Abstract
Background
Bronchopulmonary dysplasia (BPD) is characterized by an arrest in lung development and is a leading cause of morbidity in premature neonates. It has been well documented that BPD disproportionally affects males compared to females, but the molecular mechanisms behind this sex-dependent bias remain unclear. Female mice show greater preservation of alveolarization and angiogenesis when exposed to hyperoxia, accompanied by increased miR-30a expression. In this investigation, we tested the hypothesis that loss of miR-30a would result in male and female mice experiencing similar impairments in alveolarization and angiogenesis under hyperoxic conditions.
Methods
Wild-type and miR-30a−/− neonatal mice were exposed to hyperoxia [95% FiO2, postnatal day [PND1-5] or room air before being euthanized on PND21. Alveolarization, pulmonary microvascular development, differences in lung transcriptome, and miR-30a expression were assessed in lungs from WT and miR-30a−/− mice of either sex. Blood transcriptomic signatures from preterm newborns (with and without BPD) were correlated with WT and miR-30a−/− male and female lung transcriptome data.
Results
Significantly, the sex-specific differences observed in WT mice were abrogated in the miR-30a−/− mice upon exposure to hyperoxia. The loss of miR-30a expression eliminated the protective effect in females, suggesting that miR-30a plays an essential role in regulating alveolarization and angiogenesis. Transcriptome analysis by whole lung RNA-Seq revealed a significant response in the miR-30a−/− female hyperoxia-exposed lung, with enrichment of pathways related to cell cycle and neuroactive ligand–receptor interaction. Gene expression signature in the miR-30a−/− female lung associated with human BPD blood transcriptomes. Finally, we showed the spatial localization of miR-30a transcripts in the bronchiolar epithelium.
Conclusions
miR-30a could be one of the biological factors mediating the resilience of the female preterm lung to neonatal hyperoxic lung injury. A better understanding of the effects of miR-30a on pulmonary angiogenesis and alveolarization may lead to novel therapeutics for treating BPD.
Plain Language Summary
Bronchopulmonary dysplasia (BPD) is a lung condition that affects babies born prematurely, causing problems with their lung development. Interestingly, BPD tends to affect boys more than girls, but we do not fully understand why. To investigate this, we conducted a study using mice. Female mice had better lung development and blood vessel formation when exposed to high oxygen levels. We found higher expression of a molecule called miR-30a in the female mice and seemed to be protective. So, we wanted to see if removing miR-30a would have the same effect on both male and female mice. To test this, we exposed newborn mice without miR-30a and normal mice to high oxygen levels or regular room air. Interestingly, the differences between normal males and females were no longer present in the mice without miR-30a. This suggested that miR-30a plays an important role in lung development. We also identified that the female mice without miR-30a, when exposed to high oxygen, had the greatest number of genes affected, and these gene changes were like those seen in blood samples from premature babies with BPD. Finally, we report that miR-30a was in a specific part of the lung called the bronchiolar epithelium. Overall, this study suggests that miR-30a is crucial in protecting premature lungs from damage caused by high oxygen levels. By understanding how miR-30a affects lung development, we may be able to develop new treatments for BPD in the future.
Highlights
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Sex-specific differences are abrogated in neonatal miR-30a−/− mice upon exposure to hyperoxia.
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The loss of miR-30a expression eliminated the female resilience to neonatal hyperoxic lung injury.
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Pulmonary miR-30a expression could be one of the protective epigenetic mechanisms in the neonatal female lung.
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Background
Bronchopulmonary dysplasia (BPD) is characterized by an arrest in lung development with severe impairment in vascular development and alveolarization [1]. Despite recent advances in perinatal care, BPD remains a leading cause of morbidity in premature neonates [2, 3]. Infants with BPD also face a variety of long-term sequelae, including pulmonary hypertension, increased rehospitalization rates, and additional risk for pulmonary disease as adults [4,5,6,7,8]. Many pre- and post-natal factors contribute to disease pathogenesis in BPD, including exposure to postnatal hyperoxia due to the generation of reactive oxygen species [9, 10]. It has been well documented that BPD disproportionally affects males compared to females. Males are at an increased risk for developing moderate-to-severe BPD and experience higher neonatal and infant mortality rates, but the molecular mechanism behind this sex-dependent bias remains unclear [11,12,13,14,15,16,17,18].
MicroRNAs (miRs) play an important role in the post-transcriptional regulation of protein-coding genes and act primarily by destabilizing the mRNA of their target genes. miR-30a is a known pro-angiogenic miR that stimulates arteriolar branching via the downregulation of Dll4 [19, 20]. miR-30a levels are decreased in the peripheral blood of neonates with evolving and established BPD, which may be correlated with arrested lung development [21].
Mice exposed to postnatal hyperoxia develop pathognomonic features of human BPD and are used to model the disease [22,23,24]. Like their human counterparts, female mice are more resilient when exposed to hyperoxia, while males show greater arrest in alveolarization and angiogenesis [18, 25]. Previous studies found that this sexual dimorphism is accompanied by an increased pulmonary expression of microRNA-30a (miR-30a) in female mice compared to male mice exposed to hyperoxia. The findings were replicated in neonatal human pulmonary microvascular endothelial cells (HPMECs), with female endothelial cells showing higher expression of miR-30a when exposed to hyperoxia in vitro [26]. miR-30a could contribute to the resilience of the neonatal female lung when exposed to hyperoxia. In this investigation, we sought to clarify the role miR-30a plays in the previously observed sex-specific differences in lung development of mice exposed to hyperoxia. We tested the hypothesis that loss of miR-30a in mice would result in male and female mice experiencing similar impairments in alveolarization and angiogenesis when exposed to hyperoxia. The current study outlines the consequences of loss of miR-30a in neonatal hyperoxic lung injury, the sex-specific differences, and reveals the biological pathways mediating these differences, as outlined in Fig. 1. Overall, our results reveal a critical role of miR-30a in possibly mediating the sex-specific differences in BPD.
Materials and methods
Animals
All animal studies were conducted with the approval of the Institutional Animal Care and Use Committee (IACUC) of Baylor College of Medicine. Experiments were performed in accordance with relevant guidelines and regulations. Care of animals in research met the highest contemporary standards per the 8th edition of the Guide for the Care of Use of Laboratory Animals and other IACUC protocols. miR-30a−/− mice were received from Dr. Sean Hartig from Baylor College of Medicine. CRISPR/Cas9 gene editing was used to knockout the entire miR-30a gene. Wild-type (WT) and miR-30a−/− mice were bred in the animal facility and both were on the C57BL/6J background. Guide RNAs flanked the 1-kb genomic region that contains miR-30a and knockout was confirmed using qPCR analysis and DNA sequencing of the deleted region. The miR-30a−/− mice are viable and show no overt phenotypes during postnatal growth [27]. The sex of the neonatal mouse pups was determined by both anogenital distance and pigmentation in the anogenital region [28]. Sex was reconfirmed with PCR analysis for the Sry gene in genomic DNA obtained from mouse tail clips [18].
Mouse model of BPD
Exposure to hyperoxia (95% FiO2) mimics the alveolar arrest of bronchopulmonary dysplasia in mouse pups [24, 29]. Mouse pups from multiple litters were pooled before being randomly and equally redistributed by sex into two groups, one group exposed to normoxia (21% FiO2), and the other group exposed to hyperoxia (95% FiO2), within 12 h of birth for 5 days [23]. Animals were chosen at this time because neonatal mice are at the saccular stage of lung development during this period, which is approximately equivalent to 26–36 weeks in human neonates. The dams were rotated between air- and hyperoxia-exposed litters every 24 h to prevent oxygen toxicity and to eliminate maternal effects between the groups. Oxygen exposure was conducted in plexiglass chambers as previously described [18]. Mice were euthanized on postnatal day (PND) 21 after recovery in room air, as most of postnatal lung development in mice is complete by this age. miR-30a levels were most different between male and female mice after early hyperoxia exposure at PND21 with female mice showing significantly higher expressions. Hence, PND21 was chosen as the time-point for analysis of lung morphometry and gene expression signatures [26]. The control group was kept at room air for the same duration of time. 5–7 pups/genotype/treatment were included for the morphometry related studies. Data from previously published studies were used in this manuscript, including lung histology data in WT mice [18] and lung transcriptome data from male and female WT neonatal mice [25]. The WT and miR-30a−/− mice were not exposed to hyperoxia simultaneously for this study.
Lung histology
Both hyperoxia- and normoxia-exposed mice were anesthetized (100 mg/kg i.p. pentobarbital sodium), tracheas were cannulated, and lungs were fixed by instilling with 4% paraformaldehyde endotracheally at 25 cmH2O pressure for 15 min. The trachea was tied off and the lungs were removed and further fixed overnight at 4 °C, followed by dehydration in graded alcohol and embedding in paraffin.
Analysis for alveolarization
Sections (5 μm) were prepared and stained with hematoxylin and eosin (H&E). Alveolar development was evaluated by the measurement of mean linear intercept (MLI) [30]. Ten randomly selected, non-overlapping areas were photographed with bright field microscopy (40×). The photographs were overlaid with a grid and alveolar wall intersections with array lines were manually counted in a blinded fashion to prevent observer bias. Fields containing large airways and vessels were excluded. Radial alveolar count was measured as previously described [18]. Each section was analyzed in a blinded fashion to prevent observer bias by two reviewers.
Analysis for macrophages
Pulmonary macrophage count was determined based on immunofluorescence staining for F4/80 (1:500 dilution, Bio-Rad Laboratories; catalog no. MCA497GA), a macrophage-specific marker. Fifteen randomly selected, non-overlapping areas were photographed with bright field microscopy (40×). For each image captured, brown-color-stained macrophages were manually identified and counted to determine the macrophage count [18]. Each section was analyzed in a blinded fashion to prevent observer bias by two reviewers.
Analysis for pulmonary vascular development
Pulmonary vessel density was determined based on immunofluorescence staining for von Willebrand factor (vWF; 1:4000 dilution, Abcam, ab6994), an endothelial specific marker. Ten randomly selected, non-overlapping areas were photographed with bright field microscopy (20 ×). For each image captured, pulmonary vessels (< 50 um in diameter) were manually identified and counted to determine density [18]. Each section was analyzed in a blinded fashion to prevent observer bias by two reviewers.
Preparation of lung samples for transcriptomic analysis, library preparation, and sequencing
Mice were euthanized on PND21 with i.p. pentobarbital. The right ventricle was perfused with ice cold PBS, and lungs were flash frozen in liquid nitrogen until ready for total RNA extraction. Total RNA from frozen lung samples was isolated using the Zymo micro kit (Zymo Research, Irvine, CA). Sample concentration was assayed using Nanodrop-8000 (Thermo Scientific, Wilmington, DE), and quality checks were done using the NanoDrop spectrophotometer and the Agilent Bioanalyzer. Three samples of total RNA with RIN values > 8, were subjected to RNA-Seq analysis. RNA libraries were prepared with QIAseq Stranded Total RNA library Kit (Qiagen) using 1000 ng input RNA, and purity of the libraries was analyzed using the DNA 1000 tape Tapestation 4200 (Agilent). The indexed libraries were pooled and sequenced.
Analysis of RNA-Seq data
The miR-30a−/− data have been submitted to NCBI GEO (GSE213287). Previous WT samples were submitted to NCBI GEO (GSE97804). All the RNA-Seq used was trimmed for Illumina adapters and low-quality terminal base pairs using trim galore. Filtered and trimmed sequences were mapped to the mouse genome build UCSC mm10 using the STAR software [31]. Gene expression was quantified as read counts using featureCounts [32]. Further batch normalization was applied using CombatSeq [33]. Data were normalized using RUVr [34] and upper quartile normalization; the EdgeR [35] R package was used for differential gene expression analysis, with significance achieved at FDR < 0.05 and fold change exceeding 1.5x. Enriched pathways were determined using Gene Set Enrichment Analysis (GSEA) against gene set collections compiled by MSigDB [36], with significance achieved at FDR < 0.25 per the software developers' best practices. Heatmaps were generated using the R statistical system. Upset plots for gene signatures were generated using the ComplexHeatmap R package.
Analysis using GTex data
Transcriptomic profiles of 578 whole adult human lungs compiled by the Genotype-Tissue Expression (GTEx) project were downloaded. Gene symbols conserved between mouse and human were converted to the mouse symbols using Biomart. Gene signatures for each sample were computed using the summed z-scores method. First expression of each gene across all samples was converted to a z-score to determine how many standard deviations each gene was away from the mean. Next, for each sample z-scores of up-regulated genes were added, and z-scores of down-regulated genes were subtracted. Gene signature correlation was computed for all signatures using the Pearson correlation coefficient as implemented in the Python scientific library, with significance achieved for p-value < 0.05 [37].
Analysis using the human blood data
Bronchopulmonary dysplasia (BPD) blood transcriptomics from newborns were downloaded from the dataset GSE32472 [38]. Gene symbols for genes conserved between mouse and human were converted to the mouse gene symbols using Biomart. Gene signatures for each sample were computed using the summed z-scores method as described above. Correlations of summed z-scores with numerical clinical variables were computed using the Python scientific library.
Quantitative real-time PCR (qRT-PCR)
Total RNA was extracted from the lungs using the Quick-RNA MiniPrep kit (ZYMO Research, Cat# R1055) following manufacturer's instruction. RNA integrity was evaluated by Agilent 2100 bioanalyzer. cDNA was synthesized with 1 ug of total RNA using Applied Biosystems High-Capacity cDNA Reverse Transcription Kit (ThermoFisher, Cat# 4,374,966). qRT-PCR was conducted in duplicates on a 384-well plate on the Applied Biosystems QuantStudio 6 Pro system (ThermoFisher) using the Applied Biosystems TaqMan Fast Advanced Master Mix (2X) with following conditions (QuantStudio 6 Pro Fast run mode): hold 50 °C for 2 min, hold 95 °C for 20 s followed by 95 °C for 1 s and 60 °C for 20 s for 40 cycles. All gene expression assays were conducted using Applied Biosystems Taqman Probes (TaqMan® Gene Expression Assays, ThermoFisher Scientific). Genes of interest used in this study were Chl1 (Mm00483313_m1) and Cd109 (Mm00462151_m1). Three housekeeping genes, including Vcl (Mm00447745_m1), B2m (Mm00437762_m1) and Tbp (Mm01277042_m1), were selected as endogenous controls for normalization. Gene expression Ct values for both target and housekeeping genes were directly acquired by QuantStudio Design and Analysis software (DA2 software v2.6.0, ThermoFisher Scientific). The target gene expression (ΔCt value) was normalized through incorporation of the housekeeping genes B2m/Vcl/Tbp by the DA2 software. The changes in expression for genes of interest (ΔΔCt values) were calculated using the gene expression in room air values in the respective sex as reference, and the fold changes were generated using the 2−ΔΔCt method.
In situ hybridization
Mice were euthanized on PND21 with i.p. pentobarbital, lungs were inflated and fixed in 4% paraformaldehyde (PFA) for 24 h. Histomorphometry was carried out on 7-μm paraffin sections of samples (n = 3 per sex/oxygen environment for WT). Samples were stained using hematoxylin and eosin (H&E), cover slipped with Vectamount permanent mounting medium (Vector labs, Newark, CA, USA), and imaged with Leica Thunder Imager DMi8 (Leica, Nußloch, Baden-Wurttemberg, Germany). On serial sections to the sections used for H&E, we performed in situ hybridization (ISH) using the BaseScope Duplex Kit (Advanced Cell Diagnostics, Hayward, CA, USA). Samples (n = 3 per sex/oxygen environment) were treated with a miR-30a probe (Advanced Cell Diagnostics, Hayward, CA, USA) for 2 h at 4 °C. A positive control slide used a mixture of probes targeting housekeeping gene Polr2A. A negative control slide used dapB (a bacterial gene). Nuclei were counterstained with a 50% hematoxylin solution and mounted with Vectamount permanent mounting medium (Vetor labs, Newark, CA, USA). Slides were imaged using Leica Thunder Imager DMi8 (Leica, Nußloch, Baden-Wurttemberg, Germany).
Statistical analysis
GraphPad version 9 (GraphPad Software, San Diego, CA) was used for data analysis. Data were expressed as means ± SE. Differences were assessed by three-way ANOVA to test for the independent effects of sex, genotype and hyperoxia. Multiple comparison correction (Bonferroni) was performed. Differences determined by ANOVA were considered significant if p-values were less than 0.05 after correction.
Results
Sex-specific differences in alveolarization were lost in miR-30a−/− mice in the setting of neonatal hyperoxia exposure
Male and female miR-30a−/− mice were exposed to room air or hyperoxia (95% FiO2) within 12 h of birth for 5 days, during the saccular stage of lung development. After recovering in room air until PND21, lung morphometry was assessed to evaluate the effect of hyperoxia in the absence of miR-30a expression. Representative lung sections (PND21) stained with hematoxylin and eosin from WT and miR-30a−/− mice are shown in Fig. 2A. Alveolar development was quantified using mean linear intercept (MLI) and radial alveolar count (RAC) shown in Fig. 2. There was no difference between WT and miR-30a−/− mice under normoxic conditions. Statistical analysis was performed by 3-way ANOVA to account for sex, genotype, and treatment. The statistical significance of the independent variables and their interaction terms are depicted in Additional file 2: Table S1. There was a significant impact of hyperoxia exposure on both the genotypes in either sex, with an increase in MLI and decrease in RAC upon hyperoxia exposure (Fig. 2B, C). In WT mice, MLI was lower and RAC higher in females compared to males. However, this sex-specific difference was lost in miR-30a−/− mice. MLI was higher in miR-30a−/− females compared to WT females in the hyperoxia group, with no differences between miR-30a−/− males and females. For MLI, genotype, treatment, and sex also showed a main effect with all the interaction terms being significant except for 'treatment x genotype'. Genotype, treatment, but not sex, had a main effect on RAC and all the interaction terms were significant except 'genotype x treatment x sex'.
We also quantitated lung macrophages in WT and miR-30a−/− mice (Fig. 3A). At baseline, the macrophage count was decreased in WT females (compared to WT males) and in miR-30a−/− males (compared to WT males). Hyperoxia increased macrophages in the distal lung in all the hyperoxia exposed groups compared to room air controls. miR-30a−/− mice had a lower macrophage count in the distal lung compared to WT mice (Fig. 3B). Main effects were significant for sex, genotype, and treatment by 3-way ANOVA (Additional file 1: Fig. S1). The interaction term of 'sex x genotype' was also significant.
Loss of miR-30a leads to similar impairment of distal lung vascular development in male and female mice
To assess the effects of hyperoxia on vascular development in the miR-30a−/− cohort, vessel counts were quantified using anti-vWF antibodies, as described in methods. Representative lung sections from normoxia- and hyperoxia-exposed WT and miR-30a−/− mice are shown in Fig. 4A. At baseline, the vessel count was decreased in miR-30a−/− mice compared to WT mice of the same sex. As expected, there was a significant decrease (P < 0.01) in vessel count in the hyperoxia group when compared to the room air group (Fig. 4B). Vessel counts in the hyperoxia-exposed miR-30a−/− female mice were significantly lower compared to the WT female mice; the same was true for males. Statistical analysis by 3-way ANOVA showed a main effect of treatment and sex, but not genotype (Additional file 1: Fig. S1). All the interaction terms were statistically significant.
Loss of miR-30a led to significant changes in gene expression in the neonatal lung exposed to hyperoxia
The overlap and differences in gene expression and modulated biological pathways in WT and miR-30a−/− mice are highlighted in Fig. 5. The number of differentially expressed genes (DEGs; up- and down-regulated) is shown in Fig. 5A, comparing hyperoxia-exposed animals to controls in each genotype. Strikingly, the miR-30a−/− female lung had nearly 2000 up-regulated genes, substantially higher that any of the other groups, leading us to speculate that loss of miR-30a has a greater impact on the female neonatal lung compared to the male. Genes that were either unique or common to one or more genotypes are represented in Fig. 5A. Compared to total number of DEGs, there were a minority that overlapped between the genotypes and sexes. Among female mice, there were only 36 up-regulated and 8 down-regulated genes that were common between WT and miR-30a−/− mice. To quantitatively derive potential functional relationships between gene signatures, analysis of gene signature summed z-scores in full human lung transcriptomes can capture unappreciated co-regulatory relationships between genes. Whereas large collections of human lung transcriptomes from newborns would be ideal for this purpose, they are not readily available; however, the adult human lung transcriptomes compiled by the GTEx consortium are a suitable alternative [39]. To study the clustering of the lung transcriptome responses based on genotype and sex, we used transcriptome profiles of healthy human adult lung samples (n = 578) compiled by the GTEx consortium, one of the largest scale efforts to assess genotype/transcriptome relationships in phenotypically healthy individuals [37]. Summed z-scores for each human individual and each genotype signature were computed and assessed for inter-signature correlations. There was a clear separation between the miR-30a−/− hyperoxia signatures, as shown in Fig. 5B, with the female miR-30a−/− hyperoxia signature showing the most separation. Clustering of enriched biological pathways from Gene Ontology Biological Process, as determined by gene set enrichment analysis (GSEA), also revealed separation of the miR-30a−/− hyperoxia-exposed female neonatal lung compared to the other genotypes and sexes (Fig. 5C). Among the enriched pathways most induced in miR-30a−/− hyperoxia-exposed female neonatal lungs were those related to cell cycle and neuroactive ligand receptor interaction. Lipoprotein assembly and remodeling, PPAR signaling pathway, and the renin angiotensin system were enriched in the miR-30a−/− male lung (Additional file 3: Table S2). Since miR-30a would be expected to decrease the expression of target genes in the WT female hyperoxia-exposed lung, we identified biological pathways that were negatively enriched in the WT hyperoxia-exposed female lung, but positively enriched in the miR-30a−/− female lung. (Fig. 5D). Sensory perception, nervous system process, calcium ion transport, skeletal muscle contraction, and epidermis development were positively enriched in the miR-30a−/− female but negatively enriched in the WT female. Conversely, respiratory system development, collagen fibril organization, epithelial tube formation, and artery morphogenesis were negatively enriched in the miR-30a−/− female lung but positively enriched in the WT female lung.
Figure 6A highlights examples of differentially expressed genes that were upregulated in miR-30a−/− females but downregulated in the WT female upon exposure to hyperoxia compared to controls maintained in room air. We selected genes that were known miR-30a targets and down-regulated in the female WT lung but upregulated in the female miR-30a−/− lung for validation by qRT-PCR in an independent cohort of mice, similarly, exposed to hyperoxia and euthanized on PND21. One of the targets we validated was Chl1 (Cell Adhesion Molecule L1 Like), a protein that functions as an extracellular matrix and cell adhesion protein and potentiates integrin-dependent cell migration towards extracellular matrix proteins. Chl1 expression was increased in miR-30a−/− hyperoxia-exposed females compared to its room air control and compared to WT hyperoxia-exposed females (Fig. 6B). In the LungMAP database, the Chl1 gene was expressed in airway basal cells, goblet cells, and PNECs (Fig. 6D, E).
Another gene target that we validated was Cd109, which encodes a glycosyl phosphatidylinositol (GPI)-linked glycoprotein on the surface of platelets, activated T-cells, and endothelial cells. The protein negatively regulates signaling by transforming growth factor beta (TGF-beta) by binding to it. In our validation by qRT-PCR, Cd109 expression was increased in miR-30a−/− hyperoxia-exposed females compared to its room air control, compared to WT hyperoxia-exposed females, and compared to miR-30a−/− hyperoxia-exposed males (Fig. 6C). In the LungMAP database, the Cd109 gene was highly expressed in the basal cells in the human lung airway in addition to other cell types (Fig. 6D, E).
Gene expression signature in the miR-30a−/− female lung associated with human BPD blood transcriptomes
The distribution of summed z-scores for the hyperoxia gene signatures from the four genotypes at PND21 was compared to gene expression signatures obtained from the blood of human preterm neonates who developed BPD [38]. Four clinical variables were chosen: gestational age, birth weight, BPD status, and oxygen requirement at 28 days and the samples were stratified by sex (Fig. 7A). The WT female hyperoxia signature positively correlated with gestational age, and negatively with BPD status. Interestingly, the gene signature pattern in miR-30a−/− males correlated positively with both gestational age and birth weight and negatively with BPD status and oxygen therapy at 28 days. Strikingly, the transcriptomic signature from the hyperoxia-exposed miR-30a−/− female lungs had a negative correlation with gestational age and birth weight and a positive correlation with BPD status. The correlation values based on BPD disease severity are shown in Fig. 7B. Distribution of summed z-scores (y-axis) for the murine lung hyperoxia signatures were correlated with the gene signature in human newborn blood samples collected at PND28, stratified by biological sex and by BPD status (x-axis: BPD severity; no BPD, mild, moderate, and severe). A significant negative correlation with either the WT female or miR-30a−/− male hyperoxia signatures, but a significant positive correlation with the miR-30a−/− female hyperoxia signature. We next identified biological pathways that were similarly enriched between the miR-30a−/− female lung hyperoxia exposure and the human BPD patients (compared to healthy controls) but modulated in the opposite direction by hyperoxia in the WT female lung (Fig. 7C). Pathways related to keratinization, ion transport, neurotransmitter metabolic process, and regulation of vasoconstriction were positively enriched in the miR30a−/− female lung and human BPD, while histone methylation and chromatin organization were negatively enriched in both.
miR-30a was expressed in the bronchioles in the lung upon exposure to hyperoxia compared to vessels and the lung parenchyma
To delineate cell-specific expression of miR-30a in the murine lung we performed in situ hybridization in lung sections, shown in Fig. 8. The expression was mainly localized to the bronchiolar epithelial cells (Fig. 8B, C, E). Expression was also measured in the vessels and the lung parenchyma, but the expression was lower compared to the bronchiolar epithelium. Overall, the expression was higher in the female lung after exposure to hyperoxia in the bronchioles but was not statistically significant.
Discussion
Neonatal male mice show greater arrest in alveolarization and vascularization following exposure to hyperoxia when compared to females [18]. This protective effect in female mice is accompanied by increased miR-30a expression [26]. In this investigation, we examined the role of miR-30a in alveolarization and vascular development and showed that miR-30a modulates sex-specific differences in neonatal lung in hyperoxic conditions. Significantly, miR-30a−/− mice did not exhibit sex-specific differences in alveolarization and vascular development in the postnatal hyperoxia model, as previously reported in WT mice [18]. Without expression of miR-30a, both sexes suffered similar adverse impact in alveolarization and vascular development when exposed to hyperoxia.
Post-transcriptional regulation of many protein-coding genes is modulated by small noncoding RNAs, called miRNAs (miRs). They mainly act to decrease gene expression of their target genes by decreasing mRNA stability. Each miRNA can have up to hundreds of downstream target genes and individual genes can be modulated by multiple miRs. Differential expression of miRNAs could be a potential mechanism underlying sexual dimorphism in a variety of diseases. Bronchopulmonary dysplasia has a multifactorial etiology and is a disease that specifically afflicts the developing preterm lung. Males are more susceptible to the development of this disease, which suggests that sex as a biological variable plays a crucial role in its pathophysiology [40]. Many studies have emphasized the role of miRs in the pathophysiology of BPD, however they did not address the sex-specific differences in their expression or regulation [41,42,43,44,45,46,47,48,49,50]. miR-30a emerged as one of the possible factors mediating the sex-specific differences in our previous study [26]. In vivo, the hyperoxia-exposed female lung showed higher miR-30a expression and in vitro female human pulmonary microvascular endothelial cells showed increased expression of miR-30a upon exposure to hyperoxia. miR-30a has anti-inflammatory [51, 52] and anti-fibrotic [53, 54] effects in various organ systems and disease processes.
Multiple publications have investigated the role of miR-30a in pulmonary diseases. miR-30a was down-regulated in the bronchoalveolar lavage fluid and lung samples obtained from patients with idiopathic pulmonary fibrosis (IPF) [55,56,57]. The adverse phenotype observed in the miR-30a−/− lung could be attributed to many downstream targets with relevance to lung diseases including idiopathic pulmonary fibrosis, COPD, and asthma [58, 59]. miR-30a stabilizes pulmonary vessels by decreasing vascular hyperpermeability [60] and was downregulated in a model of hypoxia-induced pulmonary hypertension [61]. In a case control study, which reported the expression profiles of miRNAs in the peripheral blood of very low birth weight preterm infants, miR-30a expression was decreased both in babies with evolving BPD at 2 weeks postnatal age and at 36 weeks of post-menstrual age. [21].
We noted the macrophage count in the hyperoxia exposed miR-30a−/− lungs to be lower than hyperoxia exposed WT mice. The macrophage population within the lung is very heterogenous with unique niches and biological roles [62,63,64]. miR-30a plays a role in macrophage polarization [65,66,67] and the distinction between alveolar and interstitial macrophages in the miR-30a−/− lung and macrophage polarization state needs to be investigated in future experiments. Interestingly, pathways related to sensory perception and nervous system process were enriched in the miR-30a−/− female lung upon exposure to hyperoxia compared to the WT female lung. Among the genes upregulated in the miR-30a−/− hyperoxia- exposed female lung are those enriched in pulmonary neuroendocrine cells (PNECs). PNECs have important roles in airway physiology and immunity by producing bioactive amines and neuropeptides [68]. Many pulmonary diseases exhibit PNEC hyperplasia [69, 70]. These include genes such as chromogranin A (Chga), chromogranin B (Chgb), secretogranin-II (Scg2), Ubiquitin C-Terminal Hydrolase L1 (Uchl1), olfactory receptor genes (Olfr 78), calcitonin related genes (Calcb and Calcr) and Neural cell adhesion molecule 1 (Ncam 1) [70,71,72,73]. Tubb3 expression was also higher. Airway basal stem cells give rise to Tubb 3 + PNECs and Tubb 3 + PNECs are increased in infant diseases [73]. A study in infants with BPD also revealed a higher number of pulmonary neuroendocrine cells [74]. Basal cell markers, such as Krt5 and Trp63, were also upregulated in the miR-30a−/− hyperoxia-exposed female lung [65]. Basal cells function as tissue-specific stem cells participating in repair after lung injury. The biological relevance of these genes in the miR-30a−/− hyperoxia-exposed female mice needs to be examined in future studies. Interestingly, the neurotransmitter metabolic process was a biologic pathway enriched in the blood transcriptomic signature of preterm babies with BPD and the miR-30a−/− hyperoxia- exposed female lung.
We validated two genes (Cd109 and Chl1) that were predicted to be miR-30a targets and were upregulated in the miR-30a−/− and downregulated in the WT hyperoxia-exposed neonatal female lung. In a model of oxygen-induced retinopathy, Xu et al. reported that CD109 was among the most down-regulated proteins in hypoxic retinal endothelial cells. Overexpression of CD109 decreased, while downregulation increased endothelial cell proliferation in both human retinal and umbilical vein endothelial cells [75]. CD109 is a GPI-anchored protein that acts as a TGF-β co-receptor and a negative regulator of TGF-β signaling. It facilitates TGF-beta receptor endocytosis and subsequent degradation, thus inhibiting TGF-beta signaling [76]. Chl1 is expressed in the mouse carotid body, and loss of Chl1 decreased mortality and improved adaptation to acute hypoxia [77]. In a study involving pulmonary adaption to hypoxia at high altitude, Chl1 was one of the most downregulated genes, possibly modulating the enhanced ventilatory response after exposure to hypoxia. [78] These target genes are expressed in the airway epithelium, basal cells, and PNECs as shown from the LungMAP database. Furthermore, ISH studies from this study localized miR-30a in the bronchioles. miR-30a expression was increased in bronchial brushings, and miR-30a transcripts were localized to human bronchial epithelium [79]. PNECs are found at airway bifurcations or bronchioloalveolar junctions and serve as airway sensors to control lung immune response [68, 73]. Taken together, these data suggest a possible role of miR-30a in the pulmonary basal cells and/or PNECs.
We recognize the limitations of this current investigation. The findings in this study are from a global knock-out/loss of miR-30a. Intrapulmonary delivery strategies for inhibiting miR-30a or cell-specific loss of mir-30a would be superior to elucidate the organ-specific or cell-specific role of miR-30a. Long-term functional consequences of miR-30a loss related to lung function and pulmonary hypertension were not measured in this study. The cell-specific expression data in human lungs may be tightly associated with the developmental stage of the human lung and needs further validation. The correlation between mouse lung samples and human blood samples is not ideal, but these findings lend translational relevance of the biological role of miR-30a in BPD pathogenesis. Additionally, findings from the murine model may not translate directly to humans. However, several parallels between miR-30a expression in human patients with other lung diseases (COPD, asthma, and IPF) that possess similarities in phenotypes to BPD support the translational relevance of this miRNA [57, 59, 65]. In conclusion, we show the loss of sex-specific differences in neonatal hyperoxic lung injury after loss of miR-30a and a significant impact of miR-30a loss in the female neonatal lung. We also highlight the enrichment of genes expressed in PNECs and airway basal cells in miR-30a-/- female lungs exposed to hyperoxia.
Perspectives and significance
We believe our data present a significant advancement in explaining the molecular basis behind the sex-specific differences of neonatal hyperoxic lung injury and BPD. The primary mechanisms of miR-30a regulation and functional outcomes remain elusive. Exploring whether supplementation of miR-30a through AAV-mediated or other approaches can rescue or improve the lung injury phenotype in the murine hyperoxic lung injury model should be the focus of future research.
Conclusions
miR-30a could be one of the biological factors mediating resilience of the preterm lung to neonatal hyperoxic lung injury. A better understanding of the effects of miR-30a on pulmonary angiogenesis and alveolarization may lead to novel therapeutics for the treatment of BPD.
Availability of data and materials
The miR-30a−/− data have been submitted to NCBI GEO (GSE213287). Previous WT samples were submitted to NCBI GEO (GSE97804). The datasets used and/or analyzed during the current study are available from the corresponding author on reasonable request. Bronchopulmonary dysplasia (BPD) blood transcriptomics from newborns were downloaded from the public NCBI GEO dataset GSE32472.
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Funding
This project was supported by NIH grants R01 HL144775, R01 HL146395 and R21HD100862 to KL. SLG and CC were partially supported by The Cancer Prevention Institute of Texas (CPRIT) grants RP170005, RP210227, RP200504, NIH P30 shared resource grant CA125123, NIEHS grants P30 ES030285 and P42 ES027725, and NIMHD grant P50 MD015496. This project was supported in part by the Genomic and RNA Profiling Core at Baylor College of Medicine with funding from the NIH S10 grant (1S10OD023469). Some of the results are partly based upon data generated by the LungMAP Consortium [U01HL122642] and downloaded from (www.lungmap.net), on September 29, 2022. The LungMAP consortium and the LungMAP Data Coordinating Center (1U01HL122638) are funded by the National Heart, Lung, and Blood Institute (NHLBI).
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KL conceived and planned the experiments. XD, CL, AW and MG carried out the experiments. SG, SR, MG, and CC analyzed the data and formulated the results. SG, SR, CL, MG, BM, SH, KL, and CC contributed to the interpretation of the results. KL, CC, and SG took the lead in writing the manuscript. All authors provided critical feedback and helped shape the research, analysis, and manuscript. All authors read and approved the final manuscript.
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Additional file 1.
3-way ANOVA analysis.
Additional file 2: Table S1.
Differentially expressed genes (Hyperoxia over Room Air).
Additional file 3: Table S2.
Gene Set Enrichment Analysis (GSEA).
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Grimm, S.L., Reddick, S., Dong, X. et al. Loss of microRNA-30a and sex-specific effects on the neonatal hyperoxic lung injury. Biol Sex Differ 14, 50 (2023). https://doi.org/10.1186/s13293-023-00535-6
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DOI: https://doi.org/10.1186/s13293-023-00535-6