Significance of vascular endothelial growth factor messenger RNA expression in gastric cancer

IM To study VEGF mRNA expression in gastric carcinoma and to clarify the association of its expression with the clinicopathologic features of the disease.METHODS In situ hybridization (ISH) and histochemistry were used to examine and analyze the expression of VEGF mRNA and antigen, and microvessel count (MVC) in 28 cases of gastric carcinomatous tissue in combination with clinical materials.RESULTS Ninteen of 28 gastric carcinomas were positive for VEGF mRNA. VEGF mRNA was mainly expressed in malignant cells and not in normal epithelium of gastric mucosa. Its expression was further increased in tumor cells adjacent to tumor necrosis zones, where stromal cells expressed VEGF mRNA occasionally. There was a close correlation between MVC and VEGF mRNA positivity (P<0005). High VEGF mRNA levels were significantly associated with serosal invasion, lymph node metastasis and TNM staging (P<005, respectively).CONCLUSION VEGF mRNA expression is associated with tumor invasion and metastasis by stimulating angiogenesis in gastric carcinoma.expression; endothelial growth factor.

Expression of alpha-fetoprotein messenger RNA in BEL-7404 human hepatoma cells and effect of L-4-oxalysine on the expression

AIM To investigate alpha-fetoprotein (AFP) mRNA expression in BEL-7404 human hepatoma cells and the effect of L-4-oxalysine (OXL) on the expression.METHODS BEl-7404 human hepatoma cells were maintained in RPMI 1640 media. Human AFP cDNA probe was labelled with digoxigenin-11-dUTP by the random primer labelling method. The expression of AFP mRNA in Bel-7404 cells was determined by an in situ hybridization technique with digoxigenin-labelled human AFP cDNA probe. The positive intensities of AFP mRNA in cells were analyzed by microspectrophotometer and expressed as absorbance at 470nm. For the experiment with OXL, cells were incubated with various concentrations of the agent for 72h.RESULTS Essentially all the hepatoma cells contained AFP mRNA in the cytoplasm, although in various amounts. The specificity of the hybridization reaction was confirmed by control experiments in which the use of RNase-treated BEL-7404 cells, non-AFP-producing cells (HL-60 human leukemia cells) or a nonspecific cDNA probe resulted in negative hybridization. When the cells were treated with OXL (25, 50mg/L), the content of AFP mRNA in the cytoplasm was decreased with the inhibition percentages of 34.3% and 70.1%, respectively (P＜0.05).CONCLUSION AFP mRNA was expressed in BEL-7404 human hepatoma cells and OXL suppressed AFP mRNA expression in the cells.

Heme status affects human hepatic messenger RNA and microRNA expression

AIM:To assess effects of heme on messenger RNA(mRNA) and microRNA(miRNA) profiles of liver cells derived from humans.METHODS:We exposed human hepatoma cell line Huh-7 cells to excess iron protoporphyrin(heme)(10 μmol/L) or induced heme deficiency by addition of 4,6-dioxoheptanoic acid(500 μmol/L),a potent inhibitor of aminolevulinic acid dehydratase,for 6 h or 24 h.We harvested total RNA from the cells and performed both mRNA and miRNA array analyses,with use of Affymetrix chips,reagents,and instruments(human genome U133 plus 2.0 and miRNA 2.0 arrays).We assessed changes and their significance and interrelationships with Target Scan,Pathway Studios,and Ingenuity software.RESULTS:Changes in mRNA levels were most numerous and striking at 6 h after heme treatment but were similar and still numerous at 24 h.After 6 h of heme exposure,the increase in heme oxygenase 1 gene expression was 60-fold by mRNA and 88-fold by quantitative reverse transcription-polymerase chain reaction.We found striking changes,especially up-regulation by heme of nuclear erythroid-2 related factor-mediated oxidative stress responses,protein ubiquitination,glucocorticoid signaling,P53 signaling,and changes in RNAs that regulate intermediary metabolism.Fewer mRNAs were down-regulated by heme,and the fold decreases were less exuberant than were the increases.Notable decreases after 24 h of heme exposure were patatin-like phospholipase domain-containing protein 3(-6.5-fold),neuronal PAS domain protein 2(-1.93-fold),and protoporphyrinogen oxidase(-1.7-fold).CONCLUSION:Heme excess exhibits several toxic effects on liver and kidney,which deserve study in humans and in animal models of the human porphyrias or other disorders.

基于RNA-seq不明原因复发性流产绒毛组织mRNA基因差异性表达研究

目的:构建不明原因复发性流产(unexplained recurrent spontaneous abortion,URSA)孕妇绒毛组织的mRNA差异性表达谱并进行功能分析,为阐明URSA的发生发展机制提供依据。方法:收集2022年3月于新疆医科大学第一附属医院妇科门诊收治的4例URSA(试验组)和4例选择性终止妊娠孕妇(对照组)的绒毛组织样本。应用转录组测序技术(RNA-seq)筛选2组差异表达基因(differentially expressed genes,DEGs),并对其进行GO功能注释、KEGG通路分析及蛋白质-蛋白质相互作用(PPI)网络分析,进一步研究差异表达mRNA的功能,并筛选出URSA的关键基因。结果:RNA-seq分析共筛选出3350个DEGs,其中上调基因2259个,下调基因1091个。通过PPI网络分析,筛选出与URSA有关的前10个关键基因:TYROBP、CD74、GH1、GH2、STAT5A、HLA-DRA、STAT5B、HLA-DRB1、CISH和HLA-A。通过GO和KEGG生物学功能分析,发现差异性表达的mRNA参与到多种白细胞分化相关免疫反应通路和同种异体免疫应答等生物学过程。结论:利用RNA-seq获得的URSA的mRNA差异性表达谱,筛选出可能与URSA有关的关键基因及生物学通路,为进一步研究URSA的发病机制和诊疗靶点提供了理论依据。

参芪复方对糖尿病GK大鼠肝脏组织mRNA、lncRNA表达谱的影响

目的应用全转录组测序与实时聚合酶链锁反应(Real-time polymerase chain reaction,RT-qPCR)技术,探索参芪复方调控糖尿病GK大鼠肝脏信使RNA(messenger RNA,mRNA)、长链非编码RNA(long non-coding RNA,lncRNA)表达谱的机制研究。方法采用高脂高糖饲料建立2型糖尿病模型,将GK大鼠随机分为模型组、参芪复方组和西药组。另将10只Wistar大鼠设为空白组,予普通饲料喂养。参芪复方组大鼠予参芪复方浸膏灌胃,西药组予西格列汀混悬液灌胃,模型组及空白组灌服生理盐水。干预12周,每周检测空腹血糖(fasting blood glucose,FBG)。运用HE染色法观察大鼠肝脏组织病理形态,在空白组、模型组和参芪复方组中每组随机选取4只大鼠进行全转录组测序,构建mRNA、lncRNA差异表达谱,分析差异基因生物学功能,并进行RT-qPCR验证。结果与空白组相比,糖尿病GK大鼠FBG显著升高(P<0.05),模型组大鼠肝脏可见肝细胞排列紊乱,边界模糊,出现弥漫空泡状改变,呈中度脂肪变性,伴见炎性浸润、弥漫水肿;与模型组相比,参芪复方组大鼠FBG在12周时明显降低(P<0.05),肝脏组织排列较整齐,脂质沉积、细胞水肿及炎细胞浸润明显减轻。全转录组结果显示,与空白组相比,模型组大鼠mRNA、lncRNA表达谱存在显著差异,决定了糖尿病大鼠生理病理上的差异表现。参芪复方可广泛调控mRNA、lncRNA的差异表达,富集分析显示参芪复方通过调控多条内分泌系统及代谢过程相关信号通路改善糖尿病,包括胰岛素分泌、非酒精性脂肪性肝病、胆固醇代谢、鞘脂代谢、胰岛素抵抗等信号通路。RT-qPCR结果显示,基因Irf1、Trim30、Tmcc3、Insig1与转录组结果一致,转录组准确性较高。结论参芪复方发挥调节血糖及改善肝脏脂质沉积、水肿的作用,可能与广泛调控mRNA、lncRNA的差异表达有关。

弱精子症患者精子lncRNA与mRNA基因表达特征分析

目的:通过DNBSEQ平台测序技术构建文库,并以此来确定人类正常与弱精子症精子中lncRNA和mRNA的表达差异,并通过生物信息学方法分析其在弱精子症中的生物学意义。方法:将9份正常精液样本及9份弱精子症精液样本分组后,分离精子,提取总RNA,通过DNBSEQ测序平台检测得到RNA-seq在精子中的表达情况,通过GO富集分析和KEGG通路分析,进一步分析其相关功能情况。结果:使用DNBSEQ平台检测,每组平均产出10.64G数据,共检测到282185个RNA,包含有107009个lncRNA,其中15157个lncRNA具有表达差异,2190个lncRNA表达上调,12967个表达下调;共检测到19514个mRNA,其中13736个mRNA具有表达差异,4995个mRNA表达上调,8741个mRNA表达下调。差异基因主要富集在精子细胞膜、离子通道的功能以及精子发育、受精相关的通路上。结论:通过对弱精子症与正常精子的测序分析,鉴别出差异表达的lncRNA和mRNA,可通过胞膜离子通道对精子功能进行调控,进而导致弱精子症的发生,可为弱精子症的进一步研究提供分子基础。

妊娠期高血压病患者血清DNMT1 mRNA和LncRNA UCA1水平表达与妊娠结局的关系

目的分析妊娠期高血压疾病(hypertensive disorder complicating pregnancy,HDCP)患者血清DNA甲基转移酶1(DNA methyltransferase 1,DNMT1)信使RNA(messenger RNA,mRNA)、长链非编码RNA(long non-codingRNA,LncRNA)尿路上皮癌胚抗原1(urothelial carcinoembryonic antigen 1,UCA1)水平与妊娠结局的关系。方法选取2021年3月~2023年8月在邯郸市妇幼保健院诊治的HDCP患者195例为病例组、健康妊娠孕妇195例为对照组。收集所有孕妇临床资料并检测分娩前1天生化指标;荧光定量PCR法检测血清DNMT1 mRNA,LncRNA UCA1水平;根据病情将病例组分为妊娠期高血压(pregnancy induced hypertension,PIH)组、轻度子痫前期(preeclampsia,PE)组、重度PE组;根据HDCP患者分娩时不良妊娠结局情况分为妊娠结局良好组和妊娠结局不良组;比较对照组和病例组临床资料和生化指标、血清DNMT1 mRNA,LncRNA UCA1水平;比较不同严重程度HDCP患者血清DNMT1mRNA和LncRNA UCA1水平;比较不同妊娠结局HDCP患者临床资料和生化指标、血清DNMT1 mRNA和LncRNAUCA1水平;分析HDCP患者血清DNMT1 mRNA与LncRNA UCA1的相关性,影响HDCP患者妊娠结局的因素,血清DNMT1 mRNA和LncRNA UCA1对HDCP患者发生不良妊娠结局的预测价值。结果与对照组比较,病例组收缩压、舒张压、白细胞计数水平明显升高,血清DNMT1 mRNA(0.72±0.18 vs 1.00±0.04),LncRNA UCA1(0.61±0.16vs 1.00±0.02)水平明显降低,差异具有统计学意义(t=40.651,32.595,7.837,21.205,33.775,均P<0.001);PIH组、轻度PE组、重度PE组血清DNMT1 mRNA(0.85±0.20,0.74±0.18,0.50±0.15),LncRNA UCA1(0.77±0.18,0.58±0.16,0.43±0.13)水平依次降低,差异具有统计学意义(F=52.687,64.030,均P<0.001);HDCP患者血清DNMT1 mRNA与LncRNA UCA1呈正相关(r=0.582,P<0.001);与妊娠结局良好组比较,妊娠结局不良组HDCP严重程度较高,收缩压、舒张压、白细胞计数水平明显升高,血清DNMT1 mRNA(0.80±0.20 vs 0.59±0.15),LncRNA UCA1(0.72±0.17 vs 0.43±0.14)水平明显降低,差异具有统计学意义(χ^(2)=18.386,t=2.615~12.290,均P<0.05);重度PE[OR(95%CI)=1.708(1.193~2.445)]、收缩压[OR(95%CI)=1.495(1.090~2.049)]、舒张压[OR(95%CI)=1.621(1.076~2.442)]是影响HDCP患者发生不良妊娠结局的危险因素,DNMT1 mRNA[OR(95%CI)=0.833(0.725~0.957)],LncRNA UCA1[OR(95%CI)=0.796(0.696~0.909)]是影响HDCP患者发生不良妊娠结局的保护因素(均P<0.05);DNMT1 mRNA和LncRNA UCA1二者联合预测HDCP患者发生不良妊娠结局的曲线下面积(area under curve,AUC)大于DNMT1 mRNA及LncRNA UCA1单独预测的AUC(0.926 vs 0.832,0.844),差异具有统计学意义(Z=2.932,2.345,均P<0.05)。结论HDCP患者血清DNMT1 mRNA和LncRNA UCA1水平均较低,与病情程度、妊娠结局相关,DNMT1 mRNA联合LncRNA UCA1检测对不良妊娠结局有较佳预测效能。

基于生物信息学构建膀胱尿路上皮癌的ceRNA网络以及关键mRNA与免疫功能分析

目的构建膀胱尿路上皮癌(bladder urothelial carcinoma,BLCA)具有预后价值的内源竞争性核糖核酸(competing endogenous RNA,ceRNA)调控网络,分析关键信使RNA(messenger RNA,mRNA)与免疫功能的关系。方法UCSC Xena数据库下载404例BLCA患者和28例正常人的mRNA表达数据,通过差异分析筛选关键mRNA。ENCORI数据库中查找与关键mRNA结合的微小核糖核酸(micro RNA,miRNA)以及与miRNA结合的长链非编码核糖核酸(long non-coding RNA,LncRNA)。TCGA数据库下载miRNA和LncRNA的表达数据,对关键mRNA与所有miRNA以及mi RNA与所有LncRNA进行共表达分析,筛选出关键的miRNA和LncRNA。根据关键mRNA,miRNA和LncRNA在肿瘤患者和正常人之间表达量的差异进行生存分析,最后构建了ceRNA调控网络。借助TIMER 2.0数据库,分析关键mRNA与免疫细胞、免疫检查点(CD274,PDCD1,CTLA4)以及免疫细胞标记基因(immunomarker genes,IG)的相关性。结果筛选出关键mRNA*共22个,其中差异显著性最高的是脯氨酸3-羟化酶4(proline3-hydroxylase 4,P3H4)。在BLCA中,P3H4表达高,在高表达组患者的生存时间较短。以关键mRNA为中心环节,共筛选出33个miRNA和14个LncRNA。经过共表达分析和生存分析后,筛选出具有预后价值的关键miRNA和关键LncRNA分别为hsa-miR-151a-3p和MIR100HG。上述分析结果差异具有统计学意义(均Ρ<0.05)。综合以上结果,构建了包含1个mRNA,1个miRNA和1个LncRNA的ceRNA调控网络。免疫分析首次在BLCA肿瘤微环境中发现了与P3H4表达量呈显著正相关的双阳性T细胞。此外还有3种免疫细胞(肿瘤相关性中性粒细胞、肿瘤相关巨噬细胞、树突状细胞)、3个免疫检查点(CD274,PDCD1,CTLA4)以及15个IG与P3H4相关度显著,这些差异具有统计学意义(均Ρ<0.01)。结论该研究有助于揭示BLCA的进展机制,构建的ceRNA网络及免疫分析,可为BLCA患者的诊断、治疗、预测提供新的生物学靶点和方向。

环状RNA的成环策略及环状RNA疫苗的研究现状

环状RNA相比于线性mRNA具有合成简单、稳定性高、持续稳定表达等优点,在感染性微生物疫苗、肿瘤疫苗和蛋白替代疗法等领域具有巨大的应用潜力,近年来已经成为核酸药物领域研究的热点。RNA的环化技术是体外合成环状RNA的关键,成环策略对环化效率、免疫原性和蛋白表达量等产生重要影响,制约了环状RNA的基础研究和临床应用。本文系统综述了化学法、酶法和核酶法等几种成环策略,重点分析各成环技术的反应条件、成环工艺、环化效率和免疫原性等。目前,理想的环状RNA成环策略还面临诸多挑战,但是研究证实环状RNA在新型冠状病毒肺炎疫苗、抗肿瘤疫苗等领域比线性mRNA具有更好的稳定性和更强的免疫效应,成为一种极具潜力的新型核酸药物分子,为优化和拓展环状RNA的研究和临床应用提供参考。

IL-17 mRNA和PGE2 mRNA在口腔扁平苔藓患者中的表达水平及临床意义

目的探讨白细胞介素17(IL-17)信使RNA(mRNA)和前列腺素E2(PGE2)mRNA在口腔扁平苔藓(OLP)患者中的表达水平及临床意义。方法选取2020年3月至2021年3月宁夏医科大学总医院口腔医院收治的35例OLP患者作为试验组,另选取同期在宁夏医科大学总医院口腔医院进行阻生牙拔除的20例患者作为对照组,根据组织是否糜烂,将试验组患者分为糜烂型OLP组和非糜烂型OLP组。检测并比较糜烂型OLP组和非糜烂型OLP组患者口腔黏膜病损组织及对照组患者口腔黏膜组织的IL-17 mRNA和PGE2 mRNA表达水平,并通过视觉模拟评分法(VAS)评估OLP患者的疼痛程度,比较不同疼痛程度的OLP患者IL-17 mRNA和PGE2 mRNA表达水平。采用Pearson相关分析OLP患者IL-17 mRNA与PGE2 mRNA表达水平的相关性。采用Spearman相关分析OLP患者IL-17 mRNA和PGE2 mRNA表达水平与疼痛程度的相关性。结果非糜烂型OLP组有19例患者,糜烂型OLP组有16例患者。糜烂型OLP组IL-17 mRNA和PGE2 mRNA表达水平均高于非糜烂型OLP组和对照组,且非糜烂型OLP组均高于对照组,差异均有统计学意义(P<0.05)。试验组中无疼痛患者有5例,轻度疼痛患者有6例,中度疼痛患者有16例,重度疼痛患者有8例。无疼痛OLP患者IL-17 mRNA和PGE2 mRNA表达水平均低于轻度、中度、重度疼痛OLP患者,差异均有统计学意义(P<0.05)。Pearson相关分析结果显示,OLP患者IL-17 mRNA表达水平与PGE2 mRNA表达水平呈正相关(r=0.505,P=0.002)。Spearman相关分析结果显示,OLP患者IL-17 mRNA、PGE2 mRNA表达水平与疼痛程度均呈正相关(r=0.710、0.570,P<0.05)。结论IL-17 mRNA和PGE2 mRNA参与了OLP的发生、发展过程,并且其表达水平与OLP患者疼痛程度呈正相关。

结核病mRNA疫苗的研制策略与展望

应对危害全球人类健康的重大传染性疾病——结核病流行的严峻挑战,迫切需要研制出有效的新型结核病疫苗。虽然目前开展了多种类型的新型结核病疫苗的研制,且一些疫苗已进入临床试验研究,但至今仍未能获得可以替代传统卡介苗(BCG)的更为有效的新型疫苗。随着mRNA疫苗研制技术的突破,其研发周期短、高效、安全和生产成本低等优点,使其成为一个非常有前景的疫苗研发新方向。笔者主要就mRNA疫苗的技术原理、优势、制备技术,以及结核病mRNA疫苗的研制策略和现状等方面的研究进展进行综述,以期为结核病mRNA疫苗的研制提供参考。

信使RNA N6-甲基腺嘌呤甲基化修饰在血管性痴呆中的作用机制研究进展

信使RNA(mRNA)中的腺苷酸可发生甲基化转化为N6-甲基腺嘌呤(N6-methyladenosine,m^(6)A)进而调节mRNA的功能和代谢,这是一种高度动态可逆的表观转录组修饰方式。血管性痴呆(vascular dementia,VD)是由多种脑血管原因(如动脉粥样硬化、淀粉样改变等)引起的一种神经退行性疾病,近年来,有研究发现m^(6)A与VD的发病和进展密切相关,m^(6)A甲基化在调节神经元氧化应激、炎症反应、脑血管内皮损伤、线粒体功能障碍和突触可塑性等方面具有较大影响。文章对近几年关于m^(6)A甲基化修饰在VD中的潜在作用机制进行综述,以期为后续研究和靶向治疗VD提供新的科学思路。

mRNA疫苗制备技术在甲型流感病毒疫苗研究中的应用

禽流感病毒(Avian influenza virus,AIV)、H1N1和H3N2亚型人流感病毒(Influenza virus,IV)均属于甲型流感病毒(Influenza A virus,IAV)。IAV含有多种亚型,毒株变异快,因此IAV疫苗株需要根据当年的优势毒株进行相应的调整,这给疫苗的研制和生产带来巨大挑战。信使核糖核酸(messenger RNA,mRNA)疫苗制备工艺简单、生产时间短且容易规模化生产,在疾病预防方面具有广阔的应用前景。笔者对mRNA疫苗的种类、优化策略和IAV mRNA疫苗的研究现状进行了综述,旨在为IAV mRNA疫苗的研发提供理论参考。

基于GEO数据库联合分析高原病患者外周血差异表达miRNA及其上游转录因子和下游mRNA

目的基于GEO数据库联合分析高原病患者外周血差异表达miRNA及其上游转录因子和下游mRNA,从而基于分子层面探讨高原病潜在的发病机制。方法(1)在GEO数据库获取与高原病相关的miRNA表达谱芯片(GSE90500数据集)和mRNA表达谱芯片(GSE29977数据集),再采用R语言3.6软件limma程序包筛选差异表达miRNA和差异表达mRNA。(2)利用FunRich软件预测差异表达miRNA的下游靶基因(mRNA)和上游转录因子,并对上游转录因子进行功能富集分析。使用R语言3.6软件、DAVID数据库对下游靶基因分别进行功能和通路富集分析。(3)对GSE29977数据集的差异表达mRNA与差异表达miRNA下游靶基因取交集,并根据miRNA及其靶基因的表达关系,筛选miRNA-mRNA调控轴。结果(1)共筛选出14个差异表达miRNA及其385个下游靶基因、123个上游转录因子。差异表达miRNA主要富集的转录因子包括EGR1、RREB1、MYF5和MEF2A。(2)上游转录因子涉及的生物学过程主要包括信号转导、核酸代谢的调节、脂肪酸代谢、糖代谢、细胞因子和趋化因子介导的信号通路、细胞周期等。下游靶基因富集的生物学过程主要包括转录调控、心肌细胞增殖、血管生成和染色质重塑等,富集的信号通路主要包括PD-L1表达和PD-1免疫检查点通路、细胞衰老、MTOR信号通路、MAPK信号通路及PI3K/AKT信号通路等。(3)共筛选得到443个差异表达mRNA,与差异表达miRNA的下游靶基因取交集后获得与高原病相关的5个核心mRNA,并构建出hsa-miR-155-5p-MYO1D调控轴。结论高原病中存在多个差异表达的miRNA,其上游转录因子EGR1、RREB1、MYF5、MEF2A可能是参与调控下游靶基因转录的核心因子;差异表达miRNA的上游转录因子和下游靶基因可能通过调控基因转录、细胞增殖与凋亡、炎症过程等生物学过程,共同参与高原病的发生、发展。hsa-miR-155-5p与下游靶基因MYO1D之间的调控关系可能在高原病的发生、发展中发挥重要的作用。

Relationship between bone marrow-derived CD_(34)^+ cells expressing interleukin-5 receptor messenger RNA and asthmatic airway inflammation

BACKGROUND: Asthma is clinically related with the degree of eosinophilic inflammation. How asthmatic airway inflammation is affected is still poorly understood. So the effects of bone marrow-derived hematopoietic cells expressing CD(34) (CD(34)(+)) and interleukin-5 (IL-5) receptor messenger RNA (IL-5R mRNA+) on asthmatic airway inflammation were investigated. METHODS: Balb/c mice were sensitized and challenged by ovalbumin (OVA) to establish an asthmatic model while control mice were sensitized and exposed to sterile saline. The mice were killed at different time points after being challenged by OVA and sterile saline. Then, bronchoalveolar lavage fluid (BALF), peripheral blood (PB) and bone marrow (BM) were prepared. Eosinophils in PB (PBEOS) and BALF (BALFEOS), nuclear cells in BALF, PB and BM were counted. By flow cytometry, the percentage of CD(34)(+) cells to nucleated cells in PB, BM and the relative number of CD(34)(+) cells in PB (PBCD(34)(+)) and BM (BMCD(34)(+)) were calculated. Immunocytochemistry and in situ hybridization were used to investigate the hematopoietic cells with co-localized expression of CD(34) and IL-5R mRNA in BM (BMCD34+IL-5R mRNA+). The percentage of BMCD34+IL-5R mRNA+ to BMCD(34)(+) was calculated. RESULTS: Twelve hours after challenge by OVA, BALFEOS and PBEOS in the experimental group were significantly higher than those in the control group (P

基于微小RNA-信使RNA互作在畸形精子症中的潜在发生机制研究

目的探讨微小RNA(miRNA)-信使RNA(mRNA)互作在畸形精子症中的潜在作用及机制。方法选取2018年1—12月于江西省妇幼保健院就诊的30例畸精症患者作为观察组,另选取同期于江西省妇幼保健院工作的30名正常男性作为对照组。构建mRNA和miRNA基因表达谱,并通过京都基因和基因组百科全书(KEGG)和基因本体论(GO)富集分析后进行反转录聚合酶链式反应(RT-PCR)进一步验证。结果通过miRNA测序研究畸精症中miRNA的影响,共发现23个差异表达miRNA,同时满足log2FC|>0.585和P<0.05。23个差异表达miRNA的表达,有17个上调miRNA来自9个miRNA家族和6个下调的miRNA来自5个miRNA家族。使用KEGG和GO分析差异表达miRNA的2022个差异表达靶mRNA,共获得10条通路和9个注释簇。10条通路包括果糖和甘露糖代谢、磷酸戊糖通路、酵解/糖异生、碳代谢、氨基酸生物合成、核因子κB(NF-κB)信号通路、信号转导子和转录激活子(STATs)、丝裂原激活蛋白激酶(MAP)信号通路、Th1和Th2细胞分化、Toll样受体信号通路。注释簇1总结了3个GO术语;注释簇2总结了41个GO术语;注释簇3总结了3个GO术语;注释簇4总结了3个GO术语;注释簇5总结了3个GO术语;注释簇6总结了3个GO术语;注释集群7总结了38个GO术语;注释簇8总结了4个GO术语;注释簇9总结了10个GO术语。使用RT-PCR检测注释簇9中的3个miRNA和8个mRNA。miR-375-4-3p是上调的miRNA,而miR-31-12-5p和miR-9-6-5p是下调的miRNA。在4个GO术语中检测NF-κB、环氧合酶-2(COX-2)、前列腺素E合酶(PTGES)和基质金属蛋白酶9(MMP9)表达。在3个GO术语中检测白细胞介素(IL)-11、Spi-B转录因子(SPI1)、T细胞中表达的T-box转录因子(T-Bet)和IL-4/13A表达。RT-PCR的结果与miRNA和mRNA测序的结果一致,观察组miR-375-4-3p、NF-κB、COX-2、PTGES和IL-4/13A mRNA表达高于对照组,而miR-31-12-5p、miR-9-6-5p、MMP9、IL-11、SPI1和T-Bet mRNA表达低于对照组,差异有统计学意义(P<0.05)。结论畸精症中有23个差异表达的miRNA和2022个目标mRNAs,可使用KEGG和GO富集分析获得5条通路和7个目标mRNA炎症免疫抑制损伤相关的GO术语,miRNAs可通过miRNA-mRNA网络分析介导炎症免疫抑制损伤相关机制参与畸精症进展,但具体机制需进一步研究。

慢性镉暴露下食管鳞状细胞癌细胞的lncRNA-mRNA共表达网络分析

目的:构建食管鳞状细胞癌(ESCC)细胞在慢性低浓度镉暴露诱导下的长链非编码RNA(lncRNA)和mRNA的共表达网络,探讨关键lncRNA和mRNA在镉促ESCC演进及放化疗抵抗中的潜在功能及分子机制。方法:EC109细胞持续暴露于5μmol/L氯化镉培养12周,构建慢性镉暴露ESCC细胞模型CCT-EC109。采用Illumina NovaSeq 6000系统对暴露株CCT-EC109和亲本株EC109细胞进行全转录组测序,运用生物信息学方法分析差异lncRNA和mRNA表达谱,利用基因本体(GO)和京都基因与基因组大百科全书(KEGG)对差异lncRNA的靶基因进行功能分析,根据Pearson相关系数利用Cytoscape软件构建lncRNA-mRNA共表达网络,并对筛选的lncRNA和mRNA进行实时荧光定量PCR(qPCR)验证。结果:EC109细胞与CCT-EC109细胞存在差异表达lncRNA(DE-lncRNA) 2 794个,差异mRNA(DE-mRNA) 4 267个;DE-lncRNA的靶基因与DE-mRNA取交集,获得1 546个DE-lncRNA调控的镉暴露相关mRNA;GO分析显示这些基因主要富集在代谢过程、膜与膜封闭腔部分及催化反应等功能;KEGG分析提示Hippo信号通路是最显著富集项之一。差异表达最显著的前10个lncRNA的38个共表达mRNA构建共表达网络,经qPCR验证,与mRNA关联最多的lncRNA NONHSAT097388.2以及ECE1、EMP2、ORAT1、ZNF713在CCT-EC109中表达均下调(均为P<0.01),而MFAP5和PGF表达均升高(均为P<0.05)。结论:lncRNA-mRNA共表达网络可能在慢性镉暴露诱导ESCC细胞演进和治疗抵抗机制中发挥重要作用,相关基因有望成为镉暴露ESCC患者预后判断的潜在生物标志物和治疗靶点。

Tumor gene mutations and messenger RNA expression： correlation with clinical response to icotinib hydrochloride in non-small cell lung cancer

Background Molecular targeted drugs is now widely used in non-small cell lung cancer （NSCLC） clinical treatment. Icotinib hydrochloride is a new type of oral epidermal growth factor receptor （EGFR） tyrosine kinase inhibitors （EGFR-TKIs）. In this study, we examined the role of EGFR, K-RAS, B-RAF somatic mutations and EGFR mRNA expression in tumor specimens from advanced NSCLC patients as predicators of the efficacy of icotinib hydrochloride. Methods We analyzed tumor paraffin-embedded specimens, which were obtained from 14 of 40 patients with advanced NSCLC who enrolled in the stage I clinical trial of icotinib hydrochloride. Somatic mutations were evaluated by mutant-enriched liquidchip （MEL） technology, and EGFR mRNA expression was measured by branched DNA liquidchip （MBL） technology. Results In the 14 specimens, seven patients showed EGFR mutations, exon 19 deletion （3/7） and exon 21 point mutation （4/7）; and two patients showed K-RAS mutation. No mutations in EGFR exon 20. or B-RAF were detected. In patients with EGFR mutation, one patient developed progress disease （PD）, three patients had stable disease （SD）, two patients had partial responses （PR） and one patient had a complete response （CR）. In patients with wild-type EGFR, four patients had PD, three patients acquired SD, and none had PR/CR （P=-0.0407）. EGFR mutations were associated with better progress-free survival （PFS） （141 days vs. 61 days） but without a statistically significant difference （P=0.8597）, and median overall survival （OS） （-〉449 days vs. 140 days）. EGFR mRNA expression levels were evaluated （three high, eight moderate, one low, and two that can not be measured due to insufficient tumor tissue） and no statistically significant relationships was observed with response, PFS or OS. Conclusions The EGFR mutation rate was consistent with that reported in the Asian population, so the MEL technology is reliable for measuring EGFR mutation with high throughput and rapidity. EGFR exon 19 deletions and exon 21 point mutation are predictive biomarkers for response to icotinib hvdrochloride as second line treatment or above.

基于circRNA-miRNA-mRNA三元转录网络探讨糖尿病动脉粥样硬化小鼠模型舌象形成的机制

目的:探讨糖尿病动脉粥样硬化模型小鼠与美国癌症研究所(ICR)小鼠舌组织中差异表达的环状RNA(circRNA)、微小RNA(miRNA)及信使RNA(mRNA),构建circRNA-miRNA-mRNA三元转录网络。方法:9只ICR小鼠为对照组,9只MKR小鼠(骨骼肌特异性胰岛素样生长因子1受体功能缺失)为模型组。各组用于组织病理染色6只,基因测序3只。模型组小鼠采用N-硝基-L-精氨酸甲酯(L-NAME)腹腔注射+高脂饲料饲养。29 d后检测心电图改变、主动脉改变(HE染色)、舌面丝状乳头高度变化(HE染色)及舌面丝状乳头白细胞介素1β(IL-1β)、IL-6和IL-8的蛋白表达。使用微阵列技术筛选舌组织中差异表达的基因,进行基因本体(GO)功能分析及京都基因和基因组百科全书(KEGG)通路富集分析,采用qRT-PCR验证基因芯片结果,构建circRNA-miRNA-mRNA转录网络。结果:与对照组相比,模型组心电图出现“红旗飘飘”样改变,病理染色提示主动脉有脂质突出,舌组织出现炎症浸润,IL-1β、IL-6及IL-8蛋白表达均明显增高(P<0.01),舌面丝状乳头角化层和上皮层高度显著降低(P<0.01)。Tox2、Ncor2、Paqr6和R3hdm1基因表达的变化与微阵列结果一致(P<0.01),这些差异表达基因主要通过AGERAGE、TRP及GnRH等通路参与炎症反应、糖脂代谢紊乱及免疫细胞招募趋化等过程,由此构建28个circRNA、23个miRNA和46个mRNA组成的三元转录网络。结论:糖尿病动脉粥样硬化模型小鼠舌组织存在差异表达的circRNA和miRNA,这些差异基因可能通过circRNA-miRNA-mRNA三元转录网络系统调控糖尿病动脉粥样硬化的舌象形成。