1. Introduction
Obesity is a serious challenge of our era that is rapidly becoming a leading cause of preventable mortality worldwide. Based on the World Health Organization (WHO) report, in 2016, nearly 650 million adults were obese, and it’s projected to rise to 1.12 billion by 2030 (
Timper & Bruning, 2017). Therefore, the rising prevalence of obesity and its related diseases soon will turn into a great challenge for health systems (
Nejatbakhsh et al., 2017); particularly concerning cardiovascular diseases (
Kim, Després, & Koh, 2015), cancer (
Calle, Rodriguez, Walker-Thurmond, & Thun, 2003), type 2 diabetes, hyperlipidemia, and hypertension (
Maksvytis & Stakisaitis, 2004). Central or abdominal obesity accelerates several major risk factors for our health, including disturbances in plasma glucose, resistance to insulin, cholesterol level, low-density lipoprotein, and apolipoproteins (
Freedman et al., 1990). Moreover, abdominal obesity modifies the risk for an atherogenic lipid profile of Triglycerides (TG) (
Rakvaag et al., 2019).
Maksvytis et al. showed that the lipid profile varied depending on the Body Mass Index (BMI) (
Adams et al., 2006).
New information regarding food intake indicates the Central Nervous System (CNS), i.e., influenced by the interaction between genes and environmental factors (
Crowley, Yeo, & O'Rahilly, 2002). Hypothalamus heavily influences matching food intake to energy consumption (
Crowley et al., 2002). Based on the currently available evidence, Agouti-Related Peptide/Neuropeptide Y (AgRP/NPY) neurons and Proopiomelanocortin (POMC) influence receptors’ expression for leptin and insulin (
Timper & Bruning, 2017). Fat cells in adipose tissues release leptin, and its concentration regulates based on the metabolism of the body (
Morrison, 2009). Therefore, leptin concentration and body fat percentage are associated (
Morrison, 2009).
Moreover, leptin is known for its hunger-blocking effects; thus, it heavily influences the consumption of food (
Kozłowska et al., 2010). Therefore, the primary impact of leptin is in the hypothalamus, but it also affects other areas of the brain (
Harvey, Solovyova, & Irving, 2006). Leptin regulates our food intake and has a crucial role in multiple metabolic pathways (
Auwerx, & Staels, 1998). For example, it is well proved that leptin stimulates Triglycerides (TGs) accumulation in tissues (
Kavazarakis et al., 2001). Therefore, we can argue that leptin is associated with tissue lipid metabolism and affects the levels of lipid circulation.
Moreover, herbal medicine has positive effects on some metabolism-related disorders (
Nejatbakhsh et al., 2017), including regulating the appetite and improving hyperlipidemia (
Lemhadri, Hajji, Michel, & Eddouks, 2006), mainly through influencing the expression of insulin and leptin receptors (
Handa, Khanuja, Longo, & Rakesh, 2008). One of these herbals is Fennel (Foeniculum vulgar) extract, in which some studies have investigated its effects on metabolic pathways (
Du Plessis, Cabler, McAlister, Sabanegh, & Agarwal, 2010).
Fennel is a plant with substantial antioxidant activities (
Honardoost, Soleimanjahi, & Rajaei, 2013) that can influence (increase) satiety and (reduce) food intake (
Mathern, Raatz, Thomas, & Slavin, 2009). Fennel contains phytosterols reduce cholesterol solubilization, which decreases its absorption (
Nejatbakhsh et al., 2017).
Capasso, Savino, and Capasso (2007) suggested that fennel could delay gastrointestinal transit and reduce fat and sugar absorption. Few research has studies the relationship between fennel and lipid profile. Afiat et al. reported a minor positive change in the concentrations of serum LDL-C, HDL, and HDL (
Afiat et al., 2018).
Choi et al. demonstrated that HDL was significantly increased after the administration of fennel (
Choi & Hwang, 2004).
However, the exact mechanism of the fennel remains unknown. Thus, the present study intended to analyze the potential effects of fennel extracts on body weight and serum lipid profile and assess whether it is through leptin. Accordingly, we evaluated serum leptin concentration and leptin receptor expression in the hypothalamus of BALB/c mice.
2. Methods
Animals
The study was conducted on 35 male BALB/C mice (20-22 gram). Mice were obtained from the Animal Breeding Center of Iran University of Medical Sciences. Initially, a 12/12 h light/dark cycle was applied for all mice at a temperature of 22±2°C. Before performing the study, all protocols were approved by the Iran University of Medical Sciences (IUMS) Ethics Committee.
Fennel extract
We obtained fennel seeds stored for twelve months from the Isfahan Seed Packers Company (Isfahan, Iran). Then, seeds were grinded. Afterward, we mixed 2 g of powder with 150 ml water and was heated it. In the following, 90 mL of the solution was exposed to sterile gas. The resulting solution was poured equal volume into falcon tubes to purify the extract. Then, the falcons were centrifuged for 15 minutes using a 4400 RPM. This process was repeated daily.
Treatment
Animals have divided 35 mice into five groups (n=7/group):
Control (CO): intact animals that no injections were made on them.
Sham: mice that received solvent of fennel (Distilled water).
Fennel 50 (F50): Mice were treated with fennel (50 mg/kg; IP).
Fennel 100 (F100): Mice were treated with fennel (100 mg/kg; IP).
Fennel 200 (F200): Mice were treated with fennel (200 mg/kg; IP).
The tested animals received daily fennel extracts via Intraperitoneal (IP) injection for 2 weeks. The body weight was measured at the beginning and end of the 2 weeks of the experiment.
Measuring serum leptin & lipid concentration
After two weeks of providing interventions, mice were anesthetized to collect their blood from the heart. Next, blood fractionation was performed using a centrifuge to aliquot the serums. The following serums were prepared for analysis. ELISA kits were used to measure Serum leptin; kits were specially designed for Mouse (EASTBIOPHARM, USA). Values are reported as ng/dL of serum.
GPO-PAP enzymatic and CHOD-PAP enzymatic methods (PARS AZMUN) were used to measure serum triglyceride levels and Total Cholesterol (TC), respectively. Serum HDL level was measured by the Immunoinhibition method, and LDL concentration was derived from the Friedewald equation (
Friedewald, Levy, & Fredrickson, 1972).
Preparing tissues for the immunoassays of leptin receptors
To systemically deliver the injected solution, transcardial perfusion was used, initially with PBS, then by 4% Paraformaldehyde (PFA) mixed with PBS (pH 7.4). Dissected brains were post-fixed during the night in 4% PFA in BPS at a temperature of 4oC. After 24 h, brain tissue samples were rinsed using the ice-cold 30% sucrose in BPS. Then, samples were put into optimal cutting temperature compound (OCT, Tissue Tek) before frozen sectioning at -80oC (
Webster, 2000).
The analyses of Immunofluorescence (IFS)
Using the floor standing fully automatic cryostat, MNT-SLEE (Mainz GmbH, Germany), the brain samples were sectioned in coronal planes, each with 10 μm thickness. Then, to obtain the hypothalamus, the sections were put into poly-L-lysine coated coverslips. The next step was air-drying, which was performed for 30 min at room temperature. To rehydrate the sections, they were put into 0.1 M PBS twice, each for 10 min. Subsequently, using a blocking solution [0.1 M PBS containing 2% Bovina Serum Albumin (BSA), 1% normal goat serum, & 0.2% Triton X-100] the sections were incubated. Moreover, incubation was performed for 1h using a permeabilization buffer (10% goat serum, 0.1% Triton X-100 in PBS).
To incubate sections, we used a primary antibody at a temperature of 4°C during the night. The sections were rinsed and further incubated using secondary antibodies for snother 2 hours in antibody solution comprised of 5% goat serum and 0.05% Triton X-100 in PBS. Primary antibodies included mouse monoclonal antibodies to the leptin receptor (1:500; bio-rad). The secondary antibody (Santa Cruz Biotechnology) was used to detect leptin receptor immunostaining was FITC conjugated goat anti-mouse IgG (1:200).
All slides were counterstained using the PI (2 µg/ml) to visualize the nuclei. To obtain negative controls, either the primary or secondary antibodies were removed if no signal was observed. A fluorescence microscope (Nokia) was used for analyzing the data. Besides, a digital camera was used to capture images (Zeiss) (
Ramroodi et al., 2015;
Sarvandi et al., 2015;
Sanadgol et al., 2010).
To compare the mean values of various groups, we used the one-way Analysis of Variance (ANOVA) and Tukey’s Post Hoc Test. The obtained data were analyzed in SPSS at the significance level of P<0.05. The findings are described as Mean±Standard Error (SEM).
3. Results
Bodyweight
There was no significant difference between the research groups (
Figure 1).
Serum lipids
The mice in the fennel 100 mg/kg group had the highest decrease in cholesterol level. Besides, the TG level was decreased significantly in both fennel 100 and 200 mg/kg/day groups. Furthermore, LDL was significantly reduced in the fennel 100 mg/kg/day group. Besides, HDL was significantly enhanced in the fennel 100 mg/kg group (
Figure 2).
Fennel extract and serum leptin levels
Based on the ELISA test, fennel extract is not associated with significant changes in the serum leptin level (
Figure 3).
Effects of fennel extract on leptin receptor protein expression
Based on the collected findings, the expression of leptin receptor protein of all mice was enhanced, particularly in the fennel 50 mg/kg (
Figure 4).
4. Discussion
The global prevalence of obesity is rising and is becoming a leading cause of preventable death. Obesity contributes to numerous health problems, such as CVDs, T2D, and dyslipidemia. Moreover, it is usually associated with increased plasma triglycerides, high levels of LDL, low levels of HDL, increased blood glucose levels, insulin resistance, and increased blood pressure (
Klop, Elte, & Cabezas, 2013); it increases the risk of various chronic diseases. Moreover, obesity is associated with dyslipidemia, probably through causing insulin resistance in peripheral tissues, increasing the hepatic flux of fatty acids from dietary sources, the hydrolysis of triglycerides, and adipose tissue insulin resistance (
Klop et al., 2013).
Recently attention has increased to herbal medicine to manage some disorders (
Lemhadri et al., 2006). Fennel or Foeniculum vulgare is from the carrot family and grows widely in the Mediterranean (
Arzoo, 2017). By increasing fat and sugar metabolism, fennel helps the body lose weight. In other words, fennel dissolves fat deposits in the bloodstream as an energy source. Based on the present study’s findings, fennel could improve blood lipid profile by increasing leptin receptor expression. Fennel contains various ingredients, including phenolic compounds, fatty acids, volatile compounds, flavonoids, amino acids, and phytoestrogens (
Arzoo, 2017).
Assini et al. believed that flavonoids could effectively reduce lipid and lipoprotein. Besides, the authors reported that due to certain contents, namely naringenin and nobiletin, fennel can decline the accumulation of leptin and prevent the overproduction of lipoprotein (
Assini, Mulvihill, & Huff, 2013). A clinical trial on patients with hypercholesterolemia reported that administrating naringin (from the flavonoids family) could significantly reduce LDL of plasma, apoB, and cholesterol by >14% (
Jung et al., 2003). Animal studies developed to study metabolic syndrome and CVDs also reported the beneficial effects of flavonoids in reducing plasma lipids such as triglyceride (
Park et al., 2013). Moreover, a study has reported that applying flavonoids was associated with significant declines in total cholesterol, LDL-C, and TG (
Bao, Hu, Zhang, & Wang, 2016).
Samani and Farrokhi (2014) explored the association between cumin extract and the paraoxonase 1 activity and oxLDL. Accordingly, they reported that the flavonoids available in the seed caused decreased levels of both 1 activity and oxLDL.
Choi and Hwang (2004) found that the HDL was significantly increased after the administration of fennel. Based on the present study’s findings, fennel extract could significantly decline cholesterol, TG, and LDL. Contrarily, it caused an expanding HDL level in adult male BALB/c mice.
Trans-anethole is an active aromatic component isolated from fennel. It composes more than 80% of fennel (
Mahmoudi, Soleimani, Saidi, Khamisipour, & Azizsoltani, 2013;
Rather, Dar, Sofi, Bhat, & Qurishi, 2016). Its positive effects on appetite are proved by several studies (
Bae, Kim, Choue, & Lim, 2015). Besides, it has biologically active molecules with estrogenic activity (
Mahmoudi et al., 2013). Based on the available data, estrogens are potent regulators of energy balance. As evidenced in estrogen deficiency, hyperphagia was seen.
López and Tena Sempere (2015) believed that it has peripheral and central effects on regulating metabolic homeostasis, glucose, and lipid metabolism. Phytoestrogens are plant-derived compounds (
Chrzan & Bradford, 2007) with an extra resemblance to 17β-estradiol. The most well-characterized characteristic of phytoestrogens is binding to estrogen receptors (
Kuiper et al., 1998). However, their estrogenic activity is substantially lower than the natural estrogen hormone (
Turner, Agatonovic Kustrin, & Glass, 2007). Phytosterols can actively remove cholesterol from intestinal micelles (
Nejatbakhsh et al., 2017).
Moreover, fennel can reduce the absorption of fat and glucose levels (
Capasso, Savino, & Capasso, 2007).
Hayes et al. indicated that phytosterols could effectively reduce serum lipid in high cholesterol gerbils (
Hayes, Pronczuk, Wijendran, & Beer, 2002). The present study also revealed that fennel extract could effectively decrease cholesterol, LDL, and TG, increasing serum HDL. Therefore, fennel probably affects the metabolic process by its estrogenic effects.
Hypothalamus heavily influences food intake.
Cederroth et al. found that high phytoestrogen levels could change the expression of genes that code the peptides related to appetite hypothalami of mice (
Cederroth et al., 2007). Leptin, produced primarily by adipose tissue, has a crucial impact on food intake and energy consumption (
Nejatbakhsh et al., 2017). However, its secretion is influenced by estrogen (
Kristensen, Pedersen, & Richelsen, 1999). During the estrus cycle, serum leptin was aletered (
Tanaka et al., 2001). As reported by numerous studies, estrogen can increase leptin secretion in both humans and rats (
Tanaka et al., 2001;
Shimizu et al., 1997). Studies reported estrogen’s ability to reverse leptin secretion (
Yoneda et al., 1998;
Henson, & Castracane, 2006). However,
O’Neil, Burow, Green, McLachlan, and Henson (2001) found that estrogen could increase the promoter activity of leptin of JEG-3.
Hsu and Yen (2007) concluded that flavonoids influence the control of adipogenesis by decreasing intracellular triglyceride levels, mainly by down-regulating expression of transcription factors that control adipogenesis; leptin; C/EBPα; and PPARγ.
As a result, fennel can affect metabolism by influencing leptin secretion. In the present study, the serum level of leptin was constant; however, the expression of its receptor in the hypothalamus was increased, which translates into increased effectiveness of leptin. Research on the effects of fennel on leptin secretion is scarce. In a research on the association between fennel extracts and body weight and leptin concentration,
Nejatbakhsh et al. concluded that different doses of fennel, particularly 200 mg/kg, could increase serum leptin and decrease the weight, compared to obese animals (
Nejatbakhsh et al., 2017).
Hur, Kim, Kim, Ahn, and Ahn (2006) studied the association between fennel and body weight, serum leptin, and Food Efficiency Rate (FER). The authors found a negative association between fennel and FER in rats. Based on the collected findings, there was no association between fennel and serum leptin concentration; however, it could increase protein expression of leptin receptors in the hypothalamus, which in turn caused improved serum lipid profile. However, further studies are required to examine such association.
5. Conclusion
This study indicated that fennel extract could improve the lipid profile by influencing the leptin receptor expression. Therefore, instead of using chemical drugs that often cause adverse effects, herbal medicine can treat hyperlipidemia. The authors suggest further studies to assess the findings of the present study. Acknowledgments: This research was supported by grant No: “92-01-117-22043” from the Iran University of Medical Sciences, Tehran, Iran.
Ethical Considerations
Compliance with ethical guidelines
All protocols were approved by the Ethics Committee of the Iran University of Medical Sciences (IUMS).
Funding
This research was supported by grant No: “96-01-111-22043” from Iran University of Medical Sciences.
Authors' contributions
Conceptualization, investigation, writing - original draft, and data collection: Forogh Zakernezhad; Data analysis: Mahmood Barati and Nima Sanadgol; Writing – review & editing: Monireh Movahhedi, Ahmad Majd and Fereshteh Golab.
Conflict of interest
The authors declared no conflicts of interest.
Acknowledgments
We thank the staff of Cellular and Molecular Research Center, Iran University of Medical Sciences.
Refrences
Adams, K. F., Schatzkin, A., Harris, T. B., Kipnis, V., Mouw, T., & Ballard-Barbash, R., et al. (2006). Overweight, obesity, and mortality in a large prospective cohort of persons 50 to 71 years old. New England Journal of Medicine, 355(8), 763-78. [DOI:10.1056/NEJMoa055643] [PMID]
Afiat, M., Amini, E., Ghazanfarpour, M., Nouri, B., Mousavi, M. S., & Babakhanian, M., et al. (2018). The effect of short-term treatment with fennel on lipid profile in postmenopausal women: A randomized controlled trial. Journal of Menopausal Medicine, 24(1), 29-33. [DOI:10.6118/jmm.2018.24.1.29] [PMID] [PMCID]
Arzoo, M., P. (2017). Fennel: A brief review. European Journal of Pharmaceutical and Medical Research, 4(2), 668-75. https://www.ejpmr.com/home/abstract_id/2064
Assini, J. M., Mulvihill, E. E., & Huff, M. W. (2013). Citrus flavonoids and lipid metabolism. Current Opinion in Lipidology, 24(1), 34-40. [DOI:10.1097/MOL.0b013e32835c07fd] [PMID]
Auwerx, J., & Staels, B. (1998). Leptin. Lancet, 351(9104), 737-42. [DOI:10.1016/S0140-6736(97)06348-4] [PMID]
Bae, J., Kim, J., Choue, R., & Lim, H. (2015). Fennel (foeniculum vulgare) and fenugreek (trigonella foenum-graecum) tea drinking suppresses subjective short-term appetite in overweight women. Clinical Nutrition Research, 4(3), 168-74. [DOI:10.7762/cnr.2015.4.3.168] [PMID] [PMCID]
Bao, L., Hu, L., Zhang, Y., & Wang, Y. I. (2016). Hypolipidemic effects of flavonoids extracted from Lomatogonium rotatum. Experimental and Therapeutic Medicine, 11(4), 1417-24. [DOI:10.3892/etm.2016.3038] [PMID] [PMCID]
Calle, E. E., Rodriguez, C., Walker-Thurmond, K., & Thun, M. J. (2003). Overweight, obesity, and mortality from cancer in a prospectively studied cohort of US adults. The New England Journal of Medicine, 348(17), 1625-38. [DOI:10.1056/NEJMoa021423] [PMID]
Capasso, R., Savino, F., & Capasso, F. (2007). Effects of the herbal formulation ColiMil® on upper gastrointestinal transit in mice in vivo. Phytotherapy Research, 21(10), 999-1101. [DOI:10.1002/ptr.2192] [PMID]
Cederroth, C. R., Vinciguerra, M., Kühnem, F., Madani, R., Doerge, D. R., & Visser, T. J., et al. (2007). A phytoestrogen-rich diet increases energy expenditure and decreases adiposity in mice. Environmental Health Perspectives, 115(10), 1467-73. [DOI:10.1289/ehp.10413] [PMID] [PMCID]
Choi, E. M., & Hwang, J. K. (2004). Antiinflammatory, analgesic and antioxidant activities of the fruit of Foeniculum vulgare. Fitoterapia, 75(6), 557-65. [DOI:10.1016/j.fitote.2004.05.005] [PMID]
Chrzan, B. G., & Bradford, P. G. (2007). Phytoestrogens activate estrogen receptor β1 and estrogenic responses in human breast and bone cancer cell lines. Molecular Nutrition & Food Research, 51(2), 171-77. [DOI:10.1002/mnfr.200600091] [PMID]
Crowley, V. E. F., Yeo, G. S. H., & O’Rahilly, S. (2002). Obesity therapy: Altering the energy intake-and-expenditure balance sheet. Nature Reviews Drug Discovery, 1(4), 276-86. [DOI:10.1038/nrd770] [PMID]
Du Plessis, S. S., Cabler, S., McAlister, D. A., Sabanegh, E., & Agarwal, A. (2010). The effect of obesity on sperm disorders and male infertility. Nature Reviews Urology, 7(3), 153-61. [DOI:10.1038/nrurol.2010.6] [PMID]
Freedman, D. S., Jacobsen, S. J., Barboriak, J. J., Sobocinski, K. A., Anderson, A. J., & Kissebah, A. H., et al. (1990). Body fat distribution and male/female differences in lipids and lipoproteins. Circulation, 81(5), 1498-506. [DOI:10.1161/01.CIR.81.5.1498] [PMID]
Friedewald, W. T., Levy, R. I., & Fredrickson, D. S. (1972). Estimation of the concentration of low-density lipoprotein cholesterol in plasma, without use of the preparative ultracentrifuge. Clinical Chemistry, 18(6), 499-502. [DOI:10.1093/clinchem/18.6.499] [PMID]
Handa, S. S., Khanuja, S. P. S., Longo, G., & Rakesh, D. D. (2008). Extraction technologies for medicinal and aromatic plants (United Nations Industrial Development Organisation and the International Centre for Science and High Technology). Area Science Park Padriciano, 99, 34012. https://www.unido.org/sites/default/files/2009-10/Extraction_for_medici_0.pdf
Harvey, J., Solovyova, N., & Irving, A. (2006). Leptin and its role in hippocampal synaptic plasticity. Progress in Lipid Research, 45(5), 369-78. [DOI:10.1016/j.plipres.2006.03.001] [PMID] [PMCID]
Hayes, K. C., Pronczuk, A., Wijendran, V., & Beer, M. (2002). Free phytosterols effectively reduce plasma and liver cholesterol in gerbils fed cholesterol. The Journal of Nutrition, 132(7), 1983-8. [DOI:10.1093/jn/132.7.1983] [PMID]
Henson, M. C. & Castracane, V. D. (2006). Leptin in pregnancy: An update. Biology of Reproduction, 74(2), 218-29. [DOI:10.1095/biolreprod.105.045120] [PMID]
Honardoost, M., Soleimanjahi, H., & Rajaei, F. (2013). [Apoptosis: Programmed cell death (Persian)]. Journal of Inflammatory Disease, 17(3), 48-57. http://journal.qums.ac.ir/article-1-1492-en.html
Hsu, C. L., & Yen, G. C. (2007). Effects of flavonoids and phenolic acids on the inhibition of adipogenesis in 3T3-L1 adipocytes. Journal of Agricultural and Food Chemistry, 55(21), 8404-10. [DOI:10.1021/jf071695r] [PMID]
Hur, M. H., Kim, C., Kim, C. H., Ahn, H. C., & Ahn, H. Y. (2006). The effects of inhalation of essential oils on the body weight, food efficiency rate and serum leptin of growing SD rats. Journal of Korean Academy of Nursing, 36(2), 236-43. [DOI:10.4040/jkan.2006.36.2.236] [PMID]
Jung, U. J., Kim, H. J., Lee, J. S., Lee, M. K., Kim, H. O., & Park, E. J., et al. (2003). Naringin supplementation lowers plasma lipids and enhances erythrocyte antioxidant enzyme activities in hypercholesterolemic subjects. Clinical Nutrition, 22(6), 561-8. [DOI:10.1016/S0261-5614(03)00059-1] [PMID]
Kavazarakis, E., Moustaki, M., Gourgiotis, D., Drakatos, A., Bossios, A., & Zeis, P. M., et al. (2001). Relation of serum leptin levels to lipid profile in healthy children. Metabolism-Clinical and Experimental, 50(9), 1091-4. [DOI:10.1053/meta.2001.25606] [PMID]
Kim, S. H., Després, J. P., & Koh, K. K. (2015). Obesity and cardiovascular disease: Friend or foe? European Heart Journal, 37(48), 3560-8. [DOI:10.1093/eurheartj/ehv509] [PMID]
Klop, B., Elte, J. W. F., & Cabezas, M. C. (2013). Dyslipidemia in obesity: Mechanisms and potential targets. Nutrients, 5(4), 1218-40. [DOI:10.3390/nu5041218] [PMID] [PMCID]
Kozłowska, L., Rydzewski, A., Fiderkiewicz, B., Wasińska-Krawczyk, A., Grzechnik, A., & Rosołowska-Huszcz, D. (2010). Adiponectin, resistin and leptin response to dietary intervention in diabetic nephropathy. Journal of Renal Nutrition, 20(4), 255-62. [DOI:10.1053/j.jrn.2010.01.009] [PMID]
Kristensen, K., Pedersen, S. B., & Richelsen, B. (1999). Regulation of leptin by steroid hormones in rat adipose tissue. Biochemical and Biophysical Research Communications, 259(3), 624-30. [DOI:10.1006/bbrc.1999.0842] [PMID]
Kuiper, G. G., Lemmen, J. G., Carlsson, B., Corton, J. C., Safe, S. H., & van der Saag, P. T., et al. (1998). Interaction of estrogenic chemicals and phytoestrogens with estrogen receptor β. Endocrinology, 139(10), 4252-63. [DOI:10.1210/endo.139.10.6216] [PMID]
Lemhadri, A., Hajji, L., Michel, J. B., & Eddouks, M. (2006). Cholesterol and triglycerides lowering activities of caraway fruits in normal and streptozotocin diabetic rats. Journal of Ethnopharmacology, 106(3), 321-6. [DOI:10.1016/j.jep.2006.01.033] [PMID]
López, M., & Tena Sempere, M. (2015). Estrogens and the control of energy homeostasis: A brain perspective. Trends in Endocrinology & Metabolism, 26(8), 411-21. [DOI:10.1016/j.tem.2015.06.003] [PMID]
Mahmoudi, Z., Soleimani, M., Saidi, A., Khamisipour, G., & Azizsoltani, A. (2013). Effects of foeniculum vulgare ethanol extract on osteogenesis in human mecenchymal stem cells. Avicenna Journal of Phytomedicine, 3(2), 135-42. [PMID] [PMCID]
Maksvytis, A., & Stakisaitis, D. (2004). Impact of obesity on lipid profiles in middle-aged women. Medicina, 40(6), 553-7. [PMID]
Mathern, J. R., Raatz, S. K., Thomas, W., & Slavin, J. L. (2009). Effect of fenugreek fiber on satiety, blood glucose and insulin response and energy intake in obese subjects. Phytotherapy Research, 23(11), 1543-8. [DOI:10.1002/ptr.2795] [PMID]
Morrison, C. D., (2009). Leptin signaling in brain: A link between nutrition and cognition? Biochimica et Biophysica Acta (BBA) Biomembranes, 1792(5), 401-8. [DOI:10.1016/j.bbadis.2008.12.004] [PMID] [PMCID]
Nejatbakhsh, R., Riyahi, S., Farrokhi, A., Rostamkhani, S., Mahmazi, S., & Yazdinezhad, A., et al. (2017). Ameliorating effects of fennel and cumin extracts on sperm quality and spermatogenic cells apoptosis by inducing weight loss and reducing leptin concentration in diet-induced obese rats. Andrologia, 49(8), e12748. [DOI:10.1111/and.12748] [PMID]
O’Neil, J. S., Burow, M. E., Green, A. E., McLachlan, J. A., & Henson, M. C. (2001). Effects of estrogen on leptin gene promoter activation in MCF-7 breast cancer and JEG-3 choriocarcinoma cells: Selective regulation via estrogen receptors α and β. Molecular and Cellular Endocrinology, 176(1-2), 67-75. [DOI:10.1016/S0303-7207(01)00473-7] [PMID]
Park, H. J., Jung, U. J., Cho, S. J., Jung, H. K., Shim, S., & Choi, M. S. (2013). Citrus unshiu peel extract ameliorates hyperglycemia and hepatic steatosis by altering inflammation and hepatic glucose-and lipid-regulating enzymes in db/db mice. The Journal of Nutritional Biochemistry, 24(2), 419-27. [DOI:10.1016/j.jnutbio.2011.12.009] [PMID]
Rakvaag, E., Fuglsang-Nielsen, R., Bach Knudsen, K. E., Landberg, R., Johannesson Hjelholt, A., & Søndergaard, E., et al. (2019). Whey protein combined with low dietary fiber improves lipid profile in subjects with abdominal obesity: A randomized, controlled trial. Nutrients, 11(9), 2091. [DOI:10.3390/nu11092091] [PMID] [PMCID]
Ramroodi, N., Khani, M., Ganjali, Z., Javan, M. R., Sanadgol, N., & Khalseh, R., et al. (2015). Prophylactic effect of BIO-1211 small-molecule antagonist of VLA-4 in the EAE mouse model of multiple sclerosis. Immunological Investigations, 44(7), 694-712. [DOI:10.3109/08820139.2015.1085391] [PMID]
Rather, M. A., Dar, B. A., Sofi, S. N., Bhat, B. A., & Qurishi, M. A. (2016). Foeniculum vulgare: A comprehensive review of its traditional use, phytochemistry, pharmacology, and safety. Arabian Journal of Chemistry, 9(Suppl 2), S1574-S1583. [DOI:10.1016/j.arabjc.2012.04.011]
Samani, K. G., & Farrokhi, E. (2014). Effects of cumin extract on oxLDL, paraoxanase 1 activity, FBS, total cholesterol, triglycerides, HDL-C, LDL-C, Apo A1, and Apo B in in the patients with hypercholesterolemia. International Journal of Health Sciences, 8(1), 39-43. [DOI:10.12816/0006070] [PMID] [PMCID]
Sanadgol, N., Mostafaie, A., Bahrami, G., Mansouri, K., Ghanbari, F., & Bidmeshkipour, A. (2010). Elaidic acid sustains LPS and TNF-alpha induced ICAM-1 and VCAM-I expression on human bone marrow endothelial cells (HBMEC). Clinical Biochemistry, 43(12), 968-72. [DOI:10.1016/j.clinbiochem.2010.04.066] [PMID]
Sarvandi, S. S., Joghataei, M. T., Parivar, K., Khosravi, M., Sarveazad, A., & Sanadgol, N. (2015). In vitro differentiation of rat mesenchymal stem cells to hepatocyte lineage. Iranian Journal of Basic Medical Sciences, 18(1), 89-97. [PMID] [PMCID]
Shimizu, H., Shimomura, Y., Nakanishi, Y., Futawatari, T., Ohtani, K., & Sato, N., et al. (1997). Estrogen increases in vivo leptin production in rats and human subjects. Journal of Endocrinology, 154(2), 285-292. [DOI:10.1677/joe.0.1540285] [PMID]
Tanaka, M., Nakaya, S., Kumai, T., Watanabe, M., Tateishi, T., & Shimizu, H., et al. (2001). Effects of estrogen on serum leptin levels and leptin mRNA expression in adipose tissue in rats. Hormone Research in Paediatrics, 56(3-4), 98-104. [DOI:10.1159/000048099] [PMID]
Timper, K. & Bruning J. C. (2017). Hypothalamic circuits regulating appetite and energy homeostasis: Pathways to obesity. Disease Models & Mechanisms, 10(6), 679-89. [DOI:10.1242/dmm.026609] [PMID] [PMCID]
Turner, J. V., Agatonovic Kustrin, S., & Glass, B. D. (2007). Molecular aspects of phytoestrogen selective binding at estrogen receptors. Journal of Pharmaceutical Sciences, 96(8), 1879-85. [DOI:10.1002/jps.20987] [PMID]
Webster, D. M. (2000). Protein structure prediction: Methods and protocols. New Jersey: Humana Press Inc. https://books.google.com/books?hl=en&lr=&id=74NOmJ&oi=fnd=false
Yoneda, N., Saito, S., Kimura, M., Yamada, M., Iida, M., & Murakami T., et al. (1998). The influence of ovariectomy on ob gene expression in rats. Hormone and Metabolic Research, 30(05), 263-5. [DOI:10.1055/s-2007-978880] [PMID]