Article Text
Abstract
Introduction Gestational diabetes mellitus (GDM) is the most frequent metabolic complication during pregnancy and is associated with development of short-term and long-term complications for newborns, with large-for-gestational-age (LGA) being particularly common. Interestingly, the mechanism behind altered fetal growth in GDM is only partially understood.
Research design and methods A proteomic approach was used to analyze placental samples obtained from healthy pregnant women (n=5), patients with GDM (n=12) and with GDM and LGA (n=5). Effects of altered proteins on fetal development were tested in vitro in human embryonic stem cells (hESCs).
Results Here, we demonstrate that the placental proteome is altered in pregnant women affected by GDM with LGA, with at least 37 proteins differentially expressed to a higher degree (p<0.05) as compared with those with GDM but without LGA. Among these proteins, 10 are involved in regulating tissue differentiation and/or fetal growth and development, with bone marrow proteoglycan (PRG2) and dipeptidyl peptidase-4 (DPP-4) being highly expressed. Both PRG2 and DPP-4 altered the transcriptome profile of stem cells differentiation markers when tested in vitro in hESCs, suggesting a potential role in the onset of fetal abnormalities.
Conclusions Our findings suggest that placental dysfunction may be directly responsible for abnormal fetal growth/development during GDM. Once established on a larger population, inhibitors of the pathways involving those altered factors may be tested in conditions such as GDM and LGA, in which therapeutic approaches are still lacking.
- diabetes
- gestational
- proteomics
- placenta
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Significance of this study
What is already known about this subject?
Fetal growth abnormalities are frequent in gestational diabetes mellitus (GDM), with large-for-gestational-age (LGA) being the most common.
Placenta in GDM showed alterations in pathways linked to inflammation, oxidative stress, hypoxia, insulin resistance and metabolic complications.
What are the new findings?
Placental proteome is dysregulated in GDM, particularly in those with LGA.
Upregulation of proteoglycan (PRG2) and dipeptidyl peptidase-4 (DPP-4) was evident in GDM/LGA cohort.
PRG2 and DPP-4 alter the expression of genes relevant for human embryonic stem cells (hESCs) differentiation towards cardiac, osteogenic and endodermic progenitors.
How might these results change the focus of research or clinical practice?
PRG2 and/or DPP-4 upregulation may be involved in fetal abnormalities in GDM.
Introduction
Gestational diabetes mellitus (GDM), which affects 3%–25% of pregnancies, is defined as glucose intolerance diagnosed in pregnancy1 and is associated with the risk of developing adverse pregnancy outcomes.2 Fetal growth abnormalities are frequent in GDM, with large-for-gestational-age (LGA) being the most common, while restricted fetal growth is also observed but to a lesser extent.3 Because the placenta is the major organ responsible for fetal nourishment and growth, any alterations in the placental phenotype or function may have an impact on the fetus.4 5 Identifying new factors altered within the placenta and determining whether they affect fetal growth and health will help to clarify the pathological role of placental changes in GDM. This may also pave the way for new successful strategies in preventing, managing and treating maternal and fetal complications in GDM pregnancies. A proteomic approach has been previously employed in disease conditions, including those related to pregnancy, to screen for major molecules and pathways involved in tissue/organ damage.6–9 However, data available on the placental proteomic profile in GDM are scarce and primarily related to maternal glucose intolerance effects on placental pathways associated with insulin resistance, metabolic alterations and inflammatory/oxidative stress.8 10 11 Here, we explore whether the placental proteome is altered in GDM, particularly in those with LGA, with a specific focus on factors that may directly or indirectly control fetal growth.
Research design and methods
Sample collection and protein extraction
Placental tissues were collected from GDM with appropriate for gestational age (GDM), GDM with LGA (GDM/LGA) and healthy pregnant women (controls) who gave birth by elective caesarean section and provided informed consent according to standard operating procedures. GDM was defined based on the International Federation of Gynecology and Obstetrics guidelines.12 LGA was defined as birth weight greater than the 90th percentile according to gestational age and sex. Normal pregnancies (controls) were defined as healthy mothers with normal body mass index (BMI), pregnancy without obstetric complications, and normal fetal growth with birth weight between the 10th and the 90th percentile for Italian references.12 Proteins were extracted from 100 mg of placental tissue washed in Phosphate Buffered Saline (PBS) and minced into small pieces. Selected chorionic villi were then disrupted in liquid nitrogen and solubilized in 500 µL RIPA lysis buffer supplemented with protease inhibitor cocktail.
Liquid chromatography-tandem mass spectrometry (LC-MS/MS) analysis
Ten-microliter lysate from each sample were pooled for GDM, GDM/LGA and controls, and total protein concentration was measured. Forty micrograms of total protein from each sample was in-solution digested as previously described.13 Samples were desalted, and mass spectrometry analysis was performed in technical triplicates using Q-Exactive mass spectrometer equipped with a nanoelectrospray ion source. All MS/MS samples were analyzed using the Mascot search engine to search the UniProt_Human Proteome20180523 (93 164 sequences, 37 039 836 residues). Raw data were loaded into the MaxQuant software V.1.6.1.0, and label-free protein quantification was based on the intensities of precursors. Peptides and proteins were accepted with an false discovery rate >1%, with two minimum peptides per protein.
Bioinformatics analysis
The complete dataset of proteins was analyzed by Student’s t-test using MeV software V.4.9.0. Proteins significantly different (p<0.001) in the controls versus GDM pool and in GDM versus GDM/LGA (p<0.05) were further subjected to hierarchical clustering analysis. Search Tool for the Retrieval of Interacting Genes (STRING) V.10.5 database was used to search for protein−protein networks of differentially expressed proteins (DEPs) and later visualized in Cytoscape V.3.6.1; the BINGO plugin of Cytoscape was used for gene ontology enrichment.14
Cell culture
hESCs were a generous gift of Professor Thorsten Schlaeger lab from Harvard Medical School and were cultured in feeder independent medium (mTeSR1) on BD Matrigel hESC-qualified Matrix coated plate and maintained undifferentiated. Cells were cultured with/without human recombinant bone marrow proteoglycan (PRG2) (25 µg/mL) and dipeptidyl peptidase-4 (DPP-4) (100 ng/mL) for 72 hours and then collected for RNA extraction. Beta-lox5 human beta cell line was a generous gift from Professor Clayton Mathews, Department of Pathology, Immunology and Laboratory Medicine, University of Florida College of Medicine and were cultured with/without human recombinant DPP-4 at the concentration of 100 ng/mL, 500 ng/mL and 1 µg/mL for 72 hours.
Transcriptome profiling
Total RNA was isolated from hESC using the RNeasy Mini Kit (Qiagen, Valencia, California, USA) with on-column DNase I digestion. Next, 2 µg total RNA from each sample was reverse-transcribed using the RT2 First Strand kit (Qiagen) as previously described.15 We used the Human Stem Cell Transcription Factors RT2 Profiler PCR Arrays (PAHS-501Z) (Qiagen). The Profiler PCR Arrays measure quantitatively the expression of a panel of genes using SYBR Green-based real-time PCR. The list of genes is shown in online supplemental table 1. Statistical analysis was performed by using the software available RT2 profiler PCR Array Data Analysis (Qiagen).
Supplemental material
Quantitative reverse transcriptase PCR (qRT-PCR)
RNA from hESC and beta-lox5 was extracted using Trizol Reagent (Invitrogen), and qRT-PCR analysis was performed using TaqMan assays (Life Technologies, Grand Island, New York, USA) according to the manufacturer’s instructions. qRT-PCR data were normalized for the expression of ACTB, and ΔΔCt values were calculated. Statistical analysis compared gene expression across all cell populations via one-way analysis of variance (ANOVA) followed by Bonferroni post-test for multiple comparisons between the population of interest and all other populations. The complete list of primers used is in online supplemental table 2).
ELISA assay
DPP-4 and PRG2 levels in placental lysates of all groups of subjects were assessed using commercially available ELISA kits, according to manufacturer’s instructions (Mybiosource MBS760997-96 and MBS700931-96).
Statistical analysis
We determined that a sample size set at four would provide the proteomic study with 80% power to detect a difference of 30% in the protein expression between the two groups, with a significance level of α=0.05. Other data are presented as mean and SEM. Significance between the two groups was determined by two-tailed unpaired Student’s t-test. For multiple comparisons, the ANOVA test with Bonferroni correction was employed. Graphs were generated using GraphPad Prism V.8.2 (GraphPad Software, La Jolla, California, USA). All statistical tests were performed at the 5% significance level.
Results
Patient characteristics
The characteristics of the study populations are summarized in table 1. No differences were found with regard to maternal or gestational ages, or in placental or fetal weights in GDM versus healthy controls. Pregnant women with GDM showed higher pregravidic BMI but lower weight gain during pregnancy as compared with controls (table 1). The GDM/LGA group displayed higher fetal weight as compared with GDM, while no differences were found in maternal/gestational age, in placental weight or fetal/placenta weight ratio (table 1).
The GDM proteome profile
In order to discover novel factors that may play a role in placental function and fetal development, we first compared the placental proteomes of control and GDM subjects using an unbiased proteomics approach. Mass spectrometry identified 2103 proteins within the placenta, and MaxQuant analysis revealed a unique expression profile in GDM, consisting of 64 DEPs in GDM as compared with controls (p<0.001), 24 of which were downregulated and 40 of which were upregulated (figure 1A). Analysis of the network involving the 64 DEPs using STRING/Cytoscape showed 62 nodes and 90 edges (figure 1B). To discover possible signalling pathways affected by GDM, we underwent these 64 proteins to gene ontology enrichment analysis of biological process (GOBP) with the BINGO plug-in in Cytoscape. While some of these primarily exert protective effects on trophoblasts both in structure and function (eg, invasion, angiogenesis, oxidative stress, barrier and energy support), others were involved in fetal development (iron and nutrient transport, muscle differentiation and nutrients) and protection from fetal loss (anticoagulant and regulation of epithelial-to-mesenchymal transition). However, the aforementioned analysis did not reveal a clear molecular signature strictly related to abnormal fetal growth.
Alterations in fetal growth-related pathways in placentas of GDM with LGA
Identification of placental factors associated with LGA may provide new insights to design novel diagnostic/therapeutic strategies aimed at managing such severe fetal complications. To this end, we next compared placental proteomes of GDM/LGA and GDM using the aforementioned proteomics approach. Among the 1514 identified proteins, 37 were differentially expressed in GDM/LGA as compared with GDM (p<0.05), with 22 proteins downregulated and 15 upregulated (figure 2A). GOBP analysis revealed that 10 of these proteins are primarily involved in placental inflammation (eg, placental inflammosome, complement regulation, control of nitric oxide and histamine levels during pregnancy), fetal nutrient supply (lipid metabolism) and hormonal homeostasis (cortisol and insulin levels, and insulin-like growth factor-1 signaling) (figure 2B). Among the aforementioned proteins detected, PRG2, which controls numerous growth factors activity, was observed as the most highly abundant placental protein in GDM/LGA. Moreover, upregulated placental expression of DPP-4, a key factor in physiological regulation of glucose homeostasis, was also evident in the GDM/LGA cohort. Both PRG2 and DPP-4 protein expressions were confirmed in placental lysates by immunotargeted assays (online supplemental figure 1A and B).
Alterations of differentiation markers in hESCs cultured with PRG2 and DPP-4
To mechanistically understand the role of PRG2 and DPP-4 in fetal development, we cultured human hESC with the recombinant proteins PRG2 and DPP-4 and performed a gene expression profiling of stem cell transcription factors. Transcriptome analysis revealed significant upregulation of HOXD10, a member of the family of Hox genes involved in stem cell differentiation and embryonic limb development, in hESCs exposed to PRG2 (figure 3A). Interestingly, hESCs cultured with DPP-4 exhibited increased expression of cardiac progenitors related genes, TBX5 and IRX4, and decrease of the osteogenic differentiation marker VDR (figure 3B). Since both GDM and GDM/LGA may be associated with an increased risk for newborns to develop metabolic disorders, we explored the effects of PRG2 and DPP-4 on pathways related to hESCs differentiation into mesendoderm (ME) and definitive endoderm (DE), the first steps towards pancreatic development. Both PRG2 and DPP-4 increased stem and ME markers OCT4, ECAD and FGF4 in cultured hESCs, while endoderm markers CER1 and FOXA2 was decreased (figure 3C–F), thus suggesting a role in abnormal endocrine pancreas development and in metabolic disorders (ie, type 2 diabetes or obesity) later on. This impairment in endocrine progenitors and early-stage beta cells was further confirmed by the increased expression of NGN3, an endocrine pancreatic progenitor marker, detected in the Beta-lox5 cell line when cultured in the presence of DPP-4 (online supplemental figure 1C).
Discussion
We are herein describing an altered placental proteome in pregnant women with GDM and more importantly in those with GDM and LGA. Among proteins differentially expressed in GDM/LGA, 10 factors were linked to fetal growth/development by acting on hormone homeostasis, energy metabolism and placental nutrient transport, as previous reports suggested.16 In particular, PRG2 and DPP-4, found to be upregulated in GDM/LGA placental proteome analysis, are both involved in pregnancy17 18 and their dysregulation was shown to correlate with pregnancy-related disorders.19 As PRG2 controls several growth factors activity, its upregulation may take part to the abnormal fetal size such as that observed in GDM/LGA, while the DPP-4 increase detected in placenta may account for some growth abnormalities as well as the dysregulated glycometabolic control in the new-borns, which have been shown in literature.1 This may be of clinical interest given the availability of DPP-4 inhibitors.20 Among proteins found to be altered in GDM/LGA, dimethylarginine dimethylaminohydrolase 1 (DDAH1) was slightly downregulated, which is in line with other reports showing reduced DDAH1 expression and activity in patients with diabetes.21 As DDAH1 is responsible for asymmetric dimethylarginine (ADMA) degradation, a decrease in its expression, as that observed in our patients, may suggest an increase in ADMA levels in GDM/LGA patients as observed in other diabetic subjects, thus pointing at placenta as potential site of production in this condition.22 23 We acknowledge that our study has some limitations, included but not limited to the small number of placenta samples analyzed and the need of a larger validation of the detected proteins.
In order to prove the potential role of PRG2 and DPP-4 in fetal growth, we took advantage of hESCs, a useful tool to assess in vitro effects on fetal development. Our transcriptomic analysis revealed that PRG2 and DPP-4 alter the expression of genes relevant for hESCs differentiation toward cardiac, osteogenic and endodermic progenitors.24 25 Since DE is the precursor for endocrine pancreas development, alterations on endodermic progenitor markers may suggest an impaired generation of pancreas endocrine compartment and function, thus leading to future metabolic disorders such as obesity and type 2 diabetes, frequently observed as long-term complications in LGA children of GDM mothers.26 The mechanisms whereby these proteins may exert their effects on hESCs remains to be established. However, soluble DPP-4 is known to have intact enzymatic activity and it acts in a paracrine or endocrine manner on the targeted cells such as lymphocytes, muscle smooth cells and adipocyte, mainly through the Akt/pAkt, ERK/pERK and/or Nf-kB signaling.27–29 Several soluble factors involved in hESC self-renewal and differentiation like LIF, bFGF and BMP4 possess putative truncation site for DPP-4 and modulation of their levels due to DPP-4 activity could influence hESC physiology.30 This has recently been shown as well for SDF-1/CXCR4 axis that could be modulated by DPP-4 in different types of progenitor cells.31–33 Based on these evidences, we hypothesize that DPP-4 may exert its effect on hESC by activating signaling pathways related to hESC differentiation.
In conclusion, our data indicate that the placental proteome is dysregulated in GDM, particularly with LGA fetuses. Among these altered factors, we identified two major factors, PRG2 and DPP-4, related to pregnancy disorders, which control in vitro hESCs differentiation and may in turn directly affect embryonic development. Given the lack of therapeutic opportunities and approaches for GDM and for GDM/LGA, with diet and insulin being the sole treatments approved for these conditions, we thus envision to generate new monoclonal antibodies or fusion-proteins in order to block the activity of the upregulated proteins. DPP-4 inhibitors, available on the market as antidiabetic oral agents, represent an example of a potential inhibitor of DPP-4 enzymatic activity, which may be tested and further validated in large future trial in GDM/LGA.
Acknowledgments
We would like to thank the ‘Fondazione Romeo e Enrica Invernizzi’ for extraordinary support. Portions of this work were carried out in OMICs, an advanced mass spectrometry platform established by the Università degli Studi di Milano.
References
Supplementary materials
Supplementary Data
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Footnotes
EA and FD are joint first authors.
Contributors EA, ChM and FD designed the study, performed experiments, analyzed data, and wrote the paper; AM, CL, AJS, MBN, and VU performed experiments and analyzed data; CiM performed proteomic analysis; IP, RA, BEE, DC, FF and GZ coordinated sample collection, designed research and edited the paper; IC and PF designed research, wrote and edited the paper. PF is the guarantor of this work and, as such, had full access to all the data in the study and takes responsibility for the integrity of the data and the accuracy of the data analysis.
Funding FD is the recipient of an SID Lombardia Grant. PF is the recipient of the Italian Ministry of Health RF-2016–02362512 grant. VU is supported by a FO.DI.RI SID fellowship.
Competing interests None declared.
Patient consent for publication Not required.
Ethics approval The study protocol number 52/2010 was approved by the ASST Fatebenefratelli-Sacco Ethic Committee. Each individual enrolled provided informed consent to participate in the study.
Provenance and peer review Not commissioned; externally peer reviewed.
Data availability statement Data are available on reasonable request. All data relevant to the study are included in the article or uploaded as supplemental information. The datasets used and/or analyzed during the current study are available from the corresponding author on reasonable request.
Supplemental material This content has been supplied by the author(s). It has not been vetted by BMJ Publishing Group Limited (BMJ) and may not have been peer-reviewed. Any opinions or recommendations discussed are solely those of the author(s) and are not endorsed by BMJ. BMJ disclaims all liability and responsibility arising from any reliance placed on the content. Where the content includes any translated material, BMJ does not warrant the accuracy and reliability of the translations (including but not limited to local regulations, clinical guidelines, terminology, drug names and drug dosages), and is not responsible for any error and/or omissions arising from translation and adaptation or otherwise.