SP-A Induces Preterm Birth through Promoting Oxidative Stress via Upregulating STOX1
Received: 08-Sep-2021 / Accepted Date: 05-Oct-2021 / Published Date: 12-Oct-2021 DOI: 10.4172/1165-158X.1000211
Abstract
Preterm birth is the leading cause of infant mortality. The mechanisms that instigate preterm birth remain elusive and this makes it difficult to predict or prevent preterm birth. In this study, we found that SP-A induced the pathological damage to placenta and promoted preterm birth. Mechanismly, SP-A promoted the expression of STOX1 which further promoted the oxidative stress in placenta through inhibiting the activities of series antioxidant enzymes including SOD, CAT1 and GSH-Px. SP-A also induced dysregulation of arginine metabolism through inhibiting NOS2 and ARG2. Overexpression of STOX1 aggravated SP-A induced oxidative stress, pathological damage and preterm birth, whereas knockdown of STOX1 alleviated SP-A induced oxidative stress, pathological damage and preterm birth. Our study uncovers that SP-A induces preterm birth through promoting oxidative stress via upregulating STOX1, which provides new targets for prediction and prevention of preterm birth.
Keywords: Antioxidant, Enzymes, Corticotropin-releasing hormone, Placental cells, Oxidative stress, Necrosis, Apoptosis
Introduction
Preterm birth is defined as delivery before 37 weeks [1]. It has been reported that the global preterm birth rates are up to ten percent [2]. Preterm birth is a leading cause of neonatal death and those surviving infants have increased risks of inflammatory disorders, neurodevelopmental disorders, metabolic disorders and early-life infections [3-5]. The majorities of preterm births are spontaneous and have no identifiable cause which limited the prediction or prevention of preterm birth. Detailed understanding of the molecular mechanisms underlying preterm birth is needed.
Maternal stress has been shown to be risk factor for preterm birth [6]. Various reports reported that there is a positive association between maternal stress and Corticotropin-Releasing Hormone (CRH) level and CRH appears to mediate the relationship between maternal stress and preterm birth [7-9]. Placenta derived CRH could promote the expression of cortisol and increased cortisol could promote fetal lung secret Surfactant Protein A (SP-A). SP-A could stimulate uterine contraction through promoting the production of prostaglandins and it can also initiating inflammatory response to promote preterm birth [10-12].
Oxidative stress, defined as dysregulation between antioxidants and oxidants, has been reported to contribute to the pathology of preterm birth [13]. Excessive levels of ROS/RNS can cause cell necrosis, cell apoptosis or cell senescence from protein alterations, lipid peroxidation and DNA oxidation [14]. Several studies have reported that preterm birth is associated with lower total antioxidant status and higher total oxidant status in the maternal blood and vaginal washing fluid [15-17]. Oxidative stress is reported to induce damage to fetal membranes and placental cells which further generate uterotonic biomolecular signals that trigger labor process [13].
Storkhead box 1 (STOX1) is a transcription factor that has been shown to be related to recurrent spontaneous abortion and preeclampsia [18,19]. Overexpression of STOX1 could lead to transcriptome alterations involved in several cellular pathways and mitochondrial function is highly represented [20]. STOX1 overexpression results in improved free radical production through inhibiting the expression of a series of important antioxidant modulators, and aggravating preeclampsia [18]. However, the role of STOX1 in preterm birth has not been investigated.
In this study, we established a preterm birth model through upregulating SP-A level, housing mice under a reversed light/dark cycle to increase endogenous SP-A and intra-amniotic injection of SP-A to increase exogenous SP-A. We found that STOX1 was increased in the placenta from preterm birth group. Through knockdown of STOX1, we found that SP-A induced the pathological damage to placenta through STOX1. Mechanismly, SP-A inhibited the activities or protein levels of a series enzymes including SOD, CAT1, GSH-Px, NOS3 and ARG2 through promoting STOX1 and therefore caused increased oxidative stress in placenta and promoted the preterm birth. Our study recovers the role of STOX1 in preterm birth and provides a new target for predicting and preventing preterm birth.
Methods
Animals
BALB/c mice, aged 7-8 weeks, were purchased. The mice were housed in specific pathogen-free conditions at room temperature (22 ± 3ºC) and humidity (35 ± 5%) with light-dark cycle. All animal experiments were approved by Ganzhou People’s Hospital and all animal experiments were performed in compliance with the guide for the care and use of laboratory animals.
Induction of preterm birth
7-8 week-old BALB/c female mice were co-housed with BALB/c male mice overnight and the presence of a copulatory plug was recorded as day 0 of gestation. The pregnant mice were randomly divided into four groups including normal control group (NC group), SP-A group, SP-A+ov-STOX1 group and SP-A+si-STOX1 group. To induce stress response, the mice in SP-A group, SP-A+ov-STOX1 group and SP-A+si-STOX1 group were subjected to inverted light-dark cycles from day10 to day15 of gestation. The mice in SP-A group, SPA+ ov-STOX1 group and SP-A+si-STOX1 group were given 3ug SP-A through intra-amniotic injection at day15 of gestation. Meanwhile, mice in SP-A+ov-STOX1 group were i.v. injected with ov-STOX1 and mice in SP-A+si-STOX1 group were i.v. injected with si-STOX1. After preterm delivery, the placenta of mice was collected and analyzed.
Western blot
The placental tissues were homogenized with a tissue homogenizer and radioimmune precipitation assay lysis buffer was used to extract protein. The protein samples were then separated with 10% SDSPAGE and transferred to PVDF membranes. 5% bovine serum albumin was used to block PVDF membranes. The PVDF membranes were then incubated with primary anti-actin antibody, anti-STOX1 antibody, anti-NOS3 antibody or anti-ARG2 antibody overnight and subsequently incubated with corresponding secondary antibodies. The protein bands were imaged using an ECL reagent (Bio‑Rad laboratories, Inc.).
Immunohistochemistry
Immunohistochemistry was used to determine the expression and location of STOX1 in placenta. Tissues were fixed with 4% PFA, paraffin-embedded and sectioned into 5-μm sections. The sections were de-paraffined with xylene and rehydrated in serial ethanol baths. Citrate buffer was used for antigen retrieval, 3% of hydrogen peroxide was used to block endogenous peroxidase and 5 & BSA was used to block nonspecific binding of antibodies. The samples were incubated with anti-STOX1 primary antibody and subsequently incubated with secondary antibody. The DAB agent was used for visualization of the expression of STOX1.
H&E staining
Placental tissues were fixed with 4% PFA, embedded with paraffin and then sectioned into 5-μm sections. The samples were deparaffined with xylene and rehydrated in serial ethanol baths for hematoxylin and eosin staining. The sections were analyzed with Light microscope (Olympus).
ROS detection
The contents of Reactive Oxygen Species (ROS) were determined using CM-H2DCFDA kit according to manufacturer’s instruction. Briefly, the placental cells were loaded with 1uM CM-H2DCFDA for 30 min at room temperature. The cells were observed immediately under fluorescent microscope (Olympus).
Biochemical analysis
Placentas were homogenized and centrifuged and protein concentrations in the supernatants were measured by the method of Bradford. The activities of SOD, CAT and GSH-Px in the supernatant were determined using superoxide dismutase detection kit (njjcbio), catalase detection kit (njjcbio) and Glutathione peroxidase detection kit (njjcbio) respectively, according to manufacturer’s instructions.
Statistical analysis
Data were presented as Mean ± SD. The student’s t-test was used to analyze the difference between two groups. P <0.05 was considered statistically significant. Statistical analysis was conducted using GraphPad Prism software.
Results
SP-A induced pathological damage to placenta through promoting STOX1
It has been shown that SP-A could promote preterm birth [12]. So we established a mouse model of preterm birth through upregulating SP-A level, housing mice under a reversed light/dark cycle to increased maternal stress to increase endogenous SP-A and intra-amniotic injection of SP-A to increase exogenous SP-A. After preterm birth, the placenta was isolated and analyzed through H&E staining. We found that SP-A induced pathological damage to placenta indicated by fibrinoid necrosis of placental villi, liquefaction of interstitial effusion, nuclear embrittlement of trophoblasts and congestion of spiral artery (Figure 1). To investigate the role of STOX1 in SP-A induced preterm birth, ov-STOX1 was given to overexpress STOX1 while si-STOX1 was given to to knockdown of STOX1. And we found that STOX1 overexpression aggravated the SP-A induced pathological damage to placenta while knockdown of STOX1 alleviate the SP-A induced pathological damage to placenta (Figure 1). These results indicated that SP-A induced pathological damage to placenta through promoting STOX1. To further validate the role of STOX1 in SP-A induced preterm birth, immunohistochemistry was performed to determine the expression of STOX1 in placenta. We found that ov-STOX1 overexpressed STOX1 while si-STOX1 inhibited STOX1 in placenta effectively. More importantly, we found that SP-A promoted the expression of STOX1 in placenta. We also found that SP-A induced nuclear embrittlement of trophoblast, disappearance of interstitial tissue and excessive fibrin deposition in placenta and which is aggravated through ov-STOX1 and alleviated through si-STOX1 (Figure 2). These results further showed that SP-A promoted preterm birth through promoting STOX1.
SP-A inhibited the activities of antioxidant enzymes through STOX1
STOX1 overexpression has been reported to promote free radical production through inhibiting the expression of a series of important antioxidant modulators [18]. And oxidative stress could result in cell apoptosis, cell necrosis and cell senescence and is related to multiple diseases [13,21,22]. So we speculate that STOX1 may be involved in SP-A induced preterm birth through regulating oxidative stress. Superoxide Dismutase (SOD), Glutathione Peroxidase (GSH-Px) and Catalase (CAT) are well-known antioxidant enzymes which play important roles in antioxidant system [23]. So we investigated the activities of SOD, CAT1 and GSH-Px in placenta. We found that SP-A inhibited the activities of SOD, CAT1 and GSH-Px. Moreover, STOX1 overexpression further inhibited the activities of these antioxidant enzymes while knockdown of STOX1 rescued the activities of SOD, CAT1 and GSH-Px significantly (Figure 3). These results indicated that SP-A inhibited the activities of SOD, CAT1 and GSH-Px through STOX1.
SP-A promoted the ROS production in placenta through promoting STOX1
We further investigated the ROS levels in placentas. We found that SP-A promoted the ROS production in placenta. STOX1 overexpression further promoted the ROS level and the ROS level was decreased when STOX1 was inhibited (Figure 4). These results, combined with Figure 3, suggested that SP-A increased oxidative stress in placenta through inhibiting the activities of antioxidant enzymes via STOX1.
SP-A inhibited protein levels of NOS3 and ARG2 in placenta
We further investigated the protein levels of ARG2 and NOS3, two enzymes involved in arginine metabolism [24]. We found that SP-A inhibited the protein levels of NOS3 and ARG2. STOX1 overexpression further inhibited the protein levels of NOS3 and ARG2 while knockdown of STOX1 rescued the protein levels of NOS3 and ARG2. We also detected the activity of NOS3. Consistently, the activity of NOS3 was inhibited by SP-A. STOX1 overexpression further inhibited the activity of NOS3 activity while knockdown of STOX1 recued the activity of NOS3 (Figure 5). These results indicated that SP-A resulted in dysregulation of arginine metabolism through promoting STOX1.
Discussion
Preterm birth is a life-threaten diseases and the surviving infants are at increased risks for multiple diseases [25,26]. Despite some factors have been shown to be related to preterm birth, the majority of preterm births are spontaneous and have no identifiable cause [27,28]. Detailed understanding of the molecular mechanisms underlying preterm birth is important for prediction and prevention of preterm birth. In this study, we established a mouse model of preterm birth through intraamniotic injection of SP-A. We found that SP-A induced pathological damage to placenta. Mechanismly, SP-A promoted the expression of STOX1 and STOX1 further promoted the oxidative stress in placenta through inhibiting the activities of antioxidant enzymes. Our founding reveals a new mechanism underlying preterm birth and provides new targets for prediction and prevention of preterm birth.
Conclusion
We found that SP-A promoted the expression of STOX1 which further inhibited the activities of antioxidant enzymes, SOD, CAT1 and GSH-Px. But how STOX1 regulate the activities of SOD, CAT1 and GSH-Px need to be further investigated. We speculate that as a transcription factor, STOX1 may promote the expression of some microRNAs and these microRNAs target and downregulate the expression of antioxidant enzymes. The decreased protein level of these antioxidant enzymes result in downregulated activities in tissue homogenate. On the other hand, STOX1 may also bind with these antioxidant enzymes directly and inhibit their activities. Further study will help to recover the mechanisms underlying the effects of STOX1 on antioxidant enzymes.
Ethics Approval and Consent to Participate
The ethic approval was obtained from the Ethic Committee of Ganzhou People’s Hospital.
Consent to Publish
All of the authors have Consented to publish this research.
Availability of Data and Materials
The data are free access to available upon request.
Competing Interests
All authors declare no conflict of interest.
Funding
None.
Authors’ Contributions
Each author has made an important scientific contribution to the study and has assisted with the drafting or revising of the manuscript.
Acknowledgements
We would like to acknowledge the everyone for their helpful contributions on this paper.
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Citation: Li X, Zhang C (2021) SP-A Induces Preterm Birth through Promoting Oxidative Stress via Upregulating STOX1. Cell Mol Biol 67: 211. DOI: 10.4172/1165-158X.1000211
Copyright: © 2021 Li X, et al. This is an open-access article distributed under the terms of the Creative Commons Attribution License, which permits unrestricted use, distribution, and reproduction in any medium, provided the original author and source are credited.
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