TNF-α regulates the expression of transcription factor FoxM1 in bladder cancer and cystitis glandularis

Objective:To study the expression and significance of TNF-transcription factor M1(FoxM1)in bladder cancer and cystitis glandularis(CG).Methods:A total of 30 patients with bladder cancer admitted to our hospital and received surgical treatment from February 2017 to February 2019 were included for the study.During surgery,bladder cancer tissues and normal bladder tissues(tissues more than 5cm away from the cancer tissue center)were collected.Meanwhile,we retained 30 CG tissues from 30 CG patients who received surgical treatment in our hospital at the same time.Bladder cancer cell lines RT4 and BIU87 were cultured and treated with TNF-αat different concentrations(0nM,1nM,5nM,10nM).The expressions of TNF-αand FoxM1 in different bladder tissues were analyzed,and the effects of different concentrations of TNF-αon the expressions of FoxM1 in bladder cancer cell lines and cyclin B1 and cyclin D1 in bladder cancer cell lines were analyzed.Results:The expression levels of TNF-αand FoxM1 in normal bladder,CG and bladder cancer tissues were gradually increased,and univariate analysis of variance showed that the differences between groups were statistically significant(all P<0.05).FoxM1 expression in bladder cancer cell lines treated with TNF-αat concentrations of 0nM,1nM,5nM and 10nM showed a gradual increase trend,and one-way anova showed that the difference between the groups was statistically significant(all P<0.05).After the treatment of bladder cancer cell lines with TNF-αat concentrations of 0nM,1nM,5nM and 10nM,the expression of cyclin B1 and cyclin D1 showed a gradually increasing trend,and one-way anova showed that the difference between groups was statistically significant(all P<0.05).Conclusion:TNF-αmay play a crucial role in the occurrence and development of CG by regulating the expression of transcription factor FoxM1,and then affecting the expression of cyclin B1 and cyclin D1,which is worthy of clinical attention.

IGF_(2)BP_(1)调控lncRNA NEAT1在类风湿关节炎中的作用

目的:类风湿关节炎(rheumatoid arthritis,RA)是一种常见的全身性自身免疫疾病,可能导致关节变形和功能障碍。本研究旨在探索胰岛素样生长因子-2 mRNA结合蛋白1(insulin like growth factor 2 mRNA binding protein 1,IGF_(2)BP_(1))在RA中的表达水平,以及其对长链非编码RNA(long non-coding RNA,lncRNA)核丰富转录本1(nuclear paraspeckle assembly transcript 1,NEAT1)稳定性的影响和在RA发病机制中的作用。方法:通过GEO(Gene Expression Omnibus)数据库获取RA数据集,并将其分为正常对照组和RA组,使用R软件分析获取N^(6)-甲基腺苷(N^(6)-methyladenosine,m^(6)A)相关的甲基化酶的表达量并进行差异分析。分析差异表达的m^(6)A甲基化酶与lncRNA NEAT1的相关性。通过在线网站ENCORI预测与lncRNA NEAT1结合的蛋白质,并与lncRNA NEAT1表达相关的m^(6)A甲基化酶取交集,从而获取关键基因。通过RNA蛋白质相互作用分析实验(RNA pull-down)验证在RA滑膜细胞中NEAT1与关键基因结合的情况。通过蛋白质印迹法验证关键基因在正常滑膜细胞和RA滑膜细胞中的表达水平。在RA滑膜细胞中转染关键基因的小干扰RNA,通过real-time RT-PCR检测NEAT1在滑膜细胞中的表达水平。结果:差异分析结果显示:与正常对照组相比,共有8个m^(6)A甲基化基因在RA组中存在差异表达,其中IGF_(2)BP_(1)、甲基转移酶样蛋白14(methyltransferase 14,N^(6)-adenosine-methyltransferase subunit,MEEEL14)与lncRNA NEAT1存在相关性;ENCORI预测结果显示:共有23个蛋白质能够与lncRNA NEAT1结合,与NEAT1共表达m^(6)A甲基化酶取交集,获得NEAT1相关m^(6)A甲基化蛋白IGF_(2)BP_(1)。蛋白质印迹法显示:与正常对照组相比,RA组中IGF_(2)BP_(1)蛋白在RA滑膜细胞中表达升高(P<0.05);RNA pull-down结果显示IGF_(2)BP_(1)蛋白与NEAT1结合;real-time RT-PCR的结果表明:敲减IGF_(2)BP_(1)可显著降低NEAT1 mRNA表达水平(P<0.01)。结论:IGF_(2)BP_(1)可能通过稳定lncRNA NEAT1表达参与RA发病,调控IGF_(2)BP_(1)水平可能是一种新的治疗RA的方法。

Novel nervous and multi-system regenerative therapeutic strategies for diabetes mellitus with mTOR

Throughout the globe,diabetes mellitus（DM） is increasing in incidence with limited therapies presently available to prevent or resolve the significant complications of this disorder.DM impacts multiple organs and affects all components of the central and peripheral nervous systems that can range from dementia to diabetic neuropathy.The mechanistic target of rapamycin（m TOR） is a promising agent for the development of novel regenerative strategies for the treatment of DM.m TOR and its related signaling pathways impact multiple metabolic parameters that include cellular metabolic homeostasis,insulin resistance,insulin secretion,stem cell proliferation and differentiation,pancreatic β-cell function,and programmed cell death with apoptosis and autophagy.m TOR is central element for the protein complexes m TOR Complex 1（m TORC1） and m TOR Complex 2（m TORC2） and is a critical component for a number of signaling pathways that involve phosphoinositide 3-kinase（PI 3-K）,protein kinase B（Akt）,AMP activated protein kinase（AMPK）,silent mating type information regulation 2 homolog 1（Saccharomyces cerevisiae）（SIRT1）,Wnt1 inducible signaling pathway protein 1（WISP1）,and growth factors.As a result,m TOR represents an exciting target to offer new clinical avenues for the treatment of DM and the complications of this disease.Future studies directed to elucidate the delicate balance m TOR holds over cellular metabolism and the impact of its broad signaling pathways should foster the translation of these targets into effective clinical regimens for DM.

鸡转录增强因子-1相关基因cDNA片段的克隆及其在发育过程中的表达

目的 :克隆转录增强因子 1(transcriptionenhancerfactor 1,TEF 1)相关基因 (relatedTEF 1,RTEF 1) ,检测鸡发育过程RTEF 1基因的表达及组织分布。方法 :从 13d鸡胚骨骼肌mRNAs经RT PCR方法扩增RTEF 1的编码序列 (cDNA) ,将其克隆到 pGEM和 pUC载体并进行核苷酸序列分析。采用RT PCR技术检测鸡胚发育第9天至雏鸡孵出后 6周的骨骼肌组织中RTEF 1基因的表达 ,并测试其在 13d鸡胚和出生后 1d雏鸡的骨骼肌、心肌、脑、肝和胗等 5种组织中的存在。结果 :克隆序列分析结合GenBank检索表明 ,所克隆的cDNA片段 ( 90 0bp)与cTEF 1A序列仅相差两个碱基。应用RT PCR技术在鸡胚发育 9d至出生后 6周雏鸡的骨骼肌组织均检出了RTEF 1基因的表达 ;13d鸡胚和出生后 1d雏鸡的骨骼肌、心肌、脑、肝和胗等 5种组织中均有TEF 1相关基因的转录。结论 :克隆的cDNA片段属多种组织普遍存在的cTEF 1A。与先前检测的M CAT结合因子发生规律 (在两周前表达 )不同 ,cTEF 1A在鸡胚发育的第 9天至出生后

M2 pyruvate kinase enhances HIV-1 transcription from its long terminal repeat

Both thymocytes and tumor cells express M2 type isoenzyme of pyruvate kinase(M2PK),which is different from R type isoenzyme of pyruvate kinase(RPK)that is expressed in erythrocytes.In this report,the effect of RPK and M2PK on the transcription of human immunodeficiency virus type 1(HIV-1)was tested.The results indicated that M2PK could enhance HIV-1 transcription from its long terminal repeat(LTR)promoter,while RPK did not have such an effect.Specific down-regulation of M2PK could inhibit HIV-1 transcription from its LTR region.Furthermore,it was found that the C terminal region of M2PK is responsible for this effect.Collectively,the cellular factor M2PK that is expressed in thymocytes could facilitate the transcription of HIV-1.

Alleviating experimental pulmonary hypertension via co-delivering FoxO1 stimulus and apoptosis activator to hyperproliferating pulmonary arteries

Pulmonary hypertension(PH)is an insidious pulmonary vasculopathy with high mortality and morbidity and its underlying pathogenesis is still poorly delineated.The hyperproliferation and apoptosis resistance of pulmonary artery smooth muscle cells(PASMCs)contributes to pulmonary vascular remodeling in pulmonary hypertension,which is closely linked to the downregulation of forkhead box transcriptional factor O1(FoxO1)and apoptotic protein caspase 3(Cas-3).Here,PA-targeted co-delivery of a FoxO1 stimulus(paclitaxel,PTX)and Cas-3 was exploited to alleviate monocrotaline-induced pulmonary hypertension.The co-delivery system is prepared by loading the active protein on paclitaxel-crystal nanoparticles,followed by a glucuronic acid coating to target the glucose transporter-1 on the PASMCs.The co-loaded system(170 nm)circulates in the blood over time,accumulates in the lung,effectively targets the PAs,and profoundly regresses the remodeling of pulmonary arteries and improves hemodynamics,leading to a decrease in pulmonary arterial pressure and Fulton's index.Our mechanistic studies suggest that the targeted co-delivery system alleviates experimental pulmonary hypertension primarily via the regression of PASMC proliferation by inhibiting cell cycle progression and promoting apoptosis.Taken together,this targeted co-delivery approach offers a promising avenue to target PAs and cure the intractable vasculopathy in pulmonary hypertension.

线粒体转录复合物各因子质粒标准品的构建

目的:构建大鼠线粒体转录因子TFAM(A)、线粒体转录因子TFB1M(B1)、线粒体转录TFB2M(B2)及线粒体RNA聚合酶(POLRMT)的质粒标准品,为检测内耳细胞线粒体TFAM、TFB1M、TFB2M、POLRMT的mRNA表达水平做基础。方法:设计特异性引物和探针,提取大鼠内耳组织总mRNA逆转录成c DNA,PCR扩增、纯化目的片段,将纯化产物与p Zero Back/blunt载体重组,提取重组质粒,经测序鉴定后,用实时荧光绝对定量PCR建立标准曲线。结果:测序结果与各目的序列一致,获得良好的标准曲线(R2>0.99)。结论:成功构建了各目的基因的质粒标准品。

转录活化子1反义寡核苷酸对肺纤维化大鼠肺组织中细胞因子和胶原表达的影响

目的观察信号转导子与转录活化子1（STATI）反义寡核苷酸雾化吸入对博来霉素致肺纤维化大鼠肺组织中Ⅰ、Ⅲ型胶原，纤溶酶原激活物抑制剂-1（PAI-1），转化生长因子-β1（TGF—β1）和羟脯氨酸表达的影响。方法将45只Wistar大鼠按随机数字表法分为生理盐水组、博来霉素组和寡核苷酸组，每组15只，分别在气管内灌注并雾化吸入生理盐水、博来霉素、STAT1反义寡核苷酸。分别于雾化后第7天、第14天和第28天每组各处死5只大鼠。肺组织HE染色和Masson染色观察肺泡炎和肺纤维化改变，免疫组织化学sP法测定肺组织中TGF—β1、PAI-1表达，逆转录PCR测定肺组织中Ⅰ、Ⅲ型胶原mRNA表达，肺组织匀浆测定羟脯氨酸含量。样本均数间比较采用单因素方差分析和q检验。结果寡核苷酸组大鼠各时问点的肺泡炎和肺纤维化程度均较博来霉素组减轻。博来霉素组和寡核苷酸组大鼠肺组织中TGF—β1、PAI-1表达水平均明显高于生理盐水组，博来霉素组和寡核苷酸组大鼠雾化后第7天TGF—β1、PAI-1的积分吸光度值分别为182±12和169±12、128±11和113±13，明显高于生理盐水组的21±6和27±9，第28天时（68±7和87±7、54±8和57±8）仍高于生理盐水组（22±7和26±7）；雾化后第7天、第14天和第28天，寡核苷酸组大鼠I、Ⅲ型胶原mRNA表达水平分别为1．36±0．10、1．19±0．28、1．22±0．24和1．20±0．09、0．62±0．09、0．76±0．12，明显低于博来霉素组（3．29±0．28、2．04±0．25、1．91±0．30和1．63±0．15、1．58±0．13、1．12±0．09），寡核苷酸组大鼠肺组织中羟脯氨酸含量（mg／g）分别为3．02±0．13、3．24±0．31和3．60±0．16，明显低于博来霉素组的3．76±0．10、3．92±0．30和4．62±0．28。结论STAT1反义寡核苷酸雾化吸入能减轻博来霉素致肺纤维化大鼠肺泡炎和肺纤维化，其机制可能与抑制TGF—β1、PAl-1的表达，Ⅰ、Ⅲ型胶原mRNA表达减少，羟脯氨酸含量降低有关。