肺复方通过PI3K/Akt/Nrf2信号通路对A549/DDP细胞耐药性的影响

目的观察肺复方对人肺癌顺铂耐药株A549/DDP细胞耐药性的作用及对PI3K/Akt/Nrf2信号通路的影响。方法选用A549/DDP细胞设立不含药血清的空白对照组、肺复方组、顺铂组、联合组,流式细胞术检测各组细胞周期分布和细胞中活性氧(ROS)的变化,Western blotting和RT-PCR检测PI3K/Akt/Nrf2信号通路及下游血红素氧合酶1(HO-1)、NAD(P)H:醌氧化还原酶1(NQO1)、多药耐药相关蛋白1(MRP1)的表达变化。结果与空白对照组、顺铂组相比,联合组引起细胞G1期阻滞,增加细胞内活性氧的累积,差异具有统计学意义(P<0.05或P<0.01);与空白对照组比,肺复方组和联合组能减少Nrf2核转位,下调p-Akt、HO-1、NQO1、MRP1蛋白表达和mRNA表达水平,差异具有统计学意义(P<0.05或P<0.01)。结论肺复方能够通过调控PI3K/Akt/Nrf2信号通路增加A549/DDP细胞对顺铂的敏感性。

益气小复方通过下调lncRNA HCP5表达增强三阴性乳腺癌顺铂耐药细胞株MDA-MB-231/DDP对顺铂敏感性的机制研究

目的探讨益气小复方增强三阴性乳腺癌顺铂耐药细胞株MDA-MB-231/DDP顺铂敏感性的可能机制。方法以不同浓度的顺铂(0、2、4、8、16、32、64 mg/L)分别作用于MDA-MB-231野生、耐药细胞株24 h,噻唑蓝(MTT)比色法检测细胞增殖,鉴定耐药细胞株的顺铂耐药性。上述梯度浓度的顺铂及顺铂加固定浓度(5mg/L)益气小复方分别作用于野生、耐药细胞株及长链非编码RNA人源组织相容性白细胞抗原复合物P5(LncRNAHCP5)基因过表达、敲减的野生、耐药细胞株,MTT比色法检测细胞增殖,流式细胞仪检测细胞凋亡,实时荧光定量逆转录聚合酶链式反应(RT-qPCR)法检测HCP5mRNA表达水平,蛋白质免疫印迹(Western blot)法检测磷酸酶张力蛋白同源物(PTEN)、磷酸化蛋白激酶B(p-Akt)蛋白表达水平。结果MDA-MB-231耐药细胞株较野生细胞株顺铂耐药指数为42.4。益气小复方同顺铂联用较单独使用顺铂,对耐药细胞株的增殖抑制率及诱导细胞凋亡比率均有提高(P<0.05)。MDA-MB-231耐药细胞株较野生细胞株,lncRNAHCP5、p-Akt蛋白表达升高,PTEN蛋白表达降低(P<0.05);益气小复方可降低MDA-MB-231耐药细胞株lncRNA HCP5、p-Akt蛋白表达,提高PTEN蛋白表达(P<0.05)。结论益气小复方可能通过下调lncRNAHCP5表达而升高PTEN蛋白表达、降低p-Akt蛋白表达,进而增强MDA-MB-231耐药细胞株对顺铂的敏感性。

蒽醌修饰物KA-4s抑制SKOV3/DDP细胞增殖并诱导铁死亡

目的:探讨蒽醌修饰物KA-4s在体外对人顺铂耐药卵巢癌SKOV3/DDP细胞增殖的影响和诱导细胞铁死亡的机制。方法:将SKOV3/DDP细胞分为对照组和不同浓度(2μmol/L、5μmol/L和7μmol/L)的蒽醌修饰物KA-4s组。采用MTT法检测单药KA-4s和顺铂(DDP)对SKOV3/DDP细胞活力的影响,划痕实验检测细胞的迁移能力,线粒体绿色荧光探针(Mito-Tracker Green)检测线粒体形态改变,透射电镜观察线粒体超微结构。以铁死亡诱导剂RSL3为阳性对照组,用DCFA-DA荧光探针检测细胞内活性氧(ROS)水平,比色法检测细胞内总铁蛋白含量,western blotting检测铁死亡相关蛋白GPX4、FSP1的表达情况。结果:KA-4s和顺铂作用48 h后,卵巢癌SKOV3/DDP细胞增殖均明显受到抑制,相比顺铂,KA-4s的抑制作用更强(P<0.001),并能抑制细胞迁移。经KA-4s处理后线粒体受损,线粒体结构改变,膜密度增大,嵴减少甚至消失。与空白对照组相比,阳性RSL3组和KA-4s组SKOV3/DDP细胞内ROS水平升高(均P<0.001),5μmol/L KA-4s组总铁离子含量显著升高(P<0.001),卵巢癌SKOV3/DDP细胞中GPX4、FSP1蛋白的表达均降低(P<0.01),但正常卵巢IOSE80细胞中GPX4表达均无改变。结论:KA-4s能抑制SKOV3/DDP细胞增殖、迁移并诱导细胞铁死亡。

声带癌前病变组织中基质金属蛋白酶抑制剂-1、果蝇母亲DDP同源物4表达水平与术后复发和恶变的相关性研究

目的探讨声带癌前病变组织中基质金属蛋白酶抑制剂-1(tissue inhibitor of metalloproteinases 1,TIMP-1)、果蝇母亲DDP同源物4(drosophila mothers against DDP homolog 4,Smad4)表达水平与术后复发和恶变的相关性。方法回顾性分析2018年8月~2021年8月郑州大学第一附属医院收治的162例声带癌前病变患者的临床和病理资料,收集手术切除癌前病变组织(癌前病变组)及病变旁正常黏膜组织(对照组),采用免疫组织化学法检测组织中TIMP-1、Smad4表达情况。分析TIMP-1、Smad4阳性率与临床病理特征的关系,并采用Kaplan-Meier法和Cox回归分析法分析其对术后复发和恶变的影响。结果与对照组正常黏膜组织比较,癌前病变组的TIMP-1阳性率较高,Smad4阳性率较低(P<0.05)。不同病变范围、是否累及前连合、不同程度上皮异常增生患者的TIMP-1、Smad4阳性率存在差异(P<0.05)。术后随访时间24~60个月,中位随访时间36个月,随访期间失访患者6例,随访率96.30%(156/162),随访期间术后复发35例(21.60%),术后恶变16例(9.88%);Kaplan-Meier生存分析显示,TIMP-1阳性患者术后复发率和恶变率高于TIMP-1阴性患者(P<0.05);Smad4阴性患者术后复发率和恶变率高于Smad4阳性患者(P<0.05)。多因素Cox回归分析显示,喉咽反流、病变范围>1/2、中/重度异型增生、TIMP-1阳性、Smad4阴性是复发的独立危险因素(P<0.05),年龄>60岁、累及前连合、TIMP-1阳性、Smad4阴性是恶变的独立危险因素(P<0.05)。结论声带癌前病变组织中TIMP-1高表达、Smad4低表达,且TIMP-1阳性、Smad4阴性表达者术后复发和恶变风险较高。

mir-3168 targeted inhibition of TP53 promotes malignant transformation and cisplatin resistance of AGS and AGS/DDP gastric cancer cells

Objective:To investigate the effect of mir-3168 on the malignant transformation and cisplatin resistance of AGS and AGS/DDP gastric cancer cells,and to verify its target gene.Methods:The expression of mir-3168 in AGS and AGS/DDP gastric cancer cells was detected by qPCR,and mir-3168 mimic,inhibitor and negative control were synthesized.They were transfected into AGS and AGS/DDP gastric cancer cells,respectively.The expression of mir-3168 and TP53 mRNA was detected by qPCR.Cell viability was detected by CCK8 under gradient cisplatin treatment and non treatment,apoptosis was detected by flow cytometry,cell invasion was detected by Transwell,and TP53 protein expression was detected by western blot,The database predicted the binding sites of mir-3168 and TP53.According to the binding sites,the double luciferase experiment was used to verify the binding of mir-3168 and TP53.Results:Compared with cisplatin sensitive gastric cancer cell AGS,mir-3168 was significantly overexpressed in cisplatin resistant gastric cancer cell AGS/DDP;mir-3168 mimic promotes cisplatin resistance,proliferation and invasion of AGS and AGS/DDP gastric cancer cells,and inhibits apoptosis of AGS and AGS/DDP gastric cancer cells;mir-3168 inhibitor inhibits cisplatin resistance,proliferation and invasion of AGS and AGS/DDP gastric cancer cells,and promotes apoptosis of AGS and AGS/DDP gastric cancer cells;mir-3168 mimic inhibits the expression of TP53 mRNA and protein,and mir-3168 inhibitor promotes the expression of TP53 mRNA and protein;Targetscan database predicted that there was a binding point between mir-3168 and TP53,and the double luciferase experiment suggested that mir-3168 was bound to TP53 through the predicted binding site.Conclusion:mir-3168 may promote the malignant transformation of AGS and AGS/DDP gastric cancer cells and cisplatin resistance by targeting TP53.

华蟾素调控PI3K/AKT通路逆转卵巢癌A2780/DDP细胞顺铂耐药的作用机制

目的研究华蟾素(CBG)对人卵巢癌细胞顺铂耐药的逆转作用和机制。方法A2780细胞株及其顺铂耐药细胞株A2780/DDP是临床常见的卵巢癌细胞,故选择这两种细胞株作为研究对象。通过CCK-8法检测细胞活力,平板克隆和5-乙炔基-2′脱氧尿嘧啶核苷(EdU)实验检测细胞的增殖能力,赫斯特染色(Hoechst)法观察细胞凋亡情况,细胞划痕实验和Transwell实验评估细胞的迁移和侵袭能力,Western blot和定量逆转录PCR(RT-qPCR)法检测磷脂酰肌醇3-激酶/蛋白激酶(PI3K/AKT)信号通路和上皮-间质转化(EMT)的相关蛋白和mRNA的表达差异。结果与A2780细胞相比,A2780/DDP细胞的耐药指数分别约为5.636、5.864、5.695,采用CBG(2、4、6 mg/ml)处理A2780/DDP耐药细胞后,逆转耐药指数分别为1.617、2.570、3.461。CBG呈浓度依赖性地上调细胞凋亡水平、抑制细胞的增殖、迁移和侵袭能力(P<0.05)。Western blot结果显示:与A2780细胞相比,对照组(A2780/DDP)细胞中P-PI3K/PI3K和P-AKT/AKT的蛋白水平相对比值以及N钙黏蛋白(N-cadherin)、波形蛋白(Vimentin)、蜗牛蛋白(Snail)的蛋白表达更高,E钙黏蛋白(E-cadherin)蛋白表达更低(t_(P-PI3K/PI3K)=8.115,t_(P-AKT/AKT)=17.62、t_(N-cadherin)=6.126、t_(Vimentin)=4.001、t_(Snail)=17.333、t_(E-cadherin)=4.620,P<0.01);随着CBG剂量升高,耐药细胞中的P-PI3K、P-AKT、N-cadherin、Vimentin、Snail的蛋白表达水平降低,而E-cadherin的蛋白表达量增加(F_(P-PI3K)=268.5、F P-AKT=190.5、F_(N-cadherin)=24.02、F_(Vimentin)=57.65、F_(Snail)=87.24、F_(E-cadherin)=135.8,P<0.05)。RT-qPCR结果显示:随着CBG浓度增加,PI3K、AKT、N-cadherin、Vimentin、Snail的mRNA表达水平随之降低,相反E-cadherin的mRNA表达水平逐渐升高(F PI3K=101.1、F_(AKT)=558.3、F_(N-cadherin)=86.97、F_(Vimentin)=105.9、F_(Snail)=85.71、F_(E-cadherin)=80.96,P<0.01)。结论CBG具有逆转卵巢癌A2780/DDP细胞株顺铂耐药的作用,其机制可能与CBG调控PI3K/AKT信号通路和抑制EMT发生有关。

Cisplatin-induced activation of TGF-βsignaling contributes to drug resistance

Growing evidence suggests an association between epithelial-mesenchymal transition(EMT),a hallmark of tumor malignancy,and chemoresistance to a number of anti-cancer drugs.However,the mechanism of EMT induction in the process of acquiring anti-cancer drug resistance remains unclear.To address this issue,we obtained a number of cisplatin-resistant clones from LoVo cells and found that almost all of them lost cell-cell contacts.In these clones,the epithelial marker E-cadherin was downregulated,whereas the mesenchymal marker N-cadherin was upregulated.Moreover,the expression of EMT-related transcription factors,including Slug,was elevated.On the other hand,the upregulation of other mesenchymal marker Vimentin was weak,suggesting that the mesenchymal-like phenotypic changes occurred in these cisplatin-resistant clones.These mesenchymal-like features of cisplatin-resistant clones were partially reversed to parental epithelial-like features by treatment with transforming growth factor-β(TGF-β)receptor kinase inhibitors,indicating that TGF-βsignaling is involved in cisplatin-induced the mesenchymallike phenotypic changes.Moreover,cisplatin was observed to enhance the secretion of TGF-βinto the culture media without influencing TGF-βgene transcription.These results suggest that cisplatin may induce the mesenchymal-like phenotypic changes by enhancing TGF-βsecretion,ultimately resulting in drug resistance.

miR-125b reverses cisplatin resistance by regulating autophagy via targeting RORA/BNIP3L axis in lung adenocarcinoma

The platinum-based chemotherapy is one of the most frequently used treatment protocols for lung adenocarcinoma(LUAD),and chemoresistance,however,usually results in treatment failure and limits its application in the clinic.It has been shown that microRNAs(miRNAs)play a significant role in tumor chemoresistance.In this study,miR-125b was identified as a specific cisplatin(DDP)-resistant gene in LUAD,as indicated by the bioinformatics analysis and the real-time quantitative PCR assay.The decreased serum level of miR-125b in LUAD patients was correlated with the poor treatment response rate and short survival time.MiR-125b decreased the A549/DDP proliferation,and the multiple drug resistance-and autophagy-related protein expression levels,which were all reversed by the inhibition of miR-125b.In addition,xenografts of human tumors in nude mice were suppressed by miR-125b,demonstrating that through autophagy regulation,miR-125b could reverse the DDP resistance in LUAD cells,both in vitro and in vivo.Further mechanistic studies indicated that miR-125b directly repressed the expression levels of RORA and its downstream BNIP3L,which in turn inhibited autophagy and reversed chemoresistance.Based on these findings,miR-125b in combination with DDP might be an effective treatment option to overcome DDP resistance in LUAD.

TGF-β-regulated different iron metabolism processes in the development and cisplatin resistance of ovarian cancer

The impact of different iron metabolism processes(DIMP)on ovarian cancer remains unclear.In this study,we employed various gene chips and databases to investigate the role of DIMP in the initiation and development of ovarian cancer.cBioPortal was used to determine mutations in DIMP-associated genes in ovarian cancer.Kaplan-Meier plotter was used to examine the influence of DIMP on the prognosis of ovarian cancer.By analyzing 1669 serous ovarian cancer cases,we identified a range of mutations in iron metabolism genes,notably in those coding for the transferrin receptor(19%),melanotransferrin(19%),and ceruloplasmin(10%)in the iron import process,and glucose-6-phosphate isomerase(9%),hepcidin antimicrobial peptide(9%),metal regulatory transcription factor 1(8%),and bone morphogenetic protein 6(8%)in the iron regulation process.Compared to the unaltered group,the group with gene alterations exhibited a higher tumor mutation burden count(43 vs.54)and more advanced histologic grade(78.19%vs.87.90%).Compared to the normal ovarian counterparts,a reduction in expression was observed in 9 out of the 14 genes involved in iron utilization and 4 out of the 5 genes involved in iron export in ovarian cancer;in contrast,an increase in expression was observed in 2 out of the 3 genes involved in iron storage in ovarian cancer.Furthermore,in cisplatin-resistant cells compared to cisplatin-sensitive ones,the expression of all genes in iron storage and 13 out of 14 genes in iron import was decreased,while that of 8 out of the 10 genes in iron utilization was increased.In addition,survival curve analysis indicated that a higher expression in the majority of genes in the iron import process(12/21),or a reduced expression in most genes in the iron export process(4/5)correlated with poor progression-free survival.Additionally,TGF-βcould regulate the expression of most iron metabolism-associated genes;particularly,expression of genes involved in the iron storage process(2/2)was inhibited after TGF-β1 or TGF-β2 treatment.In conclusion,DIMP plays multifaceted roles in the initiation,chemo-resistance,and prognosis of ovarian cancer.Therapeutically targeting DIMP may pave the way for more tailored treatment approaches for ovarian cancer.

沉默NAC-1基因对人卵巢癌耐药细胞株SKOV3/DDP裸鼠移植瘤化疗敏感的影响

目的:探讨核转录因子NAC-1基因沉默对人卵巢癌耐药细胞株SKOV3/DDP裸鼠移植瘤化疗敏感性的影响。方法:采用LV4-LUC-GFP慢病毒转染建立NAC-1基因沉默SKOV3/DDP细胞株,将细胞接种到免疫缺陷小鼠皮下,建立人卵巢癌耐药细胞株SKOV3/DDP裸鼠移植瘤模型,给予顺铂化疗,比较NAC-1基因沉默对SKOV3/DDP在裸鼠体内增殖的影响。取肿瘤组织进行转录组测序,利用Illumina平台进行转录组mRNA测序,筛选差异表达基因,并进行GO和KEGG功能注释和富集分析,揭示NAC-1基因影响移植瘤化疗敏感的可能分子机制。使用STRING数据库构建DEGs编码蛋白互作网络,筛选MCC算法、Degree算法、Closeness算法3种算法共有基因作为关键基因,使用Metascape网站在线分析这些共同基因的基因功能。结果:与对照组相比,抑制NAC-1基因后裸鼠皮下肿瘤体积变小,重量减轻,差异有统计学意义(P<0.05)。转录组学分析显示,抑制NAC-1基因导致肿瘤组织中460个基因显著下调,568个基因显著上调。差异基因(DEGs)在多项GO富集类别中具有显著差异,如细胞代谢、有丝分裂、坏死、炎症、信号传递等。KEGG功能富集结果显示,NAC-1基因沉默可能影响了细胞因子-细胞因子受体相互作用、白细胞跨内皮迁移、神经活性配体-受体相互作用、细胞黏附分子、坏死、ECM受体相互作用、PI3K-Akt信号通路、NF-κB信号通路等。筛选获得的关键基因主要富集在白细胞介素的信号传导、粒细胞-巨噬细胞集落刺激因子(GM-CSF)通路、炎症反应等通路。结论:抑制NAC-1基因能提高人卵巢癌耐药细胞株SKOV3/DDP化疗敏感性,其可能通过多个信号通路影响肿瘤细胞的代谢、增殖、死亡、炎症反应等。

Celecoxib enhances the response of tumor cells to cisplatin through upregulating PUMA in non–small cell lung cancer carrying wild-type p53

Celecoxib,a cyclooxygenase-2 inhibitor,can enhance the efficacy of chemotherapy;however,its effect seems inconsistent.In this study,we investigated whether celecoxib would increase the antiproliferative effects of cisplatin in human lung cancer cells.Our data demonstrated the synergistic effects of celecoxib with cisplatin in wild-type p53 cells and their antagonistic effects inmutated or deleted p53 cells.Combination indices of 0.82 to 0.93 reflected a synergistic effect between celecoxib and cisplatin in lung cancer cells with wild-type p53.Combination indices of 1.63 to 3.00 reflected antagonism between celecoxib and cisplatin in lung cancer cells with mutated or deleted p53.Compared with that in cells with mutated or deleted p53,apoptosis significantly increased with the addition of celecoxib and cisplatin in wild-type p53 cells(P<0.05).Moreover,the results in vivo were similar to those in vitro:celecoxib combinedwith cisplatin slowed tumor growth in wild-type p53 groups and not in mutated or deleted p53 groups.In addition,celecoxib promoted p53 translocation into the nucleus and upregulated active p53 expression in wild-type p53 cells.Celecoxib combined with cisplatin upregulated PUMA(PUMA is a downstream gene of p53)after active p53 increased in wild-type p53 cells.In summary,the combination of celecoxib and cisplatin demonstrates clear synergistic effects in wild-type p53 cells and antagonistic effects inmutated or deleted p53 cells.The synergistic effect was achieved by apoptosis,induced by upregulating PUMA.Our results will provide a new treatment strategy for patients carrying wild-type p53,insensitive to cisplatin.

下调富含脯氨酸蛋白11表达对食管癌耐药细胞EC9706/DDP耐药性的影响及其机制

目的:探讨下调富含脯氨酸蛋白11(PRR11)表达对食管癌耐药细胞耐药性的影响,阐明其相关机制。方法:采用顺铂(DDP)浓度递增间断刺激人食管癌EC9706细胞建立DDP耐药细胞株EC9706/DDP,MTT法检测EC9706/DDP细胞药敏性,实时荧光定量PCR(RT-qPCR)法和Western blotting法检测EC9706/DDP细胞及其亲本EC9706细胞中PRR11 mRNA和蛋白表达水平。将EC9706/DDP细胞分为对照组、sh-NC组(转染sh-NC)、sh-PRR11组(转染sh-PRR11)、sh-NC+DDP组(转染sh-NC后用4 mg·L^(-1)DDP处理)和sh-PRR11+DDP组(转染sh-PRR11后用4 mg·L^(-1)DDP处理),RT-qPCR法检测各组细胞中PRR11 mRNA表达水平,Western blotting法检测各组细胞中PRR11、磷脂酰肌醇3-激酶(PI3K)p110α、蛋白激酶B(AKT)、磷酸化AKT(p-AKT)、P-糖蛋白(P-gp)和多药耐药相关蛋白1(MRP1)蛋白表达水平,流式细胞术检测各组细胞凋亡率。结果:成功获得DDP耐药细胞株EC9706/DDP,耐药指数为7.23±0.86。与EC9706细胞比较,EC9706/DDP细胞中PRR11 mRNA和蛋白表达水平升高(P<0.05)。分别与对照组和sh-NC组比较,sh-PRR11组细胞中PRR11 mRNA和蛋白表达水平降低(P<0.05),细胞的DDP半数抑制浓度(IC50)降低(P<0.05)。与sh-NC组比较,sh-NC+DDP组和sh-PRR11组细胞中PI3K p110α、p-AKT、P-gp和MRP1蛋白表达水平降低(P<0.05),细胞凋亡率升高(P<0.05);分别与sh-NC+DDP组和sh-PRR11组比较,sh-PRR11+DDP组细胞中PI3Kp110α、p-AKT、P-gp和MRP1蛋白表达水平降低(P<0.05),细胞凋亡率升高(P<0.05)。结论:下调EC9706/DDP耐药细胞中PRR11基因的表达,可抑制耐药相关蛋白的表达,逆转对DDP耐药,并诱导细胞凋亡,其作用机制可能与抑制PI3K/AKT信号通路激活有关。

TPX2基因沉默对膀胱癌耐药细胞株T24/DDP顺铂化疗敏感性的增强作用及其机制

目的:探讨爪蟾驱动蛋白样蛋白2靶蛋白(TPX2)基因沉默对膀胱癌耐药细胞株T24/顺铂(DDP)的化疗敏感性的影响,并阐明其作用机制。方法:采用DDP浓度梯度刺激法建立DDP耐药细胞株T24/DDP,将细胞分为T24细胞组和T24/DDP细胞组。MTT法检测各组细胞增殖活性,并根据半数抑制浓度(IC50)值计算耐药指数(RI);实时荧光定量聚合酶链式反应(RT-qPCR)法和Westernblotting法检测细胞中TPX2mRNA及蛋白表达水平。通过小干扰RNA(siRNA)沉默T24/DDP细胞中TPX2基因表达,再将细胞分为空白对照组、阴性对照干扰(si-NC)组、TPX2沉默(si-TPX2)组、si-NC+DDP(2 mg·L^(-1) DDP)组和si-TPX2+DDP(2 mg·L^(-1) DDP)组。RT-qPCR法和Western blotting法检测转染后细胞中TPX2 mRNA及蛋白表达水平,MTT法检测各组细胞增殖活性,流式细胞术检测各组凋亡细胞率和细胞周期G2/M期百分率,Transwell小室实验检测各组迁移细胞数和侵袭细胞数,Western blotting法检测各组细胞中Wnt/β-连环蛋白(β-catenin)信号通路相关蛋白β-catenin、P-糖蛋白(P-gp)、锌指蛋白转录因子1(Snail1)和Survivin蛋白表达水平。结果:成功建立膀胱癌DDP耐药细胞株T24/DDP,RI值为8.76。与T24细胞组比较,T24/DDP细胞组中TPX2 mRNA和蛋白表达水平明显升高(P<0.01)。与空白对照组和si-NC组比较,si-TPX2组T24/DDP细胞中TPX2mRNA和蛋白表达水平明显降低(P<0.01),且DDP的IC50值明显降低(P<0.01)。与si-NC组比较,si-TPX2组T24/DDP细胞凋亡率和细胞周期G2/M期百分率明显升高(P<0.01),迁移细胞数和侵袭细胞数明显降低(P<0.01),T24/DDP细胞中β-catenin、P-gp、Snail1和Survivin蛋白表达水平明显降低(P<0.01);与si-NC+DDP组比较,si-TPX2+DDP组T24/DDP细胞凋亡率和细胞周期G2/M期百分率明显升高(P<0.01),迁移细胞数和侵袭细胞数明显降低(P<0.01),T24/DDP细胞中β-catenin、P-gp、Snail1和Survivin蛋白表达水平明显降低(P<0.01)。结论:TPX2基因沉默通过抑制Wnt/β-catenin信号通路增强膀胱癌耐药细胞株T24/DDP对DDP的化疗敏感性。

补中益气汤含药血清对TGF-β介导的A549/DDP细胞Snail、E-cadherin表达的影响

目的观察补中益气汤含药血清对转化生长因子(TGF)-β1诱导前后,A549/DDP细胞Snail、E-钙黏蛋白(cadherin)表达的影响,探讨补中益气汤对A549/DDP细胞上皮-间充质转化(EMT)的干预作用。方法A549/DDP细胞分为:空白组、TGF-β1组(TGF-β15 ng/L,48 h)、中药组(10%补中益气汤含药血清)、干扰组(Snail干扰)。采用siRNA技术,运用免疫细胞化学法、Western印迹法、实时荧光定量PCR法,检测补中益气汤含药血清对A549/DDP细胞Snail、E-cadherin及mRNA水平的影响。结果与空白组比较,TGF-β1组E-cadherin及mRNA表达水平显著下调(P<0.05);与TGF-β1组比较,中药组及干扰组E-cadherin及mRNA表达水平显著上调(P<0.05)。而Snail蛋白及mRNA水平的影响呈现相反的变化趋势。结论Snail作为转录因子,可抑制E-cadherin基因的表达,诱导EMT发生,而补中益气汤含药血清可通过干预Snail蛋白及基因的表达,解除其对E-cadherin的抑制作用,从而逆转A549/DDP细胞EMT。

白杨素通过下调Annexin A3逆转人肺腺癌A549/DDP细胞顺铂的耐药性

目的观察白杨素对肺腺癌顺铂(DDP)耐药性细胞A549/DDP耐药敏感性的影响。方法取A549和A549/DDP细胞,qRT-PCR及Western blot法检测膜联蛋白A3(Annexin A3)基因及蛋白表达,CCK-8法测不同浓度白杨素(0、5、25、50、100 mmoL/L)干预后细胞生存率;将A549/DDP细胞分为A549/DDP组、白杨素组(50 mol/L)、Annexin A3过表达组(Annexin A3mimic组)、Annexin A3阴性对照组(Annexin A3 NC)、白杨素+Annexin A3mimic组,另取A549细胞正常培养作为空白对照组;CCK-8法检测细胞对DDP的半数生存浓度(IC50)及耐药指数;qRT-PCR和Western blot法检测Annexin A3基因和蛋白表达水平,流式细胞义监测细胞凋亡率,小鼠荷瘤实验检测移植瘤体积。结果不同浓度的白杨素均能时效依赖性和剂量依赖性降低A549、A549/DDP细胞生存率(P<0.05),选取50 mol/L为实验浓度作用细胞48 h;与A549细胞比较,A549/DDP细胞Annexin A mRNA及蛋白表达、对DDP的IC50、耐药指数均升高,凋亡率降低(P<0.05);与A549/DDP组比较,白杨素组细胞IC50、耐药指数、Annexin A3 mRNA及蛋白表达降低,细胞凋亡率升高(P<0.05),Annexin A3 mimic组细胞IC50、耐药指数、Annexin A3 mRNA及蛋白表达升高,细胞凋亡率降低(P<0.05);Annexin A3基因高表达可减弱A549/DDP细胞对白杨素的敏感性,降低细胞凋亡率(P<0.05);小鼠荷瘤实验证实,与单独的DDP治疗组比较,白杨素与DDP联合治疗可显著降低小鼠A549/DDP移植瘤瘤体体积(P<0.05),Annexin A3基因高表达的小鼠逆转白杨素与DDP联合治疗效果(P<0.05)。结论白杨素可能通过下调Annexin A3表达,逆转A549/DDP细胞对DDP的耐药性。

Inhibition of PI3K/Akt/m TOR signaling pathway enhances the sensitivity of the SKOV3/DDP ovarian cancer cell line to cisplatin in vitro

The activation of the PI3K/AKT/m TOR pathway plays a key role in ovarian cancer tumorigenesis, progression and chemotherapy resistance. This study aimed to explore the possible mechanism that PI-103, a dual inhibitor of phosphatidylinositide 3-kinase and m TOR, enhances the sensitivity of SKOV3/DDP ovarian cancer cell line to cisplatin chemotherapy. The results showed that PI-103 could significantly increase the sensitivity of SKVO3/DDP cells to cisplatin through inhibiting the activation of PI3K/Akt/m TOR signaling pathway and inducing cell cycle arrest and apoptosis.

Mechanism of drug resistance and reversal with ligustra-zine and cyclosporin A in cisplatin--inducedhuman epithelial ovarian cancer resistant cell line 3Ao/cDDP

Objective: To investigate the mechanism of resistance and reversal effect of ligustrazine and cyclosporin A in cisplatin--induced multidrug resistance ovarian cancer cell line 3Ao/cDDP. Methods: Using the corresponding dose calculated from clinical chemotherapy at 30 mg cisplatin per cycle, we established 3Ao/cDDP with 3Ao exposed at regular intervals and repeatedly to high-level concentration of cisplatin at 10 mg/ml for 24 hours each time. Expressions of LRP, MRP, P-gp, GSTp and TopoII were quantitatively detected with FCM. For drug resistance reversal, cyclosporin A and ligustrazine were administered singly or in combination at the maximal dose without cytotoxicity. Inhibition rates were determined by MTT assay. Results: 3Ao/cDDP was established after 4.5 months, with resistance factor 1.6 which was similar to clinical resistance degree. Low expression levels of MRP and P-gp were found in both 3Ao and 3Ao/cDDP (P>0.05), and LRP and GSTp expression levels in 3Ao/cDDP were significantly higher than those in 3Ao (P<0.005 and P<0.05, respectively), and TopoII in 3Ao/cDDP was significantly lower vs 3Ao (P<0.05). The inhibition rate of cDDP was 20.807±0.015%, cDDP plus ligustrazine 27.421±0.07% (P>0.05 vs cDDP), cDDP plus cyclosporin A 49.635±0.021% (P<0.01 vs cDDP), and cDDP plus ligustrazine and cyclosporin A 58.861±0.014% (P<0.01 vs cDDP). Conclusions: 3Ao/cDDP, induced by cisplatin and established by imitating the characteristics of clinical chemotherapy for epithelial ovarian cancer, was an ideal model for investigation of cisplatin resistance in vitro. Cisplatin resistance in 3Ao/cDDP could be accounted for by higher LRP, GSTp and lower TopoII expression and was not associated with MRP or P-gp. Ligustrazine had no significant reversal effect on cisplatin resistance, but cyclosporin A could reverse the resistance effectively.

THE EFFECT OF IRISQUINONE ON THE GLUTATHIONE SYSTEM AND MRP EXPRESSION OF CISPLATIN-RESISTANTHUMAN LUNG ADENOCARCINOMA CELL LINE (A_(549)^(DDP))

Objective: To investigate the Reversal Effect of Irisquinone (ANKA) on Cisplatin-resistant Human Lung Adenocarcinoma Cell Line (A 549 DDP ) and the change of MRP expression. Methods: MTT assay, flow cytometry, glutathione reductase recycling assay, RT-PCR were used. Results: None or low cytotoxic concentration of ANKA (10, 20, 30 μmol/L) could increase the sensitivity of A 549 DDP cells to CDDP by 8.2, 7.9 and 8.9-fold in a dose independent manner. After A 549 DDP cells was pretreated with 10 μmol/L ANKA for 12 h, CDDP cytotoxicity was increased 9.41-fold. The GSH content of the cells treated by ANKA is reduced significantly (P<0.001). The GSTπ protein expression was reduced by ANKA depended on its doses. ANKA also reduced expression of MRP protein, dependent on its dose and treating time (P<0.001). MRP mRNA expression was reduced only by 30μmol/L ANKA (P<0.05). Conclusion: The reversal effect of ANKA on A 549 DDP cell was relative to intracellular glutathione system.

基于Keap1/Nrf2信号通路针灸拮抗DDP肾损伤小鼠的作用机制

目的以顺铂(DDP)诱导肾损伤模型小鼠,通过观察针灸对肾脏组织中Kelch样环氧氯丙烷相关蛋白1(Keap1)/核因子E2相关因子2(Nrf2)信号通路的影响,阐释针灸改善DDP所致肾损伤的保护机制。方法选用清洁级雄性KM小鼠40只,随机分为4组,每组10只。在干预开始前1天,对空白组外的3组小鼠按体质量腹腔注射顺铂10 mg·kg^(-1),空白组注射同等剂量的0.9%NaCl溶液,24 h后模型即成。针刺组与艾灸组均选取“大椎”“肝俞”“肾俞”“足三里”,分别进行针刺与艾灸,每天1次,连续5天,其余2组陪同固定不予干预。禁食1天后取材,运用ELISA法检测血清中尿素氮(BUN)、肌酐(Scr)、半胱氨酸蛋白酶抑制剂(CysC)、中性粒细胞明胶酶相关脂质运载蛋白(NGAL)含量及肾脏组织中Keap1和Nrf2的含量;Western blot法及Real-time PCR法检测各组小鼠肾脏组织中Keap1和Nrf2蛋白表达及基因转录情况。结果与空白组比,模型组肾脏组织中Keap1含量、蛋白表达及mRNA相对表达均增多(P<0.05),Nrf2含量及蛋白表达减少(P<0.05),Nrf2 mRNA相对表达增多;与模型组比,针刺和艾灸组小鼠肾脏组织中Keap1含量、蛋白表达以及mRNA相对表达均减少(P<0.05);Nrf2含量、蛋白表达以及mRNA相对表达均增多(P<0.05)。结论针灸可以改善DDP肾损伤模型小鼠的肾功能,提升其抗氧化应激能力,从而改善DDP化疗所致的肾损伤,其作用机制可能与Keap1/Nrf2信号通路有关。

补中益气汤联合顺铂通过调控Wnt/β-catenin信号通路改善A549/DDP细胞耐药性的分子机制

目的:探究补中益气汤联合顺铂通过调控Wnt/β-catenin信号通路改善A549/DDP细胞耐药性的分子机制。方法:培养A549/DDP细胞并制备补中益气汤含药血清。采用siRNA沉默GSK-3β表达,检测各组A549/DDP细胞中GSK-3β蛋白的相对表达量;Western blot检测沉默GSK-3β后各组A549/DDP细胞β-catenin和Survivin表达;MTT法检测GSK-3β受抑对各组A549/DDP细胞顺铂IC_(50)的影响;采用Annexin V/PI染色法检测GSK-3β受抑对各组A549/DDP细胞凋亡的影响。结果:相较于空白对照组,siGSK-3β-592组对蛋白表达的抑制率达70%(P<0.05);RNAi技术沉默GSK-3β后,A549/DDP细胞中β-catenin和Survivin蛋白表达明显增加(P<0.05),单独顺铂治疗组与单独补中益气汤治疗组均可使β-catenin和Survivin蛋白表达明显下调(P<0.05),补中益气汤联合顺铂治疗组则可使β-catenin和Survivin蛋白表达下调更显著(P<0.05);RNAi技术沉默GSK-3β后,A549/DDP细胞顺铂IC_(50)显著升高(P<0.05),而补中益气汤仍可显著降低A549/DDP细胞的顺铂IC_(50)(P<0.05);GSK-3β表达受抑后,A549/DDP细胞的顺铂诱导凋亡率明显受抑制(P<0.05),而补中益气汤仍可明显提高A549/DDP细胞的顺铂诱导凋亡率(P<0.05)。结论:上调A549/DDP细胞中Wnt/β-catenin信号通路活性时,补中益气汤联合顺铂仍对A549/DDP细胞的顺铂耐药性有明显改善作用。