Roles of Smad3 and Smad7 in rat pancreatic stellate cells activated by transforming growth factor-beta 1

BACKGROUND: Pancreatic stellate cells (PSCs) play a major role in promoting pancreatic fibrosis. Transforming growth factor beta 1 (TGF-beta 1) is a critical mediator of this process. This study aimed to determine the expression of the Smad3 and Smad7 genes in the process of PSC activation, and explore the mechanisms of chronic pancreatitis. METHODS: The expressions of Smad3 and Smad7 in PSCs before and after TGF-beta 1 treatment were detected by reverse transcription-polymerase chain reaction and Western blotting analysis. Smad3 expression was detected in PSCs after treatment with 5 ng/ml of TGF-beta 1 for 24 hours. RESULTS: Smad7 expression was decreased in TGF-beta 1 -activated PSCs (P<0.05) in a dose-dependent manner. When TGF-beta 1 concentration reached 10 ng/ml, the expression of p-Smad3, Smad3, and Smad7 was inhibited (P<0.05). CONCLUSIONS: TGF-beta 1 promotes the expression of Smad3 and inhibits the expression of Smad7 during the activation of PSCs. In contrast, high-dose TGF-beta 1 downregulates the expression of Smad3 in completely activated PSCs.

Chondrogenesis of periodontal ligament stem cells by transforming growth factor-β3 and bone morphogenetic protein-6 in a normal healthy impacted third molar

The periodontal ligament-derived mesenchymal stem cell is regarded as a source of adult stem cells due to its multipotency.However, the proof of chondrogenic potential of the cells is scarce.Therefore,we investigated the chondrogenic differentiation capacity of periodontal ligament derived mesenchymal stem cells induced by transforming growth factor(TGF)-p3 and bone morphogenetic protein(BMP)-6.After isolation of periodontal ligament stem cells(PDLSCs) from human periodontal ligament,the cells were cultured in Dulbecco’s modified Eagle’s medium(DMEM) with 20%fetal bovine serum(FBS).A mechanical force initiated chondrogenic differentiation of the cells.For chondrogenic differentiation,10μg·LTGF-β3 or 100μg·LBMP-6 and the combination treating group for synergistic effect of the growth factors.We analyzed the PDLSCs by fluorescence-activated cell sorting and chondrogenesis were evaluated by glycosaminoglycans assay,histology,immunohistochemistry and genetic analysis.PDLSCs showed mesenchymal stem cell properties proved by FACS analysis.Glycosaminoglycans contents were increased 217%by TGF-β3 and 220%by BMP-6. The synergetic effect of TGF-β3 and BMP-6 were shown up to 281%compared to control.The combination treatment increased Sox9, aggrecan and collagen II expression compared with not only controls,but also TGF-P3 or BMP-6 single treatment dramatically.The histological analysis also indicated the chondrogenic differentiation of PDLSCs in our conditions.The results of the present study demonstrate the potential of the dental stem cell as a valuable cell source for chondrogenesis,which may be applicable for regeneration of cartilage and bone fracture in the field of cell therapy.

EDIL3 depletion suppress epithelial-mesenchymal transition of lens epithelial cells via transforming growth factor β pathway

AIM： To study the effect of discoidin I-like domaincontaining protein 3（EDIL3） depletion on the proliferation and epithelial-mesenchymal transition（EMT） in human lens epithelial cells（LECs）. METHODS： RNA interference was used to inhibit the expression of EDIL3 in human LECs in vitro. The morphology of cells was observed using an inverted microscope. Cell proliferation was assessed using Ed U kit. Cell migration was investigated using Transwell chamber and EMT of LECs was assessed using confocal microscope and Western blotting. The transforming growth factor β（TGFβ） pathway was investigated using Western blotting. RESULTS： The data showed that silencing EDIL3 expression changed LECs morphology and suppressed LECs proliferation（P〈0.05） and migration（P〈0.01）. Furthermore, the result of Western blotting showed that EDIL3 depletion reduced the expression of α-smooth muscle actin（α-SMA）（P〈0.001） and vimentin（P〈0.01）, while increased the expression of E-cadherin（P〈0.001）. EDIL3 depletion could suppress the phosphorylation of Smad2（P〈0.01） and Smad3（P〈0.01） and the activation of exracellular signal regulated kinase（ERK）（P〈0.05）. CONCLUSION： The findings indicate that EDIL3 might participate in the proliferation and EMT in LECs via TGFβ pathway and may be a potential therapeutic target for the treatment of posterior capsule opacification.

Epigallocatechin-3-gallate suppresses transforming growth factor-beta signaling by interacting with the transforming growth factor-beta typeⅡreceptor

AIM: To investigate the(-)-epigallocatechin-3-gallate(EGCG) binding to transforming growth factor-β(TGF-β) type Ⅱ receptor(TGFRⅡ).METHODS: The expression of α-smooth muscle actin(α-SMA) was used as a marker for fibrotic change inhuman lung fibroblast MRC-5 cells. The α-SMA expression level was determined by western blotting and immunohistological analysis. We examined whether the anti-fibrotic effects of EGCG on MRC-5 cells was dependent on antioxidant mechanism by using edaravone and N-acetylcysteine(NAC). The suppression effects of EGCG on Smad2/3 activation were studied by confocal fluorescence microscopy. The binding of EGCG to recombinant TGFRⅡ protein was analyzed by immunoprecipitation and affinity chromatography.RESULTS: When MRC-5 cells were treated with TGF-β, EGCG decreased the expression of α-SMA in a dose dependent manner, whereas catechin did not influence the α-SMA expression in the cells. Except for EGCG, antioxidant compounds(e.g., edaravone and NAC) had no effects on the TGF-β-induced α-SMA expression. Nuclear localization of phosphorylated Smad2/3 was observed after TGF-β treatment; however, EGCG treatment attenuated the nuclear transportation of Smad2/3 in the presence or absence of TGF-β. After a TGFRⅡ expression vector was introduced into COS-7 cells, cell lysates were untreated or treated with EGCG or catechin. The immunoprecipitation experiments using the lysates showed that EGCG dose-dependently bound to TGFRⅡ and that catechin did not at all. Affinity chromatography study indicated that EGCG would bind to TGFRⅡ.CONCLUSION: Our results demonstrate that EGCG interacts with TGFRⅡ and inhibits the expression of α-SMA via the TGF-β-Smad2/3 pathway in human lung fibroblast MRC-5 cells.

T-cell immunoglobulin mucin molecule-3, transformation growth factor β, and chemokine-12 and the prognostic status of diffuse large B-cell lymphoma

BACKGROUND The effects of T-cell immunoglobulin mucin molecule-3(Tim-3),transforming growth factor β(TGF-β),and chemokine-12(CXCL12) expression on the prognosis of patients with diffuse large B-cell lymphoma(DLBCL) have not been elucidated.AIM To examine the correlation between Tim-3,TGF-β and CXCL12 expression and DLBCL prognosis.METHODS Lymph node tissues of 97 patients with DLBCL and 93 normal-response hyperplastic lymph node tissues treated from January 2017 to May 2019 were selected as the DLBCL and control groups,respectively.The expression of Tim-3,TGF-β,and CXCL12 was detected immunohistochemically.Patients were followed up for 3 years,and progression-free survival was recorded.Cox mult-ifactorial analysis was performed to analyze the risk factors for poor prognosis.RESULTS The positive expression rates of Tim-3,TGF-β,and CXCL12 were higher in DLBCL tissues than in non-cancerous(control) tissues(P < 0.05).One-year postsurgery,the positive expression rates of Tim-3,TGF-β,and CXCL12 were higher in patients with effective treatment than in those with ineffective treatment(P < 0.05).The 3-year progression-free survival of 97 patients with DLBCL was 67.01%(65/97).Univariate analysis revealed that clinical stage,bone marrow infiltration,International Prognostic Index(IPI) score,Tim-3 positivity,TGF-β positivity,and CXCL12 positivity were associated with poor prognosis(P < 0.05).Multivariate Cox regression analysis demonstrated that clinical stage Ⅲ–Ⅳ,bone marrow infiltration,mediate-to-high-risk IPI scores,Tim-3 positivity,TGF-β positivity,and CXCL12 positivity were independent risk factors affecting prognosis(P < 0.05).CONCLUSION DLBCL tissues exhibit high positive expression of Tim-3,TGF-β,and CXCL12,and a high expression of all three indicates a poor prognosis.

入院时血清TGF-β1、Smad2、Smad3、HA、LN、PCⅢ、CⅣ水平与CHB肝纤维化严重程度的相关性及对疾病预后的预测价值

目的探讨入院时血清转化生长因子-β1(TGF-β1)、Smad同源蛋白2(Smad2)、Smad同源蛋白3(Smad3)及透明质酸(HA)、Ⅲ型前胶原(PCⅢ)、层黏连蛋白(LN)、Ⅳ型胶原(CⅣ)水平与慢性乙型肝炎(CHB)肝纤维化严重程度的相关性及联合检测对疾病预后的预测价值。方法选取河南省中医院2021年3月至2022年3月收治的78例CHB肝纤维化患者作为研究组,选择同期78名健康体检者作为对照组。比较研究组和对照组及不同肝纤维化分期、不同炎症活动分级CHB肝纤维化患者入院时血清TGF-β1、Smad2、Smad3、HA、PCⅢ、LN、CⅣ水平;分析入院时血清TGF-β1、Smad2、Smad3、HA、PCⅢ、LN、CⅣ水平与肝纤维化分期、炎症活动分级的相关性。CHB肝纤维化患者治疗3个月后,根据患者预后分为预后良好和预后不良亚组,比较预后良好和预后不良患者入院时血清TGF-β1、Smad2、Smad3、HA、PCⅢ、LN、CⅣ水平;分析入院时血清TGF-β1、Smad2、Smad3、HA、PCⅢ、LN、CⅣ水平联合检测对CHB肝纤维化患者预后不良的预测价值。结果研究组入院时血清TGF-β1、Smad2、Smad3、HA、LN、PCⅢ、CⅣ高于对照组(P<0.05);不同肝纤维化分期、炎症活动分级CHB肝纤维化患者入院时血清TGF-β1、Smad2、Smad3、HA、LN、PCⅢ、CⅣ比较:S1<S2<S3<S4、G1<G2<G3<G4,差异有统计学意义(P<0.05);入院时血清TGF-β1、Smad2、Smad3、HA、LN、PCⅢ、CⅣ水平与肝纤维化分期、炎症活动分级均呈正相关(P<0.05)。预后良好患者入院时血清TGF-β1、Smad2、Smad3、HA、LN、PCⅢ、CⅣ水平均低于预后不良患者(P<0.05);入院时血清TGF-β1、Smad2、Smad3、HA、LN、PCⅢ、CⅣ水平联合预测肝纤维化患者预后不良的曲线下面积(AUC)优于各指标单一检测(P<0.05)。结论CHB肝纤维化患者入院时血清TGF-β1、Smad2、Smad3、HA、PCⅢ、LN、CⅣ水平均呈现高表达,且与肝纤维化分期、炎症活动分级密切相关,其联合检测对CHB肝纤维化患者预后有较高的预测价值,可用于评估CHB肝纤维化患者病情严重程度和预后,为制定针对性治疗措施提供参考。

除风益损汤对兔角膜损伤后瘢痕形成及TGF-β1、Smad3、α-SMA蛋白表达的影响

目的探讨除风益损汤对兔角膜损伤后瘢痕形成及转化生长因子-β1(ransforming growth factor-beta 1,TGF-β1)、果蝇母本抗生存因子蛋白3(small mothers against decapentaplegic 3,Smad3)、α-平滑肌肌动蛋白(α-smooth muscle actin,α-SMA)蛋白表达的影响。方法取健康月龄新西兰兔48只,按随机数字法将其分成4组,每组12只,设为空白组、模型组、除风益损汤组(以下简称中药组)、重组牛碱成纤维细胞生长因子滴眼组(以下简称贝复舒组);中药组予除风益损汤灌胃,1次/d,空白组、模型组、贝复舒组予等体积生理盐水灌胃,1次/d,贝复舒组予重组牛碱成纤维细胞生长因子滴眼液滴眼,3次/d;建模后各组于7、14、28 d在高倍显微镜下观察角膜损伤修复情况,共聚焦激光断层扫描观察角膜细胞,Masson染色观察角膜组织病理改变,Western blot检测角膜组织中TGF-β1、Smad3、α-SMA蛋白表达。结果眼前节拍照:可见兔角膜7、14、28 d时中药组、贝复舒组角膜损面积伤较模型组角膜损伤面积明显减小。共聚焦激光断层扫描角膜浅层细胞:在造模后28 d,模型组呈现出大量瘢痕组织,同时存在肌成纤维细胞;中药组和贝复舒组可见成纤维细胞及角膜基质细胞,以及极少量瘢痕组织。角膜混浊度分级:与空白组比较,模型组在造模后7、14、28 d的角膜混浊分级均明显升高(P<0.01),呈时间相关性,但28 d时模型组的角膜混浊分级出现回落,与模型组相比,中药组和贝复舒组在造模后7、14、28 d的角膜混浊分级均明显降低(P<0.01),且呈时间相关性(P<0.01)。Masson切片染色:在造模后28 d,空白组可见角膜上皮整齐连续排列,基质层纤维排列整齐,染色致密,厚度均一;模型组伤口处角膜上皮细胞不连续分布,且角膜前部基质浅蓝色胶原纤维排列紊乱,呈不连续状态,厚度不一,角膜后部基质浅蓝色胶原纤维排列较混乱,呈紊乱纤维束;中药组可见角膜前部基质浅蓝色胶原纤维较模型组排列有序,稍疏松,呈连续状态,角膜后部基质浅蓝色胶原纤维排列有序;贝复舒组见角膜前部基质浅蓝色胶原纤维较模型组排列有序,稍疏松,呈连续状态,仍存在纤维束,角膜后部基质浅蓝色胶原纤维排列有序。Western blot检测:与模型组比较,中药组、贝复舒组的角膜组织中TGF-β1、Smad3、α-SMA蛋白表达在7、14、28 d时均显著降低(P<0.05)。结论除风益损汤能促进角膜损伤修复,抑制角膜瘢痕化,并对TGF-β1、Smad3、α-SMA蛋白产生影响。

雷火灸、穴位贴敷治疗慢性肾脏病3~4期的疗效及对血清TGF-β1、Klotho、FGF23水平的影响

目的:研究雷火灸、穴位贴敷治疗慢性肾脏病3~4期的疗效及对血清转化生长因子-β1(TGF-β1)、Klotho蛋白(Klotho)、成纤维生长因子23(FGF23)水平的影响。方法:2022年1月~2023年1月我院收治的慢性肾脏病3~4期患者92例,分为对照组与试验组,各46例,方法为随机数字表法。对照组予以常规西医治疗,试验组在对照组的基础上予以雷火灸、穴位贴敷治疗,两组均治疗2周。比较两组治疗2周后疗效,治疗前、治疗2周后血清TGF-β1、Klotho、FGF23水平、肾功能、免疫功能,治疗期间不良反应发生情况。结果:与对照组治疗2周后的总有效率(71.74%)比较,试验组总有效率更高(91.30%,P<0.05)。较治疗前,治疗2周后两组血清TGF-β1、FGF23、尿素氮(BUN)、血肌酐(Scr)水平,全血辅助性T细胞17(Th17)水平,24h尿蛋白定量降低,且试验组更低(P<0.05)。较治疗前,治疗2周后两组全血调节性T细胞(Treg)水平,血清免疫球蛋白G(IgG)、免疫球蛋白A(IgA)、免疫球蛋白M(IgM)、Klotho水平升高,且试验组更高(P<0.05)。治疗期间,两组不良反应发生率接近,均未影响继续治疗(P>0.05)。结论:雷火灸、穴位贴敷治疗慢性肾脏病3~4期的疗效较好,可改善肾功能、免疫功能,调节血清TGF-β1、Klotho、FGF23水平表达,降低肾脏损伤,安全性良好。

3-甲基腺嘌呤对转化生长因子-β诱导大鼠肝脏星形细胞株HSC-T6活化及自噬的影响观察

目的观察3-甲基腺嘌呤(3-MA)对转化生长因子-β(TGF-β)诱导的大鼠肝星形细胞株HSC-T6活化及自噬的影响。方法取对数生长期的HSC-T6细胞分为空白组、TGF-β+PBS组、TGF-β+3-MA组。TGF-β+3-MA组细胞加入浓度为2 ng/mL TGF-β培养72 h后加入3-MA(0.5 mg/mL)处理24 h,TGF-β+PBS组细胞加入浓度为2 ng/mL TGF-β培养72 h后加入等量PBS处理24 h,空白组加入等量PBS处理,采用实时荧光定量PCR法检测各组细胞活化标志物α-SMA、TGF-βmRNA和自噬标志物LC3、Beclin-1、Atg5 mRNA,采用Western blotting法检测各组细胞活化标志物α-SMA、TGF-β蛋白和自噬标志物LC3、Beclin-1、Atg5蛋白。结果TGF-β+PBS组、TGF-β+3-MA组细胞活化标志物α-SMA、TGF-βmRNA和蛋白均高于空白组,且TGF-β+3-MA组均低于TGF-β+PBS组(P均<0.05)。TGF-β+PBS组、TGF-β+3-MA组细胞自噬标志物LC3、Beclin-1、Atg5 mRNA和蛋白均高于空白组,且TGF-β+3-MA组均低于TGF-β+PBS组(P均<0.05)。结论3-MA可抑制TGF-β诱导的大鼠肝星形细胞株HSC-T6活化及自噬。

微RNA-196a-1-3p靶向Ras响应元件结合蛋白调控胆管癌细胞增殖的机制研究

目的探讨转化生长因子β(TGF-β)调控人胆管癌细胞系RBE细胞增殖的关键微RNA(miRNA)及其潜在的机制。方法该研究起止时间为2020年1月至2022年1月。磷酸盐缓冲液(PBS)处理为对照组,TGF-β处理为TGF-β组,TGF-β抗体处理为抗体组。检测三组RBE细胞的增殖水平。miRNA高通量测序检测三组RBE细胞的miRNA调控变化,并进行miRNA模拟物过表达筛选鉴定受TGF-β调控的影响RBE细胞增殖水平的关键miRNA。miRNA数据库(miRDB)在线分析miRNA的潜在底物,并通过小干扰RNA(siRNA)敲低筛选鉴定影响RBE细胞增殖水平的关键底物。结果相比于对照组,TGF-β组RBE细胞的增殖水平上升(1.62±0.07比2.35±0.09,P<0.05),抗体组RBE细胞的增殖水平下降(1.62±0.07比1.11±0.08,P<0.05)。过表达微RNA-196a-1-3p(miR-196a-1-3p)时,RBE细胞的增殖水平下降(P<0.05)。敲低Ras响应元件结合蛋白(RREB1)时,RBE细胞的增殖水平下降(P<0.05)。过表达miR-196a-1-3p后,RBE细胞中RREB1的信使RNA(mRNA)和蛋白水平下降(P<0.05)。敲低miR-196a-1-3p后,RBE细胞中RREB1与SMAD家族蛋白3(SMAD3)的相互作用增加。敲低SMAD3后,RBE细胞的增殖水平下降(P<0.05)。与仅敲低SMAD3相比,敲低SMAD3的同时过表达RREB1的RBE细胞的增殖水平无显著变化,并且同时敲低SMAD3和miR-196a-1-3p的RBE细胞的增殖水平无显著变化。结论TGF-β能够通过miR-196a-1-3p/RREB1/SMAD3轴促进RBE细胞增殖;miR-196a-1-3p和RREB1可作为潜在的治疗胆管癌的靶标,为针对该靶标的新药研发奠定了基础。

Flt3L、TGF-β1及EGFR与急性髓系白血病患者不良预后的关系

目的探究FMS样酪氨酸激酶3配体(Flt3L)、转化生长因子β1(TGF-β1)及表皮生长因子受体(EGFR)与急性髓系白血病(AML)患者不良预后的关系。方法选取120例首次确诊AML患者作为观察组,募集同期体检的100例健康志愿者为对照组,比较2组的Flt3L、TGF-β1及EGFR水平。观察组患者出院后随访3~12个月,根据预后情况将患者分为良好组(86例)和不良组(34例),比较2组的临床资料,采用COX模型分析上述指标与患者不良预后的关系,采用受试者工作特征(ROC)曲线探究上述指标对AML患者不良预后的预测效能。结果观察组Flt3L、TGF-β1水平低于对照组,EGFR水平高于对照组,差异有统计学意义(P<0.05)。不同预后AML患者的Flt3L、TGF-β1及EGFR水平比较差异有统计学意义(P<0.05);COX模型分析显示Flt3L、TGF-β1及EGFR水平为AML患者预后不良的独立影响因素(P<0.05)。经ROC曲线分析显示,Flt3L、TGF-β1及EGFR水平预测AML患者预后不良的AUC为0.874、0.838、0.858。结论Flt3L、TGF-β1及EGFR与AML患者不良预后相关。

CONSTRUCTING ADENO-ASSOCIATED VIRUS-TGFβ_3 AND COMPARING ITS BIOLOGICAL EFFECT ON PROTEOGLYCAN SYNTHESIS IN DEDIFFERENTIATED NUCLEUS PULPOUS CELLS WITH ADENOVIRUS-TGFβ_1

Objective To construct adeno-associated virus (AAV) expression system for transforming growth factor β3 (TGFβ3) and detect its biological effect on proteoglycan synthesis of the earlier and later dedifferentiated rabbit lumbar disc nucleus pulpous (NP) cells, which was compared with that of adenovirus (AV) expression system for TGFβ1. Methods TGFβ3 gene was obtained using PCR. Its upstream contained restriction enzyme site Kpn Ⅰ, and its downstream contained restriction enzyme site SalⅠ. Using the restriction enzyme sites of PCR product of TGFβ3 and the corresponding multiple cloning site (MCS) in plasmid AAV, TGFβ3 was subcloned into AAV. The recombinant plasmid AAV-TGFβ3 was transfected into H293 cells with LipofectamineTM 2000, and the expression of TGFβ3 gene was detected using immunofluorescent analysis. After AAV-TGFβ3 virus particle with infectious activity was packaged, TGFβ3 expression in NP cells was detected by immunoblotting, and its biological effect on proteoglycan synthesis was detected by antonopulos method and compared with that of AV-TGFβ1 in the earlier and later dedifferentiated NP cells. Results For the earlier dedifferentiated NP cells, AAV-TGFβ3 slowly and stably enhanced proteoglycan synthesis, but AV-TGFβ1 rapidly and transiently enhanced its synthesis. For the later dedifferentiated NP cells, AAV-TGFβ3 stably enhanced proteoglycan synthesis, but AV-TGFβ1 inhibited its synthesis. Conclusion AAV expression system can mediate TGFβ3 gene to be expressed stably, and AAV-TGFβ3 can enhance proteoglycan synthesis of the earlier and later dedifferentiated NP cells.

基于TGF-β1/Smad2/3信号通路探讨茴香胶囊抗支气管哮喘作用及机制

目的探讨茴香胶囊抗支气管哮喘作用及潜在机制。方法采用环磷酰胺腹腔注射法建立小鼠免疫低下模型评价茴香胶囊免疫增强作用;采用浓氨水引咳法及酚红排泄法评价茴香胶囊止咳祛痰活性;采用卵清蛋白致敏和激发方式构建支气管哮喘小鼠模型,实验过程中观察并记录小鼠体重及行为学变化;检测小鼠肺泡灌洗液(BALF)中炎症细胞计数;ELISA法检测免疫球蛋白E(IgE)、γ-干扰素(IFN-γ)、白细胞介素-4(IL-4)、白细胞介素-17A(IL^(-1)7A)、转化生长因子-β1(TGF-β1)水平;HE和Masson染色观察肺组织病理学变化;RT-qPCR、Western blot检测TGF-β1/Smad2/3通路相关蛋白表达。结果茴香胶囊可增强免疫低下小鼠的免疫功能,延长小鼠咳嗽潜伏期,减少小鼠咳嗽次数,增加小鼠气管酚红排泌量,降低支气管哮喘小鼠BALF中白细胞等炎性细胞数量,降低IgE、IL-4、IL^(-1)7A、TGF-β1水平,增加IFN-γ水平,减轻小鼠肺组织病理学变化;下调TGF-β1/Smad2/3通路相关蛋白表达。结论茴香胶囊可能通过增强机体免疫力、止咳祛痰缓解支气管哮喘小鼠哮喘症状,调节Th1/Th2失衡、降低肺组织中炎症因子水平、下调TGF-β1/Smad2/3信号通路减少气道炎症及气道重塑。

右美托咪定通过调控白细胞介素-17及转化生长因子-β1/Smad蛋白3信号通路对脂多糖诱导Ⅱ型肺泡上皮细胞损伤的影响

目的探讨右美托咪定介导白细胞介素(IL)-17对脂多糖(LPS)诱导的人Ⅱ型肺泡上皮A549细胞(以下简称“A549细胞”)炎症、增殖、迁移、上皮间质转化及转化生长因子-β1(TGF-β1)/Smad蛋白3(Smad3)信号通路的调控作用。方法体外培养A549细胞,将其分为对照组(不做干预)、LPS组(10.00μg/ml LPS)和实验组(10.00μg/ml LPS+1.25、2.50、5.00、10.00μg/ml右美托咪定),分别采用CCK-8试剂盒和反转录-聚合酶链反应(RT-qPCR)法测定细胞活力和IL-17 mRNA表达水平以筛选右美托咪定最适实验浓度;随后将细胞分为对照组、LPS组、IL-17组、右美托咪定组和IL-17+右美托咪定组,干预24 h。酶联免疫吸附试验(ELISA)检测炎症因子IL-17、IL-8和IL-6的表达水平;5-乙炔基-2'脱氧尿嘧啶核苷(EdU)试剂盒用来检测细胞增殖率;划痕实验用来检测细胞迁移率;蛋白免疫印迹(WB)法测定肺泡上皮间质转化(EMT)相关蛋白、TGF-β1/Smad3通路相关蛋白及IL-17蛋白表达水平。结果右美托咪定逆转了LPS对A549细胞活力的抑制作用和IL-17 mRNA表达水平的促进作用,且10.00μg/ml浓度的右美托咪定组的效果最好,因此选择10.00μg/ml右美托咪定用于后续实验。LPS组细胞中IL-17、IL-8、IL-6表达水平、细胞迁移率、N-钙黏蛋白、波形蛋白、纤维粘连蛋白(FN)、Smad3的磷酸化(p-Smad3)/Smad3、TGF-β1和IL-17蛋白表达水平高于对照组,差异有统计学意义(P<0.05);LPS组细胞增殖率、E-钙黏蛋白和Smad7蛋白表达水平低于对照组,差异有统计学意义(P<0.05)。IL-17+右美托咪定组IL-17、IL-8、IL-6表达水平、细胞迁移率、N-钙黏蛋白、波形蛋白、FN、p-Smad3/Smad3、TGF-β1和IL-17蛋白表达水平低于LPS组,差异有统计学意义(P<0.05);IL-17+右美托咪定组细胞增殖率、E-钙黏蛋白和Smad7蛋白表达水平高于LPS组,差异有统计学意义(P<0.05)。结论右美托咪定通过抑制IL-17的分泌恢复LPS诱导的人Ⅱ型肺泡上皮细胞损伤,促进LPS诱导的人Ⅱ型肺泡上皮细胞增殖并抑制其迁移和EMT进程,其作用机制与抑制TGF-β1/Smad3通路的信号转导有关。

血清CTRP9、TGF-β2、ANGPTL3水平与糖尿病视网膜病变的相关性分析及临床意义

目的探讨血清C1q肿瘤坏死因子相关蛋白9(CTRP9)、转化生长因子-β2(TGF-β2)、血管生成素样蛋白3(ANGPTL3)水平与糖尿病视网膜病变(DR)的相关性及临床意义。方法回顾性选取2021年9月至2023年9月医院收治的100例DR患者,其中增殖性视网膜病变(PDR)39例,非增殖性视网膜病变(NPDR)61例,分别纳入PDR组、NPDR组,另选取同期糖尿病不伴有视网膜病变患者50例,纳入对照组。比较3组血清CTRP9、TGF-β2、ANGPTL3水平,分析血清各指标与DR病情严重程度的相关性及联合检测诊断价值,并分析各指标不同水平患者发生DR的危险度。结果3组血清CTRP9、TGF-β2、ANGPTL3水平比较:PDR组>NPDR组>对照组,且各指标水平与DR病情严重程度均呈正相关(P<0.05)。入院时血清CTRP9、TGF-β2、ANGPTL3水平联合诊断DR的曲线下面积为0.899,最佳诊断敏感度为91.00%,最佳诊断特异度为88.00%,约登指数为0.790,且各指标高水平患者发生DR的危险度是低水平的1.419倍、1.239倍、1.381倍(P<0.05)。结论CTRP9、TGF-β2、ANGPTL3在DR患者血清中均呈异常高表达,各指标水平与病情严重程度均呈正相关,且联合检测对DR具有一定诊断价值,可作为临床诊断疾病、评估病情的辅助指标。

TGF-β1及其信号转导蛋白Smad23在去卵巢大鼠骨组织中的表达及意义

目的观察转化生长因子β1(TGFβ1)及其信号转导蛋白Smad23在去卵巢大鼠骨组织中的表达及意义。方法手术切除大鼠双侧卵巢。术后13周,取离体胫骨测量组织学参数髓腔面积百分率(%Ma.Ar)、骨小梁厚度(Tb.Th),用逆转录多聚酶链反应(RTPCR)检测大鼠骨组织TGFβ1mRNA的表达,用免疫组化法检测Smad23蛋白在骨组织中的定位,用Westernblot杂交法检测骨组织TGFβ1、Smad23蛋白表达。结果与对照组(Sham组)比较,模型大鼠(OVX组)骨组织Tb.Th缩小,%Ma.Ar明显增大,差异有显著性(P<0.01);OVX组TGFβ1的mRNA、蛋白及Smad23蛋白表达水平显著降低(P<0.01),Smad23蛋白广泛表达于骨组织干骺端,主要表达于骨基质表面及骨小梁周围的成骨细胞。结论TGFβ1及其信号转导蛋白Smad23可能在绝经后骨质疏松症中起重要调节作用。

脉冲染料激光对体外瘢痕成纤维细胞中TGF-β1和TGF-β3表达的影响

目的探讨不同能量脉冲染料激光(Pulsed dye laser,PDL)对体外人瘢痕成纤维细胞转化生长因子(TGF)-β1和TGF-β3表达的影响。方法按组织块法体外培养人瘢痕成纤维细胞,分别用4、6、8、10、11、12 J/cm2能量的PDL照射细胞,观察不同能量PDL对细胞周期的影响,酶联免疫吸附测定(ELLSA)法检测激光照射后TGF-β1、TGF-β3的分泌量。结果 PDL照射后,处于G1期的瘢痕成纤维细胞较对照组明显增多;不同能量PDL照射瘢痕成纤维细胞后,TGF-β1的分泌量随激光能量密度的升高而降低,TGF-β3的分泌量则增加,差异有统计学意义。结论 PDL对瘢痕的治疗作用可能与抑制细胞增殖,减少瘢痕成纤维细胞TGF-β1分泌,增加TGF-β3的分泌有关。

2型糖尿病性动脉粥样硬化大鼠血浆VEGF、TGF-β1、CTRP3的表达及辛伐他汀的干预作用

目的观察2型糖尿病性动脉粥样硬化大鼠血浆血管内皮生长因子(VEGF)、转化生长因子β1(TGF-β1)、C1q/TNF相关蛋白3(CTRP3)的表达及辛伐他汀的干预作用。方法将SD大鼠随机分为正常饮食(NC)组(n=8)、高脂饮食(HFD)组(n=8)、高脂干预(HFD+S)组(n=8)、模型(M)组(n=18)、模型干预(M+S)组(n=16)。采用链脲佐菌素+维生素D3+高脂饮食建立糖尿病动脉粥样硬化大鼠模型,HFD+S、M+S组用辛伐他汀溶液20 mg/(kg·d)灌胃进行干预,蒸馏水20 m L/(kg·d)灌胃作为对照。测定各组大鼠空腹血糖(FPG)、血脂、空腹胰岛素(FINS)、VEGF、TGF-β1、CTRP3的水平。结果 M组动脉病理可见明显粥样斑块,M+S组病变较M组明显减轻。HFD组VEGF、TGF-β1及CTRP3高于NC组;M组VEGF、TGF-β1高于NC组,VEGF高于HFD组,CTRP3低于HFD组。辛伐他汀干预后,HFD+S组TGF-β1、CTRP3高于HFD组,M+S组VEGF低于M组,且TGF-β1、CTRP3均高于M组(P<0.05)。结论 VEGF、TGF-β1、CTRP3可能参与糖尿病性动脉粥样硬化的发生,辛伐他汀除降脂外,还能下调VEGF、上调TGF-β1、CTRP3表达,并对糖尿病性动脉粥样硬化发挥保护作用。

焦亚硫酸钠对雄性小鼠肝脏Caspase-3和转化生长因子β_1表达的影响

目的研究焦亚硫酸钠对小鼠肝脏中半胱氨酸天门冬氨酸特异性蛋白酶(Caspase-3)、转化生长因子β1(TGF-β1)表达的影响。方法健康雄性昆明小鼠30只随机分为对照组10只和实验组20只,对照组小鼠给予静置自来水饮用;实验组小鼠给予10g.L-1焦亚硫酸钠溶液饮用。分别于第10天和第30天时处死各组小鼠,快速取出肝脏,Zamboni固定液固定,常规冰冻制片,免疫组织化学染色,光镜观察。结果与对照组比较,实验组小鼠肝脏中Caspase-3阳性表达增强(P<0.01),第10天时实验组变化尤为明显;而实验组小鼠肝脏中TGF-β1阳性表达与对照组比较无显著差异(P>0.05)。结论焦亚硫酸钠喂食后可引起小鼠肝脏中Caspase-3表达增高,TGF-β1无明显改变,提示焦亚硫酸钠促使小鼠肝脏中肝细胞凋亡增加。

尿毒清颗粒对糖尿病肾病大鼠肾脏抗炎抗氧化保护作用及对TGF-β_1/p38MAPK信号通路影响的研究

目的探讨尿毒清胶囊对糖尿病肾病大鼠的抗炎、抗氧化作用及对糖尿病肾病大鼠肾组织TGF-β_1/p38MAPK信号通路的影响。方法 70只雄性SD大鼠,随机分为10只正常组,60只模型组。模型组大鼠腹腔注射45 mg·kg^(-1)链脲佐菌素(STZ)造模,取造模成功的60只大鼠随机分为12只模型组,12只厄贝沙坦阳性组,12只尿毒清颗粒低剂量组(0.04 mg·kg^(-1)),12只尿毒清颗粒中剂量组(0.08 mg·kg^(-1)),12只尿毒清颗粒高剂量(0.16 mg·kg^(-1)),灌胃给药12周,模型组和空白组给予生理盐水。每周称量体质量,每周检测24 h尿蛋白量。给药治疗12周后,取血检测血尿素氮(BUN)、血清肌酐(SCr)、丙二醛(MDA)、一氧化氮(NO)、甘油三酯(TG)、超氧化物歧化酶(SOD)含量;麻醉处死大鼠,各取8只对肾组织行HE染色,观察肾组织的病理形态;并取肾组织进行RT-PCR和免疫组化观察TGF-β_1/p38MAPK信号转导等转化因子的mRNA及蛋白表达。结果与正常组比较,模型组大鼠尿蛋白及血清BUN、SCr、TG、MDA含量显著增高(P<0.05),NO、SOD含量显著降低(P<0.01),肾组织胞浆中TGF-β_1、p38MAPK、Caspase-3 mRNA及蛋白表达显著升高(P<0.05);通过治疗后,与模型组对比,尿毒清颗粒高剂量组和阳性组肾脏病理损害明显减轻,尿蛋白及血清BUN、SCr、TG、MDA含量显著降低(P<0.05),NO、SOD含量明显增高(P<0.05),肾组织内TGF-β_1、p38MAPK、Caspase-3 m RNA及蛋白表达明显减少(P<0.05)。结论尿毒清颗粒能降低24 h尿蛋白量,降低TG和MDA含量及升高NO、SOD含量,通过调控TGF-β_1/p38MAPK从而治疗糖尿病肾病的肾组织受损部位,改善肾功能和减轻病理损伤,能有效地保护糖尿病肾病组织。