Skip to main content
Hauptrubriken
CME Facharzt-Training Webinare Zeitschriften Bücher e.Medpedia Podcast
Service
Jobbörse Info & Hilfe
Fachgebiete
Anästhesiologie Allgemeinmedizin Arbeitsmedizin Augenheilkunde Chirurgie Dermatologie Gynäkologie und Geburtshilfe HNO Innere Medizin Kardiologie Neurologie Onkologie und Hämatologie Orthopädie und Unfallchirurgie Pädiatrie Pathologie Psychiatrie Radiologie Rechtsmedizin Urologie Zahnmedizin
Themen
Typ-2-Diabetes und Adipositas Klimawandel und Gesundheit Neues aus dem Markt COVID-19 Praxis und Beruf Seltene Erkrankungen GOÄ & EBM Panorama
Sammlungen
Kasuistiken Algorithmen & Infografiken Blickdiagnosen Arthropedia FlapFinder (für Dermatochirurgen) Videos Kongressberichterstattung Medizin für Apothekerinnen und Apotheker Für Ärztinnen und Ärzte in Weiterbildung Für Medizinstudierende
Erweiterte Suche
Anmelden
nach oben
BMC Complementary Medicine and Therapies
Erschienen in: BMC Complementary Medicine and Therapies 1/2023

Open Access 01.12.2023 | Research

Stevia (Stevia rebaudiana) extract ameliorates insulin resistance by regulating mitochondrial function and oxidative stress in the skeletal muscle of db/db mice

verfasst von: Jin-Young Han, Miey Park, Hae-Jeung Lee

Erschienen in: BMC Complementary Medicine and Therapies | Ausgabe 1/2023

insite
INHALT
download
DOWNLOAD
print
DRUCKEN
insite
SUCHEN

Abstract

Background

Type 2 diabetes mellitus (T2DM), a growing health problem worldwide, is a metabolic disorder characterized by hyperglycemia due to insulin resistance and defective insulin secretion by pancreatic β-cells. The skeletal muscle is a central organ that consumes most of the insulin-stimulated glucose in the body, and insulin resistance can damage muscles in T2DM. Based on a strong correlation between diabetes and muscles, we investigated the effects of stevia extract (SE) and stevioside (SV) on the skeletal muscle of diabetic db/db mice.

Methods

The mice were administered saline, metformin  (200 mg/kg/day), SE (200 and 500 mg/kg/day), and SV (40 mg/kg/day) for 35 days. During administration, we checked the levels of fasting blood glucose twice a week and conducted the oral glucose tolerance test (OGTT) and insulin tolerance test (ITT). After administration, we analyzed serum biochemical parameters, triglyceride (TG), total cholesterol (TC), insulin and antioxidant enzymes, and the cross-sectional area of skeletal muscle fibers of db/db mice. Western blots were conducted using the skeletal muscle of mice to examine the effect of SE and SV on protein expression of insulin signaling, mitochondrial function, and oxidative stress.

Results

SE and SV administration lowered the levels of fasting blood glucose, OGTT, and ITT in db/db mice. The administration also decreased serum levels of TG, TC, and insulin while increasing those of superoxide dismutase (SOD) and glutathione peroxidase (GPx). Interestingly, muscle fiber size was significantly increased in db/db mice treated with SE500 and SV. In the skeletal muscle of db/db mice, SE and SV administration activated insulin signaling by increasing the protein expression of insulin receptor substrate, Akt, and glucose transporter type 4. Furthermore, SE500 administration markedly increased the protein expression of AMP-activated protein kinase-α, sirtuin-1, and peroxisome proliferator-activated receptor-γ coactivator-1α. SV administration significantly reduced oxidative stress by down-regulating the protein expression of 4-hydroxynonenal, heme oxygenase-1, SOD, and GPx. In addition, SE500 and SV administration suppressed the expression of apoptosis-related proteins in the skeletal muscle of db/db mice.

Conclusion

SE and SV administration attenuated hyperglycemia in diabetic mice. Moreover, the administration ameliorated insulin resistance by regulating mitochondrial function and oxidative stress, increasing muscle fiber size. Overall, this study suggests that SE and SV administration may serve as a potential strategy for the treatment of diabetic muscles.
Begleitmaterial
Hinweise

Supplementary Information

The online version contains supplementary material available at https://​doi.​org/​10.​1186/​s12906-023-04033-5.

Publisher’s Note

Springer Nature remains neutral with regard to jurisdictional claims in published maps and institutional affiliations.
Abkürzungen
T2DM
Type 2 diabetes mellitus
IRS
Insulin receptor substrate
GLUT4
Glucose transporter type 4
AMPK α
AMP-activated protein kinase-α
PGC-1α
Proliferator-activated receptor-γ coactivator-1α
SIRT1
Sirtuin-1
SE
Stevia extract
SV
Stevioside
FBGLs
Fasting blood glucose levels
OGTT
Oral glucose tolerance test
ITT
Insulin tolerance test
TG
Triglyceride
TC
Total cholesterol
HOMA-IR
Homeostatic model assessment for insulin resistance
SOD
Superoxide dismutase
GPx
Glutathione peroxidase
CS
Citrate synthase
4-HNE
4-Hydroxynonenal
HO-1
Heme oxygenase-1

Introduction

Type 2 diabetes mellitus (T2DM) is one of the most common metabolic diseases worldwide [1, 2]. The pathophysiology of T2DM includes disorders of carbohydrate, lipid, and protein metabolism resulting from defects in insulin secretion and action [2, 3]. Insulin resistance leads to the disruption of glucose homeostasis, which increased glucose production in the liver and reduced glucose uptake in skeletal muscle and adipose tissue [2, 4]. Fasting and postprandial hyperglycemia cause secondary complications in various organs, such as the heart, brain, kidneys, and eyes [35]. Target drugs for diabetes have been developed, but their side effects and disadvantages are still controversial [6]. Therefore, it is essential to research using natural functional materials with low side effects for diabetes.
Skeletal muscle, a significant determinant of resting metabolic rate, accounts for 40%–50% of the total body weight [7] and consumes approximately 80% glucose stimulated by insulin [810]. An essential function of the muscle is to increase glucose transport activity via the insulin signaling cascade [11]. The binding of insulin to the insulin receptor induces insulin receptor substrate (IRS)-1 tyrosine phosphorylation. This results in the activation of Akt phosphorylation, which facilitates the translocation of glucose transporter type 4 (GLUT4) and subsequent glucose uptake into muscle cells [12, 13].
Insulin resistance decreases protein synthesis and increases protein degradation, leading to muscle atrophy and sarcopenia [14, 15]. In skeletal muscle, impaired mitochondrial function causes lipid oxidation, resulting in insulin resistance [16]. AMP-activated protein kinase-α (AMPKα), a central regulator of mitochondrial biogenesis, controls intracellular energy balance and is an essential factor in skeletal muscle atrophy [17, 18]. Deacetylation of peroxisome proliferator-activated receptor-γ coactivator-1α (PGC-1α) plays an essential role in mitochondrial biogenesis, which is regulated by sirtuin-1 (SIRT1) [19]. In addition, hyperglycemia-induced oxidative stress contributes to the reduction in insulin action [20]. The abnormal cell signaling resulting from a decreased ability to eliminate oxidative stress can lead to insulin resistance [21]. Furthermore, a persistent state of oxidative stress induces apoptosis [22], which in itself can also cause muscle atrophy [23, 24].
Stevia (Stevia rebaudiana) is a natural sweetener used as a substitute for sucrose worldwide [25]. Stevia leaves have been used as tea and medicines in many parts of the world for centuries [2528]. Several steviol glycosides, which are four-ring diterpenes, such as stevioside (SV), rebaudioside A, D, C, D, and E, dulcoside A and B, have been identified from stevia leaves [29]. This non-caloric sweetener passes through the body without being metabolized, which is why it is favored bydiet-conscious consumers and can be effectively used to treat diabetes, obesity, and cardiovascular disease [25]. SV, an abundant glycoside found in stevia leaves, is 300 times sweeter than sugar [25, 30]. Several studies have reported the therapeutic benefits of stevia and SV, lowering blood sugar, cholesterol, and triglyceride levels and exhibiting [3134], antioxidant, anti-inflammatory, and anti-cancerous properties [3537]. In addition, in vivo studies have investigated the antidiabetic effect of SV, suggesting alleviation of hyperglycemia [33, 38]. However, few studies have focused on whether stevia and SV improve insulin resistance in skeletal muscle, essential for insulin-stimulated glucose absorption. Therefore, in this study, we investigated the effect of stevia extract (SE) and its glycoside, SV, on insulin resistance and improvement mechanism in skeletal muscle in diabetic db/db mice.
In this study, we used db/db mice with severe obesity caused by leptin receptor defects to model T2DM [39]. Metformin, a T2DM medication, was used as a positive control (PC) verifying a significant reduction in blood glucose in mice [40]. This study shows that the effect of SE and SV administration on insulin resistance in skeletal muscle of diabetic mice will occur through the regulation of mitochondrial function and oxidative stress, and suggests that SE and SV administration may improve diabetic muscles compared to metformin administration.

Materials and methods

Materials

Stevia rebaudiana was registered in plant variety protection right as grant No. 6485 by Korea Seed & Variety Service in 2017, according to Plant Variety Protection Act (application No. 2015–257). Experimental research on plants was performed following the relevant guidelines and legislation [41]. Lyophilized powder of stevia leaves was obtained from Pharminogen Co. (Yongin, Kyunggi-do, Korea). Briefly, stevia leaves were dried and extracted with water at 100 °C for 3 h using a heating mantle. Next, the extract was filtered through 500 mesh filter and concentrated using vacuum evaporation. The concentrate was lyophilized to remove moisture entirely and stored at -20 °C in a powder. Stevioside (C38H60O18) was purchased from ChemFaces Biochemical Co. Ltd. (Wuhan, China).

Animal studies

Eight-week-old BKS.Cg-Dock7m + / + Leprdb/J (Heterozygous for Dock7m/ Heterozygous for Leprdb) (db/m + , negative controls) and db/db mice (BKS.Cg-Dock7m + / + Leprdb/J, homozygote) were obtained from Jackson Laboratories (Sacramento, CA, USA). Mice were allowed to adjust to a controlled environment with a 12 h light/dark cycle at 20–25 °C for two weeks. Following the acclimatization period, six non-diabetic mice (db/m +) were assigned to the control group, and 30 diabetic mice (db/db) were randomly divided into six groups as follows: (1) Negative control (N +) group, non-diabetic mice + saline; (2) Normal control (NC) group, diabetic mice + saline; (3) PC group, diabetic mice + metformin (200 mg/kg BW, p.o.); (4) SE200 group, diabetic mice + SE (SE, 200 mg/kg BW, p.o.); (5) SE500 group, diabetic mice + SE (500 mg/kg BW, p.o.); (6) SV group, diabetic mice + stevioside (SV, 40 mg/kg BW, p.o.). Saline, metformin, SE, and SV were administered by oral gavage daily for 35 days (Figure S1). Mice were weighed twice a week. All animal experiments were performed following the Guide for the Care and Use of Laboratory Animals and were approved by Gachon University (GI-ACUC-R2020012).

Fasting blood glucose levels (FBGLs), oral glucose tolerance test (OGTT), and insulin tolerance test (ITT)

Mice fasted for 3 h and the FBGLs were measured using Accu-Chek Performa (Roche Diagnostics Korea Co., Ltd., Seoul, Korea). Blood was collected from the tail vein of each mouse. On day 21 of administration, overnight-fasted mice were orally administered glucose (Dai Han Pharm. Co. Ltd., Seoul, Korea) at a concentration of 2 g/kg BW. Blood glucose levels were measured at 0, 15, 30, 60, and 120 min after oral glucose gavage. In addition, ITT was performed on day 35 in mice following fasting for 3 h. Mice were administered an intraperitoneal injection of Humulin (1 U/kg BW; Eli Lilly, Indianapolis, IN, USA) and the blood glucose level was checked at 0, 15, 30, and 60 min. Blood glucose and insulin tolerance levels were determined using the area under the curve (AUC).

Biochemical analysis

Serum triglyceride (TG) and total cholesterol (TC) levels were determined using commercial kits (Asan Pharm, Seoul, Korea), and serum insulin level was measured using an enzyme-linked immunosorbent assay (ELISA) kit (Thermo Fisher, Waltham, MA, USA). The homeostatic model assessment for insulin resistance (HOMA-IR) was calculated using the following formula: \(\mathrm{HOMA}-\mathrm{IR}=\{\mathrm{fasting insulin}\left[\frac{\mathrm{U}}{\mathrm{mL}}\right]\times \mathrm{fasting glucose}\left[\frac{\mathrm{mg}}{\mathrm{dL}}\right]\}/405\) [42]. The concentration of superoxide dismutase (SOD) and glutathione peroxidase (GPx) in mouse serum was measured using Bluegene ELISA kits (Shanghai Bluegene Biotech Co. Ltd., Shanghai, China). The biochemical experiments were conducted according to the manufacturer’s recommendations.
To determine malondialdehyde (MDA) levels, liver homogenates dissolved in 1.15% KCl (Sigma-Aldrich, St Louis, MO) were obtained from one portion of 0.05 g liver of each mouse. Then, the samples were blended with a mixed solution containing 8.1% sodium dodecyl sulfate (SDS) (iNtRON Biotechnology, Seongnam, Korea) 200 μL, 20% acetic acid (Daejung Chemical, Suwon, Korea), 1.5 mL 0.8% thiobarbituric acid (TBA) (Sigma-Aldrich, St Louis, MO) 1.5 mL, distilled water 700 μL. A 5 ml volume of n-butanol (SAMCHUN, Gyeonggi-do, Korea) and 1 ml volume of distilled water were added to mixtures, followed by incubating in a 95 °C water bath for 30 min and ice for 10 min. After centrifuging at 4,000 rpm for 10 min, MDA levels of each supernatant were measured at 532 nm.

Hematoxylin and eosin (H&E) staining and analysis of the cross-sectional area of skeletal muscle fibers

Skeletal muscle tissue samples of 3 mice in each group were fixed in 10% formalin (Sigma-Aldrich, St. Louis, MO, USA). The samples were embedded in paraffin and stained with H&E. Stained sections were visualized using an Olympus Provis AX70 microscope (Olympus, Tokyo, Japan). To analyze muscle fiber size, the cross-sectional area of the skeletal muscle in mice was calculated using ImageJ software (rsb.info.nih.gov/ij).

Western blot analysis

Gastrocnemius tissue (20 mg) was homogenized in PRO-PREP™ solution (iNtRON Biotechnology, Seongnam, Korea) containing a phosphatase inhibitor (Thermo Fisher) and incubated for 30 min on ice. Following lysis, the tissue suspension was centrifuged at 13,000 × g for 5 min at 4 °C to obtain the supernatant. Nuclear and cytoplasmic fractions were isolated using NE-PER Nuclear and Cytoplasmic Extraction Reagents (Thermo Fisher) according to the manufacturer’s instructions. Protein concentrations were measured at 595 nm using the PRO-MEASURE™ solution (iNtRON Biotechnology). Concentrations were calculated according to the manufacturer’s instructions.
Equal amounts of total protein (30 μg) were electrophoresed by sodium dodecyl sulfate polyacrylamide gel electrophoresis (SDS-PAGE) and subsequently transferred onto a polyvinylidene difluoride (PVDF) membrane. The membranes were blocked with 5% skim milk for 1 h and incubated with the following primary antibodies: p-Akt, Akt, p-IRS, IRS, p-AMPKα, AMPKα, citrate synthase (CS) (Cell Signaling Technology, Beverly, MA, USA, 1:1000), SIRT1, 4-hydroxynonenal (4-HNE), Bax, Bcl-2 (Abcam, Cambridge, MA, USA, 1:1000), Lamin B1 (Abcam, 1:10,000), α-tubulin (Abcam, 1:5000), heme oxygenase 1 (HO-1), SOD, GPx (Santa Cruz Biotechnology, Santa Cruz, CA, USA, 1:200), PGC-1α (Bioss Antibodies, Woburn, MA, USA, 1:1000), and GLUT4 (Thermo Fisher, 1:1000). After incubation with secondary antibodies for 1 h, specific bands were visualized using an enhanced chemiluminescence method (iNtRON Biotechnology) and a Quant LAS 500 system (GE Healthcare Bio-Sciences AB, Björkgatan, Uppsala, Sweden).

Statistical analysis

GraphPad Prism 5.03 (GraphPad Software Inc., La Jolla, CA, USA) was used for statistical analysis using one-way analysis of variance (ANOVA), followed by Tukey’s post-hoc test. Data were presented as the mean ± standard deviation (SD). Statistical significance was set at p < 0.05.

Results

Effect of SE on the body, subcutaneous fat, and gastrocnemius weights of db/db mice

All mice were weighed twice a week during the administration of the compounds. On the last day of the experiment, differences were noted between the diabetic groups, except for the N + mice. However, no significant difference was observed (Fig. 1a). N + mice had markedly lower subcutaneous fat than diabetic NC mice. Subcutaneous fat weight was lower in SE-treated mice than in NC mice. However, the SV group did not show a significant difference (Fig. 1b). The gastrocnemius weight was the highest in N + mice, and there was no difference between the diabetic groups (Fig. 1c). In summary, subcutaneous fat weight decreased, but gastrocnemius weight remained unchanged in SE-treated mice. Thus, in subsequent experiments, we focused on the effect of SE on skeletal muscle in diabetic mice.

Effect of SE on FBGLs, OGTT, and ITT in db/db mice

We measured the FBGLs on days 0, 3, 7, 10, 14, 17, 24, and 31. At the beginning of the experiment, there were no significant differences in the blood glucose levels of mice in the experimental groups, except the N + mice. However, on day 31, FBGLs in the experimental mice declined significantly (Fig. 2a). To investigate glucose tolerance, we performed OGTT and ITT on days 21 and 35, respectively. Compared to db/db mice, mice in the experimental groups showed improved glucose tolerance, which was also noted in the AUC of the OGTT (Fig. 2b and c). A similar pattern was observed in the ITT, where the experimental mice showed improved glucose disposal compared to the NC mice (Fig. 2d and e). The higher dose of SE appeared to be most effective for glucose disposal and insulin action.

Effect of SE on biochemical markers associated with diabetes in db/db mice

To examine the biochemical markers related to diabetes, we measured the serum TG and TC levels using the blood from the tail vein of mice. NC mice showed higher serum TG and TC levels than N + mice. TG levels were reduced in the experimental mice (Fig. 3a). Consistent with the TG results, serum TC levels were also reduced in the experimental mice, and the SE500 mice showed the lowest TC levels (Fig. 3b). Next, serum insulin and HOMA-IR levels to determine whether SE administration affects serum insulin levels. NC mice displayed elevated serum insulin concentrations compared to N + mice. The experimental mice exhibited significantly reduced serum insulin and HOMA-IR levels (Fig. 3c and d). Antioxidant enzyme content is closely related to diabetes, which is a condition attributable to excessive oxidative stress. To assess the effect of stevia on antioxidant enzyme levels, we measured the levels of SOD and GPx, which are representative antioxidant enzymes, in mice serum. NC mice exhibited lower serum SOD and GPx levels than N + mice (Fig. 3e and f). In contrast, the experimental mice showed significantly higher antioxidant enzyme levels than the NC mice, except for GPx in the SV mice. In addition, to investigate oxidative stress caused by lipid peroxides, we measured hepatic MDA levels in diabetic mice. PC mice showed significant reductions in hepatic MDA levels. In mice groups with stevia treatments, SE500 and SV mice had significantly lower MDA levels compared to NC mice (Figure S2).

Effect of SE on the size of skeletal muscle fibers in db/db mice

As mentioned before, SE administration decreased subcutaneous fat weight but did not affect gastrocnemius weight in mice. Therefore, we examined the morphological changes in skeletal muscle by H&E staining of cross-sections of skeletal muscle tissues. Muscle fiber size was significantly decreased, and degenerated fibers were observed in NC mice compared to those in N + mice (Fig. 4a and b). The cross-sectional areas of SE500 and SV mice exhibited a significant increase compared to that of NC mice.

Effect of SE on insulin signaling in skeletal muscle of db/db mice

To determine whether SE administration affects insulin metabolism in diabetic skeletal muscles, we analyzed the levels of proteins related to the insulin signaling pathway using western blotting. Serine phosphorylation of IRS, which indicates insulin resistance, was the highest in NC mice. The experimental groups showed decreased p-IRS/IRS ratios (Fig. 5a). The p-Akt/Akt ratio was lower in the NC mice than in the N + mice. In contrast, the p-Akt/Akt ratio was higher in the experimental mice than in the NC mice (Fig. 5b). Similarly, GLUT4 expression was the lowest in NC mice. There was no significant difference in GLUT4 levels between SE200 mice, but it was higher compared to that in NC mice (Fig. 5c). GLUT4 expression was significantly higher in PC, SE500, and SV-treated mice. These data suggest that the administration increases glucose transport into insulin target tissues.

Effect of SE on mitochondrial activity in skeletal muscle of db/db mice

We investigated the effect of SE administration on energy metabolism in diabetic skeletal muscle by measuring the level of energy metabolism-associated proteins in the cytoplasm and nucleus. As shown in Fig. 6a, NC mice exhibited a significantly reduced cytoplasmic p-AMPKα/AMPKα ratio compared to N + mice. AMPKα phosphorylation was markedly increased in the experimental groups compared to NC mice. The expression of cytoplasmic and nuclear SIRT1, which is enhanced by AMPKα activation, was the lowest in NC mice, whereas it was elevated in SE and SV mice (Fig. 6b and c). PGC-1α, a key mediator of mitochondrial biogenesis, also showed a similar expression to AMPKα and SIRT1 in the cytoplasm, considerably increasing SE500 mice (Fig. 6d). The expression of nuclear PGC-1α was significantly increased only in PC and SE500 mice (Fig. 6e). To determine whether SE administration affects mitochondrial content, we measured the expression of cytoplasmic CS. PC, SE, and SV-treated mice displayed increased CS expression compared to NC mice (Fig. 6f). These results suggest that mitochondrial activity is enhanced in skeletal muscle of diabetic mice treated with a high dose of SE.

Effect of SE on oxidative stress and apoptosis-related proteins in skeletal muscle of db/db mice

We analyzed the expression of proteins related to oxidative stress in diabetic skeletal muscles. The NC mice showed the highest level of 4-HNE, a typical lipid peroxidation aldehyde that can cause mitochondrial damage and apoptosis [43]. SE-treated mice did not show a significant decrease in 4-HNE expression compared to NC mice, whereas the PC and SV mice exhibited significantly reduced 4-HNE levels (Fig. 7a). Next, we analyzed the expression of cytoplasmic proteins that protect against oxidative stress. HO-1, which alleviates oxidative damage, was significantly higher in NC mice than in N + mice and was decreased in PC, SE500, and SV mice (Fig. 7b). In addition, NC mice exhibited high expression of SOD and GPx, which are critical antioxidant proteins that scavenge ROS [44]. The expression of SOD showed significant differences only in PC, SE500, and SV mice compared to that in NC mice (Fig. 7c), and GPx was decreased in all experimental mice (Fig. 7d). Overall, among the treatments, SV treatment appeared to protect against oxidative stress.
Given the chronic oxidative stress conditions, we examined the ratio of the apoptosis-related factors Bax and Bcl-2 in the diabetic skeletal muscle. The NC mice displayed an elevated Bax/Bcl-2 ratio compared to N + and experimental mice, except for SE200, which exhibited a significantly decreased ratio compared to the NC mice (Fig. 7e).

Discussion

In the current study, we investigated the effects of SE and SV administration on insulin resistance and its underlying mechanism in the skeletal muscle of diabetic mice. First, treatment of SE and SV significantly reduced hyperglycemia. Additionally, the treatment raised the levels of antioxidant enzymes while decreasing serum TG, TC, and insulin levels. The administration of metformin showed the same results. Interestingly, only mice given SE500 and SV experienced an increase in muscle fiber size. In the skeletal muscle of diabetic mice, PC, SE500, and SV administration triggered insulin signaling. In particular, SE500 administration had a notable impact on elevated mitochondrial activity. Furthermore, the study demonstrated that PC and SV treatments were associated with lowering oxidative stress. Overall, this study found that supplying SE and SV to db/db mice’s skeletal muscles ameliorated their insulin resistance and was associated with regulating mitochondrial function and oxidative stress.
The incidence of T2DM, a severe metabolic disorder, is increasing worldwide. T2DM, characterized by high blood glucose and insulin dysfunction, can damage the cardiovascular system, spleen, retina, and skeletal muscles [2, 5, 45]. Given the side effects of anti-diabetic drugs, managing diabetes with herbal medicines based on plants and natural phytochemicals such as alkaloids, polysaccharides, and flavonoids is gaining more attention [46]. In the present study, we investigated the effect of stevia, a natural sweetener, on diabetes in db/db mice.
Stevia has been used as a sweetener for decades and has been reported to have various health benefits. Some studies have investigated the health risks of stevia, including the allergenic potential of purified stevia in rats [47] and its effect in reducing fertility in female rats [48]. Nevertheless, stevia and SV which have non-caloric properties are consistently proposed as a sugar substitute in obesity and diabetes [30, 31, 33, 49, 50]. In the present study, PC, SE, and SV administration significantly suppressed the increased blood glucose, serum TG, and serum TC levels in db/db mice. In addition, we performed an OGTT to monitor peripheral disposal after oral glucose loading and insulin secretion over time [51]. The AUC of the OGTT in the treated mice was significantly lower than that in the NC group, indicating greater glucose intolerance. The results of ITT, reflecting whole-body insulin action, showed a decrease in treated mice, similar to the results of the OGTT. NC mice show hyperinsulinemia, one of the symptoms of diabetes. SE administration has been reported to reduce serum insulin levels and HOMA-IR, an indicator of hepatic insulin action [52].
Our results manifested that SE500 and SV administration increased muscle fiber size while ameliorating muscle damage. It is unclear why PC mice treated with metformin did not exhibit a substantial increase; nonetheless, a recent study found that metformin causes induces atrophy by regulating myostatin [53]. To determine whether the effects of SE and SV on muscle are related to insulin action, we investigated insulin signaling in the skeletal muscle of db/db mice. Insulin binds to IR, resulting in glucose uptake and tyrosine kinase activation, leading to IRS phosphorylation. Subsequent activation of the PI3K/Akt pathway results in the translocation of GLUT4 to the membrane, thereby mediating glucose transport [54]. One study substantiated that SV activated IR/IRS-1/Akt/GLUT 4 signaling, promoting glucose uptake in the gastrocnemius muscle of diabetic rats [55]. In this study, consistent with the metformin group, SE and SV administration was found to upregulate the expression of proteins related to insulin activity. Insulin resistance reduces muscle quality and strength, resulting in muscle atrophy [56]. It is necessary to confirm the significant overlap in molecular pathways in which sarcopenia and muscle IR are abnormally regulated [57]. Previous studies have reported that treatment with rosiglitazone and anti-myostatin antibodies increased insulin sensitivity and suppressed muscle protein degradation, and increased skeletal muscle mass and strength in mice [58, 59]. Likewise, our data showed that SE and SV administration improved insulin resistance, increasing muscle fiber size and alleviating muscle damage. Meanwhile, insulin resistance is closely associated with mitochondrial dysfunction [60]. One study reported that the enzymatic activity of mitochondrial complexes involved in oxidative phosphorylation was reduced by approximately 40% in human skeletal muscle in T2DM [61]. In mitochondrial biogenesis, PGC-1α is essential in increasing cellular ATP [62], and SIRT1-mediated PGC-1α functions to promote metabolic adaptations in tissue [63]. In the current study, PC, SE, and SV administration upregulated the protein expression of p-AMPKα/AMPKα ratio and SIRT1 and consequently activated the PGC-1α in the skeletal muscle of db/db mice. In particular, a high dose of SE effectively activated mitochondrial function. To further support the effect on mitochondria, we measured the protein expression levels of CS. PC, SE, and SV administration increased CS levels, which increased mitochondrial function and content [64]. Consequently, the administration improved insulin resistance by activating the AMPK/SIRT1/PGC-1α pathway in the skeletal muscle of db/db mice.
The activity of antioxidant proteins increases under high oxidative stress [65], such as T2DM, Alzheimer’s disease, and cardiovascular disease. SOD and GPx are key cellular antioxidant enzymes that scavenge toxic free radicals and neutralize ROS [44]. Therefore, we assessed the expression of proteins related to oxidative stress, which can affect impaired insulin action [20]. NC mice exhibited increased HO-1, SOD, and GPx protein levels, indicating that severe diabetic conditions induce oxidative stress. In contrast, PC, SE500, and SV administration suppressed the expression of these proteins. In particular, SV administration showed a strong antioxidant effect, similar to the results of other studies [20, 66, 67]. Furthermore, we investigated aberrant apoptosis, which may be caused by excessive free radicals [68]. The Bax/Bcl-2 ratio, a key role in the apoptotic pathway, was increased in diabetic mice and decreased in PC, SE500, and SV mice. These findings indicated that SE500 and SV administration decreased oxidative stress and apoptosis, which enhanced insulin sensitivity.
Several studies have been reported [6971] on the antihyperglycemic effects of stevia, or SV, in general adults. We used the skeletal muscle of diabetic mice to examine their antihyperglycemic mechanisms. According to a recent study, SV attenuated insulin resistance in rats fed a high-fat diet by activating the insulin signaling pathway in their muscles [55]. We did, however, confirm the effects of SE and SV together and found that they activated insulin signaling while also controlling mitochondrial function and oxidative stress. However, given that this study only involved a small number of animals, translating its findings into clinical practice is challenging. Future research on deeper mechanisms, including inflammation and fatty acid-induced insulin resistance, using sufficiently large numbers of animals is needed in order to completely comprehend the effects of SE and SV in diabetic muscle. Furthermore, future research may also need to be tailored for the muscles of patients with type 2 diabetes.
In this study, SE and SV administration improves insulin resistance by activating mitochondrial function through the activation AMPK/SIRT1/PGC-1α pathway and reducing oxidative stress, which increases muscle fiber size and alleviates degenerated fibers in db/db mice. Therefore, our data suggest that SE and SV may be potential nutraceuticals for the management of diabetic muscle.

Acknowledgements

Not applicable.

Declarations

The authors declare that they have no conflicts of interest and have given their consent for this manuscript's scientific content and authorship. Experimental research and field studies on plants (either cultivated or wild) were performed in accordance with the relevant guidelines and legislation. This study was conducted in accordance with the guidelines stipulated by the Ministry of Food and Drug Safety for the Care and Use of Laboratory Animals. All experimental protocols were approved by the Institutional Animal Care and Use Committee of Gachon University for the Care and Use of Laboratory Animals (GIACUC-R2020012). This study is reported in accordance with ARRIVE guidelines for animal experiments.
Not applicable.

Competing interests

The authors declare no competing interests.
Open Access This article is licensed under a Creative Commons Attribution 4.0 International License, which permits use, sharing, adaptation, distribution and reproduction in any medium or format, as long as you give appropriate credit to the original author(s) and the source, provide a link to the Creative Commons licence, and indicate if changes were made. The images or other third party material in this article are included in the article's Creative Commons licence, unless indicated otherwise in a credit line to the material. If material is not included in the article's Creative Commons licence and your intended use is not permitted by statutory regulation or exceeds the permitted use, you will need to obtain permission directly from the copyright holder. To view a copy of this licence, visit http://​creativecommons.​org/​licenses/​by/​4.​0/​. The Creative Commons Public Domain Dedication waiver (http://​creativecommons.​org/​publicdomain/​zero/​1.​0/​) applies to the data made available in this article, unless otherwise stated in a credit line to the data.

Publisher’s Note

Springer Nature remains neutral with regard to jurisdictional claims in published maps and institutional affiliations.
insite
INHALT
download
DOWNLOAD
print
DRUCKEN
Anhänge
Literatur
1.
Rowley WR, Bezold C. Creating public awareness: state 2025 diabetes forecasts. Popul Health Manag. 2012;15(4):194–200.CrossRefPubMed
2.
Zheng Y, Ley SH, Hu FB. Global aetiology and epidemiology of type 2 diabetes mellitus and its complications. Nat Rev Endocrinol. 2018;14(2):88–98.CrossRefPubMed
3.
DeFronzo RA, Ferrannini E, Groop L, Henry RR, Herman WH, Holst JJ, Hu FB, Kahn CR, Raz I, Shulman GI. Type 2 diabetes mellitus. Nat Rev Dis Primers. 2015;1(1):1–22.CrossRef
4.
5.
Papatheodorou K, Papanas N, Banach M, Papazoglou D, Edmonds M: Complications of diabetes 2016vol. 2016: Hindawi; 2016.
6.
Kanwal A, Kanwar N, Bharati S, Srivastava P, Singh SP, Amar S. Exploring new drug targets for type 2 diabetes: success, challenges and opportunities. Biomedicines. 2022;10(2):331.PubMedCentralCrossRefPubMed
7.
Zurlo F, Larson K, Bogardus C, Ravussin E. Skeletal muscle metabolism is a major determinant of resting energy expenditure. J Clin Investig. 1990;86(5):1423–7.PubMedCentralCrossRefPubMed
8.
Merz KE, Thurmond DC. Role of skeletal muscle in insulin resistance and glucose uptake. Compr Physiol. 2011;10(3):785–809.
9.
10.
DeFronzo RA, Jacot E, Jequier E, Maeder E, Wahren J, Felber J. The effect of insulin on the disposal of intravenous glucose: results from indirect calorimetry and hepatic and femoral venous catheterization. Diabetes. 1981;30(12):1000–7.CrossRefPubMed
11.
12.
Basu A, Basu R, Shah P, Vella A, Johnson CM, Nair KS, Jensen MD, Schwenk WF, Rizza RA. Effects of type 2 diabetes on the ability of insulin and glucose to regulate splanchnic and muscle glucose metabolism: evidence for a defect in hepatic glucokinase activity. Diabetes. 2000;49(2):272–83.CrossRefPubMed
13.
Del Aguila LF, Krishnan RK, Ulbrecht JS, Farrell PA, Correll PH, Lang CH, Zierath JR, Kirwan JP. Muscle damage impairs insulin stimulation of IRS-1, PI 3-kinase, and Akt-kinase in human skeletal muscle. Am J Physiol Endocrinol Metab. 2000;279(1):E206–12.CrossRefPubMed
14.
Rudrappa SS, Wilkinson DJ, Greenhaff PL, Smith K, Idris I, Atherton PJ. Human skeletal muscle disuse atrophy: effects on muscle protein synthesis, breakdown, and insulin resistance—a qualitative review. Front Physiol. 2016;7:361.PubMedCentralCrossRefPubMed
15.
Leenders M, Verdijk LB, van der Hoeven L, Adam JJ, Van Kranenburg J, Nilwik R, Van Loon LJ. Patients with type 2 diabetes show a greater decline in muscle mass, muscle strength, and functional capacity with aging. J Am Med Dir Assoc. 2013;14(8):585–92.CrossRefPubMed
16.
Kelley DE, He J, Menshikova EV, Ritov VB. Dysfunction of mitochondria in human skeletal muscle in type 2 diabetes. Diabetes. 2002;51(10):2944–50.CrossRefPubMed
17.
Liang J, Zhang H, Zeng Z, Wu L, Zhang Y, Guo Y, Lv J, Wang C, Fan J, Chen N. Lifelong aerobic exercise alleviates sarcopenia by activating autophagy and inhibiting protein degradation via the AMPK/PGC-1α signaling pathway. Metabolites. 2021;11(5):323.PubMedCentralCrossRefPubMed
18.
19.
Silvestre MFP, Viollet B, Caton P, Leclerc J, Sakakibara I, Foretz M, Holness M, Sugden M. The AMPK-SIRT signaling network regulates glucose tolerance under calorie restriction conditions. Life Sci. 2014;100(1):55–60.CrossRefPubMed
20.
Monea A, Mezei T, Popsor S, Monea M. Oxidative stress: a link between diabetes mellitus and periodontal disease. Int J Endocrinol. 2014;2014:917631.PubMedCentralCrossRefPubMed
21.
Evans JL, Maddux BA, Goldfine ID. The molecular basis for oxidative stress-induced insulin resistance. Antioxid Redox Signal. 2005;7(7–8):1040–52.CrossRefPubMed
22.
23.
Wang M, Pu D, Zhao Y, Chen J, Zhu S, Lu A, Liao Z, Sun Y, Xiao Q. Sulforaphane protects against skeletal muscle dysfunction in spontaneous type 2 diabetic db/db mice. Life Sci. 2020;255:117823.CrossRefPubMed
24.
25.
Lemus-Mondaca R, Vega-Gálvez A, Zura-Bravo L, Ah-Hen K. Stevia rebaudiana Bertoni, source of a high-potency natural sweetener: a comprehensive review on the biochemical, nutritional and functional aspects. Food Chem. 2012;132(3):1121–32.CrossRefPubMed
26.
Giuffre L, Romaniuk R, Ciarlo E. Stevia, ka’a he’e, wild sweet herb from South America-An overview. Emirates J Food Agric. 2013;25(10):746–50.CrossRef
27.
Brandle J, Starratt A, Gijzen M. Stevia rebaudiana: Its agricultural, biological, and chemical properties. Can J Plant Sci. 1998;78(4):527–36.CrossRef
28.
Carakostas MC, Curry L, Boileau A, Brusick D. Overview: the history, technical function and safety of rebaudioside A, a naturally occurring steviol glycoside, for use in food and beverages. Food Chem Toxicol. 2008;46(7):S1–10.CrossRefPubMed
29.
Chatsudthipong V, Muanprasat C. Stevioside and related compounds: therapeutic benefits beyond sweetness. Pharmacol Ther. 2009;121(1):41–54.CrossRefPubMed
30.
Goyal S. Samsher n, Goyal R: Stevia (Stevia rebaudiana) a bio-sweetener: a review. Int J Food Sci Nutr. 2010;61(1):1–10.CrossRefPubMed
31.
Atteh J, Onagbesan O, Tona K, Decuypere E, Geuns J, Buyse J. Evaluation of supplementary stevia (Stevia rebaudiana, bertoni) leaves and stevioside in broiler diets: effects on feed intake, nutrient metabolism, blood parameters and growth performance. J Anim Physiol Anim Nutr. 2008;92(6):640–9.CrossRef
32.
Aghajanyan A, Movsisyan Z, Trchounian A. Antihyperglycemic and antihyperlipidemic activity of hydroponic stevia rebaudiana aqueous extract in hyperglycemia induced by immobilization stress in rabbits. BioMed Res Int. 2017;2017:9251358.PubMedCentralCrossRefPubMed
33.
Jeppesen PB, Gregersen S, Alstrup K, Hermansen K. Stevioside induces antihyperglycaemic, insulinotropic and glucagonostatic effects in vivo: studies in the diabetic Goto-Kakizaki (GK) rats. Phytomedicine. 2002;9(1):9–14.CrossRefPubMed
34.
Jeppesen P, Gregersen S, Rolfsen S, Jepsen M, Colombo M, Agger A, Xiao J, Kruhøffer M, Ørntoft T, Hermansen K. Antihyperglycemic and blood pressure-reducing effects of stevioside in the diabetic Goto-Kakizaki rat. Metabolism. 2003;52(3):372–8.CrossRefPubMed
35.
Shivanna N, Naika M, Khanum F, Kaul VK. Antioxidant, anti-diabetic and renal protective properties of Stevia rebaudiana. J Diabetes Complications. 2013;27(2):103–13.CrossRefPubMed
36.
Sehar I, Kaul A, Bani S, Pal HC, Saxena AK. Immune up regulatory response of a non-caloric natural sweetener, stevioside. Chem Biol Interact. 2008;173(2):115–21.CrossRefPubMed
37.
Takasaki M, Konoshima T, Kozuka M, Tokuda H, Takayasu J, Nishino H, Miyakoshi M, Mizutani K, Lee K-H. Cancer preventive agents. Part 8: chemopreventive effects of stevioside and related compounds. Bioorg Med Chem. 2009;17(2):600–5.CrossRefPubMed
38.
Suzuki H, Kasai T, Sumihara M, Sugisawa H. Influence of oral administration of stevioside on levels of blood glucose and liver glycogen of intact rats. J Agric Chem Soc Japan. 1977;64:171–3.
39.
Chen H, Charlat O, Tartaglia LA, Woolf EA, Weng X, Ellis SJ, Lakey ND, Culpepper J, More KJ, Breitbart RE. Evidence that the diabetes gene encodes the leptin receptor: identification of a mutation in the leptin receptor gene in db/db mice. Cell. 1996;84(3):491–5.CrossRefPubMed
40.
Mokgalaboni K, Dludla PV, Mkandla Z, Mutize T, Nyambuya TM, Mxinwa V, et al. Differential expression of glycoprotein IV on monocyte subsets following high-fat diet feeding and the impact of short-term low-dose aspirin treatment. Metab Open. 2020;7:100047.
41.
Kilkenny C, Browne WJ, Cuthill IC, Emerson M, Altman DG. Improving bioscience research reporting: the ARRIVE guidelines for reporting animal research. J Pharmacol Pharmacother. 2010;1(2):94–9.PubMedCentralCrossRefPubMed
42.
Wallace TM, Levy JC, Matthews DR. Use and abuse of HOMA modeling. Diabetes Care. 2004;27(6):1487–95.CrossRefPubMed
43.
44.
Maritim A, Sanders A, Watkins lii J. Diabetes, oxidative stress, and antioxidants: a review. J Biochem Molec Toxicol. 2003;17(1):24–38.CrossRef
45.
Randle PJ. Regulatory interactions between lipids and carbohydrates: the glucose fatty acid cycle after 35 years. Diabetes Metab Rev. 1998;14(4):263–83.CrossRefPubMed
46.
Bhushan MS, Rao C, Ojha S, Vijayakumar M, Verma A. An analytical review of plants for anti diabetic activity with their phytoconstituent & mechanism of action. Int J Pharm Sci Res. 2010;1(1):29–46.
47.
Urban JD, Carakostas MC, Taylor SL. Steviol glycoside safety: are highly purified steviol glycoside sweeteners food allergens? Food Chem Toxicol. 2015;75:71–8.CrossRefPubMed
48.
Planas GM, Kuć J. Contraceptive properties of Stevia rebaudiana. Science. 1968;162(3857):1007–1007.CrossRefPubMed
49.
Jeppesen PB, Gregersen S, Poulsen C, Hermansen K. Stevioside acts directly on pancreatic β cells to secrete insulin: Actions independent of cyclic adenosine monophosphate and adenosine triphosphate—sensitivie K+-channel activity. Metabolism. 2000;49(2):208–14.CrossRefPubMed
50.
Geuns JM. Safety evaluation of Stevia and stevioside. Stud Nat Prod Chem. 2002;27:299–319.CrossRef
51.
Nagy C, Einwallner E. Study of in vivo glucose metabolism in high-fat diet-fed mice using oral glucose tolerance test (OGTT) and insulin tolerance test (ITT). J Vis Exp. 2018;131:e56672.
52.
Wallace T, Matthews D. The assessment of insulin resistance in man. Diabet Med. 2002;19(7):527–34.CrossRefPubMed
53.
Kang MJ, Moon JW, Lee JO, Kim JH, Jung EJ, Kim SJ, Oh JY, Wu SW, Lee PR, Park SH. Metformin induces muscle atrophy by transcriptional regulation of myostatin via HDAC6 and FoxO3a. J Cachexia Sarcopenia Muscle. 2022;13(1):605–20.CrossRefPubMed
54.
Karlsson HK, Zierath JR. Insulin signaling and glucose transport in insulin resistant human skeletal muscle. Cell Biochem Biophys. 2007;48:103–13.CrossRefPubMed
55.
Deenadayalan A, Subramanian V, Paramasivan V, Veeraraghavan VP, Rengasamy G, Coiambatore Sadagopan J, Rajagopal P, Jayaraman S. Stevioside attenuates insulin resistance in skeletal muscle by facilitating IR/IRS-1/Akt/GLUT 4 signaling pathways: an in vivo and in silico approach. Molecules. 2021;26(24):7689.PubMedCentralCrossRefPubMed
56.
Volpato S, Bianchi L, Lauretani F, Lauretani F, Bandinelli S, Guralnik JM, Zuliani G, Ferrucci L. Role of muscle mass and muscle quality in the association between diabetes and gait speed. Diabetes Care. 2012;35(8):1672–9.PubMedCentralCrossRefPubMed
57.
Cleasby ME, Jamieson PM, Atherton PJ. Insulin resistance and sarcopenia: mechanistic links between common co-morbidities. J Endocrinol. 2016;229(2):R67–81.CrossRefPubMed
58.
Camporez J-PG, Petersen MC, Abudukadier A, Moreira GV, Jurczak MJ, Friedman G, Haqq CM, Petersen KF, Shulman GI. Anti-myostatin antibody increases muscle mass and strength and improves insulin sensitivity in old mice. Proc Natl Acad Sci. 2016;113(8):2212–7.PubMedCentralCrossRefPubMed
59.
Wang X, Hu Z, Hu J, Du J, Mitch WE. Insulin resistance accelerates muscle protein degradation: activation of the ubiquitin-proteasome pathway by defects in muscle cell signaling. Endocrinology. 2006;147(9):4160–8.CrossRefPubMed
60.
Montgomery MK, Turner N. Mitochondrial dysfunction and insulin resistance: an update. Endocr Connect. 2015;4(1):R1.CrossRefPubMed
61.
Ritov VB, Menshikova EV, He J, Ferrell RE, Goodpaster BH, Kelley DE. Deficiency of subsarcolemmal mitochondria in obesity and type 2 diabetes. Diabetes. 2005;54(1):8–14.CrossRefPubMed
62.
Lehman JJ, Barger PM, Kovacs A, Saffitz JE, Medeiros DM, Kelly DP. Peroxisome proliferator–activated receptor γ coactivator-1 promotes cardiac mitochondrial biogenesis. J Clin Investig. 2000;106(7):847–56.PubMedCentralCrossRefPubMed
63.
Gerhart-Hines Z, Rodgers JT, Bare O, Lerin C, Kim SH, Mostoslavsky R, Alt FW, Wu Z, Puigserver P. Metabolic control of muscle mitochondrial function and fatty acid oxidation through SIRT1/PGC-1α. EMBO J. 2007;26(7):1913–23.PubMedCentralCrossRefPubMed
64.
Ørtenblad N, Mogensen M, Petersen I, Højlund K, Levin K, Sahlin K, Becknielsen H, Gaster M. Reduced insulin-mediated citrate synthase activity in cultured skeletal muscle cells from patients with type 2 diabetes: evidence for an intrinsic oxidative enzyme defect. Biochim Biophys. 2005;1741(1–2):206–14.CrossRef
65.
66.
Geeraert B, Crombe F, Hulsmans M, Benhabiles N, Geuns J, Holvoet P. Stevioside inhibits atherosclerosis by improving insulin signaling and antioxidant defense in obese insulin-resistant mice. Int J Obes. 2010;34(3):569–77.CrossRef
67.
Kim I-S, Yang M, Lee O-H, Kang S-N. The antioxidant activity and the bioactive compound content of Stevia rebaudiana water extracts. LWT Food Sci Technol. 2011;44(5):1328–32.CrossRef
68.
Stoian I, Oros A, Moldoveanu E. Apoptosis and free radicals. Biochem Mol Med. 1996;59(2):93–7.CrossRefPubMed
69.
Anton SD, Martin CK, Han H, Coulon S, Cefalu WT, Geiselman P, Williamson DA. Effects of stevia, aspartame, and sucrose on food intake, satiety, and postprandial glucose and insulin levels. Appetite. 2010;55(1):37–43.PubMedCentralCrossRefPubMed
70.
Curi R, Alvarez M, Bazotte RB, Botion L, Godoy J, Bracht A. Effect of Stevia rebaudiana on glucose tolerance in normal adult humans. Braz J Med Biol Res. 1986;19(6):771–4.PubMed
71.
Gregersen S, Jeppesen PB, Holst JJ, Hermansen K. Antihyperglycemic effects of stevioside in type 2 diabetic subjects. Metabolism. 2004;53(1):73–6.CrossRefPubMed
Metadaten
Titel
Stevia (Stevia rebaudiana) extract ameliorates insulin resistance by regulating mitochondrial function and oxidative stress in the skeletal muscle of db/db mice
verfasst von
Jin-Young Han
Miey Park
Hae-Jeung Lee
Publikationsdatum
01.12.2023
Verlag
BioMed Central
Erschienen in
BMC Complementary Medicine and Therapies / Ausgabe 1/2023
Elektronische ISSN: 2662-7671
DOI
https://doi.org/10.1186/s12906-023-04033-5

Weitere Artikel der Ausgabe 1/2023

BMC Complementary Medicine and Therapies 1/2023 Zur Ausgabe

Research

Cantharidin suppresses hepatocellular carcinoma development by regulating EZH2/H3K27me3-dependent cell cycle progression and antitumour immune response

Research

Effects of online mindfulness-based interventions (MBIs) on anxiety symptoms in adults: a systematic review and meta-analysis

Retraction Note

Retraction Note: Antidiabetic, antioxidant, antihyperlipidemic effect of extract of Euryale ferox salisb. With enhanced histopathology of pancreas, liver and kidney in streptozotocin induced diabetic rats

Research

Anti-obesity effect of Neoagaro-oligosaccharides with overweight and obese subjects: a 16-week, randomized, double-blind, placebo-controlled clinical trial

Research

Network module analysis and molecular docking-based study on the mechanism of astragali radix against non-small cell lung cancer

Research

The use of traditional medicine practitioner services for childhood illnesses among childbearing women: a multilevel analysis of demographic and health surveys in 32 sub-Saharan African countries