| Literature DB >> 30127828 |
Arezou Azizsoltani1,2, Khosro Piri1, Sahar Behzad3,4, Masoud Soleimani5, Mina Nekouei6, Zahra Mahmoudi7, Asad Kazemi8.
Abstract
Glycyrrhiza glabra (G. glabra) has been used as a flavoring and sweetener agent, in addition to its therapeutic properties. It is rich in phytoestrogen and may prevent osteoporosis caused by estrogen deficiency; however, there is no evidence for its effects on proliferation and osteogenesis in mesenchymal stem cells. So, we were encouraged to investigate whether the ethyl acetate extract of licorice root as a source of phytoestrogen can act similar to estrogen in cell culture. Furthermore, the analysis of the licorice extract (LE) based on HPLC-DAD-ESI-MS indicated that LE comprises phytoestrogen compounds, such as glabridin and glabrene. In this study, the effects of LE on proliferation of human bone-marrow mesenchymal stem cells (hBM-MSCs) were investigated using MTT assay. In addition, its effects on the osteogenesis were evaluated using alkaline phosphatase activity (ALP), calcium deposition, and bone specific gene expression such as ALP, osteocalcin, Runx2, and BMP-2. The quantitative gene expression was studied by real-time RT-PCR. Our results showed a significant increase in proliferation in presence of LE in concentration 10-50 µg/mL. The differentiation of hBM-MSCs increased in doses of LE (10-25 µg/mL) compared to the control group. The effects of LE were similar to those of 17β-estradiol (E2) (10-8 M) and were abolished by ICI 182,780 an antagonist of estrogen receptor (ER) (10-7), indicating that the stimulatory effects of LE occur through estrogen receptor-mediated mechanism . Taking these into account, LE may be a potential candidate for prevention of osteoporosis in menopausal women.Entities:
Keywords: Differentiation; Fabaceae; Glycyrrhiza glabra; Mesenchymal stem cell; Osteoporosis; Phytoestrogen
Year: 2018 PMID: 30127828 PMCID: PMC6094414
Source DB: PubMed Journal: Iran J Pharm Res ISSN: 1726-6882 Impact factor: 1.696
Compounds assigned in the G. glabra extract by LC-MS.
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| 1 | 13.6 | 230, 280 | Dihydroxy-glabridin | 357 | 135, 235, 339 | 341 |
| 2 | 17 | 230, 280, 340 | Hydroxy-glabrene | 337 | 161, 268, 293, 309, 322 | 339 |
| 3 | 18 | 220,280 | Hydroxy-4’-O-methylglabridin | 353 | 165, 201, 321, 309, 338 | 355 |
| 4 | 19.8 | 217, 250, 285, 325 | Glabrene | 321 | 175, 293, 306 | 323 |
| 5 | 25.5 | 280 | Hydroxy-glabridin | 339 | 135,203,221,321 | 341 |
| 6 | 26 | 230, 280 | Glabridin | 323 | 121, 135, 201 | 325 |
| 7 | 27 | 222, 250, 302 | Glabrone | 335 | 213, 291, 292, 307, 320 | 337 |
| 8 | 36 | 230, 280, 290 | Hispaglabridin A | 391 | 335 | 393 |
| 9 | 46 | 230, 280, 320 | Hispaglabridin B | 389 | 373 | 391 |
Figure 1The RP-HPLC-DAD chromatogram of the G. glabra extract at 283 nm
Figure 2The TIC chromatogram of the G. glabra extract obtained in NI mode.
Figure 3(A) Morphology of undifferentiated Mesenchymal Stem Cells. (B) Osteogenic differentiation of MSCs was visualized by Alizarin Red which stained calcium deposited in extracellular matrix . (C) adipogenic differentiation was confirmed by lipid vacuoles stained with Oil Red staining. (Magnification 10X).
Figure 4Effect of LE on the proliferation of hBM-MSCs. Cells were exposed to LE (1-100 µg/mL) and 0.1% DMSO for 48 and 72 h. Data represent mean ± SD and expressed as an Optical density. *P ˂ 0.05 significantly different compared to control (n = 4).
Figure 5Effect of LE on Alkaline phosphatase activity of hBM-MSCs. Data shown are mean ± SD. *P ˂ 0.05 vs. control (n = 5).
Figure 6Effects of LE on calcium deposition of MSCs. Data shown are mean ± SD. *P ˂ 0.05 vs. control.
Figure 7The real time RT-PCR analysis of osteoblastic genes. Changes in expression of Runx2, ALP, BMP-2 and osteocalcin were analyzed in cells, which were grown in osteogenic medium (control) plus different doses of LE or E2 with or without ICI 182,780 on day 6 and 12. Data represent mean ± SD expressed as a percentage of control. *P ˂ 0.05 significantly different compared to control (n = 4).