脓毒症并发急性肾损伤患儿血清中miR-93-5p和miR-424-5p的表达及临床意义

目的探讨血清中微小RNA-93-5p(miR-93-5p)和微小RNA-424-5p(miR-424-5p)在脓毒症并发急性肾损伤(S-AKI)患儿中的表达水平及其临床意义。方法选取2019年11月至2021年11月南阳市中心医院综合ICU收治的116例脓毒症患儿作为研究对象,根据脓毒症患儿是否并发AKI分为AKI组60例和非AKI组56例;比较两组患儿的一般资料和血清miR-93-5p、miR-424-5p及肾功能指标[血肌酐(Scr)、胱抑素C(Cys-C)]水平;采用Pearson法分析S-AKI患儿血清miR-93-5p、miR-424-5p与肾功能指标的相关性;采用多因素Logistic回归分析脓毒症患儿并发AKI的影响因素;采用受试者工作特征曲线(ROC)分析血清miR-93-5p、miR-424-5p水平对脓毒症患儿并发AKI的诊断价值。结果AKI组患儿的尿量为(1.52±0.31)mL·kg^(-1)·h^(-1)、血清miR-93-5p表达水平为0.62±0.14,均明显低于非AKI组的(1.87±0.36)mL·kg^(-1)·h^(-1)、(1.02±0.21),急性生理学与慢性健康状况评分(APACHEⅡ评分)、序贯器官衰竭评分(SOFA评分)、血清miR-424-5p表达水平、Scr、Cys-C水平分别为(17.35±5.01)分、(5.77±1.80)分、(2.36±0.51)、(182.84±43.31)μmol/L、(1.63±0.39)mg/L,明显高于非AKI组的(14.96±4.12)分、(5.10±1.41)分、(1.01±0.23)、(91.51±28.34)μmol/L、(0.96±0.28)mg/L,差异均有统计学意义(P<0.05);经Pearson法分析结果显示,S-AKI患儿血清miR-93-5p与Scr、Cys-C呈负相关(r=-0.621、-0.720,P<0.05),miR-424-5p与Scr、Cys-C呈正相关(r=0.503、0.538,P<0.05);经多因素Logistic回归分析结果显示,miR-424-5p、Scr、Cys-C是影响脓毒症患儿并发AKI的危险因素,miR-93-5p是保护因素(P<0.05);经ROC分析结果显示,血清miR-93-5p、miR-424-5p以及两者联合诊断脓毒血症患儿并发AKI的AUC分别为0.856、0.860、0.949,联合诊断的敏感度为90.00%,特异性为91.07%,两者联合优于血清miR-93-5p、miR-424-5p各自单独诊断(Z两者联合-miR-93-5p=2.897、Z两者联合-miR-424-5p=2.706,P=0.004、P=0.007)。结论S-AKI患儿血清miR-93-5p水平显著下调,miR-424-5p水平显著上调,两者联合诊断脓毒血症患儿并发AKI具有更高价值。

MicroRNA-363-5p靶向血小板反应蛋白-3调控心肌细胞肥大的作用机制研究

目的 探讨microRNA-363-5p(miR-363-5p)靶向血小板反应蛋白-3(THBS3)对心肌肥大的调节作用。方法 体外人心肌细胞(AC16)经血管紧张素Ⅱ(AngⅡ)处理复制心肌肥大体外模型,随后鬼笔环肽染色观察细胞骨架,Western blotting检测心肌肥大体外模型中胚胎期基因的蛋白表达,以确认模型复制的有效性。实时荧光定量聚合酶链反应检测心肌肥大体外模型中miR-363-5p表达。Western blotting检测肥大心肌细胞中转染miR-363-5p mimics和miR-363-5p inhibitor后,肥大相关表型的变化。双荧光素酶报告基因实验验证miR-363-5p与THBS3的3’-UTR结合作用。设计挽救实验,同时过表达THBS3与miR-363-5p,以评估THBS3是否介导miR-363-5p对心肌肥大的调控。结果 AngⅡ组细胞面积较对照组大(P <0.05),心房钠尿肽(ANP)、B型钠尿肽(BNP)、肌球蛋白β重链(β-MHC)及miR-363-5p较对照组高(P <0.05)。miR-363-5p mimics组miR-363-5p相对表达量较mimics-NC组高(P <0.05),miR-363-5p inhibitor组相对表达量较inhibitor-NC组低(P <0.05);miR-363-5p mimics组ANP、BNP、β-MHC相对表达量较mimics-NC组低(P <0.05),miR-363-5p inhibitor组相对表达量较inhibitor-NC组高(P <0.05)。miR-363-5p mimics组细胞面积较mimics-NC组小(P <0.05),miR-363-5p inhibitor组较inhibitor-NC组大(P <0.05)。miR-363-5p mimics+THBS3-WT组THBS3-WT荧光素酶活性较mimics-NC+THBS3-WT组低。mimics-NC+THBS3-MUT组与miR-363-5p mimics+THBS3-MUT组THBS3-MUT荧光素酶活性比较,差异无统计学意义(P>0.05)。miR-363-5p mimics组THBS3 mRNA和蛋白相对表达量较mimics-NC组低(P <0.05)。THBS3-OE组THBS3 mRNA和蛋白相对表达量较对照组、OE-NC组高(P <0.05)。THBS3-OE+miR-363-5p mimics组细胞面积较OE-NC+miR-363-5p mimics组大(P <0.05)。THBS3-OE+miR-363-5p mimics组ANP、BNP及β-MHC相对表达量较OE-NC+miR-363-5p mimics组高(P <0.05)。结论 过表达miR-363-5p可抑制AngⅡ对AC16细胞的促肥大作用,其机制与减少THBS3表达有关。

lncRNA NEAT1调节miR-424-5p/ELK4轴对ox-LDL诱导的血管内皮细胞损伤、Lp-PLA2和CRP水平的影响

目的:探讨长链非编码RNA核旁斑组装转录本1(lncRNA NEAT1)在氧化型低密度脂蛋白(ox-LDL)诱导的血管内皮细胞损伤中的分子机制和功能。方法:收集健康人和动脉粥样硬化(AS)病人血液标本并通过实时荧光定量逆转录聚合酶链式反应(qRT-PCR)检测血清中lncRNA NEAT1、微小RNA-424-5p(miR-424-5p)和ETS域蛋白4(ELK4)mRNA表达水平。体外培养人脐静脉内皮细胞(HUVEC),qRT-PCR和蛋白免疫印迹法(Western Blot)检测细胞中lncRNA NEAT1、miR-424-5p和ELK4表达情况;细胞计数试剂盒(CCK-8)法和膜联蛋白V-异硫氰酸荧光素/碘化丙啶(Annexin V-FITC/PI)法检测HUVEC细胞增殖活力和凋亡情况;酶联免疫吸附法(ELISA)测定HUVEC中乳酸脱氢酶(LDH)释放量、肿瘤坏死因子-α(TNF-α)和白细胞介素(IL)-1β含量、脂蛋白磷脂酶A2(Lp-PLA2)和C反应蛋白(CRP)水平;采用双荧光素酶报告基因测定lncRNA NEAT1、miR-424-5p和ELK4之间的靶向相互作用。进行动物实验以评估lncRNA NEAT1在体内AS进展中的作用。结果:lncRNA NEAT1在AS病人血清和ox-LDL诱导的HUVEC中显著上调(P<0.05)。lncRNA NEAT1的沉默可削弱ox-LDL引发的细胞毒性,降低Lp-PLA2和CRP水平,并减少ApoE^(-/-)小鼠的脂质异常分泌(P<0.05)。miR-424-5p是lncRNA NEAT1在调节ox-LDL诱导的HUVEC损伤中的功能介质,ELK4是miR-424-5p的直接靶标(P<0.05)。miR-424-5p的抑制或ELK4的过表达逆转了lncRNA NEAT1沉默对ox-LDL诱导的HUVEC细胞损伤的影响(P<0.05)。结论:沉默lncRNA NEAT1可通过调控miR-424-5p/ELK4轴保护HUVEC免受ox-LDL触发的细胞毒性,降低Lp-PLA2和CRP水平。

Urinary exosomal microRNA-145-5p and microRNA-27a-3p act as noninvasive diagnostic biomarkers for diabetic kidney disease

BACKGROUND Diabetic kidney disease(DKD),characterized by increased urinary microalbumin levels and decreased renal function,is the primary cause of end-stage renal di-sease.Its pathological mechanisms are complicated and multifactorial;Therefore,sensitive and specific biomarkers are needed.Urinary exosome originate from diverse renal cells in nephron segments and partially mirror the pathological changes in the kidney.The microRNAs(miRNAs)in urinary exosome are remark-ably stable and highly tissue-specific for the kidney.METHODS Type 2 diabetic mellitus(T2DM)patients were recruited from the Second Hospital of Hebei Medical University and were divided into two groups:DM,diabetic pa-tients without albuminuria[urinary albumin to creatinine ratio(UACR)<30 mg/g]and DKD,diabetic patients with albuminuria(UACR≥30 mg/g).Healthy subjects were the normal control(NC)group.Urinary exosomal miR-145-5p,miR-27a-3p,and miR-29c-3p,were detected using real-time quantitative polymerase chain reaction.The correlation between exosomal miRNAs and the clinical in-dexes was evaluated.The diagnostic values of exosomal miR-145-5p and miR-27a-3p in DKD were determined using receiver operating characteristic(ROC)analysis.Biological functions of miR-145-5p were investigated by performing RESULTS Urinary exosomal expression of miR-145-5p and miR-27a-3p was more upregulated in the DKD group than in the DM group(miR-145-5p:4.54±1.45 vs 1.95±0.93,P<0.001;miR-27a-3p:2.33±0.79 vs 1.71±0.76,P<0.05)and the NC group(miR-145-5p:4.54±1.45 vs 1.55±0.83,P<0.001;miR-27a-3p:2.33±0.79 vs 1.10±0.51,P<0.001).The exosomal miR-145-5p and miR-27a-3p positively correlated with albuminuria and serum creatinine and negatively correlated with the estimated glomerular filtration rate.miR-27a-3p was also closely related to blood glucose,gly-cosylated hemoglobin A1c,and low-density lipoprotein cholesterol.ROC analysis revealed that miR-145-5p had a better area under the curve of 0.88[95%confidence interval(CI):0.784-0.985,P<0.0001]in diagnosing DKD than miR-27a-3p with 0.71(95%CI:0.547-0.871,P=0.0239).Bioinformatics analysis revealed that the target genes of miR-145-5p were located in the actin filament,cytoskeleton,and extracellular exosome and were involved in the pathological processes of DKD,including apoptosis,inflammation,and fibrosis.CONCLUSION Urinary exosomal miR-145-5p and miR-27a-3p may serve as novel noninvasive diagnostic biomarkers or promising therapeutic targets for DKD.

miR-126-5p通过靶向TRAF3抑制糖氧剥夺再灌注介导的HT22细胞凋亡和炎症

目的探讨miR-126-5p通过靶向肿瘤坏死因子受体相关因子3(tumor necrosis factor receptor-associated factor 3,TRAF3)对糖氧剥夺再灌注(oxygen-glucose deprivation/reperfusion,OGD/R)介导的小鼠海马神经元细胞HT22细胞凋亡和炎症的影响。方法模拟缺血/再灌注损伤(ischemia/reperfusion,I/R)损伤在体外建立氧糖剥夺/复氧(oxygen-glucose deprivation/reperfusion,OGD/R)细胞模型,分析miR-126-5p与TRAF3靶向关系及对HT22细胞凋亡和炎症反应的影响。结果与对照组比较,OGD/R组中miR-126-5p下调而TRAF3 mRNA及蛋白水平上调,细胞存活率及Bcl-2蛋白水平降低,乳酸脱氢酶(lactate dehydrogenase,LDH)释放量、细胞凋亡率、Bax及Cleaved caspase-3蛋白水平升高(P均<0.05)。与OGD/R+mimic-NC组比较,OGD/R+miR-mimic组、OGD+miR-mimic+pcDNA组TRAF3蛋白水平、LDH释放量、细胞凋亡率、Bax及Cleaved caspase-3蛋白水平明显降低,细胞存活率及Bcl-2蛋白水平升高,而OGD+miR-mimic+pcDNA-TRAF3组各指标升高,细胞存活率明显下降(P均<0.05)。结论miR-126-5p通过靶向TRAF3,抑制OGD/R介导的HT22细胞凋亡和炎症反应,从而对神经元细胞发挥保护作用。

血清microRNA-186-5p、microRNA-328-5p表达和乳腺癌患者临床病理特征与新辅助化疗效果的关系

目的探讨血清microRNA-186-5p(miR-186-5p)、microRNA-328-5p(miR-328-5p)表达和乳腺癌患者临床病理特征与新辅助化疗效果的关系。方法选取2019年2月—2022年2月广西壮族自治区妇幼保健院收治的乳腺癌患者105例作为乳腺癌组,另随机选取该院与乳腺癌患者年龄相匹配的57例健康体检女性作为对照组。乳腺癌患者均接受新辅助化疗,根据化疗反应分为耐药组(30例)和敏感组(75例)。qRT-PCR检测血清miR-186-5p、miR-328-5p表达,比较不同临床病理特征乳腺癌患者血清miR-186-5p、miR-328-5p表达的差异,比较耐药组和敏感组血清miR-186-5p、miR-328-5p表达的差异。多因素Logistic逐步回归分析影响乳腺癌患者新辅助化疗效果的因素。绘制受试者工作特征(ROC)曲线,分析miR-186-5p、miR-328-5p预测乳腺癌患者对新辅助化疗效果的价值。结果乳腺癌组血清miR-186-5p、miR-328-5p mRNA相对表达量低于对照组(P<0.05)。T_(3)、T_(4)期、N_(1~3)期、HER2阳性乳腺癌患者血清miR-186-5p、miR-328-5p mRNA相对表达量低于T_(2)期、N_(0)期、HER2阴性乳腺癌患者(P<0.05)。耐药组血清miR-186-5p、miR-328-5p mRNA相对表达量低于敏感组(P<0.05),T_(3)、T_(4)期、N_(1~3)期占比高于敏感组(P<0.05)。N分期[OR=3.497(95%CI:1.737,7.041)]、miR-186-5p[OR=1.680(95%CI:1.169,2.415)]、miR-328-5p[OR=1.519(95%CI:1.134,2.034)]是影响乳腺癌患者新辅助化疗耐药的危险因素(P<0.05)。ROC曲线分析结果显示,miR-186-5p、miR-328-5p及两者联合预测乳腺癌患者新辅助化疗效果的敏感性分别为76.67%(95%CI:0.553,0.856)、70.00%(95%CI:0.510,0.808)、90.00%(95%CI:0.768,0.977),特异性分别为74.67%(95%CI:0.528,0.831)、76.00%(95%CI:0.544,0.840)、90.67%(95%CI:0.776,0.984)。结论乳腺癌患者血清miR-186-5p、miR-328-5p表达下调,可能与乳腺癌患者临床病理特征及化疗耐药有关,均可作为新辅助化疗疗效评估的标志物。

MiR-424-5p调控PD-1/PD-L1信号通路对弥漫大B细胞淋巴瘤细胞耐药性的影响

目的:探讨微小RNA-424-5p(mi R-424-5p)调控程序性死亡受体-1(PD-1)/程序性死亡配体-1(PD-L1)信号通路对弥漫大B细胞淋巴瘤细胞耐药性的影响。方法:诱导人弥漫大B细胞淋巴瘤细胞系CRL2631细胞构建CRL2631-CHOP耐药细胞株。RT-q PCR和Western blot分别检测CRL2631细胞和CRL2631-CHOP细胞中mi R-424-5p、PD-L1 m RNA和蛋白及多元药物抗性基因-1(MDR-1)蛋白表达水平。双荧光素酶报告基因实验验证mi R-424-5p的靶标基因。使用mi RNA模拟/干扰技术和噻唑蓝法检测CRL2631细胞和CRL2631-CHOP细胞对CHOP方案化疗药物的耐药性。结果:与CRL2631细胞相比,CRL2631-CHOP细胞对CHOP方案化疗药物的耐药性显著增高,细胞中MDR-1蛋白水平(P<0.05)、PD-L1 m RNA和蛋白水平显著增高(均P<0.001),而mi R-424-5p相对水平显著降低(P<0.001)。双荧光素酶报告基因实验结果显示,PD-L1是mi R-424-5p下游直接靶标基因(P<0.001)。转染mi R-424-5p inhibitor后,CRL2631细胞对CHOP方案化疗药物的耐药性增高,且MDR-1蛋白水平(P<0.01)、PD-L1 m RNA和蛋白水平显著增高(均P<0.01);转染mi R-424-5p mimics后,CRL2631-CHOP细胞对CHOP药物的耐药性降低,且MDR-1蛋白水平(P<0.001)、PD-L1 m RNA和蛋白水平显著降低(均P<0.001);过表达PD-L1可逆转上调mi R-424-5p对PD-L1的抑制作用(P<0.001)。结论:下调mi R-424-5p通过调控PD-1/PD-L1信号通路增强了弥漫大B细胞淋巴瘤细胞的耐药性。

紫草素调控MicroRNA-382-5p抑制人增生性瘢痕成纤维细胞纤维化

背景:目前已有研究表明紫草素具有治疗增生性瘢痕的潜力,且miRNA参与增生性瘢痕的病理机制调控,猜测紫草素有可能通过影响miRNA调控增生性瘢痕的发生发展。目的:探讨紫草素通过影响MicroRNA-382-5p对人增生性瘢痕成纤维细胞纤维化的作用机制。方法:收集宁夏医科大学总医院烧伤整形外科提供的增生性瘢痕组织及瘢痕旁正常皮肤组织(瘢痕旁3 cm以内),并分别分离出人增生性瘢痕成纤维细胞和正常成纤维细胞用于后续实验。苏木精-伊红染色鉴定正常皮肤和增生性瘢痕;免疫荧光鉴定成纤维细胞;采用实时荧光定量PCR从组织水平检测MicroRNA-382-5p相对表达水平。将增生性瘢痕成纤维细胞随机分为紫草素组(紫草素溶于二甲基亚砜配成浓度为13.46μmol/L的药物干预细胞24 h)、二甲基亚砜组、MicroRNA-382-5p阴性对照组、MicroRNA-382-5p抑制组、紫草素+MicroRNA-382-5p阴性对照组及紫草素+MicroRNA-382-5p过表达组。实时荧光定量PCR检测Ⅰ型胶原蛋白α1、Ⅲ型胶原蛋白α1和α-平滑肌肌动蛋白mRNA表达;Western blot检测Ⅰ型胶原蛋白α1、Ⅲ型胶原蛋白α1和α-平滑肌肌动蛋白的蛋白表达;CCK-8法检测细胞活性;划痕实验检测细胞迁移能力。结果与结论:①与正常皮肤成纤维细胞相比,增生性瘢痕成纤维细胞增殖活性更强(P<0.01);②与二甲基亚砜组相比,紫草素组可以下调增生性瘢痕成纤维细胞中Ⅰ型胶原蛋白α1、Ⅲ型胶原蛋白α1和α-平滑肌肌动蛋白的表达水平(mRNA:P<0.01,蛋白:P<0.01),并抑制增生性瘢痕成纤维细胞迁移(P<0.05);③与正常皮肤相比,MicroRNA-382-5p在增生性瘢痕中呈高表达(P<0.01),且紫草素能下调增生性瘢痕成纤维细胞中MicroRNA-382-5p的表达(P<0.01);④敲低MicroRNA-382-5p能下调增生性瘢痕成纤维细胞中Ⅰ型胶原蛋白α1、Ⅲ型胶原蛋白α1和α-平滑肌肌动蛋白的表达水平(mRNA:P<0.01,蛋白:P<0.01),并抑制增生性瘢痕成纤维细胞迁移(P<0.05);⑤过表达MicroRNA-382-5p能上调在紫草素影响下增生性瘢痕成纤维细胞中Ⅰ型胶原蛋白α1、Ⅲ型胶原蛋白α1和α-平滑肌肌动蛋白的表达水平(mRNA:P<0.01,蛋白:P<0.01),并促进增生性瘢痕成纤维细胞迁移(P<0.01);⑥提示紫草素可通过下调MicroRNA-382-5p的表达抑制增生性瘢痕成纤维细胞的纤维化和迁移。

MiRNA-145-5p inhibits gastric cancer progression via the serpin family E member 1-extracellular signal-regulated kinase-1/2 axis

BACKGROUND MicroRNAs(miRNAs)regulate gene expression and play a critical role in cancer physiology.However,there is still a limited understanding of the function and regulatory mechanism of miRNAs in gastric cancer(GC).AIM To investigate the role and molecular mechanism of miRNA-145-5p(miR145-5p)in the progression of GC.METHODS Real-time polymerase chain reaction(RT-PCR)was used to detect miRNA expression in human GC tissues and cells.The ability of cancer cells to migrate and invade was assessed using wound-healing and transwell assays,respectively.Cell proliferation was measured using cell counting kit-8 and colony formation assays,and apoptosis was evaluated using flow cytometry.Expression of the epithelial-mesenchymal transition(EMT)-associated protein was determined by Western blot.Targets of miR-145-5p were predicated using bioinformatics analysis and verified using a dual-luciferase reporter system.Serpin family E member 1(SERPINE1)expression in GC tissues and cells was evaluated using RT-PCR and immunohistochemical staining.The correlation between SERPINE1 expression and overall patient survival was determined using Kaplan-Meier plot analysis.The association between SERPINE1 and GC progression was also tested.A rescue experiment of SERPINE1 overexpression was conducted to verify the relationship between this protein and miR-145-5p.The mechanism by which miR-145-5p influences GC progression was further explored by assessing tumor formation in nude mice.RESULTS GC tissues and cells had reduced miR-145-5p expression and SERPINE1 was identified as a direct target of this miRNA.Overexpression of miR-145-5p was associated with decreased GC cell proliferation,invasion,migration,and EMT,and these effects were reversed by forcing SERPINE1 expression.Kaplan-Meier plot analysis revealed that patients with higher SERPINE1 expression had a shorter survival rate than those with lower SERPINE1 expression.Nude mouse tumorigenesis experiments confirmed that miR-145-5p targets SERPINE1 to regulate extracellular signal-regulated kinase-1/2(ERK1/2).CONCLUSION This study found that miR-145-5p inhibits tumor progression and is expressed in lower amounts in patients with GC.MiR-145-5p was found to affect GC cell proliferation,migration,and invasion by negatively regulating SERPINE1 levels and controlling the ERK1/2 pathway.

Exercise-induced modulation of miR-149-5p and MMP9 in LPS-triggered diabetic myoblast ER stress: licorice glycoside E as a potential therapeutic target

Background:This study explores the relationship between endoplasmic reticulum(ER)stress and diabetes,particularly focusing on the impact of physical exercise on ER stress mechanisms and identifying potential therapeutic drugs and targets for diabetes-related sepsis.The research also incorporates traditional physical therapy perspectives,emphasizing the genomic insights gained from exercise therapy in disease management and prevention.Methods:Gene analysis was conducted on the GSE168796 and GSE94717 datasets to identify ER stress-related genes.Gene interactions and immune cell correlations were mapped using GeneCard and STRING databases.A screening of 2,456 compounds from the TCMSP database was performed to identify potential therapeutic agents,with a focus on their docking potential.Techniques such as luciferase reporter gene assay and RNA interference were used to examine the interactions between microRNA-149-5p and MMP9.Results:The study identified 2,006 differentially expressed genes and 616 miRNAs.Key genes like MMP9,TNF-α,and IL1B were linked to an immunosuppressive state.Licorice glycoside E demonstrated high affinity for MMP9,suggesting its potential effectiveness in treating diabetes.The constructed miRNA network highlighted the regulatory roles of MMP9,IL1B,IFNG,and TNF-α.Experimental evidence confirmed the binding of microRNA-149-5p to MMP9,impacting apoptosis in diabetic cells.Conclusion:The findings highlight the regulatory role of microRNA-149-5p in managing MMP9,a crucial gene in diabetes pathophysiology.Licorice glycoside E emerges as a promising treatment option for diabetes,especially targeting MMP9 affected by ER stress.The study also underscores the significance of physical exercise in modulating ER stress pathways in diabetes management,bridging traditional physical therapy and modern scientific understanding.Our study has limitations.It focuses on the microRNA-149-5p-MMP9 network in sepsis,using cell-based methods without animal or clinical trials.Despite strong in vitro findings,in vivo studies are needed to confirm licorice glycoside E’s therapeutic potential and understand the microRNA-149-5p-MMP9 dynamics in real conditions.

妊娠糖尿病患者血清microRNA-873-5p、ZEB1与胰岛素抵抗、母婴结局的相关性研究

目的探究妊娠糖尿病(GDM)患者血清microRNA-873-5p(miR-873-5p)、E盒结合锌指蛋白1(ZEB1)与胰岛素抵抗、母婴结局的相关性。方法选取连云港市第一人民医院2021年1月—2022年6月收治的137例GDM患者为研究组,另选取同期该院体检且一般资料与研究组患者相匹配的137例健康孕妇为对照组。实时荧光定量聚合酶链反应(q RT-PCR)检测两组研究对象血清miR-873-5p、ZEB1的表达;Pearson法分析GDM患者血清miR-873-5p、ZEB1与胰岛素抵抗指数(HOMA-IR)的相关性;多因素一般Logistic回归分析影响GDM患者母婴结局的相关因素;绘制受试者工作特征(ROC)曲线分析miR-873-5p、ZEB1对GDM患者母婴不良结局的预测效能。结果研究组患者的空腹血糖(FPG)、空腹胰岛素(FINS)及HOMA-IR均高于对照组(P<0.05);研究组患者血清miR-873-5p、ZEB1水平均高于对照组(P<0.05);Pearson法分析结果显示,GDM患者血清miR-873-5p表达(r=0.754,P=0.000)、ZEB1表达(r=0.771,P=0.000)与HOMA-IR均呈正相关;母婴不良结局组的GDM患者血清miR-873-5p、ZEB1表达均高于良好结局组(P<0.05);FPG[OR=1.366(95%CI:1.065,1.752)]、FINS[OR=1.619(95%CI:1.214,2.160)]、HOMA-IR[OR=1.550(95%CI:1.146,2.096)]、miR-873-5p[OR=1.772(95%CI:1.250,2.512)]及ZEB1[OR=1.512(95%CI:1.050,2.177)]均为GDM患者发生母婴不良结局的危险因素(P<0.05);血清miR-873-5p、ZEB1及两者联合预测GDM患者发生母婴不良结局的敏感性分别为71.11%(95%CI:0.670,0.821)、66.67%(95%CI:0.620,0.715)和65.89%(95%CI:0.617,0.727),特异性分别为70.65%(95%CI:0.670,0.821)、85.87%(95%CI:0.775,0.897)和88.04%(95%CI:0.785,0.910),两者联合检测对GDM患者的母婴结局具有较高的特异性。结论GDM患者血清miR-873-5p、ZEB1表达与胰岛素抵抗密切相关,并且两者联合检测对GDM患者的母婴结局具有较好的预测效能。

麻防犀角地黄汤通过调控microRNA-491-5p影响PI3K/Akt/mTOR通路治疗银屑病的机制

目的 观察麻防犀角地黄汤对银屑病小鼠模型的影响,探讨麻防犀角地黄汤治疗银屑病的作用机制。方法 构建咪喹莫特银屑病小鼠模型,灌胃给药麻防犀角地黄汤,观察模型外观及组织病理学改变,Real time PCR检测皮损组织中microRNA-491-5p、PI3K、Akt、mTOR mRNA的表达,Western blot检测皮损组织中PI3K、p-PI3K、Akt、p-Akt、mTOR、p-mTOR蛋白的表达。结果 麻防犀角地黄汤能改善小鼠皮损、PASI评分、耳廓外缘厚度、组织病理、体质量等指标,上调microRNA-491-5p mRNA的表达,下调PI3K、Akt、mTOR mRNA的表达量,抑制p-PI3K、p-Akt、p-mTOR的蛋白表达,并表现出部分量效相关性。结论 麻防犀角地黄汤可能通过调控microRNA-491-5p影响PI3K/Akt/mTOR信号通路在银屑病的治疗中发挥作用。

microRNA-424-5p对人胃癌细胞SGC-7901自噬的影响及机制

目的研究microRNA-424-5p(miR-424-5p)对人胃癌细胞SGC-7901自噬的影响及可能机制。方法培养人正常胃黏膜上皮细胞GES和人胃癌细胞SGC-7901,应用实时定量PCR方法检测miR-424-5p的表达水平;应用Lipofectamine LTX试剂将化学合成的miR-424-5p agomir和miR-424-5p antagomir转染人胃癌细胞SGC-7901,验证转染效率后应用MTT方法检测细胞活力;应用免疫荧光法检测自噬标记物微管相关蛋白轻链-3(LC3)和自噬降解底物p62/SQSTM1在SGC-7901细胞的分布;应用Western blot方法检测LC3-Ⅱ、p62/SQSTM1和自噬相关蛋白Beclin1的蛋白表达水平。结果 miR-424-5p在人胃癌细胞SGC-7901中呈低表达,miR-424-5p过表达显著抑制人胃癌细胞SGC-7901的细胞活力,miR-424-5p表达沉默的作用效果与之相反。miR-424-5p过表达后自噬标记物LC3在SGC-7901细胞的胞浆内呈点状分布,荧光表达显著增强,并且LC3-II的蛋白表达水平显著上调,同时伴有自噬降解底物p62/SQSTM1在细胞浆内荧光表达显著减弱,蛋白表达下调,此外,自噬相关蛋白Beclin1的蛋白表达水平显著上调;miR-424-5p表达沉默的作用效果与之相反。结论 miR-424-5p过表达明显抑制人胃癌细胞SGC-7901的细胞活力,诱导细胞发生自噬,其机制之一可能与自噬相关蛋白Beclin1上调有关。

MicroRNA-129-5p、SOX4在宫颈癌组织中的表达及其与患者临床病理特征、预后的关系

目的 探讨宫颈癌组织中micro RNA-129-5p(mi R-129-5p)、性别决定区Y框蛋白4(SOX4)表达与临床病理特征及预后的关系。方法 选取2017年6月-2019年8月湖北民族大学附属民大医院101例宫颈癌患者的宫颈癌组织、癌旁组织标本及其临床资料,根据患者生存情况将其分为生存组79例和死亡组22例。采用免疫组织化学法检测SOX4蛋白阳性表达,采用实时荧光定量聚合酶链反应(q RT-PCR)检测mi R-129-5p m RNA相对表达量。绘制Kaplan-Meier曲线分析mi R-129-5p、SOX4表达与宫颈癌患者3年生存率的关系;采用多因素Cox回归分析宫颈癌患者预后的影响因素。结果 宫颈癌组织mi R-129-5p m RNA相对表达量低于癌旁组织(P<0.05),SOX4蛋白阳性表达率高于癌旁组织(P<0.05)。FIGO分期Ⅱ期、低分化、有淋巴结转移的宫颈癌患者组织中mi R-129-5p高表达、SOX4蛋白阳性表达率高于FIGO分期Ⅰ期、中/高分化、无淋巴结转移患者(P<0.05)。mi R-129-5p低表达患者3年生存率低于mi R-129-5p高表达患者(P<0.05);SOX4蛋白阳性表达患者3年生存率低于SOX4蛋白阴性表达患者(P<0.05)。死亡组FIGO分期Ⅱ期患者比例高于生存组(P<0.05)。SOX4蛋白阳性表达[■=2.793(95%CI:1.495,5.219)]是宫颈癌患者3年内死亡的危险因素,mi R-129-5p高表达[■=0.809(95%CI:0.700,0.935)]是宫颈癌患者3年内死亡的保护因素(P<0.05)。结论 宫颈癌组织中mi R-129-5p表达降低、SOX4表达升高,两者表达与FIGO分期、分化程度、淋巴结转移及3年预后有关,有可作为预后评估的生物标志物。

微小RNA-424-5P靶向调控HMGA1基因对胃癌细胞生长、侵袭的影响

目的 研究微小RNA(miR)-424-5P对高迁移率族蛋白(HMG)A1的靶向调控及对胃癌细胞增殖、迁移的作用。方法 将人胃癌BGC-823细胞复苏后,应用10%胎牛血清,在5%二氧化碳和37℃培养箱中进行培养,应用miR-424-5P抑制物(inhibitor)转染的BGC-823细胞列为anti-miR-424-5P组。应用阴性对照进行转染的BGC-823细胞列为anti-NC组,不进行转染的BGC-823细胞列为对照组,细胞转染后各组继续在培养箱中培养。应用qRT-聚合酶链反应(PCR)检测各组miR-424-5P的相对表达水平;应用四甲基噻唑蓝(MTT)研究miR-424-5P对细胞增殖的影响;应用划痕实验检测miR-424-5P对细胞迁移的影响;应用transwell实验研究miR-424-5P对细胞侵袭的影响。应用免疫印迹实验对各组HMGA1蛋白相对表达水平进行检测。结果 转染48 h后qRT-PCR结果表明,anti-miR-424-5P组miR-424-5P相对表达量明显低于对照组和anti-NC组(P<0.05)。对BGC-823细胞进行转染48 h后,miR-424-5P OD值显著低于anti-NC组和对照组(P<0.05)。与anti-NC组和对照组相比,anti-miR-424-5P组迁移距离显著较低(P<0.05)。与anti-NC组和对照组相比,anti-miR-424-5P组迁移数量显著较少(P<0.05)。与对照组和anti-NC组比较,anti-miR-424-5P组HMGA1蛋白的表达水平显著较高(P<0.05)。结论 miR-424-5P能够靶向调控HMGA1对胃癌细胞的生长、侵袭,可为胃癌的治疗提供新的靶点和治疗策略。

miR-424-5p在急性髓系白血病中的表达及临床意义

目的探讨miR-424-5p在急性髓系白血病(acute myeloid leukemia,AML)患者中的表达及临床意义。方法选择2018年1月至2019年12月于西安交通大学第二附属医院血液内科就诊的58例AML患者骨髓标本作为研究对象,同时收集13例缺铁性贫血(irondeficiency anemia,IDA)患者的骨髓标本作为对照,通过实时定量PCR方法检测两组骨髓标本中miR-424-5p的相对表达量。通过受试者工作特征曲线(receiver operating characteristic curve,ROC)分析miR-424-5p对AML的诊断价值。总结58例AML患者miR-424-5p表达谱及临床资料,用Kaplan-Meier法分析miR-424-5p与AML总体生存期(overall survival,OS)的关系,并分析其表达水平与临床资料的相关性。建立COX比例风险模型进行多因素分析。利用在线数据库预测miR-424-5p下游通路,探究miR-424-5p在AML发病中可能发挥的作用机制。结果miR-424-5p在初发AML患者中低表达(P=0.002),其表达量与患者年龄、外周血白细胞数有关(P<0.05)。ROC曲线下面积为0.776,95%CI为0.663~0.889,可有效区分AML患者和IDA患者。分析临床资料发现miR-424-5p的表达水平降低和患者的OS延长显著相关(P=0.005)。建立COX比例风险模型,结果显示miR-424-5p表达量在模型中有统计学意义(P<0.05),且miR-424-5p表达量>12.478患者发生死亡的风险是≤12.478患者的3.315倍。StarbaseV2.0数据库预测发现miR-424-5p的靶基因可能通过TRAIL信号通路参与AML的发生发展。结论miR-424-5p在初发AML患者中低表达,具有一定的辅助诊断价值,其表达水平与AML患者年龄、外周血白细胞数相关,表达水平升高与AML患者的预后不良显著相关,有望成为AML的潜在预后标志物。

MicroRNA-122-5P通过靶向MMP-9抑制TPA诱导的SW480细胞侵袭迁移能力

目的:研究miR-122-5p对TPA诱导人结直肠癌SW480细胞MMP-9表达及侵袭迁移的影响。方法:利用生物信息学筛选结直肠癌差异基因,预测其靶基因miRNA。用TPA(100nM)处理SW480细胞,通过RT-qPCR、Western blot法检测基因和蛋白表达水平;明胶酶谱法检测MMP-9细胞外分泌情况;Transwell检测细胞侵袭和迁移能力。结果:MMP-9在结肠癌组织中高表达,筛选出上游靶基因miR-122-5P;TPA诱导MMP-9 mRNA表达呈时间依赖性上调(P<0.01),诱导miR-122-5p的表达下调(P<0.01);过表达miR-122-5p明显下调TPA诱导的MMP-9 mRNA和蛋白表达(P<0.05),且MMP-9胞外分泌减少,细胞的侵袭、迁移能力显著下降(P<0.01)。结论:miR-122-5p可能通过调控TPA诱导MMP-9的表达,进而抑制结直肠癌SW480细胞侵袭和迁移能力,为克服结直肠癌转移研究提供新的思路。

MicroRNA-766-5p靶向SCAI对宫颈癌细胞增殖、周期和凋亡的作用

目的研究MicroRNA-766-5p靶向肿瘤细胞侵袭抑制因子(SCAI)对宫颈癌细胞增殖、周期和凋亡的作用。方法选取人宫颈癌MCF-7细胞模型;CCK8检测细胞增殖;流式细胞术分析细胞周期;Western blot检测细胞周期和凋亡相关蛋白表达。结果MicroRNA-766-5p靶向SCAI高效抑制人宫颈癌MCF-7细胞增殖,48 h处理的IC50为(49.33±7.02)nmol/L。低、高药物浓度实验组减少B细胞特性莫洛尼鼠白血病病毒插入位点1(BMI-1)和细胞周期素D1(CyclinD1)、细胞周期蛋白D1(CyclinD1),增加细胞周期素B1(CyclinB1)和P21,G2/M期周期阻滞,促进促凋亡蛋白[Bcl-2相关X蛋白(Bax)、裂解型多聚ADP-核糖聚合酶(c-PARP)]和抑制凋亡蛋白Bcl-2表达。结论MicroRNA-766-5p靶向SCAI能抑制宫颈癌细胞增殖,促进细胞周期阻滞和凋亡。

MicroRNA-409-5p Inhibits GIST Tumorigenesis and Improves Imatinib Resistance by Targeting KDM4D Expression

Objective Gastrointestinal stromal tumors(GISTs)can rapidly proliferate through angiogenesis.Previous studies indicated the potential influence of microRNA on the progression of tumor immature angiogenesis.This study aimed to explore the specific mechanism by which microRNA-409-5p(miR-409-5p)contributes to GIST.Methods To identify genes potentially involved in the development and progression of GIST,the differences of miR-409-5p between tumors and adjacent tissues were first analyzed.Following this analysis,target genes were predicted.To further investigate the function of miRNA in GIST cells,two GIST cell lines(GIST-T1 and GIST882)were transfected with lentiviruses that stably expressed miR-409-5p and scrambled miRNA(negative control).Later,the cells were subjected to Western blotting and ELSA to determine any differences in angiogenesis-related genes.Results In GISTs,there was a decrease in the expression levels of miR-409-5p compared to the adjacent tissues.It was observed that the upregulation of miR-409-5p in GIST cell lines effectively inhibited the proteins hypoxia-inducible transcription factor 1β(HIF1β)and vascular endothelial growth factor A(VEGF-A).Further investigations revealed that miR-409-5p acted as an inhibitor of angiogenesis by binding to the 3′-UTR of Lysine-specific demethylase 4D(KDM4D)mRNA.Moreover,the combination of miR-409-5p with imatinib enhanced its inhibitory effect on angiogenesis.Conclusion This study demonstrated that the miRNA-409-5p/KDM4D/HIF1β/VEGF-A signaling pathway could serve as a novel target for the development of therapeutic strategies for the treatment of imatinib-resistance in GIST patients.

MicroRNA-183-5p在动脉粥样硬化患者中的表达及其临床意义

目的分析microRNA-183-5p(miR-183-5p)在动脉粥样硬化患者中的表达及其临床意义。方法选取2021年1月—2022年8月四川省人民医院收治的经血管造影确诊的103例动脉粥样硬化患者为研究组,选取同期该院年龄相当的90例健康体检者为健康组。采用实时荧光定量聚合酶链反应(qRT-PCR)检测两组患者血清miR-183-5p的表达,绘制受试者工作特征(ROC)曲线,分析miR-183-5p在动脉粥样硬化中的诊断价值。结果研究组血清miR-183-5p mRNA相对表达量高于健康组(P<0.05);研究组中高Gensini积分组患者血清miR-183-5p mRNA相对表达量高于低Gensini积分组(P<0.05);Pearson相关性分析结果显示,miR-183-5p与C反应蛋白、颈动脉内中膜厚度及Gensini积分呈正相关(r=0.664、0.571和0.712,均P<0.05);ROC曲线分析结果显示,miR-183-5p诊断动脉粥样硬化的截断值为2.08,敏感性和特异性分别为87.8%(95%CI:0.832,0.924)和91.6%(95%CI:0.877,0.955)。结论动脉粥样硬化患者血清miR-183-5p高表达,能够辅助区分冠状动脉狭窄程度,可作为动脉粥样硬化临床诊断的重要生物标志物。