Abstract
Uterine glands are essential for pregnancy in mice and likely humans, because they secrete or transport bioactive substances that regulate uterine receptivity for blastocyst implantation. In mice, the uterus becomes receptive to blastocyst implantation on day 4, but is refractory by day 5. Here, blastocysts could be recovered from progesterone-induced uterine gland (PUGKO) but not wildtype (WT) mice on day 5 post-mating. Anti-adhesive Muc1 protein and microvilli were present on the luminal epithelium of PUGKO but not WT uteri. A number of known uterine receptivity genes and gland-specific genes were altered in the PUGKO uterus. Next, the uterus and uterine luminal fluid (ULF) were obtained from WT and PUGKO mice on day 3, 4 and 5. Transcriptome analysis revealed that 580 genes were decreased in the PUGKO uterus, however ULF secrotome analysis revealed that many proteins and several amino acids were increased in the PUGKO ULF. Of note, many proteins encoded by many gland-specific genes were not identified in the ULF of WT mice. These results support the ideas that uterine glands secrete factors that regulate ULF homeostasis and interact with other cell types in the uterus to influence uterine receptivity and blastocyst implantation for the establishment of pregnancy.
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Introduction
In humans and rodents, implantation involves blastocyst apposition, attachment, and adhesion to the luminal epithelium (LE) followed by infiltration and growth of the trophectoderm into the decidualizing stroma1. This complex process requires an intricate dialogue between an implantation-competent blastocyst and a receptive uterus2. Uterine receptivity can be defined as the state of the endometrium when it is ready to support blastocyst implantation and establishment of pregnancy. In humans, the inability of the uterus to achieve a receptive status is likely a major cause of infertility3,4,5. In mice, blastocysts enter the uterus by the morning of gestational day (GD) 4, and the endometrium becomes receptive by the afternoon of day 42,6. By the afternoon of GD 5, the uterus is non-receptive and refractory to blastocyst implantation7. The implantation process is initiated by blastocyst trophectoderm apposition and attachment to the LE on GD 4. By GD 5, the LE cells at the implantation sites undergo apoptosis or entosis, allowing the motile blastocyst trophectoderm to contact stromal cells and initiate decidualizations8,9. Stromal cell decidualization is important for regulating blastocyst implantation and formation of a functional placenta10.
Uterine function is primarily regulated by the ovarian steroid hormones estrogen and progesterone11. Under their influence, the LE, glandular epithelia (GE), and stroma express genes important for uterine receptivity and blastocyst implantation, including cytokines, growth factors, and lipid mediators2,12,13,14. The phenotype of mouse models lacking uterine glands emphasized the importance of endometrial glands and, by inference, their secretions for blastocyst implantation15,16,17,18,19. Deficient glandular activity, usually described as a secretory phase defect, is hypothesized to be a significant underlying cause of early pregnancy failure in women3,7. Secretions present in the uterine lumen of mice are not well characterized, but likely contain amino acids, glucose, proteins, and other substances based on studies of uterine luminal fluid (ULF) in humans and domestic animals20,21,22,23,24. The first GE-derived factor found to be essential for pregnancy in mice was leukemia inhibitory factor (LIF). Lif is expressed in the GE in response to the nidatory surge of estrogen from the ovary on GD 3.5, and Lif null mice are infertile and exhibit defects in uterine receptivity, blastocyst implantation and stromal cell decidualization25. Additional studies of several mouse models lacking uterine glands provide further evidence that the GE and their secretions have important biological roles in blastocyst implantation and stromal cell decidualization17,18,26,27,28. However, how uterine glands regulate those fundamental processes important for the establishment and maintenance of pregnancy is not well understood.
A series of studies are presented here to further understand the infertility of progesterone-induced uterine gland knockout (PUGKO) mice and contributions of the endometrial GE to the uterine transcriptome and ULF secretome. PUGKO mice are generated by exposing neonatal C57BL/6 mice to progesterone from postnatal days 2 to 1018,29. That exposure regimen permanently inhibits differentiation of GE in the uterus, which normally beings during the second week of life, but does not affect the differentiation of other reproductive tract structures such as the ovary, oviduct, vagina or cervix. The resulting mice have normal estrous cycles as adults, but are infertile and exhibit defects in blastocyst implantation and stromal cell decidualization17,18,19. Results of these studies support the ideas that uterine glands impact uterine gene expression and ULF homeostasis and play an important role in uterine receptivity and blastocyst implantation for establishment of pregnancy.
Results
PUGKO mice lack endometrial glands
Forkhead box A2 (FOXA2) is a transcription factor that is expressed solely in the GE of both neonatal and adult mouse uteri27,30. In day of pseudopregnancy 4 (DOPP 4) wildtype (WT) mice, immunoreactive FOXA2 protein was detected in the nuclei of GE cells in the endometrium and was not present in other uterine cell types (LE, stroma or myometrium) (Fig. 1). In contrast, uteri from DOPP 4 PUGKO mice were completely devoid of immunoreactive FOXA2 protein. With the exception of glands, there was no consistent morphological or histological differences between the adult WT and PUGKO uteri.
Embryo implantation is defective in PUGKO mice
A reciprocal embryo transfer experiment was performed between WT and PUGKO mice. Both WT and PUGKO mice were mated to intact males, and blastocysts were recovered from the uterine lumen on GD 4. Blastocysts from WT mice were transferred into DOPP 3 WT or PUGKO recipient mice, and blastocysts were also transferred from PUGKO mice into DOPP 3 WT recipient mice. Blastocyst implantation sites were visualized 72 hours later (GD 6) by intravenous injection of Evans blue dye, which accumulates at sites of embryo implantation due to increased vascular permeability31. Implantation sites were observed in WT recipient mice receiving blastocysts from either WT or PUGKO mice (Fig. 2A). The number of implantation sites observed did not differ between WT recipients receiving WT blastocysts and those receiving PUGKO blastocysts (P > 0.05). An average of 8 (range 5–11) and 7.6 (range 4–10) implantations were observed in WT recipients of WT blastocysts and those receiving PUGKO blastocysts, respectively. Further, the diameter of the implantation sites was not different (P > 0.05) in WT recipients of WT blastocysts (2.8 ± 0.2 mm) and those receiving PUGKO blastocysts (2.5 ± 0.1 mm). Blastocyst implantation sites were not observed in any PUGKO recipient mouse receiving WT blastocysts (Fig. 2A).
By the afternoon of GD 5, blastocysts are firmly attached to the LE within implantation crypts and can no longer be flushed from the uterus32. Both WT and PUGKO mice were mated to males of proven fertility, and the uterus was gently flushed on the afternoon of GD 4 or 5 (GD 1 = observation of vaginal plug) (Fig. 2B). On GD 4, blastocysts were recovered from both WT and PUGKO mice. In contrast, blastocysts could be recovered in the uterine flush from PUGKO but not WT mice on GD 5. These results support the idea that the blastocyst fails to attach or adhere to the uterine LE in PUGKO mice.
Uterine receptivity is defective in PUGKO mice
Expression of the anti-adhesive glycoprotein mucin one (MUC1) on the LE is considered an important indicator of uterine receptivity33. As the uterus achieves receptivity, MUC1 expression is decreased on the LE between GD 3 and 4, and persistent MUC1 is indicative of a nonreceptive uterus. In uteri of WT mice on the afternoon of DOPP 4, immunoreactive MUC1 protein was abundant on the apical surface of the GE, but absent from the LE (Fig. 3A). In contrast, MUC1 protein remained abundant on the LE of uteri from PUGKO mice.
Another important parameter for acquisition of uterine receptivity is membrane transformation of the uterine LE. The presence of long microvilli on the LE apical surface indicates a lack of receptivity, as a marked flattening of these microvilli occurs prior to implantation34. Transmission electron microscopy (TEM) revealed that, in contrast to WT uteri, the LE of PUGKO uteri fail to undergo microvilli flattening, indicating impaired uterine receptivity (Fig. 3B). As illustrated in Fig. 3B, the number and length of microvilli (MV) were substantially greater on the apical surface of the LE of PUGKO uteri. Microvilli were almost two-fold longer (P < 0.05) on the LE of PUGKO (0.77 ± 0.04 μm) as compared to WT (0.40 ± 0.04 μm) uteri. The persistent MUC1 protein and lack of membrane transformation clearly indicate that the LE of the PUGKO uterus is not receptive to blastocyst implantation.
Uterine receptivity in mice also requires dynamic changes in gene expression in the uterine epithelia as well as stroma2,6,35. Receptivity and implantation-associated genes that are expressed in the LE (Hbegf, Ihh, Msx1, Sfrp4, Wnt7a), GE (Lif, Ihh, Msx1, Prss29, Spink3), LE and GE (Ihh, Msx1), and/or stroma (Nog, Sfrp4) were quantified in the uteri from bred WT and PUGKO mice by qPCR (Fig. 4). The abundance of GE-expressed (Ihh) and GE-specific genes (Lif, Prss29, Spink3) were substantially reduced or absent (P < 0.05) in the PUGKO uterus. Expression of Hbegf, Nog and Sfrp4 were also decreased (P < 0.05) in the PUGKO uterus on GD 5. In contrast, expression of Msx1 and Wnt7a were not different (P > 0.05) (Fig. 4).
Transcriptomic analysis of uterine receptivity in pseudopregnant mice
Pseudopregnant mice experience the same changes in uterine gene expression as early pregnant mice6, and samples of the ULF can be obtained without blastocysts36. Therefore, uteri were obtained from WT and PUGKO mice on DOPP 3 (pre-receptive), 4 (receptive), and 5 (post-receptive). The lumen of each uterus was gently flushed with PBS to obtain ULF, and the uterus and ULF were frozen for subsequent analysis. First, total RNA was extracted from the uteri and sequenced. Transcriptome analysis revealed dynamic changes in gene expression in WT mice (Fig. 5A and Supplemental Table 1). Expression of 157 genes (83 increased, 74 decreased) changed (P < 0.05) from DOPP 3 to 4 (Fig. 5B and Supplemental Table 1). The top 10 protein coding genes increased from DOPP 3 to 4 were Prss28, Prss29, 8430408G22Rik, Pip, Atp6v0d2, Lrat, Prss35, Cyp26a1, Guca2b, and Slc46a2 (Table 1). Of note, Prss28 and Prss29 are only expressed in the GE of the uterus30,37. The top 10 protein coding genes decreased from DOPP 3 to 4 were BC048679, Clca3, Sprr2f, Ltf, Ppp1r1b, Gstm7, Rdh1, Sprr2g, Gpr128, Gcnt, and S100a9 (Table 1). Between DOPP 4 and 5, expression of 104 genes (31 increased, 73 decreased) changed (P < 0.05) in the WT uterus (Fig. 5B and Supplemental Table 1). The top 10 protein coding genes increased from DOPP 4 to 5 were Gm10263, Gm10260, Gtsf1, Glp1r, H2-q10, Gm21830, Hyal3, Gpr81, C130074G19Rik, and Armcx4 (Table 2). The top 10 protein coding genes decreased from DOPP 4 to 5 were Rps2-ps13, Gm26619, Gm102063 Gm10260, H2-Ea-Ps, Gm12328, H2-Bl, RP23-184F1.2, Gtsf1, and Glp1r (Table 2).
Hierarchical clustering based on weighted gene co-expression network analysis identified an extensive modular network pattern of genes in WT uteri that substantially differed in PUGKO uteri (Fig. 6). The present study identified 21 of the top 25 differentially expressed genes (i.e., Spink3, Cxcl15, Cyp3a25, Tmprss11g) previously identified in the uteri of WT and PUGKO mice on DOPP 4 by microarray37. Here, the expression of 1,210 genes differed in uteri of WT and PUGKO mice from DOPP 3 to 5 (Supplemental Table 2). Expression of 444 genes were more abundant and 580 genes less abundant in PUGKO as compared to WT uteri (Fig. 5B). Of the 580 decreased genes, 253 genes were not expressed (RPKM < 1) in the PUGKO uterus (Fig. 5C). Many of those 253 genes are exclusively expressed in the GE (i.e., Cxcl15, Foxa2, Sox9, Spink3) or abundantly expressed in the GE but also expressed in other cell types (i.e., Fgf9, Lrat, Prss35)2,30. Integration with uterine cell specific transcriptomic data previously published by our lab37 illustrated that 24% and 29% of the genes absent from the PUGKO uterus on DOPP 3 and 4, respectively, were enriched in the GE of WT mice. Expression of 26 of the 253 absent genes in the PUGKO uterus (i.e., Prss28, Prss29, Pip, Serpina3n) increased (P < 0.05) between DOPP 3 to 4 in WT mice, whereas expression of only 4 of the 253 genes (H2-Ea-ps, H2-Q10, Hyal3, Gpr81) increased (P < 0.05) from DOPP 4 to 5 in WT mice (Supplemental Table 1).
Bioinformatics analyses, including gene ontology (GO) and pathway analyses, were conducted on differentially expressed genes to predict functionally impacted pathways. Genes with decreased expression in the PUGKO compared to WT uterus were largely associated with cellular and stimulus-response related activities (Table 3). The genes expressed in WT but not in PUGKO uteri are mostly enriched in gene ontologies associated with metabolism (Table 3). Expression changes of the two gene sets were further analyzed for scoring differential regulation of pathways using a method that incorporates pathway topology and the magnitude of gene expression changes38. Genes expressed in WT but not PUGKO uteri, were associated with pathways such as complement and coagulation cascades (Supplementary Figure 1), different amino acid metabolic pathways, Wnt signaling, and dopaminergic synapses. Genes with decreased expression in PUGKO compared to WT uteri are associated with pathways including cell cycle and amino acid and nucleotide metabolism. Specific pathways such as synapse pathways (serotonergic and dopaminergic), cell adhesion and tryptophan metabolism are commonly associated with both differentially expressed gene sets. Furthermore, subsets of the differentially expressed genes are associated with bicluster expression patterns (similar expression changes by subset of genes among subset of samples), suggesting tightly coordinated local cross-talk among the differentially expressed genes. The global cross-talk among all the discovered differentially expressed genes displayed topological variations between WT and PUGKO uteri (Supplementary Figure 2), which reaffirms alterations in transcriptional networks of genes in the uteri of PUGKO compared to WT mice (Fig. 6).
Proteins in the ULF
Uterine GE synthesize and secrete or transport bioactive substances, including proteins, amino acids and glucose, into the uterine lumen17,18,19,27,28. Proteins in the ULF of DOPP 3, 4 and 5 WT and PUGKO mice were identified and quantified using mass spectrometry. A total of 1,359 proteins were detected in WT ULF based on spectral count data (Supplemental Table 3). As summarized in Table 4, the most abundant proteins detected in WT ULF on all DOPP were serum proteins including albumin (Alb), alpha 2 macroglobin (A2m), and complement C3 (C3). Of particular note, several secreted proteins known to be expressed only by the GE of the uterus (e.g., LIF, PRSS28, PRSS29, SPINK3) were not found in the ULF of WT mice.
Further analyses of the proteomics data considered proteins with a minimum of 4 unique spectral counts in 4 of the 5 ULF samples. Using that criteria, WT mice ULF contained 120 proteins on DOPP 3, 36 proteins on DOPP 4, and 40 proteins on DOPP 5 (Fig. 7A and Supplemental Table 4). Integration of uterine transcriptome and ULF proteome data from WT mice found that 100 of the 124 ULF proteins are encoded by genes expressed in the uterus. Thus, 24 of the ULF proteins originate from serum such as albumin and hemoglobin. Between DOPP 3 and 4 in WT mice, the abundance of 26 proteins changed (P < 0.05) in the ULF (12 increased, 24 decreased) (Fig. 7B). In contrast, only 6 proteins changed from DOPP 4 to 5 (2 proteins increased, 4 decreased) in WT ULF (Fig. 7B and Supplemental Table 4).
Unexpectedly, the ULF of PUGKO mice contained more proteins, particularly on DOPP 4 and 5, compared to WT ULF (Fig. 7C and D and Supplemental Table 5). In fact, few proteins were less abundant in the ULF of PUGKO as compared to WT mouse uteri, including 4 proteins on DOPP 3 (CALB1, HBA1, KRT19, KRT9), 8 proteins on DOPP 4 (APOE, HMGB1, SERPINA3K, SOD1, TMSB10, TMSB4X, TPM4, VCL), and 7 proteins on DOPP 5 (HMGB1, SOD1, VIM, FASN, HSPB1, TMSB10, TPM4) (Supplemental Table 4). Of those, only 12 proteins (APOE, CALB1, FASN, HMGB1, KRT19, SOD1, TMSB10, TMSB4X, TPM4, VIN) were encoded by genes expressed in the uterine GE based on transcriptomic data.
Select nutrients in the ULF
Glucose is an important energy source required for development to the blastocyst stage and may regulate trophectoderm activation for implantation in mice39,40. As shown in Fig. 8, glucose concentrations increased (P < 0.05) in the ULF of WT mice from DOPP 3 to 4 and remained elevated on DOPP 5. In contrast, glucose concentrations were higher on DOPP 3 and lower on DOPP 5 (P < 0.05, day x type) in the ULF of PUGKO mice. Transcriptomic analysis of the glycolytic and gluconeogenesis pathway found differences in only two solute carriers (Slc2a1 and Slc2a3) on DOPP 5. Interestingly, phosphoenolpyruvate carboxykinase 1 (Pck1), a major control point in gluconeogenesis, is decreased in the PUGKO uterus during the peri-implantation period. Further, Pck1 was previously identified as a GE enriched gene on DOPP 437.
Select amino acids are also important for blastocyst implantation, and those nutrients are transported into the uterine lumen by solute carrier transporter proteins41,42. Trophectoderm outgrowth of the mouse blastocyst in vitro and likely implantation in vivo requires amino acids. Concentrations of amino acids in the ULF of WT mice changed (P < 0.05, day) from DOPP 3 to 5 (Table 5), and Glu, Asn, Ser, Gln, Gly, Thr, Cit, Arg, b-Ala, Tau, Trp, Met, Val, Orn, and Lys increased from DOPP 3 to 4. Many amino acids were more abundant (P < 0.05) in PUGKO than WT ULF on DOPP 3, 4 and 5 (Fig. 9). None of the amino acids were lower (P > 0.10) in the ULF of PUGKO as compared to WT ULF on DOPP 4, but Ser was lower (P < 0.05) on DOPP 3, and Gln and Arg were lower on DOPP 5 (Fig. 9).
Discussion
The present study confirmed that progesterone treatment permanently ablates the differentiation of GE in the neonatal uterus, resulting in an adult uterus that lacks detectable FOXA2 protein and thus glands. Mouse models with substantially reduced or absent uterine glands exhibit a subfertile or infertile phenotype due to defects in blastocyst implantation17,18,26,27,28,43,44. In the present study, morphologically normal blastocysts were recovered from the PUGKO uterus on GD 4 and 5, and GD 4 blastocysts from PUGKO mice could implant when transferred into the uterus of WT mice. Thus, the pituitary, ovary, oviduct, and vagina appear to function normally in PUGKO mice. Our previous study found that spatiotemporal patterns of steroid receptor expression (ESR1, PGR) and several steroid hormone-regulated genes were not altered in the uterus of pseudopregnant PUGKO mice17. Thus, the defects in blastocyst implantation in PUGKO mice can be ascribed to inadequate uterine receptivity and/or blastocyst trophectoderm attachment and motility, which are critical processes in implantation for establishment of pregnancy in mice and humans. Results from the present studies clearly support the idea that the blastocyst trophectoderm is unable to attach and adhere to the uterine LE of PUGKO mice, since blastocysts could be recovered by flushing the uterine lumen of PUGKO but not WT mice on GD 5. In mice, structural and molecular changes in the uterine LE occur between GD 3 and 4 that render it receptive to blastocyst implantation2. The first steps in implantation involve the apposition and adhesion of the blastocyst trophectoderm to the uterine LE. The removal of anti-adhesive MUC1 protein from the glycocalyx of the LE prior to implantation facilitates interaction of the trophectoderm with the LE45. Microvilli also become less numerous and pronounced as the LE cells lose polarity46. Thus, the uterine LE failed to undergo changes associated with development of receptivity in PUGKO mice, because persistent MUC1 protein and microvilli were observed on the LE. A similar phenotype was reported for the LE in uteri of Lif null mice47. Lif is expressed specifically in the uterine GE in response to the nidatory surge in estrogen from the ovary48. The implantation and decidualization defects in Lif null mice could be rescued by intraperitoneal injection of a single dose of recombinant LIF 25. Thus, it would be interesting to determine if intraperitoneal injections of recombinant Lif can rescue infertility of glandless mice, such as PUGKO and aglandular Foxa2 conditional knockout mice. A number of other genes with known or proposed functions in uterine receptivity and decidualization were also reduced or ablated in the PUGKO uterus, including Ihh, Nog, Prss28, Prss29, Sfrp4 and Spink3. Both PUGKO and Foxa2 conditional knockout mice have defects in stromal cell decidualization based on results of artificial induced deciduoma formation17,27. Injection of LIF into the uterine lumen was unable to rescue decidualization in PUGKO mice17 and only partially rescued decidualization in Foxa2 conditional knockout mice27. In both of those studies, the route of LIF administration may be an important issue given the inability of LIF to be detected in the ULF proteome in the current study.
Transcriptome analysis identified profound changes in uterine gene expression due to the absence of glands, as 444 genes were increased and 580 genes decreased in the PUGKO as compared to WT uterus from DOPP 3 to 5. Bioinformatics analyses revealed that many of the genes decreased or absent in the PUGKO uterus and expressed in the WT uterus are involved in biological processes known or predicted to be important for the establishment of pregnancy, including metabolic processes, transport and response to stimulus. The cell-specific expression and function of the majority of those differentially expressed in the mouse uterus are not known. Of the 580 genes with decreased expression in pseudopregnant PUGKO uteri, a few are known to be expressed solely in the GE including Cxcl15, Foxa2, Prss28, Spink3, and Sox927,30,37,49. Many of the genes reduced or absent in the PUGKO uterus encode secreted proteins, including LIF, CXCL15, SERPINA3, TMPRSS13, SPRINK3, SERPINB11, PIP, HPX, FGA, MMP7, CALCA, SELENBP1, WNT7B, LYZ, PRSS28, PRSS29. Of particular note, several cytochrome P450 (CYPs) genes (Cyp26a1, Cyp2f2, Cyp3a16, Cyp3a25, Cyp3a57, Cyp3a59), proteases (Mmp7, Prss28, Prss29, Tmprss11a, Tmprss11g, Tmprss13, Tmprss2, Tmprss4) and solute carriers (Slc) (Slc12a3, Slc12a6, Slc13a2, Slc1a5, Slc22a4, Slc24a4, Slc26a7, Slc2a1, Slc36a2, Slc39a2, Slc39a4, Slc39a8, Slc44a3, Slc46a2, Slc5a8) were less abundant in the PUGKO uterus. Cyp genes encode heme‐containing membrane enzymes in the endoplasmic reticulum or mitochondrial inner membrane that regulate hormone and cholesterol synthesis as well vitamin D metabolism and retinoic acid signaling50,51. Progesterone induces Cyp26a1 expression in the mouse uterus52, and Cyp26a1 mRNA is higher in the secretory phase than in the proliferative phase endometrium of women53.Cyp26a1 is a metabolizing enzyme catalyzing trans-retinoic acid to more polar metabolites54. Retinoic acid regulates the differentiation of the uterine epithelium55 and the expression of matrix metalloproteases (Mmps)56, which are involved in the remodeling of the extracellular matrix of the uterus in preparation for pregnancy57. Solute carrier proteins are membrane transporters that control the uptake and delivery of crucial compounds such as glucose and amino acids across epithelia58. Several amino acid transporters (Slc1a1, Slc1a5, Slc36a2), facilitated glucose transporters (Slc2a1, Slc2a3), and sodium/glucose cotransporters (Slc5a5, Slc5a8, Slc5a11) were altered in the PUGKO uterus. Glucose metabolism is important for the preparation of the epithelium and stroma for embryo implantation during early pregnancy40. Differences in the amount of glucose in the uterine lumen found between WT and PUGKO mice were likely not supraphysiological24 and did not affect the ability of day 3 embryos from the PUGKO to implant after transfer to a WT uterus. Amino acid transport is important for blastocyst implantation, and in vitro studies found leucine and arginine regulate trophoblast motility in the preimplantation mouse embryo41,42,59. Collectively, the decrease in specific secreted factors, enzymes and transporters in the uterus of PUGKO mice may also contribute to deficient uterine receptivity and defects in blastocyst implantation.
For several decades, the glands of the uterus have been hypothesized to predominantly transport or secrete factors in an apical manner into the uterine lumen and, in that way, regulate survival and growth of the blastocyst for establishment of pregnancy. The present study challenges that idea, because the dynamic changes in uterine gene expression from DOPP 3 to 5 were not reflected in the proteins and amino acids present in the ULF. Indeed, genes altered in the PUGKO uterus are expressed in many different cell types of the uterus in addition to the GE, suggesting that the glands communicate with many different cell types in the uterus. Remarkably, archetypal GE-derived factors (LIF, PRSS28, PRSS29, SPINK3) were not detected in the ULF using mass spectrometry. Although this could be due to technical limitations in terms of sensitivity, we were also unable to detect LIF protein in the ULF of WT mice using a commercially available ELISA assay (data not shown). This result suggests that LIF and other GE-specific genes encoding secreted proteins may be preferentially secreted basally from the glands and act on the stroma and LE or other cells that express Lif receptors (LIFR). Similar to Lif, Spink3 is also expressed exclusively in GE of the mouse uterus, yet SPINK3 protein was observed in the LE and decidualizing stromal cells as well as uterine glands49. Of note, SPINK3 protein was also not detected in the ULF of WT mice in the present study. Collectively, these observations support the idea that the GE synthesizes and secretes many factors basolaterally that act on the stroma and LE to create a unique microenvironment for blastocyst implantation in the antimesometrial area of the uterus where the GE are developmentally located and implantation crypt forms in a successful pregnancy. Future studies are needed to determine the role of the uterine glands and their secretions in paracrine interactions with the LE, stroma and decidual cells60.
This study is the first comprehensive investigation of the uterine luminal secretome (glucose, amino acids, proteins) in pseudopregnant or pregnant mice. The results found that dynamic changes in the ULF secretome do not occur in association with the development of uterine receptivity. This finding starkly contrasts with analysis of the ULF secretome during early pregnancy in large animals such as cattle, sheep and pigs22,61,62. Results of the present study to support the idea that uterine GE have a primarily biological role in homeostasis of the ULF, because many proteins and most amino acids were more abundant in ULF from PUGKO than WT mice. Thus, the amino acids (leucine and arginine) and glucose implicated in activation of mouse blastocyst trophectoderm motility and invasiveness were clearly not deficient in the PUGKO uterus. Although the PUGKO mice had detectable differences in ULF protein, amino acids and glucose in DOPP 3 to 5, no single protein or amino acid or glucose was completely deficient or substantially altered to a supraphysiological level. Clearly, pre-implantation embryos require optimal regulation of cellular metabolism via nutrients supplied in vitro or in vivo63. Mouse and human embryos in vitro are dependent on glucose and it is required for the blastocyst expansion and hatching, but substantial increased glucose in vitro and in vivo delayed embryo development and increased embryo death64,65,66,67,68. Whether or not the altered ULF secretome found in the ULF of PUGKO mice programs the embryo is not known, although GD 4 blastocysts from PUGKO mice exhibited normal implantation in WT uteri. Given that blastocysts from mated PUGKO mice are essentially in developmental delay, it would be interesting to transfer GD 6 or 8 PUGKO blastocysts into GD 4 WT mice to determine their developmental fate.
Collectively, studies of PUGKO and Foxa2 conditional knockout mice strongly support the hypothesis that secreted factors from the GE are essential for development of uterine receptivity, blastocyst implantation and establishment of pregnancy. Knowledge about the function of most adult GE-specific genes other than LIF is limited. Therefore, the transcriptome and secretome analysis conducted here provides an important framework for future investigations into the biological roles of endometrial glands and their secretions in uterine function, homeostasis, and establishment of pregnancy. These studies are important, as they may lead to critical knowledge important to solve pregnancy loss and complications in women.
Methods
Animals
All animal procedures were approved by the Institutional Animal Care and Use Committee of Washington State University and the University of Missouri-Columbia and conducted according to their guidelines for the care and use of laboratory animals. Female PUGKO mice were produced as previously described18. Briefly, all C57BL/6 J females in a litter received subcutaneous injections of progesterone (50 μg/g body weight in sesame oil) from postnatal days 2 through 10 (day 0 = birth).
Adult (6–10 week old) C57BL/6 J wildtype and PUGKO females were mated with fertile or vasectomized males to induce pregnancy or pseudopregnancy, respectively. Uteri on days 3, 4, and 5 (day 1 = vaginal plug) were collected for histology and RNA analysis. One uterine horn was fixed in 4% paraformaldehyde in PBS (pH 7.2) at room temperature for 16 h, dehydrated through a series of ethanol and embedded in paraffin for histology. The remaining uterine horn was snap frozen in liquid nitrogen and stored at −80 °C.
Uterine luminal fluid was collected from mice on DOPP 3, 4, and 5 using a previously described method24. The female reproductive tract was excised immediately following euthanasia and washed with ice cold PBS, patted dry, and placed under ice cold mineral oil. The cervix and oviduct were removed and retrograde flushing of uterus was performed from the uterotubal junction after 30 μl of sterile PBS was instilled into the uterine lumen. Samples were transferred to a 0.6 ml tube and centrifuged for 5 min at 3,000 × g. The oil-free PBS was stored at −80 °C for proteome, amino acid or glucose analysis.
Embryo transfer
Wildtype (WT) and PUGKO females were bred to fertile males. Uteri were flushed on day 4 after mating with M2 medium (EMD Millipore) to recover blastocysts. Pseudopregnant recipients were generated by mating females with vasectomized males. Day 4 blastocysts from WT or PUGKO mice were transferred into day 3 uteri of WT or PUGKO psuedopregnant recipients (n = 6 blastocysts per uterine horn). Implantation sites were visualized 72 hours later (day 6) by intravenous injection of 1% Evans blue dye (Sigma-Aldrich Corp., St Louis, MO) into the tail vein 5 min before necropsy.
Immunohistochemistry
Localization of a specific proteins was performed using a previously described method18. Briefly, fixed uteri were sectioned (5 μm), mounted on slides, deparaffinized, and rehydrated in a graded alcohol series. Antigen retrieval was performed by incubating sections for 10 min in boiling 10 mM citrate buffer (pH 6.0). Sections were blocked with 10% normal goat serum in PBS (pH 7.2) and incubated with an antibody to FOXA2 (1.2 μg/ml; LS-C 138006, LifeSpan Biosciences) or MUC1 (1.0 μg/ml; NB120-15481, Novus Biological) overnight at 4 °C. Sections were washed in PBS and incubated with biotinylated secondary antibody (5 μg/ml; Vector Laboratories, Burlingame, CA) for 1 h at 37 °C. Immunoreactive protein was visualized using a Vectastain ABC kit (Vector Laboratories) and diaminobenzidine tetrahydrochloride as the chromagen. Sections were lightly counterstained with hematoxylin before affixing coverslips with Permount.
Transmission electron microscopy
Uterine horns from DOPP 5 WT and PUGKO mice (n = 3 per type) were fixed in 2% paraformaldehyde/2% glutaraldehyde in 0.1 M cacodylate buffer overnight at 4 °C, rinsed three times in 0.1 M cacodylate buffer and post fixed in 1% OsO4 overnight at 4 °C. Samples were rinsed three times in 0.1 M cacodylate buffer prior to dehydration in an ethanol series, then infiltrated with acetone, embedded in Spurr’s resin and polymerized at 70 °C. Sections were cut to a thickness of 85 nm using an ultramicrotome (Ultracut UCT, Leica Microsystems) and a diamond knife (Diatome). These sections were post-stained using Sato’s triple lead solution stain69 and 5% aqueous uranyl acetate. Images were acquired with a JEOL JEM 1400 transmission electron microscope (JEOL) at 80 kV on a Gatan Ultrascan 1000 CCD (Gatan, Inc.) at the Univeristy of Missouri Electron Microscopy Core Facility. After importing into ImageJ 1.49 v, measurements of 10 microvilli from 4 different images were determined for each mouse uterus.
RNA extraction and real-time PCR
RNA was isolated from uterine samples (n = 4 mice per day and type) using the RNeasy plus mini kit (Qiagen). To eliminate genomic DNA contamination, RNA was treated with DNase I (Qiagen) on-column during RNA isolation. The quantity and purity of total RNA were determined by spectrometry. Total RNA (1 μg) from each sample was reverse transcribed in a total reaction volume of 20 μl using iScript RT supermix (BioRad). Reverse transcription was performed as follows: 5 min at 25 °C; 30 min at 42 °C; and 5 min at 85 °C. Control reactions in the absence of reverse transcriptase were prepared for each sample to test for genomic DNA contamination. The resulting cDNA was stored at −20 °C for further analysis.
Real-time PCR was performed using a CFX384 Touch Real Time System with SsoAdvanced Universal SYBR Green Supermix (BioRad). PrimePCR primers (Bio-Rad) for the quantification of selected genes were used (Hegf1, Ihh, Lif, Msx1, Noggin, Sfrp4, Wnt7a). Each sample was analyzed in duplicate with the following conditions for 40 cycles: 95 °C for 30 sec; 95 °C for 5 sec; and 60 °C for 30 sec. A dissociation curve was generated at the end of amplification to ensure that a single product was amplified. PCR without template and template substituted with total RNA were used as negative controls. The threshold line was set in the linear region of the amplification plot above the baseline. Quantification cycle (Cq) values were determined as the cycle number in which the threshold line intersected the amplification curve.
RNA-sequencing analysis
DOPP 3, 4, and 5 uteri from WT and PUGKO mice (n = 4 mice per treatment) were homogenized in RLT plus buffer and RNA was isolated using RNeasy Plus mini kit (Qiagen). Samples of total RNA (5 μg) were depleted of ribosomal RNA using Ribominus Eukaryote System v2 (Ambion). Ion Total RNA-seq Kit v2 (Life Technologies) was used to construct strand-specific sequencing libraries from ribosomal-depleted samples (20 ng), with several deviations from the protocol. Enzymatic RNA fragmentation was carried out at 37 °C for 90 sec. Fragmented RNA was purified using 1.03 AMPure XP beads (Beckman-Coulter Genomics). The cDNA and final libraries were purified with 0.83 AMPure XP beads. Emulsion PCR was performed on an Ion One Touch 2 instrument (Life Technologies), using the Ion P1 Template OT2 200 v3 reagents. Sequencing beads were quantified and evaluated by flow cytometry using a Guava Easy Cyte (Millipore) with Sybr Gold (Molecular Bioprobes) before loading on an Ion P1 semiconductor sequencing chip. Libraries (n = 4) were sequenced on an Ion Proton using Ion P1 200 v3 sequencing reagents (Life Technologies) at the Washington State University Molecular Biology and Genomics Core. The barcoded libraries were pooled at three per chip for sequencing. Base calling and primary analysis were performed using Torrent Suite 4.0.2 (Life Technologies).
Unmapped BAM files were imported into CLC Genomics Workbench (7.0.4, CLC bio, Aarhus, Denmark). Sequence quality was verified by inspection of quality control reports and samples were processed using CLC Genomics Server (6.0, CLC bio). Reads were quality trimmed (error probability 0.01) with default parameters and mapped to the RefSeq assembly (Mus musculus GRCm38.p1). Alignment BAM files were exported for read quantification of genes using FeatureCounts70. Data were deposited in the Gene Expression Omnibus database (GEO, in process).
Differential expression analyses between sample groups were performed by fitting the expression data to a generalized linear model using edgeR-robust71. Differentially expressed genes (FDR P < 0.10) were further subjected to weighted correlation network analysis (using R package WGCNA) to identify changes in expression modules (transcriptional networks).
Network analysis were performed using Aracane 2 algorithm. Visualization was done using cytoscape (http://apps.cytoscape.org/apps/aracne). Functional prediction of genes corresponding to those expression modules were assessed by mapping the genes to KEGG (Kyota Encyclopedia of Genes and Genomes) pathways as well GO (Gene Ontology) databases using tools (KEGGscape and BINGO) included in Cytoscape.
Genes that were decreased or absent in PUGKO as compared to WT mice were further analyzed to predict gene functions, pathways and networks. Pathway analysis was performed by topology-based prediction method38 implemented in R-bioconductor package ToPAseq72. Over-representation of gene-ontology (GO terms) were analyzed using BINGO tool73. Biclusters analysis of gene expression was performed using the Order-preserving Submatrix Algorithm (OPSM) which predict large submatrices from expression data74 with the BicAT tool75.
Mass spectrometry analysis
Uterine luminal fluid was collected from WT and PUGKO mice on DOPP 3, 4, and 5 (n = 5 mice per treatment). Mass spectrometry analyses were performed by the University of California-Davis Proteomics Center. Proteins were precipitated from the ULF samples using the ProteoExtract Protein Precipitation Kit (Calbiochem). The protein pellet was then solubilized in 100 μL of 6 M urea. Dithiothreitol (DTT; 200 mM) was added to a final concentration of 5 mM, and samples were incubated for 30 min at 37 °C. Next, 20 mM iodoacetamide (IAA) was added to a final concentration of 15 mM and incubated for 30 min at room temp, followed by the addition of 20 μL DTT to quench the IAA. Trypsin/Lys-C (Promega) was added to the sample and incubated for 4 hours at 37 °C. Samples were then diluted to at least 1 M urea by the addition of 50 mM AMBIC and digested overnight at 37 °C. The following day, samples were desalted using Macro Spin Column (Nest Group).
Digested peptides were analyzed by LC-MS/MS on a Thermo Scientific Q Exactive Orbitrap Mass spectrometer in conjunction Proxeon Easy-nLC II HPLC (Thermo Scientific) and Proxeon nanospray source. The digested peptides were loaded a 100 μm × 25 mm Magic C18 100 Å 5U reverse phase trap where they were desalted online before being separated using a 75 μm × 150 mm Magic C18 200 Å 3U reverse phase column. Peptides were eluted using a 90 min gradient with a flow rate of 300 nl per min. An MS survey scan was obtained for the m/z range 300–1600, MS/MS spectra were acquired using a top 15 method, where the top 15 ions in the MS spectra were subjected to HCD (High Energy Collisional Dissociation). An isolation mass window of 2.0 m/z was for the precursor ion selection, and normalized collision energy of 27% was used for fragmentation. A five second duration was used for the dynamic exclusion.
Tandem mass spectra were extracted and charge state deconvoluted by Proteome Discoverer (Thermo Scientific). All MS/MS samples were analyzed using X! Tandem (The GPM, thegpm.org; version TORNADO (2013.02.01.1)). X! Tandem was set up to search Mus musculus Proteome database, the cRAP database of common laboratory contaminants (www.thegpm.org/crap; 114 entries) plus an equal number of reverse protein sequences assuming the digestion enzyme trypsin. X! Tandem was searched with a fragment ion mass tolerance of 20 parts per million (ppm) and a parent ion tolerance of 20 ppm. The IAA derivative of cysteine was specified in X! Tandem as a fixed modification. Deamidation of asparagine and glutamine, oxidation of methionine and tryptophan, sulphone of methionine, tryptophan oxidation to formylkynurenin of tryptophan and acetylation of the n-terminus were specified in X! Tandem as variable modifications.
Scaffold (version Scaffold 4.0.6.1, Proteome Software Inc., Portland, OR) was used to validate MS/MS based peptide and protein identifications. Peptide identifications were accepted if they exceeded specific database search engine thresholds. X! Tandem identifications required at least –Log (Expect Scores) scores of greater than 1.2 with a mass accuracy of 5 ppm. Protein identifications were accepted if they contained at least 2 identified peptides. Using the parameters above, the decoy False Discovery Rate (FDR) was calculated to be 1.1% on the protein level and 0.0% on the spectrum level76. The minimum number of unique peptides was set at 2 in order for a protein to be identified. Peptide threshold was set at 95% peptide probability, with +2 accepted charge, and parent mass tolerance of 10 parts per million. Further analysis was conducted on peptides identified as exclusive and unique to each protein following the removal of protein clusters. Additional filtering of proteins with 4 or more spectral counts in at least 4 of the 5 samples was applied to compile final lists. Total spectrum counts for proteins were used for comparisons and statistical analysis. FDR was adjusted using the Benjamini-Hochberg procedure to identify significance based on Fisher’s exact test results.
Glucose analyses
Glucose was quantified in samples of ULF from WT and PUGKO mice on DOPP 3, 4 and 5 (n = 5 mice per day and type) using a fluorometric glucose assay kit (ab65333; Abcam). Each sample was assayed in duplicate. The total recoverable amount of glucose was calculated by multiplying concentrations in the uterine flushing by volume of uterine flushing.
Amino acid analysis
Amino acids, except for proline, were determined in samples of ULF from WT and PUGKO mice on DOPP 3, 4 and 5 (n = 5 mice per day and type) by fluorometric HPLC methods involving precolumn derivatization with o-phthaldialdehyde as previously described for ovine ULF77. Briefly, ULF samples were deproteinized with an equal volume of 1.5 M HClO4 followed by addition of 2 M K2CO3. Amino acids in the extract were determined by fluorometric HPLC methods involving precolumn derivatization with o-phthaldialdehyde as described previously78. The integration of chromatographic peaks was performed using Millenium-32 Software (Waters, Milford, MA). The total recoverable amount of each amino acid was calculated by multiplying concentrations in the uterine flushing by volume of uterine flushing.
Statistical analysis
All quantitative data was subjected to least-squares analysis of variance using the general linear models procedures of the Statistical Analysis System (SAS Institute) to determine the effects of day, type (WT or PUGKO), and their interaction. In all the analyses, error terms used in tests of significance were identified according to the expectation of the mean squares for error. Significance (P < 0.05) was determined by probability differences of least-squares means. For analysis of real-time PCR data, the Ct values of the target mRNA were analyzed for effects of day, type (WT or PUGKO), and their interaction (day x type) with the Gapdh, Actb and Hprt values used as covariates. Real-time PCR data are presented as fold change relative to the mRNA level in uteri from the control mice. Probability values < 0.05 were taken to indicate statistical significance.
Additional Information
How to cite this article: Kelleher, A. M. et al. Uterine glands impact uterine receptivity, luminal fluid homeostasis and blastocyst implantation. Sci. Rep. 6, 38078; doi: 10.1038/srep38078 (2016).
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Acknowledgements
The authors appreciate the efforts of Dr. Mark Wildung in the Washington State University Genomics Core and Dr. Brian Mooney in the University of Missouri Proteomics Core.
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A.K. and T.E.S. conceived the experiments, A.K. conducted the experiments, G.W.B., S.B. and G.W. helped analyze the results. All authors reviewed the manuscript.
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Kelleher, A., Burns, G., Behura, S. et al. Uterine glands impact uterine receptivity, luminal fluid homeostasis and blastocyst implantation. Sci Rep 6, 38078 (2016). https://doi.org/10.1038/srep38078
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