombinant insulin-like growth factor 2 (IGF2) (positive control), or different concentrations of recombinant CLCF1 (5, 10, 25, and 50 ng/mL). Scale bar, 100 µm.(K) Quantification showing the proportion of EdU-positive cells among cTnT-positive cells (CM) after treatment of BSA, CLCF1 recombinant protein, or recombinant IGF2 (n = 4 per each group; **p < 0.01, ****p < 0.0001).See also Figure S7.