7 research outputs found
λ§μ΄μ½ νλμ°μ μν μ·λμΈν¬μ£Ό μ¬λ©Έμ κΈ°μ
Get PDFλͺ©μ : Mycophenolic acid (MPA)λ μ·μ₯μ΄μμ ν¬ν¨ν λ€μν μ’
λ₯μ μ₯κΈ°μ΄μμ μ¬μ©λλ λ©΄μμ΅μ μ λ‘ inosine monophosphate dehydrogenase (IMPDH)μ μ νμ μ΄κ³ λΉκ²½μμ μΈ μ΅μ μ μ΄λ μ·λμΈν¬μ£Όμμλ μΈν¬ μ¬λ©Έμ μ λνλ€κ³ μλ €μ Έ μλ€. λ³Έ μ°κ΅¬μμλ μΈμλ¦°μ λΆλΉνλ μ·λ μΈν¬μ£ΌμΈ HIT-T15 μΈν¬λ₯Ό μ¬μ©νμ¬, MPAκ° μΈν¬ μ¬λ©Έμ μΌμΌν€λ κΈ°μ μ κ·λͺ
νκ³ μ νμλ€. λ°©λ²: μΈν¬μ£Όλ American Type Culture Collectionμμ ꡬμ
νμμΌλ©° 10% fetal bovine serumμ΄ ν¬ν¨λ RPMI-1640μ μ¬μ©νμ¬ λ°°μνμλ€. μΈν¬ νμ±μ methylthiazoletetrazolium (MTT) assay, μΈν¬ μ¬λ©Έμ annexin Vμ PI μΌμλ², mitogen-activated protein kinase (MAPK) νμ±νμ caspase-3 λΆμ μ Western blot λΆμμΌλ‘ μΈ‘μ νμλ€. κ²°κ³Ό: MPA 1ΞΌMκ³Ό 10ΞΌMμ μ²λ¦¬νμμ λ MTT, caspase-3 λΆμ κ·Έλ¦¬κ³ annexin V μΌμμ΄ 24μκ°μ λλ μμ‘΄μ μΌλ‘ μ¦κ°νμμΌλ©°, μ΄λ μΈλΆμμ ν¨κ» ν¬μ¬ν guanosine 500ΞΌMμ μνμ¬ λΆλΆμ μΌλ‘ ν볡λμμΌλ adenosine 500ΞΌM ν¬μ¬μμλ λ³νκ° μμλ€. λν MPAλ extracellular-regulated protein kinase (ERK), p38 MAPK κ·Έλ¦¬κ³ c-jun N-terminal protein kinase (JNK)μ νμ±νλ₯Ό 8μκ°κ³Ό 24μκ°μμ μ¦κ°μμΌ°κ³ guanosine ν¬μ¬λ μ΄λ₯Ό λΆλΆμ μΌλ‘ ν볡μμΌ°λ€. ERKμ μ΅μ μ μΈ PD98059, p38 MAPK μ΅μ μ μΈ SB203580 κ·Έλ¦¬κ³ JNK μ΅μ μ μΈ SP600125λ MPAμ ν¨κ» μ²λ¦¬νμμ λ κ° μκ°μ μ¦κ°λ MAPK νμ±μ κ°μμμΌ°μ§λ§ MTTμ caspase-3 λΆμ μ μ΄ν΄λ³Έ κ²°κ³Ό PD98059λ μν₯μ΄ μμμΌλ©° SB203580μ μΈν¬μ¬λ©Έμ μ¦κ°μμΌ°κ³ , SP600125λ§μ΄ MPAκ° μΌμΌν¨ μΈν¬ μ¬λ©Έμ μΌλΆ νμμμΌ°λ€. Pan-caspase μ΅μ μ μΈ Z-VAD-FMK λν μΈν¬ μ¬λ©Έμ νμμμΌ°λ€. κ²°λ‘ : MPAλ MAPK νμ±μ IMPDH μμ‘΄μ μΌλ‘ μ¦κ°μν€μ§λ§, ERKlμ p38 MAPKμλ μκ΄μμ΄, JNK νμ±νλ₯Ό ν΅ν caspase-3 μ¦κ°μ κ²½λ‘λ‘ μ·λ μΈν¬ μ¬λ©Έμ μ λν¨μ μ μ μμλ€.ope
Mechanisms involved in the inhibitory effects of mycophenolic acid on the PDGF-induced proliferation of vascular smo
No full textμκ³Όνκ³Ό/λ°μ¬[νκΈ]
νκ΄ννκ·Ό μΈν¬μ μ¦μμ μ₯κΈ°μ΄μν λ°μνλ νκ΄κ²½νμ¦μ΄λ λλ§₯κ²½νμ¦μ λ°μκ³Ό μ§νμ μ€μν μν μ νλ€. Mycophenolic acid (MPA)λ κ°λ ₯ν λ©΄μμ΅μ μ λ‘μ νκ΄ννκ·Ό μΈν¬μ μ¦μλ μ΅μ νλ€. λ³Έ μ°κ΅¬μμλ ν°μ₯μ μ¬λ νκ΄ννκ·Ό μΈν¬λ₯Ό μ΄μ©νμ¬ platelet-derived growth factor (PDGF)λ‘ μ λν μΈν¬μ¦μμ λν MPAμ μμ© κΈ°μ μ μ°κ΅¬νμλ€.
μΌμ°¨λ°°μν ν°μ₯μ μ¬λ νκ΄ννκ·Ό μΈν¬λ₯Ό PDGF-BB 10 ng/mlλ‘ μκ·Ήνμκ³ , MPAλ₯Ό λΉλ‘―ν κ° μ νΈμ λ¬ μ΅μ μ λ PDGFλ₯Ό ν¬μ¬νκΈ° 1μκ° μ λΆν° ν¬μ¬νμλ€. μΈν¬μ μ¦μμ [H3]-thymidine incorporation, methyl- thiazoletetrazolium (MTT), proliferating cell nuclear antigen (PCNA) νν, NAD(P)H oxidase subunitμ mRNA ννμ RT-PCR, dichlorofluorescein (DCF)μ λ―Όκ°ν μΈν¬λ΄ νμ±μ°μμ‘±μ FACS, κ³Όμ°νμμ(H2O2) λλλ potassium iodide λ², κ·Έλ¦¬κ³ PDGF μμ©μ²΄-Ξ² (Tyr 751), rac1, Akt, ERK 1/2 λ° p38 MAPK νμ±νλ Western blot λΆμ λ°©λ²μ μ¬μ©νμλ€.
PDGF 10 ng/ml ν¬μ¬ ν ν°μ₯ νκ΄ννκ·Ό μΈν¬μ μ¦μ, PDGF μμ©μ²΄μ Akt νμ±ν, μΈν¬λ΄ νμ±μ°μμ‘±, ERK 1/2μ p38 MAPK νμ±ν λ° NAD(P)H oxidase subunit μ€ rac1μ νμ±νλΏλ§ μλλΌ p22phoxμ MOX1μ mRNA ννμ΄ λμ‘°κ΅°μ λΉνμ¬ μ μνκ² μ¦κ°νμλ€. MPAλ PDGFμ μν μΈν¬ μ¦μμ μ©λμμ‘΄μ μΌλ‘ μ΅μ νμμΌλ©°, μΈλΆμμ ν¬μ¬ν guanosine 100ΞΌMμ MPAμ μν μ¦μμ΅μ ν¨κ³Όλ₯Ό λΆλΆμ μΌλ‘ ν볡μμΌ°λ€. μΈν¬λ΄ μ νΈμ λ¬κ³μ λνμ¬ MPAλ PDGF μμ©μ²΄-Ξ² (Tyr 751) νμ±νμλ μν₯μ μ£Όμ§ μμμΌλ, Akt νμ±ν, rac1μ νμ±ν, p22phoxμ MOX1μ mRNA ννμ μν₯ μ‘°μ , μΈν¬λ΄ νμ±μ°μμ‘± λ° ERK 1/2μ p38 MAPK νμ±νλ₯Ό ν΅κ³μ μΌλ‘ μ μνκ² μ΅μ νμλ€. λν, MPAλ H2O2λ₯Ό μ κ±°νμλ€. Wortmannin (PI3K μ΅μ μ ), diphenyleniodonium (NAD(P)H μ΅μ μ ) λ° NACμ trolox (νμ°νμ )λ PDGFμ μν ERK 1/2μ p38 MAPK νμ±νμ μΈν¬μ¦μμ μ΅μ νμλ€. PD98059 (MEK μ΅μ μ )μ p38 I (p38 MAPK μ΅μ μ )λ PDGFμ μν νκ΄ννκ·Ό μΈν¬μ μ¦μμ νμ νκ² μ΅μ νμλ€. μ¬λμ νκ΄ννκ·Ό μΈν¬μμλ MPAλ PDGFμ μν μΈν¬λ΄ νμ±μ°μμ‘± λ° ERK 1/2μ p38 MAPKμ νμ±νλ₯Ό μ΅μ νμλ€.
κ²°λ‘ μ μΌλ‘, λ³Έ μ°κ΅¬κ²°κ³Όλ MPAκ° μΈν¬λ΄ guanosine μμ± μ΅μ , Akt νμ±ν μ΅μ λ° νμ°ν ν¨κ³Όλ₯Ό ν΅ν MAPK νμ±ν μ΅μ λ₯Ό κ²½μ νμ¬ PDGFμ μν νκ΄ννκ·Ό μΈν¬μ μ¦μμ μ΅μ ν¨μ μμ¬νμλ€. MPAμ νμ°ν ν¨κ³Όλ H2O2μ λν μ§μ μ μ κ±°ν¨κ³Όμ NAD(P)H oxidase μ΅μ μ κΈ°μΈν¨μ μμ¬νμλ€.
[μλ¬Έ]Vascular smooth muscle cell (VSMC) proliferation plays an important role in the development and progression of chronic allograft vasculopathy as in atherosclerosis. Mycophenolic acid (MPA), an immunosupressive agent, inhibits VSMC proliferation. In this study, the mechanisms involved in anti-proliferative effect of MPA was examined.
Primary rat and human VSMCs were stimulated with platelet-derived growth factor (PDGF)-BB 10 ng/ml in the presence or absence of MPA (10 nM ο½ 100 ΞΌM). The effect of known inhibitors of signaling molecules involved in VSMC proliferation were compared with that of MPA to confirm the involvement of each signaling molecule. Cell proliferation was assessed by [H3]-thymidine incorporation, methyl- thiazoletetrazolium (MTT), and proliferating cell nuclear antigen (PCNA) expression, NAD(P)H oxidase subunits mRNA expression by reverse transcription-polymerase chain reaction, dichlorofluorescein (DCF)- sensitive cellular reactive oxygen species (ROS) by FACS, hydrogen peroxide (H2O2) concentration by iodometric analysis, and the activation of PDGF receptor-Ξ² (Tyr 751), rac1, Akt, ERK 1/2, and p38 MAPK by Western blot analysis.
PDGF increased cell proliferation and cellualr ROS, activation of PDGF receptor, Akt, rac1, ERK 1/2, and p38 MAPK, and expression of p22phox and MOX1 mRNA, compared to control. MPA inhibited PDGF-induced VSMC proliferation in a dose-dependent manner. Exogenously administered guanosine partially rescued cell proliferation inhibited by MPA. MPA also inhibited PDGF-induced up-regulation of Akt and rac1 phosphorylation, p22phox and MOX1 mRNA expression, cellualr ROS, and ERK 1/2 and p38 MAPK phosphorylation. However, MPA did not affect PDGF receptor-Ξ² (Tyr 751) phosphorylation, suggesting that MPA''s anti-proliferative effect is independent on PDGF receptor activation. MPA directly scavenged H2O2. Wortmannin (PI3K inhibitor), diphenyleneiodonium (DPI, NAD(P)H oxidase inhibitor), N-acetylcysteine and trolox (anti-oxidants) all inhibited PDGF-induced ERK 1/2 and p38 MAPK activation and cell proliferation. PD98059 (MEK inhibitor) and p38 I (p38 MAPK inhibitor) inhibited PDGF-induced cell proliferation. In human VSMCs, MPA also suppressed PDGF-induced cellular ROS and activation of ERK 1/2 and p38 MAPK.
In conclusion, these results suggest that MPA inhibits PDGF-induced VSMC proliferation through inhibiting de novo synthesis of guanosine, Akt activation, and cellular ROS leading to ERK 1/2 and p38 MAPK activation. Both direct scavenging and inhibiting NAD(P)H oxidase appear to be involved in anti-oxidative effect of MPA.ope
Mechanisms Involved in the Inhibitory Effects of Mycophenolic Acid on the PDGF-induced Proliferation of Vascular Smooth Muscle Cells
No full textBackground: Vascular smooth muscle cell (VSMC) proliferation plays an important role in the development and progression of chronic allograft vasculopathy as in atherosclerosis. We already reported that mycophenolic acid (MPA) inhibited VSMC proliferation, cellular reactive oxygen species (ROS) and mitogen-activated protein kinases (MAPK) in human VSMCs. In this study, we examined further molecular mechanisms involved in the anti-proliferative effect of MPA in rat VSMCs.
Methods: Primary rat VSMCs were stimulated with PDGF-BB 10 ng/mL in the presence or absence of MPA and various kinds of cell signaling inhibitors. Cell proliferation was assessed by [HΒ³]- thymidine incorporation, NAD(P)H oxidase subunits mRNA expression by RT-PCR, dichlorofluorescein- sensitive cellular ROS by FACS, and the activation of PDGF receptor-Ξ² (Tyr 751), rac1, and MAPK by Western blot analysis.
Results: PDGF increased cell proliferation and cellular ROS, activation of PDGF receptor-Ξ² (Tyr 751), rac1, expression of p22phox and MOX1 mRNA, ERK 1/2, and p38 MAPK, compared to control. MPA inhibited up-regulation of rac1 phosphorylation, p22phox and MOX1 mRNA expression, cellular ROS, and phosphorylation of ERK 1/2 and p38 MAPK. However, MPA did not affect PDGF receptor-Ξ² (Tyr 751) activation. Wortmannin, diphenyleniodonium (DPI), trolox, and NAC, each inhibited PDGF- induced ERK 1/2 and p38 MAPK activation. PD98059 and p38 MAPK inhibitor also inhibited PDGF-induced cell proliferation.
Conclusion: These results suggest that MPA inhibits PDGF-induced VSMC proliferation through inhibiting NAD(P)H oxidase-dependent cellular ROS leading to ERK 1/2 and p38 MAPK activation.ope
An Implementation of an GPGPU-based Digital Channel Selector and a Matched Filter for a Distributed Spectrum Sensing Node
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Effects of Mycophenolic Acid and Rapamycin on PDGF-induced Mesangial Cell Proliferation and Extracellular Matrix Production
No full textPurpose: Excess proliferation and extracellular matrix (ECM) accumulation of mesenchymal cells such as vascular smooth muscle cells (VSMC) and glomerular mesangial cells cause chronic allograft nephropathy showing transplant vascular sclerosis and glomerulosclerosis. Mycophenolic acid (MPA) and rapamycin (RPM) are well known as strong inhibitors of VSMC proliferation, but their effects on the glomerular mesangial cells are not yet clearly understood. This study examined the effects of MPA or RPM on PDGF-induced proliferation and ECM accumulation in rat glomerular mesangial cells.
Methods: Mesangial cells isolated from the glomeruli of Sprague-Dawley rats were cultured with DMEM containing 20% fetal bovine serum. Growth arrested and synchronized cells were administered with test drugs (MPA10 nM~10microM , RPM 0.1 nM~1microM) before the addition of PDGF 10 ng/mL. Cell proliferation was assessed by [3H]thymidine incorporation, collagen by [3H]proline incorporation, and fibronectin, ERK, and p38 MAPK by Western blot analysis.
Results: PDGF increased mesangial cell proliferation by 4.64-fold. Compared to stimulated control, MPA above 500 nM and RPM above 10 nM showed a significant inhibitory effect in a dose- dependent manner. The IC50 of MPA and RPM against PDGF-induced mesangial cell proliferation were around 500 nM and 100 nM, respectively. The collagen synthesis was also inhibited by MPA and RPM, but the fibronectin secretion was inhibited by MPA alone. The proliferation of mesangial cell correlated with activation of ERK and p38 MAPK. MPA, but not RPM, inhibited ERK and p38 MAPK activation.
Conclusion: This study demonstrated that MPA and RPM significantly inhibited PDGF-induced proliferation and ECM production in rat glomerular mesangial cells. The inhibitory effects of MPA, but not RPM, are correlated with ERK and p38 MAPK.ope
Mycophenolic Acid Inhibits Oleic AcidβInduced Vascular Smooth Muscle Cell Activation by Inhibiting Cellular Reactive Oxygen Species
No full textBACKGROUND:
Vascular smooth muscle cell (VSMC) proliferation and matrix protein accumulation play important roles in the development and progression of chronic allograft vasculopathy. Mycophenolic acid (MPA) inhibits various types of mesenchymal cell proliferation and cellular reactive oxygen species (ROS) are involved in the anti-proliferative effect of MPA. In this study, we investigated the effects of MPA on oleic acid (OA)-induced VSMC proliferation and the role of ROS in this process.
METHODS:
Primary VSMCs from Sprague-Dawley rats were stimulated with 100 microM OA, with or without MPA (0.1- 10 microM) or 5 mM N-acetylcysteine (NAC) for one hour prior to the addition of OA. Cell proliferation was measured by methylthiazoletetrazolium (MTT) assays, proliferating cell nuclear antigen (PCNA) expression, and fibronectin secretion by Western blot analysis, and dichlorofluorescein (DCF)-sensitive cellular ROS by fluorescence-activated cell scanning (FACS).
RESULTS:
OA (100 microM) increased cell proliferation, as measured by MTT (by 1.6-fold), PCNA expression, fibronectin secretion, and cellular ROS (by 1.6-fold). Treatment with MPA dose-dependently inhibited OA-induced VSMC proliferation, fibronectin secretion, and cellular ROS. Treatment with 5 mM NAC also inhibited OA-induced rat VSMC activation.
CONCLUSIONS:
These results suggest that MPA inhibits OA-induced VSMC proliferation and matrix protein synthesis partially by inhibiting cellular ROS.ope
