Beneficial Effect Of Thymelaea Hirsuta On Pancreatic Islet Degeneration, Renal Fibrosis, And Liver Damages

Sanae Abid, Hassane Mekhfifi, Abderrahim Ziyyat, Abdekhaleq Legssyer, Mohammed Aziz, and Mohamed Bnouham

Laboratory of Bioresources, Biotechnology, Ethnopharmacology and Health, Department of Biology, Faculty of Sciences,

University Mohamed Ist, Bd: Mohamed VI, BP: 717, Oujda 60000, Morocco

Contact: joanna.jia@wecistanche.com / WhatsApp: 008618081934791

Objective. In Morocco, +ymelaea hirsute (T. hirsute) (Thymelaeacea) is a medicinal plant widely used to treat and prevent diabetes. The present study aimed to evaluate the medium-term antidiabetic effect of aqueous extract (AqTh) and ethyl acetate fraction (EaTh) of Th and to investigate their putative protective effect on pancreatic islet degeneration, diabetic nephropathy, and liver damage in streptozotocin (STZ)-diabetic rats. Methods. Experimental diabetes in rats was induced by a single intraperitoneal injection of 50 mg/kg of STZ. During the treatment period (4 weeks), 200 mg/kg AqTh and 50 mg/kg EaTh were orally administrated daily to STZ-diabetic rats. A group of parameters including fasting blood glucose, biochemical parameters, and intestinal α-glucosidase inhibition were studied. Furthermore, the histological study of the pancreas, kidney, liver, and aorta was also realized. Results. At the end of the treatment, both AqTh and EaTh had normalized fasting blood glucose to 1.08 and 1.25 g/l, respectively. AqTh has also reduced urinary creatinine and HbAc1. The EaTh showed inhibitory activity against intestinalα-glucosidase, whereas AqTh did not have this inhibitory effect. Furthermore, pancreas hematoxylin and eosin staining showed that AqTh or EaTh prevents pancreatic islet cell degeneration. As the same kidney, Masson’s trichrome staining has shown significant prevention of renal fibrosis in AqTh- or EaTh-treated diabetic rats. On the other hand, liver hematoxylin and eosin staining showed that AqTh and EaTh prevent liver damage. Conclusion. We conclude that medium-term administration of AqTh and EaTh exerts a significant antihyperglycemic effect in STZ-diabetic rats possibly through intestinal α-glucosidase inhibition and protection against pancreatic islet cell damage. Moreover, AqTh and EaTh treatment prevent nephropathy and liver complications in STZ-diabetic rats.

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Introduction

Diabetes mellitus is the most common endocrine disease. The incidence of this disease is increasing at an alarming rate (4-5%) [1]. Untreated or noncontrolled, noninsulin-dependent type 2 diabetes (DM2) can cause several complications such as cardiovascular diseases and diabetic nephropathy, and it may lead to insulin-dependent type 1 diabetes (DM1).

Diabetic nephropathy is one of the important complications of diabetes, and it is the main reason for the increased number of patients with end-stage renal disease(ESRD) [2], which require kidney dialysis or a kidney transplant for the patient to live.

Therefore, the management of diabetes is becoming very important to avoid its serious metabolic outcomes such as nephropathy.

Nowadays, the treatment of diabetes involves diet control, exercise, the use of insulin and/or hypoglycemic drugs, and also the use of medicinal plants as complementary alternative medicine. Several medicinal plants have shown a crucial antihyperglycemic effect with minimal side effects [3–5], For this reason, the World Health Organization (WHO) has called great attention to the rational use of traditional and natural medicines for treating diabetes [6].

In Morocco, more than 100 medicinal plants are used to treat and prevent diabetes [7–10]. The antihyperglycemic and antidiabetic activity of numerous extracts and products of these plants (Ammi visnaga Lam., Globularia alum, Nigella sativa, and Olea europaea var.) have been confifirmed[9].

T. hirsuta is a medicinal plant traditionally used for the prevention and management of diabetes, in northeastern Morocco [8]. Previous pharmacological studies have demonstrated the acute antihyperglycemic effect of the AqTh and EaTh [11–13]. However, the medium-term antidiabetic effect of these two T. hirsuta extracts has not yet been established. Therefore, the aim of the present study is to evaluate for the first time the medium-term antidiabetic activity of the AqTh and EaTh and to investigate their putative protective effect on pancreatic islet degeneration, diabetic nephropathy, liver steatosis, and aorta complications in STZ-induced diabetic rats.

2. Materials and Methods

2.1.Chemicals and Reagents.

Glucose Autokit was purchased from BioSystems (Spain). STZ was purchased from SigmaAldrich (China). Acarbose (Glucor 50) was obtained from Bayer Schering Pharma (Casablanca, Morocco). Sucrose was purchased from Prolabo (groupe Rhone-Poulenc) (EEC). Pentobarbital was obtained from CEVA Sante Animale (LaBallasti`ere). Anthrone (C14H10O) was purchased from across Organics. Paraffiffiffin wax was purchased from FlukaChemika (Switzerland). Eosin (C20H6Br4Na2O5) was obtained from Riedel-de Haen (Seelze), and hematoxylin was obtained from BDH Chemicals Ltd. (Poole England). Fuchsin acid was purchased from Acros Organics (NewJersey, USA), phosphomolybdic acid was purchased from Sigma-Aldrich (PF, Steinheim), and light green was purchased from Sigma-Aldrich (MO, USA).

2.2. Animals.

Wistar rats of both genders, initially weighing150–250 g (8-9 weeks), were obtained from the animal house of the Department of Biology of the Faculty of Sciences(Oujda, Morocco). The study has been carried out along the“Principles of Laboratory Animal Care” [14]. They were maintained under standard laboratory conditions (light/dark cycle of 12/12 h and temperature of 23 + 2°C with 3 rats per cage with access to food and water. To collect urine and determine water and food intake, rats were maintained in metabolic cages.

2.3. Induction of Diabetes.

After 14 h fasting, the rats were intraperitoneally injected with a single dose of STZ (50 mg/kg BW), prepared in a fresh and cold sodium citrate buffer(0.1 M citric acid and 0.1 M trisodium citrate dihydrate) at PH4.5, to induce diabetes [15]. After 1 week, rats with a fasting blood glucose range of 1.26–2 g/l were considered type 2 diabetic and they were included in the study.

2.4. Preparation of Plant Sample.

T. hirsuta was purchased from a traditional market in Oujda (Oriental Morocco) and was authenticated by a botanist in the Department of Biology (Faculty of Sciences, Oujda, Morocco), and a voucher specimen (HUMPOM137) was deposited at the plant section of the Herbarium University Mohamed Premier of Oujda, Morocco (HUMPO).

T. hirsuta's aerial parts were first cleaned and washed with water and then dried at 40°C overnight in the oven. To prepare AqTh, 140 g of T. hirsuta aerial parts was infused in2 L of distilled water for 3 hours. The AqTh yield was4.53%. The EaThwas prepared as described in our previous study [13].

2.5. Experimental Design.

The rats were randomly divided into five groups (5 or 6 rats per group): normal control rats(administered only with distilled water), diabetic control rats (administered only with distilled water), diabetic rats treated with 10 mg/kg BW of acarbose (standard hypoglycemic drug), diabetic rats treated with 50 mg/kg of EaTh, and diabetic rats treated with 200 mg/kg BW of AqTh. Optimal doses were determined based on our previous studies [13]and from preliminary tests. All rats were treated once daily for 4 weeks. The body weight was recorded every day. The water and food intake and urine volume were monitored before and after treatment, and glycosuria has measured at the end of the treatment. Fasting blood glucose was examined before the treatment (week 0) and after 1, 2, 3, and 4weeks of treatment. The inhibition of α-glucosidase, in vivo, was studied the day before rats were sacrificed. After the 4weeks of treatment, all the animals were anesthetized by50 mg/kg of pentobarbital, after 14 h of fasting. Then, the blood was collected, by cardiac puncture, and immediately centrifuged at 3000 tour/min for 10 min. *e serum was then stored at −20°C until biochemical analysis (total cholesterol and triglycerides). The kidney, liver, aorta, heart, and pancreas were removed, weighted (kidney liver, and heart), and then fixed (kidney, liver, aorta, and pancreas) in 10%formalin for the histological study. A liver sample was stored at −20°C for glycogen content assay.

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2.6. Estimation of Fasting Blood Glucose.

During the treatment period, the fasting glycemia was quantified weekly. After 14 h of fasting, blood was removed from the tail veins, under light ether anesthesia, using microcapillaries. Then, it was centrifuged at 5000 ×g for 10 min, and glycemia was estimated in the serum using a commercial glucose kit(BioSystems, Spain) based on the glucose oxidase peroxidase method [16].

2.7. α-Glucosidase Inhibition, in vivo Study.

The day before the sacrifice, the rats deprived of food for 14 h were used to monitor the α-glucosidase inhibition, in vivo. 30 min prior to oral sucrose load (2 g/kg), each group was administrated by the dose corresponding to its treatment. The blood was collected, from the tail, vein using microcapillaries, just before the test dose administration (−30 min), immediately before sucrose load (0 min), and at 30, 60, and 120 min after sucrose load. After centrifugation at 5000 ×g/10 min, the plasma glucose level was determined by the glucose oxidase peroxidase method [17].

2.8. Extraction and Determination of Hepatic Glycogen.

Weighed samples of liver tissues (0.3–0.5 g) from all groups were used to extract glycogen according to Ong and Khoo[18]. Liver samples were first crushed, homogenized with2 ml of 30% potassium hydroxide (KOH), and boiled at100°C/30 min. Then, for precipitating glycogen, the mixture was treated twice with 4 ml 95% ethanol, and each time, the mixture was stored at 4°C/30 min. After centrifugation at3000 tours/min/15 min, the pellet was washed with 8 ml 95%ethanol and then centrifuged at 3000 tours/min/15 min. The glycogen obtained was solubilized in 1 ml distilled water. The glycogen concentration was monitored using an anthrone reagent. The optic density was read at 625 nm.

2.9. Biochemical Assays.

Glycosuria was measured by a commercial Autokit (BioSystems, Spain) based on the glucose oxidase peroxidase method. Glycosylated hemoglobin(HbA1c) was estimated using a commercial kit (Cal-tech diagnostics, INC, USA), and cholesterol was determined using commercial assay kits (SGM- Italia, Roma, Italy). Triglycerides and urinary creatinine were estimated using commercial assay kits (Bio Sud Diagnostic S.R.L, Ricerca, Italy).

2.10. Histopathology.

After 3 ± 1 day’s period of fixation in 10%formalin, the pancreas, kidney, liver, and aorta tissues were washed with distilled water for 20 min. Then, they were dehydrated with increasing ethanol title (30% for 30 min,70% for 30 min, 95% for 30 min, and 2 ×100% for 60 min, respectively). After an enlightenment step in toluene(2 ×120 min), organs were included by the mixture parafintoluene (1V/1V) for 90 min, then by paraffin (2 ×120 min). Finally, the organs were embedded in paraffin before sectioning at 7 μm (microtome Leitz 1512). Pancreas and liver sections were stained with hematoxylin and eosin. Kidney and aorta sections were stained with Masson’s trichrome to show fifibrosis/collagen.

Before staining with hematoxylin and eosin, the sections were deparaffinized and incubated in toluene (2 × 5 min), then hydrated by decreasing ethanol title (100%, 95%, and70%, respectively) for 5 min. Then, for hematoxylin and eosin staining, after 20 min of washing, cell nuclei were stained with immersed in hematoxylin for 5 min, followed by 15 min of washing with water. To stain cytoplasm, the sections were immersed in 1% eosin for 5 min, then washed for 2 min. After coloration, sections were dehydrated with100% ethanol (2 ×1/2 min) and toluene (2 × 2 min). Masson's trichrome staining, after the hydration, kidney, and aorta sections were refi fixed in Bouin’s solution for 1hour/56°C. Then, after 10 min washing, sections were stained in Weigert’s iron hematoxylin for 2 min. After 10 min rinsing, sections were immersed in fuchsin acid for 3 min, and after 10 min washing, they were differentiated phosphomolybdic acid for 15 min. To stain collagen, sections were transferred directly to light green for 15 min. After2 min differentiation in 1% acetic acid, sections were dehydrated through 95% and 100% ethanol for 1 min each and then cleared in toluene (2 ×1 min) [19–21].

Finally, sections stained on lamellas were mounted paramount. After drying, the microscopic observation was made using the 40x objective ocular system of OlympusTokyo (Japan) light microscope.

To determine the drug’s effect on pancreas tissue, pancreatic islet cell number and diameter were calculated. To quantify collagen in kidney sections, results were scored from zero to three (0: no collagen, 1: weak collagen, 2:moderate collagen, and 3: strong collagen) [22]. The treatment effect on the aorta was evaluated by measuring the aorta diameter, and liver damage was elucidated by the development of lipid droplets.

2.11. Statistical Analysis.

All the values were expressed as mean ± SEM. The statistical analysis and comparison of means were performed using the unpaired Student test to compare two groups’ means and paired Student test to compare two means inside the same group. To determine the protective drug effect on the kidneys and liver, the chi-square test was used. p values <0.05 were considered significant.

3. Results

3.1. Effect of Drug Treatment on Fasting Blood Glucose in STZ-

Induced Diabetic Rats. In untreated diabetic control rats, significant fasting blood glucose elevation was observed compared to normal control rats. Treatment with 200 mg/kg AqTh decreased blood glucose level from the 1st-week of administration, and this effect was significant at the 3rd(p < 0.001) and 4th week (p < 0.05) compared to untreated diabetic rats. Treatment with 50 mg/kg EaTh reduced hyperglycemia from the 2nd week, and this effect was significant (p < 0.05) in the 3rd and 4th weeks. On the 2nd, 3rd, and 4thweek, Ea* effect was statistically similar to that of 10 mg/kg acarbose (Figure 1).

3.2. Effect of Drugs on α-Glucosidase Activity, in vivo Study.

In normal control rats, blood glucose was increased to1.48 g/l.30 min after sucrose loading and then it returns to normal value at 120 min whereas, in untreated diabetic rats, glycemia was increased to 2.76 g/l at 30 min of sucrose loading to achieve 2.85 g/l at 120 min. 50 mg/kg EaTh has significantly (p < 0.05) prevented the hyperglycemia induced by sucrose loading at 30 and 60 min compared with untreated diabetic rats. In the 200 mg/kg AqTh group, an anti-hyperglycemic effect was shown. Blood glucose levels reached 2.63 g/l and 2.70 g/l at 30 and 60 min, respectively, and they decreased to 2.21 g/l at 120 min. 10 mg/kg acarbose has significantly (p < 0.01) prevented the hyperglycemia induced by sucrose loading at 30, 60, and 120 min compared to diabetic control. The effect of acarbose was statistically similar to EaThTheffffect (Figure 2).

3.3. Effect of Drug

Treatment on BodyWeight, Food, and water intake. The body weight gain by untreated diabetic rats was significantly (p < 0.05) decreased compared with normal rats. AqTh has signifificantly (p < 0.05) prevented bodyweight fall compared with untreated diabetic rats. EaTh- and acarbose-treated rats did not signifificantly (p > 0.05) change the body weight gain compared to untreated diabetic rats. At the end of treatment, water intake did not change in untreated diabetic rats, AqTh, EaTh, and acarbose group compared to the data before treatment whereas food intake was signifificantly increased in diabetic rats and AqTh-, EaTh-, and acarbose-treated rats (p < 0.05, p < 0.05, p < 0.05, a dp < 0.01, respectively) compared to before drug administration (Table 1).

3.4. Effect of Drug Treatment on Urinary Parameters.

After the 4-week treatment period, urinary creatinine and glycosuria were signifificantly increased (p < 0.05 andp < 0.001, respectively) in untreated diabetic rats when compared to normal rats. Oral administration of AqTh has decreased signifificantly (p < 0.05) urinary creatinine compared to untreated diabetic rats, but no significant difference has been observed in glycosuria when compared with untreated diabetic rats. EaTh treatment has prevented urinary creatinine increase compared to normal rats; however, EaTh did not change signifificantly glycosuria. On the other hand, the AqTh and EaTh effect on urinary creatinine and glycosuria was statistically similar to that of 10 mg/kg acarbose. Finally, there was no significant difference in urinary volume when comparing data before and after treatment with AqTh, EaTh, or acarbose (Table 2).

3.5. Effect of Drug Treatment on Biochemical Parameters.

After the 4-week treatment period, HbA1c was signifificantlyincreased (p < 0.05), in untreated diabetic rats, when compared to normal rats. Oral administration of AqTh has prevented HbA1c elevation compared to normal rats. At the end of the treatment period, liver glycogen quantity wassignifificantly decreased (p < 0.05) in untreated diabetic rats when compared to normal rats. Aq* and Ea* treatments have shown no significant effect on liver glycogen compared to untreated diabetic rats whereas acarbose treatment did not change liver glycogen quantity compared to normal rats. Finally, total cholesterol and triglycerides results show that there is no significant change after AqTh, EaTh, or acarbose treatment compared to normal and diabetic rats (Table 3).

3.6. Effect of Drug Treatment on OrganWeight.

Table 4 shows liver, kidney, and heart weight at the end of the treatment period. Results indicate that kidney weight was signifificantlyincreased in untreated diabetic rats as compared to normal rats. Treatment with 200 mg/kg AqTh or 50 mg/kg EaTh did not change liver, kidney, and heart weight when compared to untreated diabetic rats whereas there is a significant elevation in liver and heart weight of acarbose-treated rats compared to untreated diabetic rats.

3.7. Histopathological Observation

3.7.1. Pancreas Changes.

Light microscopic observation of pancreatic islet cells from normal rats shows a normal histological appearance with a large diameter and high granulation density (Figure 3). In untreated diabetic rats, significant reduction of diameter and islet cell number(p < 0.001 and p < 0.01, respectively) was observed. Treatments with 200 mg/kg AqTh have signifificantly prevented the reduction of diameter and cell number of Langerhans islet(p < 0.01 and p < 0.05, respectively). At the same, 50 mg/kg EaTh has signifificantly (p < 0.05) protected diameter and cell number against reduction. Treatment with 10 mg/kg acarbose has prevented signifificantly (p < 0.05) the reduction of the islet cell number.

3.7.2. Kidney Changes.

The Masson staining marks in blue/green collagen fibers, in brown nuclei, in red muscle fiber cytoplasm, and in orange blood cells. Minimal tubulointerstitial collagen was observed in the normal group(Figure 4). A significant increase (p < 0.01) of tubulointerstitial collagen was detected in untreated diabetic rats.Treatment with 200 mg/kg AqTh and 50 mg/kg EaTh has prevented signifificantly (p < 0.001 and p < 0.05, respectively)the tubulointerstitial collagen compared to untreated diabetic rats, but 10 mg/kg acarbose treatment did not changesignifificantly (p > 0.05) this tubulointerstitial collagen. On the other hand, glomeruli collagen was observed in 33.3% of normal rats. In diabetic rats, glomeruli collagen was detected in all rats (100%). Treatment with 200 mg/kg AqTh has significantly reduced (p < 0.05) glomeruli collagen to 40%,but Ea* and acarbose did not (Figure 4).

3.7.3. Liver Changes.

Examination of hematoxylin and eosin-stained sections showed that normal rats had a normal histological appearance. In untreated diabetic rats, an important degenerative change in the liver tissue was observed. Lipid droplets were appeared in all the rats (100%). Treatment with 200 mg/kg AqTh and 50 mg/kg EaTh has signifificantly (p < 0.05) attenuated this effect. The percentage of protection was 60 and 50%, respectively. However, 10 mg/kg acarbose treatment did not attenuate this liver damage(Figure 5).

3.7.4. Aorta Changes.

Light microscopic observation shows that untreated diabetic rats had normal aorta diameter compared to normal rats. Treatment with 200 mg/kg AqTh,50 mg/kg EaTh, or 10 mg/kg acarbose did not signifificantlychange aorta diameter compared to normal and diabetic rats(Figure 6).

4. Discussion

In this study, we demonstrated for the first time the anti-diabetic effect of T. hirsuta medium-term administration (4weeks) and its prevention of renal and liver complications inSTZ-induced diabetic rats.

Our results indicated that the medium-term treatment with 200 mg/kg AqTh or 50 mg/kg EaTh decreases significantly fasting blood glucose in STZ-treated diabetic rats compared with STZ-untreated diabetic rats. EaTh has shown a similar α-glucosidase inhibitory activity when compared to 10 mg/kg acarbose, but AqTh has not inhibited α-glucosidase activity after sucrose loading. These results indicate that the medium-term antihyperglycemic effect of Ea* is related to intestinal α-glucosidase inhibition. So, this finding confirms our previous results [13]whereas the antidiabetic effect of Aq* seems to be related to another mechanism than the α-glucosidase pathway. In addition, we have observed a reduction in HbAc1 levels inAq*-treated diabetic rats while Ea* treatment did not change HbAc1 levels when compared to untreated diabetic rats. This explains why α-glucosidase inhibitors are often prescribed with other antidiabetic drugs in diabetic treatment.

Histopathological study of the sections of the pancreas showed that the administration of AqTh and EaTh for 4weeks signifificantly increases the diameter and cell number in Langerhans islets. Similar studies had proved that many plant extracts signifificantly restored the diameter of islets and the number of β cells in diabetic rats [23–25].

Consequently, the plausible mechanism of action ofAqTh in controlling the blood glucose level might be the enhancement of secretion of insulin from pancreatic β-cells. As with other possible mechanisms, the AqTh may sensitize the insulin receptor to insulin or stimulate the stem cells of the islets of Langerhans in the pancreas of STZ-induced diabetic rats [25].

Therefore, we conclude that the antihyperglycemicphytochemical compounds present in AqTh are different from those of EaTh.

Many studies proved that secondary metabolites such as flavonoids, tannins, and terpenoids have potential inhibitory effects on alpha-glucosidase [26–28]. In a previous study by our team, a polyphenol-rich fraction of T. hirsutahas demonstrated a potent anti-diabetic effect in diabetic rats[29]. Thus, the α-glucosidase inhibitory action of EaTh is due probably to the presence of flavonoids.

It is well known that diabetes is associated with macrovascular and microvascular complications such as nephropathy. Statistics showed that of all dialysis patients, diabetics represent 20.6% in 2001 against 13.1% in 1995 and6.9% in 1989. The mortality rate of patients on dialysis is insignificantly higher in diabetics than in nondiabetes (241.4/1000 vs. 153.99/1000 person-years) [30]. The average survival of type 2 diabetes entering dialysis is approximately 3 years [31, 32]. Diabetic nephropathy is characterized by the accumulation of some proteins such as collagen in the glomerular mesangium and in the tubulointerstitial space that lead to renal fibrosis and so to renal failure [33–35]. In this study, we have demonstrated that medium-term oral administration of 200 mg/kg AqTh or50 mg/kg EaTh prevents urinary creatinine increase and tubulointerstitial renal collagen when compared to untreated diabetic rats as shown in kidney histopathological results. These findings demonstrate that AqTh and EaThcould protect against renal fibrosis through the inhibition of the extracellular matrix (ECM) protein accumulation. These results are similar to other ethnopharmacological studies which demonstrated that garlic and Sclerocaryabirrea ameliorate the process of renal fibrosis in diabetic nephropathy [36, 37]. The protective effect against renal ECM protein accumulation is due to the inhibition of the protein kinase B/mammalian target of the rapamycin(PKB/mTOR) signaling pathway [38]. Recent research studies had demonstrated that the activation of PKB causes the activation of mTORC1 and its downstream proteinp70S6K, which are critical regulators of cell growth, cell proliferation, and protein synthesis [39, 40].

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Consequently, the management of diabetes mellitus with AqTh and EaTh compounds could have helpful effects on renal function in diabetic patients

Evidence suggests that in diabetic rats, a complex alteration in the activities of antioxidant enzymes was observed [41]. This alteration leads to tissue damage and plays an important role in the pathogenesis of diabetic complications. In the present study, liver histopathological results show that untreated diabetic rats develop liver steatosis characterized by lipid droplets. Other studies found that the liver was necrotized in STZ-induced diabetic rats [42]. STZ is considered a classic model of diabetes induction because it provokes toxicity to pancreatic β-cells and cellular death [43], resulting in hypoinsulinemia and hyperglycemia. Insulin plays an important metabolic role as a suppressor of lipolysis in adipose tissue [44]. Thus, hypoinsulinemia in diabetes leads to an increased release of free fatty acids (FFAs) in the bloodstream [45] and the influx of acids into the liver. Intrahepatic triglyceride accumulation occurs when the influx of lipids to the liver surpasses the hepatic capacity to export triglycerides to the bloodstream [45] which causes the development of hepatic steatosis as a diabetic complication [46].

In the present study, the histopathological data show that the medium-term oral administration of 200 mg/kg AqTh or 50 mg/kg EaTh protects signifificantly the liver under steatosis via decreasing lipid droplet accumulation. Similar findings were reported by Eliza et al. [47]where Costus speciosus decreased hepatic disorder. In addition, other studies showed that Camellia oleifera seedameliorates hepatic steatosis via the regulation of FFA [48]and curcumin reduces steatohepatitis and lipid deposition through being an antioxidant and exerting anti-inflammatory and free radical scavenger In roles [49]. However, acarbose treatment did not have this liver-protective propriety. This confirms the side effect of this drug on the liver [50].

Furthermore, T. hirsuta contains sterols, coumarins, terpenes, tannins, aliphatic alcohol, lactone, alkanes, and alkanols [51]. Interestingly, AqTh and EaTh anti-hyperglycemic and antidiabetic effects might be due to the presence of these phytochemicals or other unknown compounds.

5. Conclusions

In conclusion, our study has shown that the medium-term administration of AqTh and EaTh of T. hirsuta had the potential to decrease blood glucose in STZ-induced diabetic rats. The antihyperglycemic effect of EaTh may be partially explained by the inhibition of intestinal α-glucosidase activity. And the AqTh antihyperglycemic activity can be attributed to the stimulation of insulin secretion from pancreatic islet cells. In addition, AqTh and EaTh have shown a crucial preventive effect against renal fibrosis and liver steatosis complications. Thus, these findings suggest that AqTh and EaTh could be considered an efficient oral antidiabetic treatment. Currently, our studies are focused on the isolation and identification of the active compounds of EaTh and AqTh, which are responsible for the antidiabetic effect ofT. hirsuta.

Abbreviations

AqTh: Aqueous extract of +ymelaea hirsuta

DM1: Type 1 diabetes

DM2: Type 2 diabetes

EaTh: Ethyl acetate fraction of +ymelaea hirsuta

ECM: Extracellular matrix

ESRD: End-stage renal disease

FFA: Free fatty acid

mTOR: Mammalian target of rapamycin

PKB: Protein kinase B

STZ: Streptozotocin

T. hirsuta: +ymelaea hirsuta

UMPO: Herbarium University Mohamed Premier of

Oujda, Morocco

WHO: World Health Organization.

Data Availability

The data used to support the findings of this study are available on request from the authors.

Conflicts of Interest

The authors declare that there are no conflicts of interest.

Acknowledgments

The authors wish to express their appreciation to Ramdaoui Karim and Badraoui Mustapha for their technical assistance.

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From: ' Beneficial Effect of Thymelaea hirsuta on Pancreatic Islet Degeneration, Renal Fibrosis, and Liver Damages' Sanae Abid

---The Scientifific World Journal