Killing effect and mIFN-γ expression of gene-viral therapeutic system CNHK300-mIFN-γ on malignant tumor cells in vitro

AIM: To investigate the cytotoxicity and mouse IFN-γ (mIFN-γ) expression of oncolytic adenovirus CNHK300-mIFN-γ (CNHK300-Mγ) containing mIFN-γ gene in malignant tumor cells in vitro . METHODS: Human lung cancer cell line A549, human liver cancer cell line SMMC-7721, human pancreatic cancer cell line PANC-1, and human normal fibroblast line BJ were cultured and treated with CNHK300-Mγ, CNHK300, ONYX-015 or AdEasy-mIFN-γ (AdEasy-Mγ). TCID₅₀ assay was used to evaluate the replication ability of CNHK300-Mγ, CNHK300 and ONYX-015 in carcinoma cell lines and normal cell line, and the cytotoxicity was evaluated by cytopathic effect assay and MTT assay. The mIFN-γ expression in the supernatant was detected by ELISA after CNHK300-Mγ or AdEasy-Mγ infection in carcinoma cell lines and normal cell line. RESULTS: The tumor-specific replication ability and cytotoxicity of CNHK300-Mγ were similar to those of CNHK300. The IC₅₀ was as low as MOI of 0.47 pfu/cell for A549 cells, 0.074 pfu/cell for SMMC-7721 cells, 0.532 pfu/cell for PANC-1 cells and was as high as MOI of 281.73 pfu/cell for BJ cells. CNHK300-Mγ was a more powerful killer of malignant tumor cells than ONYX-015 (P<0.01). The tumor cells infected with CNHK300-Mγ efficiently expressed mIFN-γ in vitro and mIFN-γ largely increased as the time prolonged in A549, SMMC-7721 and PANC-1 cells. The mIFN-γ expression in the carcinoma cell lines infected with CNHK300-Mγ was much higher than that in the cells infected with AdEasy-Mγ (P<0.01), but was similar to that in the normal cell line (P>0.05). CONCLUSION: CNHK300-Mγ selectively replicates and effectively promotes the expression of mIFN-γ in carcinoma cells, and specifically kills the tumor cells.     

Effects of rosiglitazone,a PPARγ ligand,on chemoprevention of MNNG-induced gastric cancer in rats

AIM: To examine the chemo-preventive effects of peroxisome proliferator-activated receptor γ(PPARγ) ligand rosiglitazone (RSG) on a rat model of gastric carcinogenesis induced by chemical carcinogen N-methyl-N’-nitro-N-nitrosoguanidine (MNNG). We also attempted to identify novel anti-cancer mechanisms of rosiglitazone.METHODS: Ninety male Wistar rats were randomly allocated into six groups: group A (control group); group B (MNNG group); group C, D and E (RSG group, given different concentrations of rosiglitazone). The treatment procedures were terminated at 40th week. Stomach was harvested and gastric carcinoma was verified by histology. The gastric cancer incidence in different groups was calculated. To elucidate the mechanisms underlying the chemo-preventive effects of PPARγ ligand, we examine the gene expression profiles of MNNG induced gastric cancer and the rosiglitazone treated gastric cancer with Uniset Rat I Bioarray microarray.RESULTS: Incidence of gastric cancer in group A-E was 0% (0/10), 70% (14/20), 15% (3/20), 30% (6/20) and 30% (6/20), respectively. Gastric cancer incidence in group C, D and E was significantly lower than that in group B (P<0.01). A gene that showed prominent responses in rosiglitazone treated group was identified. The hypertension-related, calcium-regulated gene (HCaRG) was significantly upregulated in rat gastric carcinoma in rosiglitazone treated group when compared to MNNG group. The expression of HCaRG was down-regulated in human gastric cancerous tissue. CONCLUSION: PPARγ ligand rosiglitazone has a potent chemo-preventive effect against gastric cancer development in rats. Upregulation of HCaRG may be one of the mechanisms underlying the chemo-preventive effect of rosiglitazone in gastric cancer.     

Effects of simvastatin on proliferation of esophageal cancer cells through NF-κB p65 pathway

AIM To investigate the effects of simvastatin （SIM） on the proliferation of esophageal cancer Eca109 cells through NF-κB p65 pathway. METHODS Esophageal cancer Eca109 cells were cultured in vitro and treated with SIM at different concentrations （2 , 4, 8, 16 and 32 μmol/L）. The proliferation of Eca109 cells was measured by MTT assay and plate colony formation assay. The proliferation-related protein levels of cyclin D1, c-Myc, NF-κB p65 （p65） and IκB-α in the esophageal cancer Eca109 cells were determined by Western blot. ELISA was used to detect the levels of tumor necrosis factor α （TNF-α） and interleukin-6 （IL-6） in the culture supernatant of Eca109 cells. RESULTS Compared with control group, the inhibitory effects of SIM at 2 , 4 , 8 and 16 μmol/L on the viability of Eca109 cells were increased in a concentration-dependent and time-dependent manners （P<0.05）. Simultaneously, the inhibitory rates of SIM at 16 and 32 μmol/L on the viability of Eca109 cells showed no significant difference （P>0.05）. The inhibitory rates of SIM at 16 μmol/L on the viability of esophageal cancer cells was 50.61% at 48 h, which was closed to half of the inhibitory dose IC₅₀, and it was used as the optimum concentration and time for follow-up experiments. Compared with control group, the plate colony formation rate of Eca109 cells, the protein levels of cyclinD1, c-Myc, nuclear p65, TNF-α and IL-6 in 8 and 16 μmol/L groups were decreased, while the levels of cytosolic p65 and IκB-α proteins were increased （P<0.05）. No significant difference of plate colony formation rate in Eca109 cells, and the protein levels of cyclin D1, c-Myc, nuclear and cytoplasmic p65, IκB-α, TNF-α and IL-6 between 16 μmol/L SIM group and 32 μmol/L SIM group was observed （P>0.05）. CONCLUSION Simvastatin inhibits the proliferation of esophageal cancer Eca109 cells, and its mechanism may be related to up-regulation of IκB-α, down-regulation of cyclinD1 and c-myc, inhibition of p65 nuclear translocation, and the expression of TNF-α and IL-6 downstream of NF-κB p65 pathway.     

Influence of IFN-γ combined with M-pred on human embryonic lung fibroblasts

AIM: To look for a better method to deal with interstitial lung disease, interferon-gamma (IFN-γ) combined with methylprednisolone (M-pred) to influence human embryonic lung fibroblast on proliferation, collagen synthesis and the expression of transforming growth factor-β1 (TGF-β1) protein and mRNA were investigated. METHODS: Exponentially growing cells were preincubated for 48 h before harvested. The microculture tetrazolium (MTT) assay was used to measure the inhibition ratios of M-pred combined with different concentrations of IFN-γ. The expression of proliferation cell nuclear antigen (PCNA) was detected by immunocytochemical analysis. Hydroxyproline kit was adopted to detect collagen synthesis. The expressions of TGF-β1 mRNA and protein were detected respectively by RT-PCR and Western blotting. RESULTS: Methylprednisolone, IFN-γ as well as the combination of methylprednisolone and IFN-γ inhibited the proliferation of HELF and the expression of PCNA in comparison with control group (P<0.05). That also decreased the expression of hydroxyproline, inhibited the expression of TGF-β1 mRNA and protein (P<0.05). The effectiveness of IFN-γ became stronger when the concentration increased. The synergistic effect between IFN-γ and methylprednisolone was observed (P<0.05). CONCLUSION: The combination effect of IFN-γ and methylprednisolone is augmented compared with using IFN-γ or methylprednisolone alone, suggesting that the combination use of both drugs has better anti-fibrous degeneration effect than use either alone.     

Effects of zanthoxylum seed oilA2 on NF-кB signaling pathway and inflammatory factor in lung tissue of asthmatic mice

AIM: To investigate the dynamic influence of zanthoxylum seed oilA2 (ZSOA2) on NF-кB signaling pathway and inflammatory factor in pulmonary tissue of asthmatic mice. METHODS: The suspensoid (0.2 mL containing 20% albumin hydroxide and 10% ovalbumin) was administered by intraperitoneal injection to sensitize the BALB/c mice on day 1, then 0.4% ovalbumin solution (50 μL in phosphate buffer fluid) was dripped into the respiratory tract through nasal cavity to establish the asthmatic mouse model. After dripped ovalbumin for 24 h, 48 h, 3 d, 7 d and 14 d, the mice were killed at specified time points. The contents of interleukin-4 (IL-4), interleukin-5 (IL-5) and interferon-γ (IFN-γ) in bronchoalveolar lavage fluid (BALF) were determined by ELISA. The pathological changes of the lung tissues were observed with HE staining. The inflammatory cell counts were conducted by Eosin staining. The protein levels of adhesion molecule and the molecules of NF-κB signaling pathway in lung tissues were determined by Western blotting. RESULTS: In ZSOA2 treated mice, the pathological injury of the lung was significantly attenuated as compared to the model mice, the counts of eosinophils and lymphocytes were reduced obviously in lung bronchial area of asthmatic mice at all observed time points (P<0.05). The levels of IL-5 and IL-4 decreased and IFN-γ increased in BALF. The results of Western blotting showed that ZSOA2 down-regulated the protein levels of intercellular adhesion molecule-1, vascular cell adhesion molecule-1, I kappa B kinase alpha-α and phosphorylation inhibitory-κB. ZSOA2 also up-regulated the protein levels of tumor necrosis factor receptor 1 and phosphorylation nuclear factor-kappaB in lung tissue at all observed time points. CONCLUSION: ZSOA2 has therapeutic effect on asthma by down-regulating the protein expression of IκB-β and p-IκB, inhibiting the releases of cytokines and chemotactic factors, and attenuating the infiltration of inflammatory cells in the lungs of ovalbumin challenged asthma mice.     

Effects of HIF-1α/SDF-1 signaling axis on hypoxia-induced migration and adhesion of progenitor cells

AIM: To observe the expression of hypoxia-inducible factor-1alpha (HIF-1α) and stromal cell-derived factor 1 (SDF-1) in pulmonary artery endothelial cells (PAECs) of SD rats and to investigate the role of HIF-1α/SDF-1 signaling axis on hypoxia-induced migration and adhesion of progenitor cells to PAECs. METHODS: Immunomagnetic beads were used to separate and purify the CD34⁺/CXCR4⁺ progenitor cells derived from the peripheral circulation of SD rats. The expression of HIF-1α and SDF-1 in PAECs exposed to hypoxia (1% O₂, 5% CO₂ and 94% N₂) was detected by immunofluorescence, Western blotting and ELISA. The migration index and adhesion rate were measured in the progenitor cells, which were subjected to the following different treatments: (1) normoxia (21% O₂); (2) hypoxia 12 h; (3) hypoxia 12 h +HIF-1α inhibitor (2ME2); (4) hypoxia 12 h+SDF-1 neutralizing antibody; (5) hypoxia 12 h+2ME2+SDF-1 neutralizing antibody.RESULTS: The expression of HIF-1α and SDF-1 in PAECs was effectively induced by the hypoxic exposure, and both of them reached the peak levels after 12 h of hypoxic treatment (P<0.01), while administration of 2ME2 decreased the hypoxia-induced SDF-1 expression (P<0.05). Treatment of the PAECs with 2ME2 or SDF-1 neutralizing antibody attenuated the migration index and adhesion rate of progenitor cells to the PAECs (P<0.05). CONCLUSION: There is a HIF-1α/SDF-1 signaling axis in hypoxia-exposed PAECs, which may play a crucial role in the migration and adhesion of progenitor cells to PAECs.     

Regulatory effect of NOX-4 on PI3K signaling pathway in TGF-β1-induced collagenⅠsynthesis from lung cancer cells

AIM: To investigate the regulatory effect of NADPH oxidase-4 (NOX-4) on PI3K signaling pathway in transforming growth factor-β1 (TGF-β1)-induced collagen type I (collagen I)synthesis from lung cancer cells and the mechanisms. METHODS: Human lung cancer A549 cells were cultured in vitro and stimulated with TGF-β1. The expression of NOX family and collagen family at mRNA and protein levels as well as the PI3K class I catalytic subunits and the activation of PI3K signaling pathway was measured. A549 cells were pre-treated with NOX-4 inhibitor diphenyleneiodonium (DPI), and the expression of collagen I at mRNA level as well as the PI3K class I catalytic subunits and the activation of PI3K signaling pathway was measured upon TGF-β1 stimulation. RESULTS: TGF-β1 stimulated the expression of NOX-4 and collagen I at mRNA and protein levels as well as the expression of PIK3CD and the activation of PI3K signaling pathway at a dose-and time-dependent manner. NOX-4 inhibitor DPI partly reversed TGF-β1-induced collagen I expression. Inhibition of NOX-4 down-regulated the degree of TGF-β1-stimulated activation of PI3K signaling pathway without effect on the expression of PIK3CD. CONCLUSION: NOX-4 participates in TGF-β1-induced collagenⅠsynthesis from lung cancer cells via regulating the activation of PI3K signaling pathway. TGF-β1/NOX-4/PI3K signaling pathway axis acts as a regulatory role in collagenⅠsynthesis from lung cancer cells.     

Effects of phosphorylation-defective retinoic acid receptor α1 on proli-feration of human multiple myeloma cells in vitro

AIM: To investigate the effect of phosphorylation-defective retinoic acid receptor α1 (RARα1) on the proliferation of human multiple myeloma cells. METHODS: The mRNA expression of RARα subtypes in U266 cells was detected by RT-PCR. Lentiviral plasmid construction, viral production, titer determination and cell transfection were carried out by the general methods of molecular biology. Proliferation analysis was performed with CCK-8 assay. The U266 cells were treated with all-trans retinoic acid (ATRA,0~100 μmol/L) or transfected with lentivirus RARαS77A. The expression levels of proliferation-related proteins, P53 and Rb, in U266 cells treated with ATRA or transfected with lentivirus RARαS77A were detected by Western blotting. RESULTS: RARα1 was positively expressed in U266 cells and RARα2 expression was negative. ATRA significantly inhibited the proliferation of U266 cells in a dose- and time-dependent manner. Proliferation of U266 cells was significantly inhibited 48 h after transfection with lentivirus RARαS77A, and the inhibitory rate was 15.16%±3.84%. The up-regulated expression of Rb and down-regulated expression of P53 were detected in U266 cells not only in the cells treated with ATRA, but also in the cells transfected with lentivirus RARαS77A. CONCLUSION: Phosphorylation-defective RARα1 (RARαS77A) mimics the growth inhibitory effect of ATRA on U266 cells that express RARα1 (+) and RARα2 (-) via down-regulating the expression of P53 and up-regulating the expression of Rb, suggesting that the antiproliferative effect of ATRA is mainly mediated by decreasing the phosphorylation of RARα1.     

Effects of berberine on IL-1 or tumour necrosis factor induced polymorphonuclear leucocyte－endothelium adhesion

AIM:To investigate the effect of berberine on IL-1 or tumour necrosis factor (TNF) induced polymorphonuclear leucocyte(PMN)-endothelium adhesion and adhesion molecules.METHODS:Based on the model of human umbilical vein endothelial cell (HUVEC), this study adopted Rose Bengal Stain, cell ELISA, immunocyto-chemical techniques to investigate the effect of berberine on PMN-endothelium adhesion and the expression of cell adhesion molecules (CAMs).RESULTS:Berberine inhibited IL-1, TNF-induced HUVEC adhesion for PMN when pretreated HUVEC and antagonised IL-1, TNF-induced upregulation of ICAM-1 on HUVEC. Meanwhile, TNF-stimulated PMN adhesion for HUVEC and CD18 upexpression on PMN was diminished in the presence of berberine.CONCLUSION: Inhibite PMN-endothelium adhesion by downregulating the CAMs expression to inhibite PMN migration across endothelium is one of the mechanisms of antiinflammation of berberine.     

Influence of siRNA-mediated PPARγ gene knockdown on invasion ability of chorioepithelioma JEG-3 cells

AIM: To investigate the effect of peroxisome proliferator-activated receptor γ(PPARγ) on the invasion ability of trophoblasts. METHODS: A segment of PPARγ siRNA was synthesized. Three groups were designed: experiment group, negative control group and blank control group. The PPARγ siRNA was transfected into JEG-3 cells. Real-time quantitive PCR was used to detect the mRNA levels of PPARγ and mucin-1(MUC1). The Transwell culture inserts were used to detect the invasion ability of JEG-3 cells 24 h after treated with PPARγ siRNA. RESULTS: After transfected with PPARγ siRNA, the mRNA expression levels of PPARγ and MUC1 were significantly depressed by (75.0±0.8)% and (65.0±1.3)% (P<0.05),respectively, and the invasion ability of JEG-3 cells was significantly strengthened (P<0.05). CONCLUSION: The depression of PPARγ gene down-regulates the expression of MUC1, and affects the invasion ability of trophoblasts, indicating that PPARγ may regulate the invasion of trophoblasts by MUC1 and involve in the development of placental defects such as preeclampsia.     

Effects of aldosterone on expression of angiotensin Ⅱ receptors in cultured rat mesangial cells

AIM: To investigate the effect of aldosterone (ALD) on the mRNA expression of angiotensin Ⅱ (Ang II) type 1 (AT-1a R and AT-1bR) and 2 (AT-2R) receptors in cultured rat mesangial cells (RMCs) treated with high glucose. METHODS: Rat mesangial cells were cultured in high glucose medium containing different concentrations of ALD (10-8-10-6 mol/L). The antagonists of ALD and Ang II receptors including pironolactone (10-7 mol/L, aldosterone receptor antagonist, SPI), losartan (10-7 mol/L, Ang II type 1 receptor blocker, Los) or PD123319 (10-9 mol/L, Ang II type 2 receptor antagonist, PD) were added in the cell culture for 12 h. The control cells were only treated with high (30 mmol/L) or normal (5.6 mmol/L) glucose medium. The viability and proliferation of the RMCs were evaluated by MTT assay. The mRNA expression of AT-1aR, AT-1b R and AT-2R was detected by semi-quantitative RT- PCR. The expression of MCP-1 in cultured RMCs was detected by ELISA. RESULTS: The mRNA expression of AT-1aR, AT-1b R and AT-2R was increased significantly by treatment with ALD in a dose-dependent manner (1.62-1.77, 9.61-9.89 and 7.26-7.35 folds of high glucose control, respectively, P<0.01). SPI significantly reduced the mRNA expression of AT-1aR and AT-1b R (P<0.01) but not affected the mRNA expression of AT-2R. The ratio of AT-1aR/AT-1b R in cultured RMCs treated with high glucose decreased significantly after stimulated with ALD (P<0.01). However, the effect of ALD was inhibited by SPI (P<0.01). Aldosterone treatment induced a significant upregulation of MCP-1 expression in a dose-dependent manner, and previous treatment with spironolactone, losartan or PD123319 abolished this aldosterone-induced MCP-1 expression. CONCLUSION: The results suggest that aldosterone is involved in the inflammatory response by up-regulating the expression of AT-1aR, AT-1bR and AT-2R, changing the proportion of AT-1R subtype, and inducing MCP-1 overproduction in cultured RMCs treated with high glucose.     

Effects of thrombospondin 1 on rat cardiac fibroblasts induced by transforming growth factor β1

AIM:To investigate the effects of thrombospondin 1 on transforming growth factor β₁ induced rat cardiac fibroblasts (CFs). METHODS: CFs of neonatal Sprague -Dawley (SD) rats were isolated with the method of digestion and differential anchoring velocity. The proliferation and collagen synthesis of rat CFs were observed with MTT and hydroxyproline. The expression of TSP-1mRNA was analyzed by RT-PCR.RESULTS: The dose and time-dependent effects of TGF-β₁ were observed. Expression of TSP-1 was increased significantly (P<0.01). Stimulation of CFs with TGF-β₁ (20 μg/L, 24 h) significantly increased CFs proliferation and collagen synthesis (P<0.01). TSP-1 antisense oligonucleotide effectively inhibited TGF-β₁ induced CFs proliferation and collagen synthesis (P<0.01).CONCLUSION:The proliferation and collagen synthesis of CFs induced by TGF-β₁ are inhibited by TSP-1 antisense oligonucleotide, which may exert helpful effect on anti-fibrosis.     

Effect of IL-1β and IL-6 on expression of nerve growth factor in human nucleus pulposus cells

AIM: To determine the effect of interleukin-1β(IL-1β)and IL-6 on the expression of nerve growth factor (NGF) by human nucleus pulposus (NP) cells. METHODS: The NP cells from the normal disc of operative patients with scoliosis were isolated, cultured and identified. After 7 days preculture, the NP cells were treated with IL-1β (10 μg/L, 50 μg/L) or IL-6 (10 μg/L, 50 μg/L) for 48 h in the experimental groups and 0.3% PBS was used in the control groups. The expression of NGF was detected by the methods of immunohistochemistry, semi-quantitative RT-PCR and Western blotting.RESULTS: The NP cells were chondrocyte-like cellular morphology with positive staining of toluidine blue, safranine O and anti-collagen II antibody. The NP cells cultured in monolayer showed immunoreactivity to NGF either in control condition or in experimental group. IL-1β and IL-6 up-regulated the mRNA expression of NGF and the protein production of NGF. The effect of this up-regulation was higher by treating with IL-6 than by treating with IL-1β in the same concentration.CONCLUSION: Our results demonstrate that the proinflammatory cytokines IL-1β and IL-6 stimulate the production of NGF in NP cells. The effect of IL-6 is more significant than that of IL-1β.     

Effects of erigeron breviscapine on nuclear factor-κB expression following lung ischemia-reperfusion injury

AIM: To investigate the effects of erigeron breviscapine on nuclear factor-κB (NF-κB) expression following lung ischemia-reperfusion (I/R) injury in rats. METHODS: Thirty-two male Sprague-Dawley rats were randomized into four groups with 8 animals in each group: sham operation group (I), I/R group (II), erigeron 25 mg/kg group (III) and erigeron 50 mg/kg group (IV). A lung I/R injury rat model was established in situ. I/R injury consisted of 45 min of lung cross-clamping followed by 2 h of reperfusion; sham operation animals had a thoracotomy only. The wet-to-dry weight ratio (W /D), myeloperoxidase (MPO) of lung tissue, the content of nuclear NF-κB p65 were detected by immunohistochemical staining and Western blotting. The histopathological changes of lung tissue were observed under light microscopy. Electron microscopic evaluation was done on randomly selected lungs of two rats in each group at the end of the experiment. RESULTS: Compared to sham operation group, W /D and MPO in the I/R group increased significantly after reperfusion, and the expression of NF-κB in nucleus was up-regulated. As compared with I/R group, the level of NF-κB decreased in group III and IV. Also the changes of W /D and MPO were ameliorated as compared with group II. There was significant difference between group III and IV. CONCLUSION: Erigeron breviscapine reduced I/R lung injury through suppressing the activation of NF-κB and subsequent neutrophils accumulation.     

Effects of methionine-induced hyperhomocysteinemia on protein C,antithrombin-Ⅲ and von willebrand factor

AIM:To observe the effects of methionine-induced hyperhomocysteinemia on protein C(PC),ant ithrombin-(AT-)and von willebrand factor(vWF).METHODS:Eighteen New Zealand rabbits were randomized as methionine group(group M,n=9)and control(group C,n=9),which were fed with methionine-rich diet(600 mg/d)and regular diet respectively for sixteen weeks.By the end of sixteen weeks,the serum biochemistry and PC,AT-and vWF in plasma were determined and vWF expression of endothelial cel s of aorta were examined.RESULTS:In group M,the levels of methionine(29.97±5.34 mol/L)and homocysteine(13.30±2.19mol/L)in serum were signif icantly higher than those(14.48±1.97 mol/L and 5.36 1.19 mol/L,respectively,P<0.01)of group C.The levels of AT-and PC of group M were signif icantly lower than those of group C(P<0.01).The level of vWF in plasma of group M was higher than that of group C(P<0.01).Immunohisto chemistry showed that vWF expression in endothelial cells of aorta was decreased.CONCLUSION:Methionine-induced hyperhomocysteinemia had promot ive ef ects on coagulat ion and inhibiting effects on antioagulation.     

Effects of α-MSH on the Ca2+ channels of primary DMNV cells and effects of anti-apoptosis on primary DMNV cells after activation of melanocortin receptors

AIM: α-MSH is elevated in patients with inflammatory bowel disease and has been implicated as an inflammatory mediator. The purpose of this study was to investigate effects of α-MSH on the Ca2+ channels of primary DMNV cells, the effects of gastrointestinal inflammation on the dorsal motor nucleus of the vagus in rats, as well as the effects of proinflammatory cytokines and α-MSH on neurons from the dorsal motor nucleus of the vagus in vitro. METHODS: In vitro studies the primary culture of neurons from the dorsal motor nucleus of the vagus was performed. Single-cell cytoplasmic calcium transients were determined using the fluorescence dye fura-2-AM. Cell proliferation and apoptosis were measured by enzyme-linked immunosorbent assay. RESULTS: MC4R mRNA was expressed in the DMNV cells of normal rats. Activation of MC4R promoted the calcium influx of primary DMNV cells. The addition of α-MSH to thrombin or trypsin resulted in significant decreases in apoptosis compared to thrombin or trypsin alone. CONCLUSION: Functionally active α-MSH receptors are linked to Ca2+ channels in DMNV neurons. In cultured DMNV cells, α-MSH attenuates neuronal apoptosis and reverses inhibition of cellular proliferation.