Hsa_circRNA_102610 upregulation in Crohn’s disease promotes transforming growth factor-β1-induced epithelial-mesenchymal transition via sponging of hsa-miR-130a-3p

BACKGROUND The incidence of inflammatory bowel disease,a chronic intestinal inflammatory disorder that includes Crohn’s disease(CD)and ulcerative colitis,is rising.Circular RNAs are considered valuable diagnostic biomarkers for CD.Current evidence supports the views that epithelial-mesenchymal transition(EMT)plays an important role in CD pathogenesis,and that hsa-miR-130a-3p can inhibit transforming growth factor-β1(TGF-β1)-induced EMT.Our previous study revealed that hsa_circRNA_102610 was upregulated in CD patients.Moreover,we predicted an interaction between hsa_circRNA_102610 and hsa-miR-130a-3p.Thus,we hypothesized that hsa_circRNA_102610 may play roles in the proliferation and EMT of intestinal epithelial cells by sponging hsa-miR-130a-3p to participate in the pathogenesis of CD.AIM To explore the mechanism of hsa_circRNA_102610 in the pathogenesis of CD.METHODS The relative expression levels of hsa_circRNA_102610 and hsa-miR-130a-3p in patients were detected by quantitative reverse transcription-polymerase chain reaction.The proliferation of human intestinal epithelial cells(HIECs)and normal-derived colon mucosa cell line 460(NCM460)cells was detected by cell counting kit-8,5-ethynyl-2’-deoxyuridine staining and cell cycle assays following overexpression or downregulation of hsa_circRNA_102610.Cell proliferation assays were performed as described above in a rescue experiment with hsa-miR-130a-3p mimics.The interaction of hsa_circRNA_102610 and hsa-miR-130a-3p was verified by fluorescence in situ hybridization and dual luciferase reporter assays.The relative expression levels of CyclinD1,mothers against decapentaplegic homolog 4(SMAD4),E-cadherin,N-cadherin and Vimentin were detected by western blotting following hsa_circRNA_102610 overexpression,TGF-β1-induced EMT or hsa-miR-130a-3p mimic transfection(in rescue experiments).RESULTS Upregulation of hsa_circRNA_102610 was determined to be positively correlated with elevated fecal calprotectin levels in CD(r=0.359,P=0.007)by Pearson correlation analysis.Hsa_circRNA_102610 promoted the proliferation of HIECs and NCM460 cells,while hsa-miR-130a-3p reversed the cell proliferationpromoting effects of hsa_circRNA_102610.Fluorescence in situ hybridization and dual luciferase reporter assays showed that hsa_circRNA_102610 directly bound hsa-miR-130a-3p in NCM460 and 293T cells.An inverse correlation between downregulation of hsa-miR-130a-3p and upregulation of hsa_circRNA_102610 in CD patients was observed(r=-0.290,P=0.024)by Pearson correlation analysis.Moreover,overexpression of hsa_circRNA_102610 promoted SMAD4 and CyclinD1 protein expression validated by western-blotting.Furthermore,overexpression of hsa_circRNA_102610 promoted TGF-β1 induced EMT in HIECs and NCM460 cells via targeting of hsa-miR-130a-3p,with increased expression of Vimentin and N-cadherin and decreased expression of E-cadherin.CONCLUSION Hsa_circRNA_102610 upregulation in CD patients could promote the proliferation and EMT of intestinal epithelial cells via sponging of hsa-miR-130a-3p.

Multiple roles of mothers against decapentaplegic homolog 4 in tumorigenesis, stem cells, drug resistance, and cancer therapy

The transforming growth factor(TGF)-βsignaling pathway controls many cellular processes,including proliferation,differentiation,and apoptosis.Abnormalities in the TGF-βsignaling pathway and its components are closely related to the occurrence of many human diseases,including cancer.Mothers against decapentaplegic homolog 4(Smad4),also known as deleted in pancreatic cancer locus 4,is a typical tumor suppressor candidate gene locating at q21.1 of human chromosome 18 and the common mediator of the TGF-β/Smad and bone morphogenetic protein/Smad signaling pathways.It is believed that Smad4 inactivation correlates with the development of tumors and stem cell fate decisions.Smad4 also interacts with cytokines,miRNAs,and other signaling pathways,jointly regulating cell behavior.However,the regulatory function of Smad4 in tumorigenesis,stem cells,and drug resistance is currently controversial.In addition,Smad4 represents an attractive therapeutic target for cancer.Elucidating the specific role of Smad4 is important for understanding the mechanism of tumorigenesis and cancer treatment.Here,we review the identification and characterization of Smad4,the canonical TGF-β/Smad pathway,as well as the multiple roles of Smad4 in tumorigenesis,stem cells,and drug resistance.Furthermore,we provide novel insights into the prospects of Smad4-targeted cancer therapy and the challenges that it will face in the future.

Regulation of transforming growth factor-β signaling as a therapeutic approach to treating colorectal cancer

According to data from 2020,Slovakia has long been among the top five countries with the highest incidence rate of colorectal cancer(CRC)worldwide,and the rate is continuing to rise every year.In approximately 80%of CRC cases,allelic loss(loss of heterozygosity,LOH)occurs in the long arm of chromosome 18q.The most important genes that can be silenced by 18q LOH or mutations are small mothers against decapentaplegic homolog(SMAD)2 and SMAD4,which are intracellular mediators of transforming growth factor(TGF)-βsuperfamily signals.TGF-βplays an important role in the pro-oncogenic processes,including such properties as invasion,epithelial-mesenchymal transition(commonly known as EMT),promotion of angiogenesis,and immunomodulatory effects.Several recent studies have reported that activation of TGF-βsignaling is related to drug resistance in CRC.Because the mechanisms of drug resistance are different between patients in different stages of CRC,personalized treatment is more effective.Therefore,knowledge of the activation and inhibition of factors that affect the TGF-βsignaling pathway is very important.

褐藻聚合酚下调TGF-β_(1)/Smads信号通路抑制大肠癌细胞增殖与侵袭

目的探讨褐藻聚合酚(PFFE-A)对大肠癌细胞增殖与侵袭的影响,以及其对转化生长因子β_(1)(TGF-β_(1))及母体抗生物皮肤生长因子同源物2/3(Smad2/3)通路的调控作用。方法细胞分组:依次以50、100、150μmol·L-1的小、中、大剂量的PFFE-A干预细胞,另设立正常对照组细胞。5-乙炔基-2'脱氧尿苷(EdU)染色检测细胞的增殖;Transwell小室检测细胞的侵袭能力;异种种植结肠癌裸鼠模型检测细胞的体内生长与转移能力;实时荧光定量聚合酶链反应(RT-qPCR)检测细胞中上皮间质转化(EMT)相关基因的表达;Western blotting检测细胞中TGF-β_(1)、p-Smad2/3的表达水平。结果与正常对照组比较,PFFE-A小、中、大剂量组细胞的增殖率、侵袭细胞数、肿瘤瘤体质量、病灶转移比例、神经型钙黏附蛋白(N-cadherin)的mRNA的表达、TGF-β_(1)和p-Smad2/3的表达明显下降(P<0.05),E-钙黏蛋白(E-cadherin)的mRNA的表达明显升高(P<0.05),具有明显的剂量依赖性(P<0.05)。结论PFFE-A能抑制肿瘤细胞的EMT过程,抑制大肠癌细胞HT29的体外增殖与侵袭能力,下调其体内生长与转移的能力,这可能是通过下调TGF-β_(1)/Smads信号实现的。

TGF-β1和Smad2在胃癌中的表达及意义

目的:检测TGF-β1和Smad2信号在胃癌中的表达,探讨TGF-β1和Smad2在胃癌发生、发展中的作用.方法:采用免疫蛋白印迹(Westernblot)和实时定量PCR检测45例胃癌组织及相应正常组织TGF-β1、Smad2蛋白及mRNA的表达,比较正常对照、癌组织中上述二者表达的差异,并进行统计学分析.结果:TGF-β1在胃癌组织中阳性表达率为77.8%(35/45),在正常组织中为33.3%(15/45),二者比较差异显著(P<0.05);Smd2蛋白在胃癌组织中阳性表达率为73.3%(33/45),在正常组织中为26.7%(12/45),二者比较有显著差异(P<0.05);TGF-β1、Smad2mRNA在胃组织中阳性表达率分别为88.9%(40/45)、84.4%(38/45),均显著高于正常组织(P<0.05).胃癌组织中TGF-β1、Smad2蛋白的表达与病理分级、浸润深度、淋巴结转移、脉管侵犯相关(P<0.05).结论:TGF-β1和Smad2可能在胃癌的发生、发展中发挥作用,并与胃癌的侵袭、转移相关.

硬尖神香草提取物对哮喘幼鼠气道重塑的作用机制

目的探讨硬尖神香草提取物通过转化生长因子-β_(1)(transforming growth factor-β_(1),TGF-β_(1))/母亲信号蛋白同源物(Mothers against decapentaplegic homologs,Smads)通路调控上皮-间质转化(epithelial-mesenchymal transformation,EMT)对哮喘幼鼠气道重塑的作用。方法将幼鼠随机分为模型组、硬尖神香草(提取物)低剂量组(25 mg·kg^(-1))和硬尖神香草高剂量组(50 mg·kg^(-1))及阳性药物组(二羟丙茶碱,20 mg·kg^(-1)),各20只,另设对照组。比较支气管肺泡灌洗液(bronchoalveolar lavage fluid,BALF)各类炎症细胞数及细胞因子白细胞介素-4(interleukin-4,IL-4)、基质金属蛋白酶9(matrix metalloproteinase 9,MMP-9)和肿瘤坏死因子-α(tumor necrosis factor-α,TNF-α)的水平,HE染色观察肺组织病变,比较肺组织气道壁、平滑肌厚度,对比E钙黏蛋白(E-cadherin)、α-平滑肌肌动蛋白(α-smooth muscle actin,α-SMA)、TGF-β_(1)、母亲信号蛋白同源物2(Mothers against decapentaplegic homolog 2,Smad2)以及母亲信号蛋白同源物3(Smad3)mRNA与蛋白的表达水平。结果与对照组比较,模型组嗜酸性粒细胞(eosinophil,EOS)、中性粒细胞(neutrophil,NEU)、淋巴细胞(lymphocyte,LYM)细胞数、支气管气道壁、平滑肌厚度、IL-4、TNF-α、MMP-9水平以及α-SMA、TGF-β_(1) mRNA与α-SMA、TGF-β_(1)、p-Smad2和p-Smad3蛋白水平均升高,E-cadherin mRNA与蛋白水平降低(P<0.05);与模型组比较,硬尖神香草低剂量组和高剂量组、阳性药物组的EOS、NEU、LYM细胞数、支气管气道壁、平滑肌厚度、IL-4、TNF-α、MMP-9以及E-cadherin mRNA和蛋白水平均升高,α-SMA、TGF-β_(1) mRNA、α-SMA、TGF-β_(1)、p-Smad2与p-Smad3蛋白水平均降低(P<0.05);且各指标水平变化规律是阳性药物组最明显,硬尖神香草高剂量组次之,硬尖神香草低剂量组最弱(P<0.05);HE结果显示,硬尖神香草低剂量和高剂量组、阳性药物组肺组织支气管气道损伤较模型组出现不同程度改善,硬尖神香草高剂量组和阳性药物组改善明显。结论硬尖神香草提取物能有效抑制哮喘幼鼠气道重塑,可能通过调控TGF-β_(1)/Smads通路调控相关mRNA和蛋白的表达,抑制EMT发挥作用。

二苯乙烯苷对糖尿病大鼠肾脏沉默信息调节因子2同源体和TGF-β_1蛋白的影响

目的探讨二苯乙烯苷(TSG)对糖尿病大鼠肾脏沉默信息调节因子2(SIRT1)和转化生长因子-β1(TGF-β1)蛋白的影响。方法以链脲佐菌素腹腔注射建立糖尿病大鼠模型和高糖刺激大鼠肾系膜细胞株为研究对象,全自动生化分析仪测定生化指标,比色法检测细胞培养液中的超氧化物歧化酶(SOD)和谷胱甘肽(GSH)的活性、丙二醛(MDA)含量的变化,四甲基偶氮唑蓝(MTT)测定肾小球系膜细胞(GMCs)增殖活性,Western印迹检测大鼠肾脏和系膜细胞中SIRT1和TGF-β1蛋白表达。结果糖尿病肾病(DN)组大鼠的24 h尿蛋白定量、肾脏肥大指数、三酰甘油(TG)、总胆固醇(TC)、血尿素氮(BUN)、血肌酐(C r)与对照组比较明显增加(P<0.01),而TSG能明显改善上述指标,并改善大鼠抗氧化应激能力。TSG能明显增加糖尿病大鼠肾脏和高糖环境下系膜细胞SIRT1蛋白表达,并抑制TGF-β1蛋白表达。结论 TSG对DN具有保护作用,其作用机制可能通过提高机体抗氧化应激能力,调节SIRT1活性,并抑制肾脏TGF-β1蛋白表达而减少DN损害。

转化生长因子β1诱导心肌成纤维细胞转分化过程中Hedgehog信号通路的作用机制

背景:近年来越来越多的研究表明Hedghog信号通路异常活化广泛参与全身多组织器官疾病的损伤修复过程,但其在心肌纤维化中的相关作用尚不明确。目的:研究阻断Hedgehog-Gli信号通路对转化生长因子β1诱导的心肌成纤维细胞上皮间质转分化过程的影响。方法:①动物实验:左冠状动脉结扎法建立小鼠心肌梗死模型,苏木精-伊红和Masson染色法观察梗死后3,7,14 d心肌组织的病理改变,用RT-PCR、Western blot和免疫荧光法检测不同时段Gli1 mRNA及蛋白的时空表达,RT-PCR和免疫荧光定量检测加入特异性阻断剂后Gli1的mRNA及蛋白的时空表达变化。②细胞实验:差速贴壁法原代培养SD乳鼠心肌成纤维细胞,采用不同质量浓度(0,1,5,10μg/L)转化生长因子β1刺激心肌成纤维细胞,RT-PCR、Western blot检测Gli1 mRNA及蛋白表达,选用10μg/L的转化生长因子β1诱导心肌成纤维细胞24 h,免疫荧光法检测Gli1蛋白时空表达及上皮间质转分化标记物的表达。分别采用GANT61和Cyclopamine特异性阻断Hedgehog信号通路中的Gli1和Smo 24 h后,加入10μg/L转化生长因子β1,RT-PCR检测Gli1 mRNA表达变化,荧光免疫法检测Gli1的时空表达以及上皮间质转分化标记物的表达变化。结果与结论:①动物实验结果:随着梗死后时间延长,小鼠心肌Gli1的mRNA和蛋白表达水平逐渐升高,而加入Hedgehog通路特异性阻断剂后梗死组织中Gli1的mRNA及蛋白表达均有下降。②细胞实验结果:采用转化生长因子β1刺激后,心肌成纤维细胞上皮间质转化为肌成纤维细胞(特异性标记物a-SMA阳性);随着转化生长因子β1干预剂量增加,Gli1的mRNA及蛋白表达逐渐增加。采用阻断剂特异性阻断Hedgehog信号通路中的Gli1和Smo 24 h后,Gli1的mRNA和蛋白表达均受抑制,同时伴有上皮间质转化发生的生物标记物E-Cadherin和Vimentin的表达改变,证实发生了上皮间质转化。③结合体内及体外实验,共同证实了Hedgehog-Gli信号通路参与心肌纤维化及心肌成纤维细胞转分化发生发展过程。

Gli-1信号通路对TGF-β1诱导的人胃癌细胞上皮间质转化和侵袭的影响

目的:探讨核转录因子神经胶质瘤关联癌基因同源物1(glioma associated oncogene homolog 1,Gli-1)对转化生长因子-β1(transforming growth factor-β1,TGF-β1)诱导的人胃癌SGC-7901细胞发生上皮间质转化(epithelial-mesenchymal transition,EMT)的作用机制。方法:体外采用10 ng/ml TGF-β1对胃癌SGC-7901细胞进行处理,使用倒置显微镜观察细胞形态变化,RT-PCR和Western blot检测EMT上皮表型蛋白E-cadherin和间质表型蛋白Vimentin的表达水平; Transwell细胞侵袭实验检测细胞侵袭能力变化,检测TGF-β1对SGC-7901细胞发生EMT的影响;同时采用RT-PCR和Western blot检测Gli-1的mRNA和蛋白表达水平。随后进一步采用Gli-1基因特异性阻断剂GANT 61阻断Gli-1表达,并使用TGF-β1(10 ng/ml)对SGC-7901细胞进行处理,RT-PCR和Western blot检测Gli-1、E-cadherin和Vimentin mRNA及其蛋白表达水平的改变,并使用Transwell细胞侵袭实验检测阻断Gli-1对SGC-7901细胞侵袭能力的影响。结果:TGF-β1可以诱导人胃癌SGC-7901细胞发生上皮间质转化并促进细胞侵袭。TGF-β1可以在mRNA和蛋白水平下调上皮表型蛋白E-cadherin的表达、提高Gli-1和间质表型蛋白Vimentin的表达。TGF-β1可以明显提高SGC-7901细胞侵袭,而阻断Gli-1后可以抑制TGF-β1诱导的人胃癌SGC-7901细胞上皮间质转化和细胞侵袭。结论:胃癌SGC-7901细胞中Gli-1可能参与TGF-β1介导的EMT的发生,Gli-1可能作为胃癌基因治疗中的有效靶点发挥作用。

转化生长因子β1对大鼠髓核细胞凋亡影响的实验研究

目的 :探讨转化生长因子β1(transforming growth factor-β1,TGF-β1)对大鼠髓核细胞凋亡的影响以及其作用机制。方法:采用序贯酶消化法分离培养SD大鼠髓核细胞(nucleus pulposus cells,NPCs),实验用第3代培养的NPCs,分为6组:A组,空白对照组,用DMEM培养基常规培养,不加任何处理;B组,用含有终浓度为20ng/ml肿瘤坏死因子α(tumor necrosis factorα,TNF-α)的DMEM培养基培养;C组,用含有终浓度为50ng/ml TNF-α的DMEM培养基培养;D组,用含有终浓度为100ng/ml TNF-α的DMEM培养基培养;E组,用同时含有终浓度为100ng/ml TNF-α和10ng/ml TGF-β1的DMEM培养基培养;F组,在E组培养基的基础上加TGF-β1/smad通路抑制剂SB431542(设置终浓度为10μmol/L)进行培养。培养12h后,Cell Counting Kit-8(CCK-8)法检测细胞增殖活性,逆转录聚合酶链式反应(reverse transcription-polymerase chain reaction,RTPCR)检测各组细胞中基质金属蛋白酶3(matrix metalloproteinases 3,MMP3)、凋亡相关蛋白(bcl-2-associated x protein,Bax)、蛋白聚糖(ACAN)、Ⅱ型胶原(CollagenⅡ)m RNA相对表达量,Western blot检测各组细胞中MMP3、Bax、ACAN、CollagenⅡ、磷酸化的smad3蛋白(phosphorylate drosophila mothers against decapentaplegic protein 3,p-smad3)和Runt相关转录因子2(Runt-related transcription factor 2,Runx2)蛋白表达量。结果 :与A组相比,不同剂量的TNF-α(B^D组)均能够促进MMP3(B^D组依次为0.652+0.015、0.899+0.018、1.026+0.023)和Bax(B^D组依次为0.725+0.058、0.928+0.018和1.138+0.019)的表达,诱导髓核细胞的凋亡,并且呈现剂量依赖性关系。与D组相比,E组MMP3(0.568+0.015)和Bax(0.626+0.024)表达下调,ACAN(1.056+0.014)、CollagenⅡ(1.098+0.032)、p-smad3和Runx2表达量增高,差异有统计意义(P<0.05)。与E组相比,F组MMP3(1.015+0.015)和Bax(1.126+0.024)表达上调,ACAN(0.314+0.023)、CollagenⅡ(0.299+0.0.19)、p-smad3和Runx2表达量下降,差异有统计意义(P<0.05)。结论 :TGF-β1可能是通过激活smad/Runx2通路来拮抗TNF-α诱导的大鼠髓核细胞凋亡。

FKBP11下调对肾癌细胞增殖、迁移、侵袭及TGF-β_(1)/Smad3通路的影响

目的 探讨下调FK506结合蛋白11(FKBP11)对肾细胞癌(RCC)细胞增殖、迁移、侵袭的影响及对转化生长因子-β_(1)(TGF-β_(1))/Smad同源物3(Smad3)通路的作用。方法 2020年3月—2021年3月于武汉大学人民医院生物实验室进行实验。采用实时荧光定量PCR(qRT-PCR)和免疫印迹(Western-blot)法测定人正常肾小管上皮细胞系(HK-2)和RCC细胞系(A498、ACHN、CaKi-1、786-O)中FKBP11的mRNA和蛋白表达水平。将786-O细胞分为空白组(不转染)、对照组(转染阴性对照siRNA)、si-FKBP11组(转染si-FKBP11)和si-FKBP11+LY364947组(转染si-FKBP11同时加入TGF-β_(1)/Smad3通路抑制剂LY364947),采用qRT-PCR和Western-blot检测各组细胞中FKBP11 mRNA和蛋白表达水平,CCK-8法和集落形成实验检测细胞的增殖活力,Transwell小室检测细胞的侵袭和迁移能力,Western-blot检测各组细胞中增殖细胞核抗原(PCNA)、E-钙黏蛋白(E-cadherin)、波形蛋白(Vimentin)、凋亡抑制蛋白(Twist)、锌指转录因子(Snail)、TGF-β_(1)、Smad3及磷酸化Smad3 (p-Smad3)蛋白表达水平。结果 与正常肾小管上皮细胞系HK-2比较,RCC细胞系A498、ACHN、CaKi-1、786-O中FKBP11 mRNA和蛋白表达水平显著上调(P<0.05),且在786-O细胞中表达最高。与对照组比较,si-FKBP11组细胞中FKBP11 mRNA和蛋白表达水平、细胞增殖能力、细胞侵袭和迁移能力及PCNA、Vimentin、Twist、Snail、TGF-β_(1)和p-Smad3蛋白水平显著降低,E-cadherin蛋白水平显著增高(P<0.05);与si-FKBP11组比较,si-FKBP11+LY364947组细胞增殖能力、细胞侵袭和迁移能力以及PCNA、Vimentin、Twist、Snail、TGF-β_(1)和p-Smad3蛋白水平显著降低,E-cadherin蛋白水平显著增高(P<0.05);而空白组与对照组上述各项指标变化比较差异均无统计学意义(P>0.05)。结论 FKBP11下调可通过抑制TGF-β_(1)/Smad3通路激活进而抑制RCC细胞增殖、侵袭和迁移。

藏药灰兜巴对糖尿病肾病大鼠TGF-β1/Smads信号通路的影响

目的研究灰兜巴对糖尿病肾病(DN)大鼠转化生长因子β1/细胞转导分子(TGF-β1/Smads)信号通路的影响。方法将SD大鼠随机分为对照组、模型组、灰兜巴提取物高剂量(200 mg·kg^-1)组、中剂量(100 mg·kg^-1)组和低剂量(50 mg·kg^-1)组,3个剂量组大鼠灌胃灰兜巴提取物,对照组灌胃生理盐水,连续灌胃20 d。采用酶联免疫吸附(Elisa)法测定转化生长因子-β1(TGF-β1)、细胞信号转导分子2(Smad2)、细胞信号转导分子3(Smad3)、细胞信号转导分子7(Smad7)和结缔组织生长因子(CTGF)的蛋白表达,用实时荧光定量PCR(qPCR)测定TGF-β1、Smad2、Smad3、Smad7和CTGF的基因表达。结果藏药灰兜巴能明显降低TGF-β1、Smad2、Smad3、Smad7和CTGF的蛋白表达和基因表达(P<0.05)。结论藏药灰兜巴能阻断TGF-β1/Smads信号通路,对DN大鼠具有一定的保护作用。

Upregulated DJ-1 Promotes Renal Tubular EMT by Suppressing Cytoplasmic PTEN Expression and Akt Activation

Recently,phosphatase and tensin homolog deleted on chromosome 10（PTEN） is suggested as a new agent in the fighting against fibrogenesis.In tumor,DJ-1 is identified as a negative regulator of PTEN.But the expression of DJ-1 and the regulation of PTEN in fibrosis are unclear.Renal fibrosis was induced in 5/6 subtotal nephrectomy rat model.Human proximal tubular epithelial cells（HKC） were treated with transforming growth factor-beta 1（TGF-β1）,or transfected with DJ-1 or PTEN.Confocal microscope was used to investigate the localization of DJ-1 and PTEN.The selective phosphoinositide-3 kinase（PI3K） inhibitor,LY294002,was administered to inhibit PI3K pathway.The DJ-1 and PTEN expression,markers of epithelial-mesenchymal transition（EMT） and Akt phosphorylation were measured by RT-PCR,Western blotting or immunocytochemistry.In vitro,after HKC cells were stimulated with 10 ng/mL TGF-β1 for 72 h,the expression of DJ-1 was increased,and that of PTEN was decreased.In vivo,the same results were identified in 5/6-nephrectomized rats.In normal HKC cells,most of DJ-1 protein localized in cytoplasm,and little in nucleus.TGF-β1 upregulated DJ-1 expression in both cytoplasma and nuclei.In contrary,TGF-β1 emptied cytoplasmic PTEN protein into nucleus.Overexpression of DJ-1 decreased the expression of PTEN,promoted the activation of Akt and the expression of vimentin,and also led to the loss of cytoplasmic PTEN.Contrarily,overexpression of PTEN protected HKC cells from TGF-β1-induced EMT.In conclusion,DJ-1 is upregulated in renal fibrosis and DJ-1 mediates EMT by suppressing cytoplasmic PTEN expression and Akt activation.

肠炎清对溃疡性结肠炎大鼠TGF-β_(1)/Smad3/ERK通路的影响

目的:观察肠炎清对溃疡性结肠炎(UC)大鼠的保护作用及对TGF-β_(1)/Smad3/ERK信号通路的调控作用。方法:将25只雌性SD大鼠随机分为5组:空白对照组、模型组、美沙拉嗪组、肠炎清低剂量组和肠炎清高剂量组,除空白对照组外,其余大鼠均采用2,4,6三硝基苯磺酸(TNBS)诱导,建立UC模型。造模24 h后,模型组、空白对照组分别用0.9%生理盐水灌胃;美沙拉嗪对照组以30 mg/kg艾迪莎混悬液灌胃;肠炎清高剂量组以147.2 g/kg肠炎清灌胃;肠炎清低剂量组以36.8 g/kg肠炎清灌胃;1次/d,时间固定,持续7 d。检测结肠黏膜组织中转化生长因子(TGF)-β_(1)、Smad3、胞外信号调节激酶(ERK)磷酸化的水平及TGF-β_(1)信号通路活化的程度。结果:模型组ERK表达水平最低,低于溶媒对照组、美沙拉嗪组、肠炎清高剂量组和低剂量组,肠炎清剂量组该指标水平随剂量升高而上升,且高剂量肠炎清组ERK表达水平显著高于模型组。模型组TGF-β_(1)和Smad3高于美沙拉嗪组组、空白对照组和肠炎清低剂量组及高剂量组。结论:肠炎清对UC大鼠肠黏膜具有保护作用,其机制可能与通过下调TGF-β_(1)-Smad3通路,提高ERK表达有关。

MiR-23b通过调节TGF-β1/SMAD3信号通路对博莱霉素所致大鼠肺纤维化及自噬水平的影响

目的:探究miR-23b通过调节转化生长因子-β1(transforming growth factorβ,TGF-β1)/SMAD同源物3(mothers against decapentaplegic homolog 3,SMAD3)信号通路对博莱霉素(bleomycin,BLM)所致大鼠肺纤维化(pulmonary fibrosis,PF)及自噬水平的影响。方法:采用BLM诱导大鼠PF模型,并分为对照组、PF组、agomiR-阴性对照(negative control,NC)组和agomiR-23b组。通过生物信息学预测及双荧光素酶实验验证miR-23b对SMAD3的调控作用;用苏木精-伊红(hematoxylineosin stain,HE)和Masson染色观察大鼠肺组织病理学改变,免疫组织化学染色观察大鼠肺组织Ⅰ型胶原蛋白(collagen-Ⅰ)、α-平滑肌肌动蛋白(α-smooth muscle actin,α-SMA)、酵母自噬相关基因6(autophagy related protein 6,ATG6)的哺乳动物同源体(beclin-1)、轻链3-Ⅱ(light chain 3-Ⅱ,LC3-II)的表达,实时荧光定量聚合酶链式反应(real-time fluorescent quantitative polymerase chain reaction,RT-qPCR)检测肺组织中miR-23b和SMAD3 mRNA的表达,蛋白质印迹法检测肺组织中TGF-β1、SMAD3和SMAD7的蛋白质表达。将人肺成纤维细胞(HFL1)分为对照组、PF组、agomiR-NC组和agomiR-23b组;用RT-qPCR检测各组细胞中miR-23b和SMAD3 mRNA的表达,Transwell小室实验检测各组细胞迁移和侵袭能力,透射电镜观察各组细胞自噬泡的形成。结果:与对照组相比,PF组和agomiR-NC组PF程度更严重;肺组织SMAD3 mRNA以及collagen-Ⅰ、α-SMA、TGF-β1和SMAD3蛋白表达水平明显升高,miR-23b以及beclin-1、LC3-Ⅱ和SMAD7蛋白表达水平明显降低;HFL1细胞SMAD3 mRNA表达水平以及迁移和侵袭能力提高,自噬活性降低(均P<0.05)。与PF组相比,agomiR-23b组大鼠PF程度得到有效改善;肺组织collagen-Ⅰ、α-SMA、TGF-β1和SMAD3蛋白表达水平明显降低,beclin-1、LC3-Ⅱ和SMAD7蛋白表达水平明显升高;HFL1细胞迁移、侵袭能力降低,自噬活性增强(P<0.05)。结论:MiR-23b通过靶向抑制SMAD3的表达抑制肺成纤维细胞的迁移,降低PF程度,并提高自噬活性;其机制可能与调控TGF-β1/SMAD3通路有关。

白花蛇舌草醇提物对矽肺大鼠肺组织TGF-β1、Smad、MMP-2表达的影响

目的探究白花蛇舌草醇提物对矽肺大鼠肺组织转化生长因子-β1(TGF-β1)、母亲DPP同源物(Smad)、基质金属蛋白酶2(MMP-2)表达的影响。方法以气管内滴注二氧化硅混悬液的方法构建矽肺大鼠模型60只,随机分为模型组、白花蛇舌草醇提物低(1.5 g/kg)、中(3 g/kg)、高(6 g/kg)剂量组、吡非尼酮(100 mg/kg)组,每组12只,另选取12只大鼠气管内滴注等剂量生理盐水作为对照组。采用药物干预后,检测大鼠肺功能,比较其指标:每分通气量(MV)、呼气峰流值(PEF)、吸气阻力(Ri);检测各组大鼠双肺质量及其脏器系数;免疫组织化学染色检测各组大鼠肺组织淋巴细胞浸润情况,比较各组淋巴细胞功能相关抗原-1(LFA-1)阳性细胞比例;天狼星红染色检测各组大鼠肺组织胶原沉积及纤维化变性情况,比较胶原容积分数(CVF);采用试剂盒检测大鼠血清白细胞介素-18(IL-18)、环氧化酶-2(COX-2)、TGF-β1水平;蛋白免疫印迹法检测大鼠肺组织TGF-β1、Smad、MMP-2蛋白表达情况。结果与对照组相比,模型组大鼠MV、PEF显著降低,Ri、双肺质量及其脏器系数、肺组织LFA-1阳性细胞比例、CVF、血清IL-18、COX-2及TGF-β1水平、肺组织TGF-β1、Smad及MMP-2蛋白表达水平显著升高,差异均有统计学意义(P<0.05)。与模型组相比,白花蛇舌草醇提物低、中、高剂量组和吡非尼酮组大鼠MV、PEF均升高,Ri、双肺质量及其脏器系数、肺组织LFA-1阳性细胞比例、CVF、血清IL-18、COX-2及TGF-β1水平、肺组织TGF-β1、Smad及MMP-2蛋白表达水平均降低,差异均有统计学意义(P<0.05),且白花蛇舌草醇提物随剂量升高而作用增强并呈剂量依赖性(P<0.05)。白花蛇舌草醇提物高剂量组与吡非尼酮组相比,大鼠各指标水平无明显变化,差异无统计学意义(P>0.05)。结论白花蛇舌草醇提物可抑制肺组织TGF-β1、Smad、MMP-2表达,降低矽肺大鼠炎性因子水平,减轻肺组织炎症反应损伤和纤维化变性,修复肺功能。

Gli1对TGF-β1诱导的肾小管上皮细胞间质转分化和胶原合成的影响

目的探讨锌指转录因子1(Gli1)对转化生长因子-β1(TGF-β1)诱导的肾小管上皮细胞间质转分化和胶原合成的影响。方法培养肾小管上皮细胞NRK-52E,分为Control、TGF-β1(TGF-β1诱导)、sh-NC+TGF-β1(转染阴性对照shRNA,TGF-β1处理)和sh-Gli1+TGF-β1(转染Gli1 shRNA,TGF-β1处理)组共4组,应用qRT-PCR和Western blot分别检测细胞中Gli1表达水平,ELISA检测细胞培养液上清中纤维连接蛋白(FN)和Ⅰ型胶原酶(ColⅠ)水平,Western blot检测细胞中α-平滑肌肌动蛋白(α-SMA)和Ras相关C3肉毒素底物1(Rac1)蛋白表达水平。结果TGF-β1组肾小管上皮细胞中Gli1 mRNA和蛋白表达量均高于Control组;肾小管上皮细胞中Gli1 mRNA和蛋白表达量,TGF-β1和sh-NC+TGF-β1组均高于sh-Gli1+TGF-β1组;FN和ColⅠ水平,Control组均低于TGF-β1、sh-NC+TGF-β1和sh-Gli1+TGF-β1组,TGF-β1和sh-NC+TGF-β1组均高于sh-Gli1+TGF-β1组;α-SMA和Rac1蛋白表达,Control组均低于TGF-β1、sh-NC+TGF-β1和sh-Gli1+TGF-β1组,TGF-β1和sh-NC+TGF-β1组均高于sh-Gli1+TGF-β1组,差异有统计学意义(P<0.05或P<0.01)。结论下调Gli1减弱TGF-β1条件下肾小管上皮细胞间质转分化和胶原合成水平。

CCDC134调控人牙髓干细胞成骨分化

目的探讨CCDC134(coiled⁃coil domain containing 134)对人牙髓干细胞(human dental pulp stem cells,hDPSCs)成骨分化功能的调控作用。方法从牙髓组织中,分离培养hDPSCs,并分别以NC⁃CCDC134、shCCDC134、CCDC134慢病毒转染hDPSCs,分为空白对照组、阴性对照组、CCDC134下调组(shCCDC134)、CCDC134过表达组(CCDC134)。流式细胞术检测hDPSCs表面标志物Stro⁃1、CD105、CD34、CD45;甲苯胺蓝染色检测克隆形成;碱性磷酸酶(alkaline phosphatase,ALP)染色检测ALP表达;茜素红染色检测矿化结节形成;油红染色检测成脂能力;qPCR检测CCDC134、Runt相关转录因子2(Runt⁃related transcription factor 2,RUNX2)、骨钙素(osteocalcin,OCN)、骨形态发生蛋白⁃2(bone morphogenetic protein⁃2,BMP⁃2)、Smad家族成员1(mothers against decapentaplegic homolog 1,SMAD1)的mRNA水平表达;蛋白印迹法检测CCDC134、RUNX2、OCN、BMP⁃2、SMAD1蛋白表达水平。进一步以BMP⁃2信号激活剂(BMP⁃2)和抑制剂(Dorsomorphin)分别干预CCDC134下调及上调的hDPSCs(分组为:shCCDC134、shCCDC134+BMP⁃2、CCDC134、CCDC134+Dorsomorphin),细胞聚合体移植于裸鼠皮下2个月,HE染色法检测新骨形成。结果hDPSCs高表达间充质干细胞表面标志物,低表达造血干细胞表面标志物。与空白对照组相比,成骨诱导的hDPSCs中CCDC134的表达升高;与阴性对照组相比,shCCDC134组CCDC134的表达降低,CCDC134组的表达升高(P<0.05);shCCDC134组的矿化结节减少、成骨相关基因和蛋白表达降低(P<0.05),CCDC134组的指标升高(P<0.05);shCCDC134组的BMP⁃2/SMAD1信号通路的相关表达降低,CCDC134组表达升高(P<0.05)。与shCCDC134组相比,shCCDC134+BMP⁃2组成骨相关基因和蛋白表达升高、裸鼠皮下新骨形成增加(P<0.05),与CCDC134组相比,CCDC134+Dorsomorphin组以上指标降低(P<0.05)。结论CCDC134通过调控BMP⁃2/SMAD1信号通路促进hDPSCs成骨分化。

Possible mechanisms associated with immune escape and apoptosis on anti-hepatocellular carcinoma effect of Mu Ji Fang granules

BACKGROUND Hepatocellular carcinoma(HCC)is one of the most common digestive system cancers with high mortality rates worldwide.The main ingredients in Mu Ji Fang Granules(MJF)are alkaloids,flavonoids,and polysaccharides.MJF has been used in the clinical treatment of hepatitis,cirrhosis and HCC for more than 30 years.Few previous studies have focused on the mechanism of MJF on tumor immunology in the treatment of HCC.AIM To explore the mechanism of action of MJF on tumor immunology in the treatment of HCC.METHODS The absorbable ingredients of MJF were identified using Molecule Network related to High Performance Liquid Chromatography-Electron Spray Ionization-Time of Flight-Mass Spectrometry,and hub potential anti-HCC targets were screened using network pharmacology and pathway enrichment analysis.Forty male mice were randomly divided into the Blank,Model,and MJF groups(1.8,5.4,and 10.8 g/kg/d)following 7 d of oral administration.Average body weight gain,spleen and thymus indices were calculated,tumor tissues were stained with hematoxylin and eosin,and Interferon gamma(IFN-γ),Tumor necrosis factorα(TNF-α),Interleukin-2,aspartate aminotransferase,alanine aminotransferase,alpha-fetoprotein(AFP),Fas,and FasL were measured by Enzyme-linked Immunosorbent Assay.Relevant mRNA expression of Bax and Bcl2 was evaluated by Real Time Quantitative PCR(RTqPCR)and protein expression of Transforming growth factorβ1(TGF-β1)and Mothers against decapentaplegic homolog(SMAD)4 was assessed by Western blotting.The HepG2 cell line was treated with 10 mg/mL,20 mg/mL,30 mg/mL,40 mg/mL of MJF,and another 3 groups were treated with TGF-β1 inhibitor(LY364947)and different doses of MJF.Relevant mRNA expression of TNF-α,IFN-γ,Bax and Bcl2 was evaluated by RT-qPCR and protein expression of TGF-β1,SMAD2,p-SMAD2,SMAD4,and SMAD7 was assessed by Western blotting.RESULTS It was shown that MJF improved body weight gain and tumor inhibition rate in H22 tumorbearing mice,protected immune organs and liver function,reduced the HCC indicator AFP,affected immunity and apoptosis,and up-regulated the TGF-β1/SMAD signaling pathway,by increasing the relative expression of TGF-β1,SMAD2,p-SMAD2 and SMAD4 and decreasing SMAD7,reducing immune factors TNF-αand IFN-γ,decreasing apoptosis cytokines Fas,FasL and Bcl2/Bax,and inhibiting the effect of LY364947 in HepG2 cells.CONCLUSION MJF inhibits HCC by activating the TGF-β1/SMAD signaling pathway,and affecting immune and apoptotic cytokines,which may be due to MJF adjusting immune escape and apoptosis.

川芎嗪对胶质瘤干细胞裸鼠皮下移植瘤生长、TGF-β信号通路和上皮-间质转化的影响

目的:探讨川芎嗪对胶质瘤干细胞(GSCs)裸鼠皮下移植瘤生长、转化生长因子β(TGF-β)信号通路和上皮-间质转化(EMT)的影响,为胶质瘤临床治疗药物的选择提供参考。方法:收集人脑胶质瘤细胞系U87细胞,培养、分离、富集并鉴定GSCs。40只雌性BALB/c裸鼠,建立GSCs裸鼠皮下移植瘤模型,成模后随机分为模型组和低、中及高剂量川芎嗪组,每组10只。低、中和高剂量川芎嗪组裸鼠每3 d腹腔注射给药1次,给药剂量分别为1.5、3.0和6.0 mg·kg^(-1),模型组裸鼠仅腹腔注射等量生理盐水,连续15 d。测量各组裸鼠移植瘤体积,称瘤质量,计算瘤质量抑制率,绘制肿瘤生长曲线。HE染色观察各组裸鼠肿瘤组织病理形态表现,实时荧光定量PCR(RT-qPCR)法检测各组裸鼠肿瘤组织中TGF-β1和TGF-β受体Ⅰ(TβRⅠ)mRNA表达水平,Western blotting法检测各组裸鼠肿瘤组织中TGF-β1、TβRⅠ、母亲DPP同源物2/3(Smad2/3)、磷酸化Smad2/3(p-Smad2/3)、E-钙黏蛋白(E-cadherin)、TWIST家族bHLH转录因子1 (TWIST1)、波形蛋白(Vimentin)及锌指蛋白(Snail)表达水平。结果:在U87细胞中成功富集并分离获得GSCs,免疫荧光染色可见干细胞标志物CD133阳性表达。与模型组比较,低、中和高剂量川芎嗪组裸鼠移植瘤体积均减小(P<0.05),且呈剂量依赖性;移植瘤质量均降低(P<0.05),且呈剂量依赖性;低、中和高剂量川芎嗪组瘤质量抑制率逐渐增大,分别为12.72%、39.90%和55.36%。HE染色观察,模型组裸鼠肿瘤组织细胞形态良好,连接紧密,生长密度高,核异型性明显;低、中和高剂量川芎嗪组裸鼠肿瘤组织结构紊乱,细胞密度逐渐降低,核固缩和核裂解逐渐明显,组织坏死区逐渐增大,且随着川芎嗪剂量的增加,上述改善逐渐明显。RT-qRCR法检测,与模型组比较,低、中和高剂量川芎嗪组裸鼠移植瘤组织中TGF-β1和TβRⅠmRNA表达水平均降低(P<0.05),且呈剂量依赖性。Western blotting法检测,与模型组比较,低、中和高剂量川芎嗪组裸鼠皮下移植瘤组织中E-cadherin蛋白表达水平均升高(P<0.05),TWIST1、Vimentin、Snail、TGF-β1、TβRⅠ和p-Smad2/3蛋白表达水平均降低(P<0.05),且呈剂量依赖性。结论:川芎嗪可发挥对GSCs裸鼠皮下移植瘤生长的抑制作用,同时可干扰TGF-β1/Smad2/3信号激活和EMT诱导。