Growth and survival of the mammalian embryo within the uterine environment depends on the placenta, a highly complex vascularized organ comprised of both maternal and foetal tissues. Recent experiments demonstrate that the zinc finger transcriptional repressor Prdm1/Blimp1 is essential for specification of spiral artery trophoblast giant cells (SpA-TGCs) that invade and remodel maternal blood vessels. To learn more about functional contributions made by Blimp1+ cell lineages here we perform the first single-cell RNA-seq analysis of the placenta. Cell types of both foetal and maternal origin are profiled. Comparisons with microarray datasets from mutant placenta and in vitro differentiated trophoblast stem cells allow us to identify Blimp1-dependent transcripts enriched in SpA-TGCs. Our experiments provide new insights into the functionally distinct cell types present at the maternal–foetal interface and advance our knowledge of dynamic gene expression patterns controlling placental morphogenesis and vascular mimicry.
Placenta development is a highly dynamic process that requires coordinately regulated growth of the foetal capillary network in concert with expansion, and extensive remodelling of the maternal uterine vasculature by the invading embryonic trophoblasts. This specialized organ is essential for gas and nutrient exchange, production of hormones that regulate maternal and foetal physiology, and maternal tolerance of the foetal allograft.
Shortly after implantation the trophectoderm (TE) layer of the blastocyst expands and differentiates to form the extraembryonic ectoderm (ExE) and the ectoplacental cone (EPC), which in turn gives rise to the spongiotrophoblast (SpT) layer adjacent to maternal blood spaces. Subsequent placental morphogenesis leads to formation of a diverse set of trophoblast cell types distinguishable by localization, morphology and marker gene expression. A discrete trophoblast subset migrates into the maternal decidua to replace the lining of the spiral arteries and become spiral artery-associated trophoblast giant cells (SpA-TGCs). In addition, derivatives of the ExE-derived chorionic ectoderm give rise to subtypes that closely interact with foetal endothelial cells within the labyrinth region. Formation of these specialized trophoblast cell types is essential to insure adequate blood flow within the placenta during pregnancy. Defective remodelling of the maternal vasculature has been associated with preeclampsia, intrauterine growth restriction and miscarriage1,2.
The zinc finger transcriptional repressor Prdm1/Blimp1, originally identified as a silencer of β-interferon gene expression and a master regulator of plasma cell differentiation, controls cell fate decisions in the developing embryo and governs tissue homoeostasis in multiple cell types in the adult organism3. Developmental arrest of Prdm1 mutant embryos at around embryonic day 10.5 (E10.5) is due to placental defects. Prdm1 expression has been described in EPC-derived diploid trophoblasts and terminally differentiated giant cell types, including SpA-TGCs and glycogen trophoblasts (GlyTs), as well as endothelial cells within the labyrinth, and as yet ill-characterized maternal cells overlying the SpT4. Blimp1 function is required for specification of SpA-TGCs, proper expansion of the labyrinth region of the placenta and remodelling of the maternal vasculature4. Our microarray profiling of Prdm1 mutant vs wild type E9.5 placenta revealed dramatically reduced expression of SpA-TGC-specific markers.
The principal confounding factor intrinsic to previous tissue-wide studies is the loss of cell type-specific expression data among the population average. In all likelihood, the signal-to-noise ratio in our experiments examining Blimp1-dependent transcripts in the placenta was substantially dampened by contributions from Blimp1-independent cell types. Recent advances in RNA-seq technology have made it possible to profile gene expression at a single-cell level. This technology is proving to be a particularly powerful tool for the analysis of complex tissues containing diverse cell populations. For example, elegant single-cell RNA-seq (scRNA-seq) experiments recently identified molecularly distinct cell types within the distal lung epithelium5.
Here we exploit scRNA-seq methodology to profile Prdm1+ cell subpopulations in the developing placenta. Our data reveal differences between conventional foetal endothelial cells and so-called “vascular mimicry” functions performed by invading trophoblasts that remodel maternal spiral arteries. We describe transcriptional signatures characteristic of decidual stromal cells and uterine natural killer (uNK) cells present at the maternal–foetal interface, as well as trophoblast subsets responsible for hormone production during pregnancy. Collectively our data provides a blueprint for understanding transcriptional networks and signalling cues underlying trophoblast invasion and vascularity, and will be a valuable resource for future studies of mammalian placentation.
Isolation of Prdm1+ single cells from E9.5 placentae
We previously found that Prdm1 is expressed in SpA-TGCs, GlyTs, a percentage of proliferative diploid trophoblasts within the SpT layer, foetal endothelial cells of the labyrinth, as well as undefined cell types of maternal origin within the decidua4. To characterize unique transcriptional signatures of diverse cell types in the developing placenta, we decided to profile Blimp1+ subpopulations by scRNA-seq. A Prdm1-Venus fluorescent BAC transgenic reporter previously used to study primordial germ cells in vitro and in vivo6,7 is strongly expressed in the placenta. Histological experiments confirmed co-expression of the paternally inherited Prdm1-Venus and our previously described LacZ knock-in reporter alleles4 in invasive TGCs, diploid trophoblasts, as well as a subset of endothelial cells in the labyrinth. In addition, ectopic Venus transgene expression was occasionally observed in LacZ negative cells (Fig. 1a).
Recent lineage tracing experiments revealed Prdm1 expression in a subset of proliferative diploid trophoblasts representing SpA-TGC progenitors4. Tfap2c and Gjb3 are known to be expressed in diploid trophoblasts and loss-of-function mutants display precocious trophoblast differentiation8,9,10. Immunostaining of Prdm1LacZ placenta for the Gjb3 gene product Cx31 revealed considerable overlap between LacZ and Cx31 expression in diploid Prdm1+ trophoblasts within the SpT (Fig. 1a). Thus, Tfap2c and Gjb3 are promising candidate marker genes for identification of SpA-TGC progenitors.
To isolate cells for scRNA-seq analysis, we carefully trimmed away maternal decidual tissue and enzymatically dissociated E9.5 placentae from embryos expressing the paternally derived Venus transgene. By flow cytometry we detected two distinct populations, namely R2 consisting of small single cells, and R3 consisting of cell clusters and large cells visible in forward/side scatter profiles (Fig. 1b). Venus+ cells, present in both regions were enriched by sorting (Method #1). Single diploid Venus+ cells were recovered within R2. In contrast, R3 contained Venus+ cells in small clusters. In addition, Hoechst 33342 staining identified TGCs containing large nuclei (Fig. 1b). However, recovery of Venus+ TGCs was disappointingly low, presumably due to their fragile nature.
To enrich for Venus+ TGCs we dissected the distal tip of the SpT layer together with the surrounding maternal tissue, followed by gentle enzymatic digestion (Fig. 1b). This alternative method (#2) yielded both large Venus+ cells, and Venus– maternal cells localized at the foetal–maternal interface (Fig. 1b). As summarized in Table 1, a total of 448 single cells or clusters of diploid cells were selected for further analysis. cDNAs (complementary DNAs) were initially screened for expression of Prdm1, Venus, Prl7b1, Tfap2c and Gjb3 to distinguish maternal vs foetal populations, and identify putative SpA-TGCs and their progenitors. Using these selection criteria 78 samples including those positive for Prdm1+; Venus+ (embryonic), Prl7b1, Tfap2c or Gjb3, as well as 18 of 39 Prdm1+; Venus– (maternal) samples were chosen for scRNA-seq analysis.
Single-cell RNA-seq identifies discrete Prdm1+ cell types
Hierarchical clustering of the data revealed two distinct groups, each containing three clear subdivisions designated 1A–C and 2A–C (Fig. 2a). Principle component analysis (PCA) using all 15,402 detected genes revealed the same six distinct groups. Interestingly, group 2C contains numerous single cells together with the cell clusters recovered from R3, suggesting these correspond to the same cell type (Table 2). To further explore relationships between these six groups and identify genes that best describe the variance in the dataset, we performed linear dimensional reduction, followed by PCA on the resulting 1,007 genes (Fig. 2b). The top principle components reveal similarities shared between groups 1A and 2A, groups 1C and 2B, and a subset of group 2B with group 2C (Fig. 2b). In addition, we performed t-distributed stochastic neighbour embedding (tSNE) analysis using RaceID11. This methodology similarly identified the same six groups (Supplementary Fig. 1). Identification of genes significantly enriched in each group highlighted common features within these groups (Fig. 2c and Supplementary Data 1).
Comparisons with well-characterized marker genes subsequently allowed us to identify individual cell types represented by these groups. Endogenous Prdm1 transcripts were detectable in cells of all six groups (though only in a small minority of group 2B), (Fig. 3a). Paternally inherited Prdm1-Venus transcripts were selectively present in groups 1C–2C. Groups 1A and 1B are therefore of maternal origin. Group 1A expresses high levels of decidual stroma markers including Prl8a2 (ref. 12) and Cryab13 (Fig. 3b). Analysis of the markers Eomes and Cd244 (ref. 14) strongly suggests that group 1B corresponds to uNK cells (Fig. 3b). Consistent with this possibility, immunostaining experiments demonstrate that Eomes+ cells co-express the uNK cell marker Dolichos biflorus agglutinin lectin (DBA) (Supplementary Fig. 2a).
Venus+ group 1C cells of foetal origin express high levels of three generic trophoblast markers Krt8, Tfap2c and Gata3. In addition, group 1C expresses high levels of Prl7d1, reported to be widely expressed across diverse trophoblast subtypes12 (Fig. 3c). Interestingly expression of Gjb3 and Prl7d1 seems to be mutually exclusive, suggesting that Gjb3 expression may be restricted to an immature subpopulation, whereas Prl7d1 is a marker of differentiating trophoblasts.
Group 1C cells were also found to be strongly express Blimp1-dependent markers Prl7b1 and Rgs5 (Fig. 3a)4 suggesting these cells represent either invasive SpA-TGCs or GlyTs. To distinguish SpA-TGCs vs GlyTs, we analysed several additional members of the rodent Prolactin (Prl) gene family, known to be expressed by distinct trophoblast subtypes12. Group 1C cells express high levels of Prl2c2, Prl2c3, Prl2c5 and Prl5a1, known to be strongly expressed in SpA-TGCs, but not GlyTs (Supplementary Fig. 3a). In addition, group 1C cells express the vascular signalling receptor Kdr (formerly Flk1/Vegfr2; Fig. 3d)15. Interestingly X-gal staining experiments demonstrate expression of a paternally inherited Kdr.LacZ reporter15 in SpA-TGCs as well as foetal endothelial cells, confirming that group 1C contains SpA-TGCs (Fig. 3d).
We found that group 2A Venus+; Prdm1+ cells weakly co-express Krt8 and Prl7d1 (Fig. 3a,c). Downregulated Krt8 expression has been linked to endoreduplication in parietal TGCs (P-TGCs)16. Consistent with their endoreduplicating cell status, group 2A cells express high levels of multiple histones, (Supplementary Fig. 3b). Prdm1+ P-TGCs were not previously observed at E9.5 (ref. 4). However, we found here that Prdm1+ P-TGCs were detectable at slightly later stages, in E12.5 placenta (Fig. 3e). It is therefore tempting to speculate that these moderately sized group 2A cells, largely devoid of Prl gene expression correspond to immature Prdm1+ P-TGCs. Group 2B diploid cells strongly express trophoblast markers including Gjb3, and as discussed below appear to represent TGC progenitors. The group 2C Venus+ cells, expressing high levels of Kdr, but low levels of trophoblast markers, and in all likelihood correspond to Prdm1+ allantoic endothelial cells (Fig. 3d).
Intriguingly, numerous transcripts were expressed by both group 2A (large cells of foetal origin) and 1A (decidual stromal cells), including the decidual marker genes Prl8a2 and Cryab (Figs 2c and 3b). To exclude technical issues such as the presence of doublets or cross-contamination during single-cell isolation, we expanded the analysis to identify additional transcripts. The results shown in Supplementary Fig. 4 clearly demonstrate that many of the group 1A highly expressed genes are entirely absent from group 2A. While it is formally possible that these surprising results could potentially reflect fusion of a subpopulation of foetal TGCs with maternal decidual cells, we suggest that the more plausible explanation is that these curious findings reflect bona fide transcriptional signatures of the discrete group 1A and group 2A cells both influenced by common signalling events at the maternal–foetal interface. It will be interesting to compare 1A and 2A transcriptional signatures as documented in the present report with additional pregnancy single-cell RNA-seq datasets as they become available.
Evidence that group 2B are trophoblast progenitors
Self-renewing, multipotent trophoblast stem (TS) cells derived from either blastocysts or the ExE differentiate in vitro to form mature trophoblast cell types17. To further characterize about the cell types defined by our scRNA-seq dataset and learn more about Blimp1-dependent transcripts we isolated a panel of wild type and Prdm1-deficient TS cell lines. Western blot and immunostaining experiments demonstrate Prdm1/Blimp1 expression is upregulated by day 2 of differentiation in diploid trophoblasts and maintained in a subset of TGCs that undergo endoreduplication (Fig. 4a and Supplementary Fig. 5a). Gjb3 expression is readily detectable in wild type control TS cells whereas the SpA-TGC marker Prl7b1 appears later as Gjb3 declines (Fig. 4b).
To test the hypothesis that Gjb3+ diploid cells are progenitor trophoblasts, while large Prl7b1+ cells are terminally differentiated, TGCs we performed a microarray timecourse and then analysed the expression characteristics of genes enriched in groups 2B and 1C. Group 2B cells display a clear bias towards genes showing highest expression in TS cells or early differentiation, consistent with the idea that these are trophoblast progenitors (Fig. 4c). To further explore this possibility we assessed expression of cell cycle markers18 represented in our scRNA-seq dataset. Both foetal endothelial cells (2C) and Gjb3+ trophoblasts (2B) showed the highest expression of cell cycle genes (Fig. 4d). Collectively the results demonstrate that group 2B cells bear all the expected hallmarks of trophoblast progenitors.
To distinguish SpA-TGCs from Gjb3+ trophoblast progenitors we compared genes enriched in groups 1C and 2B. We found that markers strongly expressed by invasive trophoblasts, Cts7, Cts8 (ref. 19) and Tpbpa20 are absent in Gjb3+ trophoblasts (Fig. 5a). Interestingly, Gjb3+ trophoblasts display enriched expression of genes with deleterious placental loss-of-function phenotypes (Fig. 5b).
Identification of SpA-TGC-enriched Blimp1-dependent genes
Next we examined our microarray data to search for Blimp1-dependent transcripts. The profiles of wild type and Prdm1 mutant TS cells were initially indistinguishable. However, significant divergence was observed subsequently in differentiating cultures (Supplementary Fig. 5b). As expected Blimp1-deficient TGCs fail to express the SpA-TGC marker Prl7b1 (Fig. 4b). Functional analysis of transcripts downregulated in Prdm1–/– trophoblasts showed strong enrichment for genes required for blood vessel and extraembryonic tissue development, as well as normal embryonic growth (Supplementary Fig. 5c). Moreover, comparison of the present microarray dataset with results of our previous profiling experiments analysing wild type vs mutant E9.5 placenta4 revealed a small subset of overlapping downregulated transcripts including several SpA-TGC marker genes, that is, Prl7b1 and Rgs5 (Supplementary Fig. 5d).
We exploited our scRNA-seq dataset to directly compare Blimp1-dependent genes expressed by SpA-TGCs or Gjb3+ progenitor trophoblasts (Fig. 5c). As shown in Fig. 5d numerous Blimp1-dependent transcripts detectable in differentiating TS cell cultures, including Plxnd1 and Pla2g4d show SpA-TGC-enriched expression in vivo. Thus their absence in Prdm1 mutants probably reflects selective loss of the SpA-TGC lineage.
Functionality predicted by cell type-specific transcription
The six cell types defined by our scRNA-seq analysis and their corresponding marker gene expression fits well with their defined size differences, that is, large TGCs vs relatively small endothelial cells (Table 2). Consistent with the identification of group 1C as SpA-TGCs and group 2B as immature trophoblast progenitors both these cell populations show strikingly similar expression profiles (Fig. 2b). Interestingly, 3 of the 12 group 2B cells express genes characteristic of group 2C endothelial cells (orange box in Fig. 2c), highlighting the functional similarities between trophoblasts and endothelial cells21. Notably, the one exceptional small cell within group 1C expressing high levels of Gjb3 together with low levels of Prl7b1 and Prl7d1, potentially represents a SpA-TGC progenitor undergoing terminal differentiation (Fig. 3a,c).
Functional annotation analysis of the genes differentially expressed by each of the six groups provides insight into their distinct functional activities. For example, the decidual stromal cell transcriptome governs placental morphogenesis, differentiation, blood vessel morphology and regulation of endothelial behaviour through sphingolipid metabolism. Interestingly, we found the peptide hormone Adm is highly expressed in this cell population (Fig. 6b). Adm, previously identified as a P-TGC marker is also a key regulator of uNK cells22. uNK cells are thought to destroy the surrounding vascular smooth muscle cells and restrict the extent of SpA-TGC invasion during spiral artery remodelling23,24. The present results strongly suggest that decidual stromal cells, also regulate Adm-mediated recruitment of uNK cells. Group 2A cells express Adm and the P-TGC marker Cyp11a1 (ref. 25) (Supplementary Fig. 3c). Mature P-TGCs were recently shown to express the cell–cell adhesion molecule Cd34 (ref. 26). Interestingly group 2A cells similarly express Cd34, consistent with the possibility they represent immature P-TGCs (Fig. 7a).
The cell type-specific transcriptional signatures described here refine our understanding of the pathways controlling placental vascularity. For example, Wnt4 (ref. 27) and the Angiopoietins Angpt2 (ref. 28) and Angpt4 (ref. 29) were found to be highly expressed in the decidual stroma (Fig. 6b), whereas the Angiopoietin receptors Tek and Tie1, as well as Cd34 and pericyte recruitment factor Pdgfb30, largely restricted to endothelial cells were undetectable in SpA-TGCs (Fig. 7a). On the other hand, numerous other endothelial cell markers were expressed at similar levels in both SpA-TGCs and endothelial cells, for example, Flt4 and Pecam1 (Fig. 7a,b and Supplementary Fig. 3d). Overall our experiments have identified a plethora of novel genes regulating placental development and trophoblast function. Figure 8 presents a summary overview of the cell type-specific transcriptional signatures defined in the present report.
Gene targeting studies have revealed essential functions performed by key transcription factors, signalling molecules and membrane glycoproteins controlling cell–cell interactions during placental development31. Changes in gene expression profiles associated with many of these loss-of-function phenotypes have also been characterized via microarray experiments. Our recent experiments demonstrate that developmental arrest of Prdm1 mutant embryos at around E10.5 is associated with loss of the invasive SpA-TGC cell lineage4. In addition, lineage tracing experiments identified a population of proliferating Blimp1+ diploid cells present within the SpT that give rise to mature SpA-TGCs, canal TGCs and GlyTs.
The SpA-TGC lineage mediates key functions during pregnancy including decidual invasion, vascular mimicry leading to increased blood flow, evasion of maternal immune response, and hormonal regulation of maternal physiology and behaviour. However, isolation and characterization of this crucially important mature TGC subset has been technically challenging due to their fragile nature and intimate association with the maternal vasculature. Consequently, the transcriptional programmes governing their complex behaviour remain ill defined. The present scRNA-seq analysis provides new insights into their cell type-specific transcriptional signatures and defines the key functionally distinct cell subpopulations present at the maternal–foetal interface, as summarized in Fig. 8.
We identified a number of transcripts selectively expressed by SpA-TGCs, including genes consistent with their invasion, vascular and endocrine functions (Figs 5c,d and 7c). Pak1 is known to promote trophoblast invasion in gestational trophoblastic disease in human32. Nitric oxide production via Nos1 promotes vasodilation and increased blood flow. The peptide hormone Agrp is linked to obesity and enhanced appetite33. The semaphorin receptor Plxnd1 expressed in both endothelial cells and SpA-TGCs, regulates Vegf signalling34 by promoting expression of soluble Flt1 (sFlt1), a Vegf decoy receptor, to limit angiogenic potential35. sFlt1 is known to be produced by SpA-TGCs36. Two Blimp1-dependent phospholipase A2 family enzymes, Pla2g4d and Pla2g4f, potentially act downstream Vegf receptor Kdr to promote production of the vasodilator prostacyclin37. The hypoxia-induced extracellular matrix remodelling factor P4ha2 (ref. 38), marker of tumour vasculature Igfbp7 (ref. 39), as well as Gpc1, a co-receptor for heparin-binding growth factors such as FGFs and modulator of angiogenesis and metastasis of human and mouse tumours40 were also downregulated in the absence of Blimp1. Interestingly, the present experiments demonstrate for the first time that SpA-TGCs express the Vegf receptor Kdr. Recent studies have shown that Vegf activates Blimp1 expression in tumour vasculature41. It will be interesting to learn whether Vegf signalling similarly upregulates Blimp1 expression during SpA-TGC specification.
Our results clearly demonstrate that SpA-TGCs are well equipped to suppress harmful consequences of vascular remodelling. The galectin Lgals9 attenuates immune response by signalling via its receptor Havcr2 on immune cells (Supplementary Fig. 3e)42. In addition, Gpr77/C5ar2 proposed to be a decoy receptor involved in evasion of the complement pathway43, as well as Ccbp2/Ackr2, a decoy receptor thought to prevent spontaneous miscarriage by attenuating inflammatory responses44, both G-protein coupled receptor family genes, were found to be specifically expressed by SpA-TGCs (Figs 6a and 7c). SpA-TGCs strongly express both Entpd1 and Procr known to prevent thrombosis and inflammation (Fig. 5a)45,46. Procr loss-of-function mutants exhibit mid-gestation lethality due to placental thrombosis.
Comparisons of uNK cells profiled here with splenic NK1.1+ RNA-seq datasets strengthens the idea that uNK cells represent a unique NK subset. NK marker genes including Eomes, Cd122, Cd123 and Prf1 (perforin)14 were strongly expressed, but group 1B (uNK) cells lack expression of numerous other genes associated with NK activation (Supplementary Fig. 2b). Ifnγ is known to be a Blimp1 target in T effector cells3 and human NK cells47. Consistent with repressed cytolytic function, here we found Blimp1+ uNK cells express low levels of Ifnγ compared with splenic NK cells. It will be interesting to further investigate NK cell heterogeneity using scRNA-seq technology.
Recent advances in microfluidics and automation technologies have proven invaluable for profiling single cells with similar sizes and morphological characteristics in studies where prior enrichment for rare cell types and maintenance of viability were not complicating factors48,49. However, diverse cell subsets within the placenta display vastly different sizes and adhesion properties. Here TGCs exhibiting a broad range of morphologically distinct features were manually isolated. The present experiments provide the first comprehensive survey of gene expression profiles in individual placental cell types. Our data establishes hierarchical relationships between these cell type-specific transcriptional profiles, and reveals numerous novel marker genes for future study of placental development. Building on previous placental disruption methods50,51, here we established reliable methods suitable for isolating cell types of interest, subsequently selected by brute force screening of libraries for marker genes. The present study provides new insights into key aspects of mammalian placental development, while informing future experimentation into vascular mimicry, immune tolerance and hormone signalling.
The Prdm1BEH null allele, Prdm1Cre-nLacZ, Prdm1-Venus and KdrLacZ mouse strains were genotyped according to published protocols4,6,15,52. Males from the various reporter strains (C57BL/6J, 2–4 months of age) were crossed with wild type females (CD-1 from Charles River Laboratories, 6–12 weeks of age) to ensure reporter gene expression marked only tissues of embryonic origin. Experiments were performed in accordance with Home Office regulations.
TS cell culture and differentiation
TS cell lines were derived from individual blastocysts obtained from Prdm1+/BEHx Prdm1+/BEHintercrosses and genotyped as previously described17,52. TS cells were adapted for growth under defined conditions53. To induce differentiation trypsinized TS cells were plated in the absence of FGF4, TGFβ1 and heparin sulphate. Four independent cell lines of each genotype were used for all experiments.
For immunohistochemistry tissue was fixed in 4% paraformaldehyde (PFA) in PBS overnight at 4 °C, paraffin embedded and sectioned (6 μm). For immunofluorescence tissue was fixed overnight in 1% PFA in PBS at 4 °C, cryo-protected in 30% sucrose, embedded in O.C.T. Compound (Tissue-Tek) and sectioned (10 μm). In some instances X-gal staining was performed on cryosections followed by immunostaining. For immunostaining, sections were blocked for 1 h in 5% foetal bovine serum/0.2% bovine serum albumin in PBS at room temperature followed by overnight incubation with primary antibody in blocking buffer at 4 °C. For immunostaining of cells grown on Matrigel-coated glass coverslips, samples were fixed in 4% PFA in PBS for 10 min at room temperature, permeabilised with 2.5% Triton-X100 in PBS for 10 min, blocked with 10% Donkey serum for 1 h followed by overnight incubation with primary antibody in blocking buffer at 4 °C. Primary antibodies were detected by incubation with an appropriate secondary, and in some cases a tertiary Alexa Fluor-conjugated antibody (Molecular probes). Sections were mounted in VECTASHIELD containing DAPI (Vector Laboratories). Primary antibodies used were rabbit anti-GFP (Invitrogen, A-31851, 1:500), rabbit anti-Cx31 (Alpha Diagnostics, CX31-A, 1:200), monoclonal rat anti-Blimp1 (clone 5E7, Santa Cruz SC-130917, 1:500) and rabbit anti-Eomes (Abcam, ab23345, 1:100).
For in situ hybridization tissue was fixed overnight in 4% PFA, dehydrated in ethanol, paraffin embedded, and sectioned (6 μm). Riboprobe synthesis and RNA in situ hybridization was performed according to standard protocols using mid-plane sections. For Adm and Angpt4 PCR fragments amplified from E9.5 placenta were cloned into pBlueScript KS- using primers indicated in Supplementary Table 1 prior to probe synthesis. IMAGE clone 3966337 was used for Cd34. The Flt4 probe was a kind gift from Heiko Lickert.
Isolation of single cells and cell clusters
Placentae from CD-1 females mated to Prdm1-Venus males were harvested at E9.5 and the yolk sac and decidual tissue trimmed away being careful to leave the labyrinth and SpT layers intact. Prdm1-Venus+ placentae were identified by fluorescent imaging of the corresponding embryo.
Pools of three placentae were finely minced with spring scissors and digested in Liberase TM (Roche, 0.325 Wunsch u ml−1) and DNase 1 (Sigma-Aldrich, 20 Kunitz u ml−1) in DMEM supplemented with 15% FCS, 10% Medium NCTC-109 (Gibco), 15 mM HEPES, 0.1 mM non-essential amino acids, 2 mM Glutamine and 1% Hybri-Max OPI Media Supplement (Sigma-Aldrich). Digestion was performed for 45 min at 37 °C in a shaking incubator. Samples were vigorously pipetted every 10 min to assist tissue disassociation.
After centrifugation, cell pellets were resuspended, incubated in Accumax (Sigma-Aldrich) for 10 min at 37 °C then filtered through 100 μm mesh. Venus+ single diploid cells, diploid cell clusters and giant cells were gated on forward vs side scatter profiles and GFP fluorescence using a MoFlo XDP Flow cytometer (Beckman Coulter). Viable cells were identified by 7AAD exclusion. High-resolution images were captured using an ImageStreamX Mk II imaging flow cytometer (AMNIS) and analysed using IDEAS software (AMNIS).
Due to low recovery of Venus+ giant cells using FACS, giant cells were also manually picked from SpT tissue after enzymatic disassociation. To enrich for Venus+ TGCs, the distal tip of the SpT layer proximal to the maternal artery was used.
Preparation of single-cell cDNAs and sequencing
Cell suspensions were diluted to low density and single cells or clusters of 2–3 cells specifically selected under phase-contrast microscopy and picked directly into lysis buffer by mouth pipette, followed by synthesis and amplification of cDNA precisely as previously described54. To identify potential cells of interest, qPCR was performed using QuantiTect SYBR Green PCR kits on a Rotor-Gene Q (QIAGEN) using primer pairs detailed in Supplementary Table 1. Purified cDNAs from cells of interest were then subjected to Illumina sequence library preparation and sequencing on an Illumina HiSeq 2500.
RNA-seq data analysis
Sequence reads were mapped to the mm9 mouse genome release with Stampy using default parameters55. Read pairs with identical outer coordinates were reduced to a single pair. Numbers of remaining properly paired reads per sample are reported in Supplementary Table 2. Reads were then assigned to gene annotations of Ensembl release 67 using HTSeq-count56. To normalize raw gene intensities between libraries, scaling factors were calculated using a trimmed mean of M-values between each pair of samples within the six identified groups using edgeR57. Hierarchical clustering was performed in R. Further analysis was performed using Seurat, an R package for single-cell genomics, which has been extensively described previously49,58. We filtered out cells expressing <3,000 genes, and genes detected in <3 cells. This resulted in 78 cells expressing a total of 15,402 genes. Details of number of genes detected per cell per group are provided in Supplementary Fig. 6. Dimensional reduction was performed and significant principle components (P<1 × 10−2) identified on the basis of 200 random samplings, each time permuting 1% of genes. PCA projection was then performed and the top 300 significant genes (P≤1 × 10−5) from each significant principle component selected giving a total of 1,007 genes describing the variance in the dataset. Significant genes identified by this method were used for PCA using princomp in R. Genes significantly enriched in each group revealed by hierarchical clustering were identified using the t-test algorithm in Seurat (P≤1 × 10−3 was considered significant). Identification of cell groups using RaceID and t-distributed stochastic neighbour embedding was performed using the spearman clustering metric11. Functional annotation of the resulting gene lists relative to KEGG Pathways, Wikipathways, mammalian phenotype and Gene Ontology terms was performed with WebGestalt using default parameters59. Endothelial markers referred to in Fig. 7a,b were defined by Takase et al.60.
Western blot analysis
Cell lysates were analysed by western blot, using a rat anti-Blimp1 monoclonal antibody (Santa Cruz, sc-130917, 1:500) and rabbit anti-Tubulin polyclonal antibody (Santa Cruz, sc-9104, 1:1,000). All uncropped western blots can be found in the Supplementary Fig. 7.
TS and TG cells were directly lysed on plates at the indicated timepoints and total RNA prepared with an RNeasy MiniKit (Qiagen) with DNase treatment according manufacturers protocol. Microarray experiments were performed using Illumina Mouse WG-6 v2 Expression BeadChips. Microarray data was analysed using rank-invariant normalization and Mann–Whitney options of the Gene Error Model Expression Analysis Module V1.6.0 of GenomeStudio V2009 (Illumina). K-means clustering was performed using Cluster 3.0 (ref 61). Phenotypic analysis of differentially expressed genes was performed using Enrichr62.
Single cell RNA-seq and microarray data have been deposited in the NCBI Gene Expression Omnibus (GEO) database under accession code GSE74410.
How to cite this article: Nelson, A. C. et al. Single-cell RNA-seq reveals cell type-specific transcriptional signatures at the maternal–foetal interface during pregnancy. Nat. Commun. 7:11414 doi: 10.1038/ncomms11414 (2016).
Gene Expression Omnibus
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We thank Ita Costello for valuable advice and discussions, Nigel Rust for excellent assistance with FACS sorting, Janet Rossant for KdrLacZ mice, Xin Sun for performing in situ hybridizations and the High-Throughput Genomics Group at the Wellcome Trust Centre for Human Genetics for generating the microarray and sequencing data (funded by Wellcome Trust Grant 090532/Z/09/Z). This work was funded by Programme Grants 059312 (EJR) and 089157 (EKB) from the Wellcome Trust. E.J.R. is a Wellcome Trust Principal Research Fellow.
The authors declare no competing financial interests.
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Nelson, A., Mould, A., Bikoff, E. et al. Single-cell RNA-seq reveals cell type-specific transcriptional signatures at the maternal–foetal interface during pregnancy. Nat Commun 7, 11414 (2016). https://doi.org/10.1038/ncomms11414
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