Expression of Thyroid Transcription Factor-1(TTF-1)in Lung Carcinomas and Its Correlations with Apoptosis and Angiogenesis

OBJECTIVE To investigate the correlations between the expression of thyroid transcription factor-1 （TTF-1） and apoptosis and angiogenesis in lung carcinomas. METHODS A 829 microarray of the paraffin tissue chips was constructed, which contained 196 lung carcinomas, 10 normal lung tissues, and 1 muscular tissue. Terminal deoxynucleotidyl transferase mediated nick end labeling （TUNEL） and immunohistochemical SP method were used to detect apoptosis and expression of TTF-1 and CD34 in different types of lung carcinomas. A Leica Q500 MC image analysis system was used to measure and calculate TTF-1 positive unit （PU）, apoptotic index （AI） and microvessel density （MVD）. RESULTS AI of lung small cell carcinoma and large cell carcinoma were smaller than those of lung adenocarcinoma and squamous cell carcinoma （P = 0.000）. AI of lung carcinomas with lymph node metastases was smaller than that of those without （P = 0.039）. AI of lung carcinomas in TNM stage I-IV was smaller than that in stage I （P = 0.008）. The PU of the TTF-1 was negatively correlated with AI in small cell lung carcinoma （r = -0.752, P = 0.000）. MVD of lung carcinomas without lymph node metastases was smaller than that of those with lymph node metastasis （P = 0.031）. MVD of lung carcinomas in TNM stage I was smaller than that in stage I-IV （P = 0.040）. The PU of TTF-1 was positively correlated with MVD in lung adenocarcinoma （r = 0.708, P = 0.000）. CONCLUSION There is a negative correlation between TTF-1 PU and AI in small cell lung carcinoma. TTF-1 PU and AI may be correlated with each other. There is a positive correlation between TTF-1 PU and MVD in lung adenocarcinoma. TTF-1 may induce the development of lung adenocarcinoma by inducing tumor angiogenesis.

Reliability of a Tissue Microarray in Detecting Thyroid Transcription Factor-1 Protein in Lung Carcinomas

OBJECTIVE To compare the expression of the thyroid transcription factor-1 （TTF-1） in human normal adult type Ⅱ alveolar epithelial cells, embryonic pneumocytes and cancer cells of lung carcinoma and metastatic lymph nodes using a tissue microarray （TMA） along with paired conventional full sections, and to investigate the reliability of tissue microarrays in detecting protein expression in lung carcinoma. METHODS A lung carcinoma TMA including 765 cores was constructed. TTF-1 protein expression in both TMA and paired conventional full sections were detected by the immunohistochemical SP method using a monoclonal antibody to TTF-1. A PU （Positive Unit） of TTF-1 protein was assessed quantitatively by the Leica Q500MC image analysis system with results from the paired conventional full sections as controls. RESULTS There was no significance between TMA and paired conventional full sections in TTF-1 expression in different nuclei of the lung tissue. CONCLUSION TTF-1 protein expression in lung carcinoma detected by TMA was highly concordant with that of paired full sections. TMA is a reliable method in detecting protein expression.

Exosome-mediated transfer of circRNA563 promoting hepatocellular carcinoma by targeting the microRNA148a-3p/metal-regulatory transcription factor-1 pathway

BACKGROUND Mesenchymal stem cells(MSCs)exert anti-oncogenic effects via exosomes containing non-coding RNA(ncRNA),which play important roles in tumor biology.Our preliminary study identified the interaction of the ncRNA hsa_-circ_0000563(circ563)and the circ563-associated miR-148a-3p in exosomes,as miR-148a-3p and its target metal-regulatory transcription factor-1(MTF-1)are implicated in hepatocellular carcinoma(HCC)progression.AIM To identify the clinical significance,functional implications,and mechanisms of circ563 in HCC.METHODS The expression levels of miR-148a-3p and MTF-1 in exosomes derived from MSC and HCC cells were compared,and their effects on HCC cells were assessed.Using a dual-luciferase reporter assay,miR-148a-3p was identified as an associated microRNA of circ563,whose role in HCC regulation was assessed in vitro and in vivo.RESULTS The silencing of circ563 blocked the HCC cell proliferation and invasion and induced apoptosis.Co-culturing of HCC cells with MSC-derived exosomes following circ563 overexpression promoted cell proliferation and metastasis and elicited changes in miR-148a-3p and MTF-1 expression.The tumor-promoting effects of circ563 were partially suppressed by miR-148a-3p overexpression or MTF-1 depletion.Xenograft experiments performed in nude mice confirmed that circ563-enriched exosomes facilitated tumor growth by upregulating the expression of MTF-1.In HCC tissues,circ563 expression was negatively correlated with miR-148a-3p expression but positively correlated with MTF-1 levels.CONCLUSION MSCs may exhibit anti-HCC activity through the exosomal circ563/miR-148a-3p/MTF-1 pathway,while exosomes can transmit circ563 to promote oncogenic behavior by competitively binding to miR-148a-3p to activate MTF-1.

Optimized thyroid transcription factor-1 core promoter-driven microRNA-7 expression effectively inhibits the growth of human non-small-cell lung cancer cells

Targeted gene therapy has become a promising approach for lung cancer treatment.In our previous work,we reported that the targeted expression of microRNA-7(miR-7)operated by thyroid transcription factor-1(TTF-1)promoter inhibited the growth of human lung cancer cells in vitro and in vivo;however,the intervention efficiency needed to be further improved.In this study,we identified the core promoter of TTF-1(from-1299 bp to-871 bp)by 5’deletion assay and screened out the putative transcription factors nuclear factor-1(NF-1)and activator protein-1(AP-1).Further analysis revealed that the expression level of NF-1,but not AP-1,was positively connected with the activation of TTF-1 core promoter in human non-small-cell lung cancer(NSCLC)cells.Moreover,the silencing of NF-1 could reduce the expression level of miR-7 operated by TTF-1 core promoter.Of note,we optimized four distinct sequences to form additional NF-1-binding sites(TGGCA)in the sequence of TTF-1 core promoter(termed asTTF-1 promoter),and verified the binding efficiency of NF-1 on theTTF-1 promoter by electrophoretic mobility shift assay(EMSA).As expected,theTTF-1 promoter could more effectively drive miR-7 expression and inhibit the growth of human NSCLC cells in vitro,accompanied by a reduced transduction of NADH dehydrogenase(ubiquinone)1αsubcomplex 4(NDUFA4)/protein kinase B(Akt)pathway.Consistently,TTF-1 promoter-driven miR-7expression could also effectively abrogate the growth and metastasis of tumor cells in a murine xenograft model of human NSCLC.Finally,no significant changes were detected in the biological indicators or the histology of some important tissues and organs,including heart,liver,and spleen.On the whole,our study revealed that the optimized TTF-1 promoter could more effectively operate miR-7 to influence the growth of human NSCLC cells,providing a new basis for the development of microRNA-based targeting gene therapy against clinical lung cancer.

共表达甲状腺转录因子1与p40的非小细胞肺癌患者临床病理特征分析

目的探讨共表达甲状腺转录因子1(TTF-1)和p40的非小细胞肺癌(NSCLC)患者的临床病理特征。方法收集7例共表达TTF-1和p40的NSCLC患者的资料,回顾性分析其临床特征、病理形态、免疫表型及分子特征,并复习相关文献。结果患者中位年龄58岁,多为男性且吸烟者;影像显示为外周型肿块。肿瘤细胞呈实性巢状排列,瘤细胞呈圆形、卵圆形或多角形,胞质透明或嗜酸性,核分裂象>10个/10HPF;3例可见脉管内癌栓。同一群肿瘤细胞同时表达TTF-1和p40,CK7、p63、CK5/6和napsinA呈灶性或弥漫表达,增殖指数Ki-67阳性10%~90%。2例采用ARMS-PCR法分别检测到表皮生长因子受体(EGFR)18号外显子G719A/S/C突变和21号外显子L858R突变,1例采用二代测序法检测到TPM3-ROS1融合突变和ROS1(G2032R)突变。随访1~46个月,2例患者分别于22、46个月死亡,3例患者出现颈部淋巴结或脑转移。结论共表达TTF-1和p40的NSCLC具有独特的临床病理特征,临床进展快,预后差,可能是一种新的肿瘤实体。

P40及TTF-1共表达非小细胞肺癌7例临床病理分析

目的:P40及甲状腺转录因子1(thyroid transcription factor-1,TTF-1)被广泛应用于肺鳞状细胞癌和肺腺癌的鉴别诊断,两者共表达的非小细胞肺癌(non-small cell lung cancer,NSCLC)病例则极为罕见。本研究旨在探讨P40及TTF-1共表达NSCLC的临床及病理学特点。方法:收集山东大学附属威海市立医院2019年5月至2023年9月确诊的7例P40及TTF-1共表达NSCLC患者,分析其临床及病理学特点,采用基因检测及免疫组织化学染色检测相关指标表达情况,并随访患者。结果:7例患者均为男性,年龄57~80(中位数71)岁,除1例外其余6例均有吸烟史;6例患者肿瘤为外周型,1例为中央型;肿物长径为2.0~8.5(中位数5.8)cm。5例患者出现肿瘤转移。2例病死患者第1次确诊至死亡的时间间隔分别为12和55个月。HE染色示肿瘤分化差,肿瘤细胞排列紧密,呈片状、巢团样分布,可见坏死及炎细胞浸润,肿瘤细胞大小不一,形态多样,细胞质多呈嗜酸性,细胞核大,形状不规则,核仁易见。免疫组织化学染色可见P40、TTF-1、P63、细胞角蛋白(cytokeratin,CK)7、CK5/6广泛阳性表达,而天冬氨酸肽酶A(Napsin A)基本上为阴性表达。基因检测除1例为TP53突变外,其余无突变。结论:P40及TTF-1共表达NSCLC是一种罕见的亚型,其发病率低,但恶性程度高,好发于有吸烟史的老年人,大部分病例发现时即偏向晚期,病理结果显示其为既不属于腺癌也不属于鳞状细胞癌的低分化肿瘤。

分化型甲状腺癌组织中TTF-1、Galectin-3表达水平与患者临床表现、预后的关系

目的 探讨分化型甲状腺癌(DTC)组织中甲状腺转录因子-1(TTF-1)、半乳糖凝集素-3(Galectin-3)表达水平与患者临床表现、预后的关系。方法 选取2017年1月1日至2020年5月30日该院收治的76例DTC患者作为研究对象,将手术过程中取得的癌组织标本纳入DTC组(n=76),将对应的癌旁组织标本纳入癌旁组(n=76)。免疫组化法检测TTF-1、Galectin-3在DTC组及癌旁组的表达情况,并分析TTF-1、Galectin-3表达水平与DTC患者临床病理特征的关系。采用多因素Cox回归分析探讨影响DTC患者预后的相关因素。结果 DTC组TTF-1、Galectin-3阳性表达率高于癌旁组,差异有统计学意义(P<0.05)。TNM分期为Ⅲ~Ⅳ期、低分化、组织分型为甲状腺乳头状癌、有淋巴结转移的DTC患者TTF-1阳性表达率、Galectin-3阳性表达率高于TNM分期为Ⅰ~Ⅱ期、中/高分化、组织分型为甲状腺滤泡癌、无淋巴结转移的DTC患者,差异有统计学意义(P<0.05)。TTF-1阴性、Galectin-3阴性DTC患者的3年总生存率高于TTF-1阳性、Galectin-3阳性DTC患者,差异有统计学意义(P<0.05)。多因素Cox回归分析结果显示,有淋巴结转移、TTF-1阳性、Galectin-3阳性是DTC患者预后的影响因素(P<0.05)。结论 TTF-1、Galectin-3与DTC患者TNM分期、分化程度、组织分型、淋巴结转移及3年生存率有关,对DTC患者病情判断及预后评估有重要参考价值。

囊腔型肺癌患者CT影像特征及其与甲状腺转录因子-1表达的关系研究

目的探究囊腔型肺癌患者CT影像特征与甲状腺转录因子-1(TTF-1)的关系。方法回顾性分析123例囊腔型肺癌患者的临床资料,均行CT影像学检查。根据甲状腺转录因子-1(TTF-1)的表达情况分为TTF-1高表达组(n=58)以及TTF-1中/低表达组(n=65)。结果两组CT影像学特征比较结果显示,其中囊腔形态、是否存在血管造影征、支气管充气征、毛刺、肺部蜂窝征、磨玻璃征在两组中的占比存在统计学差异(P<0.05);腔内分隔、胸膜凹陷的病例数占比差异无统计学意义(P>0.05)。相关性分析结果显示,囊腔型肺癌患者CT影像学特征与TTF-1的表达不存在显著相关性(P>0.05)。结论TTF-1表达阳性患者与阴性患者的部分CT影像学特征的病例数占比存在差异,但相关性分析结果为不存在相关性。

LncRNA MIAT、LASP1蛋白在甲状腺癌组织中的表达及与预后的相关性

目的探讨长链非编码RNA心肌梗死相关转录本(LncRNA MIAT)、LIM和SH3蛋白1(LASP1)蛋白在甲状腺癌组织内的表达水平及与预后的关系。方法选取63例甲状腺癌患者,收集其癌组织、癌旁正常组织,测定LncRNA MIAT、LASP1蛋白表达水平,并进行对比分析;同时分析LncRNA MIAT、LASP1蛋白表达与甲状腺癌患者临床病理特征的关系;另随访3年,分析LncRNA MIAT、LASP1蛋白表达与甲状腺癌患者预后的关系。结果癌组织LncRNA MIAT相对表达量与LASP1蛋白阳性表达率均高于癌旁正常组织,有统计学差异(P<0.05)。LncRNA MIAT、LASP1蛋白表达与甲状腺癌患者的淋巴结转移、临床分期有关,有统计学差异(P<0.05);LncRNA MIAT高表达、LASP1蛋白阳性表达患者的3年生存率低于LncRNA MIAT低表达、LASP1蛋白阴性表达患者,有统计学差异(P<0.05)。结论LncRNA MIAT、LASP1蛋白在甲状腺癌组织中表现为高水平,其表达水平与患者临床分期、淋巴结转移有关,且表达水平越高,患者预后越差。

肝细胞癌患者癌组织TTF-1、p53、p63表达变化及其对术后生存的影响

目的探讨肝细胞癌(HCC)患者癌组织甲状腺转录因子(TTF)-1、p53和p63表达变化及其对术后生存的影响。方法2019年1月~2021年12月我院收治的HCC患者56例,均行肝内肿瘤切除术治疗,术后随访2年。采用免疫组化法检测癌组织和癌旁组织TTF-1、p53和p63表达。结果HCC患者癌组织TTF-1表达阳性率为33.9%,显著低于癌旁组织的73.2%(P<0.05),而p53和p63表达阳性率分别为76.8%和64.3%,显著高于癌旁组织的7.1%和32.1%(P<0.05);34例Ⅰ~Ⅱ期和19例高分化肿瘤患者癌组织TTF-1阳性率分别为47.1%和63.1%,显著高于22例Ⅲ~Ⅳ期和37例中/低分化者的13.6%和18.9%(P<0.05);Ⅲ~Ⅳ期肿瘤、38例有淋巴结转移、21例低分化肿瘤和22例有门静脉癌栓的HCC患者癌组织p53阳性率分别为95.4%、89.5%、100.0%和95.4%,显著高于Ⅰ~Ⅱ期肿瘤、无淋巴结转移、中/高分化和无门静脉癌栓者(分别为64.7%、50.0%、59.5%和64.7%,P<0.05);Ⅲ~Ⅳ期肿瘤、有淋巴结转移和低分化肿瘤组织p63阳性率分别为86.4%、73.7%和85.7%,显著高于Ⅰ~Ⅱ期、无淋巴结转移和中/高分化者的50.0%、44.4%和48.7%(P<0.05);19例TTF-1阳性者1 a和2 a生存率分别为84.2%和73.3%,显著高于37例阴性者的51.4%和35.1%(P<0.05);43例p53阳性者1 a和2 a生存率分别为53.5%和39.3%,显著低于13例阴性者的92.3%和76.9%(P<0.05);36例p63阳性者1 a和2 a生存率分别为47.2%和33.3%,显著低于20例阴性者的90.0%和75.0%(P<0.05)。结论HCC患者癌组织TTF-1阳性表达率较低,而p53和p63阳性表达率较高,而它们都可能在HCC发病过程中起作用,并影响患者生存率,值得进一步研究。

胸腔积液沉渣包埋组织TTF-1、Galectin-3的表达水平与肺腺癌恶性生物学行为间的关系

目的探讨胸腔积液沉渣包埋组织甲状腺转录因子1(TTF-1)、半乳糖凝集素-3(Galectin-3)的表达水平与肺腺癌恶性生物学行为间的关系。方法选取2020年10月至2023年3月在该院就诊的肺腺癌患者163例,根据分化程度分为高分化组(26例)、中分化组(78例)、低分化组(59例)。对比3组胸腔积液沉渣包埋组织TTF-1、Galectin-3及恶性生物学行为相关基因(p16基因mRNA)表达水平,Spearman秩相关系数分析胸腔积液沉渣包埋组织TTF-1、Galectin-3与p16基因mRNA表达水平的相关性,多元线性回归分析胸腔积液沉渣包埋组织TTF-1、Galectin-3与p16基因mRNA表达水平间的依存关系,限制性立方样条图分析胸腔积液沉渣包埋组织TTF-1、Galectin-3与p16基因mRNA表达水平间的剂量-效应关系。结果低分化组胸腔积液沉渣包埋组织TTF-1、Galectin-3表达水平高于中分化组、高分化组,p16基因mRNA表达水平低于中分化组、高分化组,中分化组胸腔积液沉渣包埋组织TTF-1、Galectin-3表达水平高于高分化组,p16基因mRNA表达水平低于高分化组,差异有统计学意义(P<0.05);胸腔积液沉渣包埋组织TTF-1(r=-0.752,P<0.001)、Galectin-3(r=-0.811,P<0.001)表达水平与p16基因mRNA表达水平呈负相关;胸腔积液沉渣包埋组织Galectin-3表达水平与p16基因mRNA表达水平间无线性依存关系(P>0.05),胸腔积液沉渣包埋组织TTF-1表达水平与p16基因mRNA表达水平间有线性依存关系(P=0.049);当胸腔积液沉渣包埋组织TTF-1表达水平<4分、胸腔积液沉渣包埋组织Galectin-3表达水平<3分时,对p16基因mRNA表达作用最显著。结论胸腔积液沉渣包埋组织TTF-1、Galectin-3表达水平与肺腺癌恶性生物学行为关系密切,早期检测对临床实现精准干预避免病情恶化具有重要意义。

TTF-1和P40共表达的非小细胞肺癌2例并文献复习

分析2例共表达甲状腺转录因子1(thyroid transcription factor-1,TTF-1)和蛋白40(protein 40,P40)的非小细胞肺癌(non-small cell lung cancer,NSCLC)患者的临床病理学特征。2例患者均为老年男性,均有长期吸烟史,并伴有胸闷、胸痛、咳嗽等呼吸道症状;CT检查提示肺癌;镜下瘤细胞呈巢团状分布,具有类似鳞状上皮分化特征,可观察到细胞边界和细胞间连接,无腺腔结构和黏液。2例细胞角蛋白(cytokeratin,CK)7、TTF-1、CK5/6、P40、P63均呈弥漫强阳性,P53均呈突变型表达模式,无整合酶相互作用分子-1(integrase interactor-1,Ini-1)和染色质重塑复合物核心催化亚基-1(brahma-related gene 1,BRG-1)表达缺失,细胞增殖指数Ki-67增高。2例均发生肿瘤蛋白53(tumor protein 53,TP53)基因突变。同时具有腺上皮和鳞状上皮分化免疫表型的NSCLC极为罕见,迄今为止8篇文献(含本研究在内)共报道的12例共表达TTF-1和P40的NSCLC病例中,10例检测到TP53基因突变。因病例数极少,2021年世界卫生组织胸部肿瘤分类未提出确切的诊断分型和预后建议,仍需要更多的病例报道补充。

卵巢癌组织中TTF-1、CyclinD1的表达及其与淋巴管生成关系的研究

目的探讨甲状腺转录因子1(TTF-1)和细胞周期蛋白D1(CyclinD1)在卵巢癌组织中的表达情况,分析其与淋巴管生成的关系。方法收集60例卵巢癌组织样本和20例经病理检查证实的正常卵巢组织。制备组织切片进行TTF-1、CyclinD1和D2-40免疫组织化学(免疫组化)染色,基于半定量积分法评价TTF-1、CyclinD1染色结果。依据Weidner评价方法评估D2-40染色结果,计算淋巴管密度(LVD)。结果TTF-1和CyclinD1的阳性表达率在卵巢癌组织中分别为58%和83%,均高于其在正常卵巢组织中的5%和10%(P均<0.001)。病理分期Ⅲ~Ⅳ期、淋巴结转移阳性、腹膜转移阳性、T3~T4期、N1期和M1期的卵巢癌组织中TTF-1及CyclinD1的阳性表达率较高(P均<0.05);患者年龄、组织学类型与卵巢癌组织中TTF-1及CyclinD1的阳性表达率无关(P均>0.05)。病理分期Ⅲ~Ⅳ期、淋巴结转移阳性、腹膜转移阳性的卵巢癌组织LVD较高(P均<0.05)。卵巢癌组织中TTF-1、CyclinD1阳性表达者的LVD均高于阴性表达者(P均<0.05)。结论TTF-1与CyclinD1在卵巢癌组织中呈现高表达。卵巢癌病情较重、出现淋巴管生成和转移者的TTF-1和CyclinD1表达较高。TTF-1和CyclinD1可作为卵巢癌干预的潜在新靶点。

西格列汀通过上调TTF-1/SP-B通路对LPS诱导小鼠急性肺损伤的保护作用

目的 探讨小鼠急性肺损伤(acute lung injury,ALI)状态下DPP4(dipeptidyl peptidase 4 inhibitor,DPP4I)抑制剂西格列汀对肺组织的保护作用及潜在的分子机制。方法 将32只雄性BALB/C小鼠随机分为对照组、DPP4抑制剂西格列汀组(DPP4I组)、内毒素组(LPS组)和LPS+DPP4I组,每组8只。采用气道内注射LPS建立小鼠ALI模型,72 h后获取标本,通过HE染色观察肺组织病理学改变及损伤评分,采用Diff-Quik染色对肺泡灌洗液(alveolar larage fluid,BALF)中炎症细胞分类计数,使用湿/干比(W/D)检测肺水肿程度,使用qPCR和western blotting法分析肺组织中甲状腺转录因子-1(thyroid transcription Factor 1,TTF-1)和表面活性物质相关蛋白-B(surfactant-associated protein-B,SP-B)的mRNA和蛋白表达水平。结果 小鼠气道内注射LPS干预72 h后,肺组织出现明显的病理学改变,肺损伤评分增加,肺水肿指标W/D显著升高,BALF中细胞总数、中性粒细胞数、巨噬细胞数和淋巴细胞数明显增多,肺组织中TTF-1和SP-B的mRNA和蛋白表达水平明显降低,差异均有统计学意义(P <0.05)。对照组与DPP4I组未见明显病理改变。与LPS组相比,LPS+DPP4I组小鼠的肺组织病理改变程度、肺损伤评分、W/D比值、BALF中细胞总数、中性粒细胞数、巨噬细胞数和淋巴细胞数均明显更低,肺组织TTF-1和SP-B的mRNA和蛋白表达水平均明显更高(P <0.05)。结论 在小鼠ALI模型中DPP4抑制剂西格列汀可能通过上调肺组织TTF-1促进SP-B分泌,减轻肺损伤和炎症反应水平,为DPP4I应用于急性呼吸窘迫综合征(acute respiratory distress syndrome,ARDS)的临床治疗奠定了实验基础。

甲状腺转录因子-1表达联合超声检查对甲状腺乳头状癌侵袭性的预测价值

目的:探讨甲状腺乳头状癌(PTC)甲状腺转录因子-1(TTF-1)的表达情况,评价TTF-1结合超声特征预测PTC侵袭性的价值。方法:回顾性收集行PTC术前超声引导下细针抽吸穿刺(FNA)并接受手术治疗、有病理结果的344例患者的临床资料,根据是否伴颈部淋巴结转移(CLNM)及周边软组织转移分为转移组228例和未转移组116例。通过单因素卡方检验和多因素logistics回归分析其与TTF-1、病灶与甲状腺被膜关系、病灶钙化、病灶血流分布之间的相关性。采用ROC曲线评价各危险因素对甲状腺乳头状癌侵袭性的预测价值。结果:TTF-1表达、病灶内微钙化及病灶血流信号呈周边分布均与PTC伴CLNM及周边软组织转移独立相关(均P<0.05)。结论:TTF-1是预测PTC侵袭性的潜在分子标志物。TTF-1结合超声特征对预测PTC的侵袭性非常有价值。

Mechanism of ELL-associated factor 2 and vasohibin 1 regulating invasion,migration,and angiogenesis in colorectal cancer

BACKGROUND As a novel endogenous anti-angiogenic molecule, vasohibin 1(VASH1) is not only expressed in tumor stroma, but also in tumor tissue. Moreover, studies have shown that VASH1 may be a prognostic marker in colorectal cancer(CRC). Knockdown of VASH1 enhanced transforming growth factor-β1(TGF-β1)/Smad3 pathway activity and type Ⅰ/Ⅲ collagen production. Our previous findings suggest that ELL-associated factor 2(EAF2) may play a tumor suppressor and protective role in the development and progression of CRC by regulating signal transducer and activator of transcription 3(STAT3)/TGF-β1 signaling pathway. However, the functional role and mechanism of VASH1-mediated TGF-β1 related pathway in CRC has not been elucidated.AIM To investigate the expression of VASH1 in CRC and its correlation with the expression of EAF2. Furthermore, we studied the functional role and mechanism of VASH1 involved in the regulation and protection of EAF2 in CRC cells in vitro.METHODS We collected colorectal adenocarcinoma and corresponding adjacent tissues to investigate the clinical expression of EAF2 protein and VASH1 protein in patients with advanced CRC. Following, we investigated the effect and mechanism of EAF2 and VASH1 on the invasion, migration and angiogenesis of CRC cells in vitro using plasmid transfection.RESULTS Our findings indicated that EAF2 was down-regulated and VASH1 was upregulated in advanced CRC tissue compared to normal colorectal tissue. KaplanMeier survival analysis showed that the higher EAF2 Level group and the lower VASH1 Level group had a higher survival rate. Overexpression of EAF2 might inhibit the activity of STAT3/TGF-β1 pathway by up-regulating the expression of VASH1, and then weaken the invasion, migration and angiogenesis of CRC cells.CONCLUSION This study suggests that EAF2 and VASH1 may serve as new diagnostic and prognostic markers for CRC, and provide a clinical basis for exploring new biomarkers for CRC. This study complements the mechanism of EAF2 in CRC cells, enriches the role and mechanism of CRC cellderived VASH1, and provides a new possible subtype of CRC as a therapeutic target of STAT3/TGF-β1 pathway.

甲状腺微小癌患者血清TSH、TTF-1与超声造影参数相关性及联合检测价值

目的探讨甲状腺微小癌患者血清促甲状腺激素(TSH)、甲状腺转录因子-1(TTF-1)与超声造影参数相关性及联合检测价值。方法前瞻性选取河北省残疾人康复中心和哈励逊国际和平医院2018年8月至2020年8月甲状腺微小癌患者106例作为恶性组,另选取同期良性甲状腺结节患者106例作为良性组。比较两组血清TSH、TTF-1、超声造影参数[造影剂峰值强度(PI)、达峰时间(TTP)、时间-强度曲线下面积(TIC-AUC)],分析血清TSH、TTF-1与超声造影参数相关性,评价血清TSH、TTF-1、超声造影参数单独及联合诊断甲状腺微小癌价值,分析血清TSH、TTF-1、超声造影参数与病理特征的关系。结果恶性组血清TSH、TTF-1高于良性组,PI、TIC-AUC低于良性组,TTP长于良性组(P<0.05);血清TSH、TTF-1与PI、TIC-AUC呈负相关,与TTP呈正相关(P<0.05);血清TSH、TTF-1联合PI、TIC-AUC、TTP诊断甲状腺微小癌的AUC为0.914(95%CI:0.868~0.948),敏感度为87.74%,特异度为84.91%,明显优于各指标单独诊断;血清TSH、TTF-1、TTP与肿瘤直径、淋巴结转移、腺外浸润呈正相关,与分化程度呈负相关,PI、TIC-AUC与肿瘤直径、淋巴结转移、腺外浸润呈负相关,与分化程度呈正相关(P<0.05)。结论甲状腺微小癌患者血清TSH、TTF-1与超声造影参数PI、AUC、TTP显著相关,联合检测可作为临床诊断的重要途径,且与多项病理特征密切相关,能为临床评估病理进展提供有效信息。

高频彩色多普勒超声联合血清lncRNA OIP5-AS1在甲状腺癌诊断中的应用价值

目的探讨高频彩色多普勒超声(CDFI)联合血清长链非编码RNA Opa相互作用蛋白5反义转录本1(lncRNA OIP5-AS1)对甲状腺癌的诊断价值。方法选择2019年6月~2021年12月在本院就诊的175例甲状腺病变患者为观察对象,其中甲状腺癌患者93例,甲状腺良性病变患者82例,另选择同期健康体检人员90例作为对照组。分析患者CDFI表现特征,RT-qPCR检测血清lncRNA OIP5-AS1水平,ROC曲线分析血清lncRNA OIP5-AS1对甲状腺癌的诊断价值,评价CDFI联合血清lncRNA OIP5-AS1对甲状腺癌的诊断效能。结果病理诊断共206个结节,其中115个为恶性结节,91个为良性结节;175例患者中有147例为单发结节,28例为多发结节。病理诊断115个恶性结节中,CDFI检查出93个恶性结节,病理诊断91个良性结节中,CDFI检查出72个良性结节;病理诊断93例甲状腺癌与82例甲状腺良性病变中,CDFI检查出甲状腺癌73例与甲状腺良性病变65例。对照组、甲状腺良性病变、甲状腺癌患者血清lncRNA OIP5-AS1表达水平分别为(1.05±0.16)、(1.10±0.18)、(1.76±0.32),三组之间比较差异有统计学意义(F=267.827,P<0.05),对照组与甲状腺良性病变患者血清lncRNA OIP5-AS1表达水平比较差异无统计学意义(P>0.05);血清lncRNA OIP5-AS1诊断甲状腺癌的截断值为1.31,ROC曲线下面积(AUC)为0.868(95%CI 0.809~0.915),灵敏度为79.57%,特异度为81.71%,准确度为80.57%,CDFI诊断甲状腺癌的AUC为0.789(95%CI 0.721~0.847),灵敏度为78.49%、特异度为79.27%,准确度为78.86%,CDFI、血清lncRNA OIP5-AS1联合诊断甲状腺癌的AUC为0.913(95%CI 0.861~0.950),灵敏度为89.27%、特异度为76.82%,准确度为83.73%,其诊断效能显著高于CDFI、血清lncRNA OIP5-AS1单独检测。结论CDFI联合血清lncRNA OIP5-AS1对甲状腺癌诊断有较高的临床价值。

转录因子CREB3L1在甲状腺癌组织中的表达及生物学意义

目的探讨转录因子环腺苷酸响应元件结合蛋白3-样1(CREB3L1)在甲状腺癌(THCA)组织中的表达及其临床意义。方法从GEO、ArrayExpress、SRA、TCGA等数据库检索下载CREB3L1 mRNA在THCA组织中的表达谱,应用Wilcoxon非参数检验检测CREB3L1 mRNA在THCA组织和正常甲状腺组织中表达水平的差异;计算CREB3L1表达值的标准化均数差(SMD)及汇总受试者工作特征(SROC)曲线下面积等指标,综合评估CREB3L1 mRNA在THCA组织中的表达水平及其对THCA的区分能力。用上述数据集批量获取CREB3L1在THCA组织中的相关过表达基因,应用CistromeDB预测CREB3L1转录靶基因,用clusterProfiler对CREB3L1在THCA组织中的相关过表达基因、CREB3L1转录靶标交集基因进行基因本体和京都基因与基因组百科全书功能注释。在THPA数据库中查看CREB3L1蛋白在THCA组织中的表达水平。结果与正常甲状腺组织比较,THCA组织中CREB3L1蛋白表达水平呈上调趋势。基于基因芯片、高通量测序数据集共纳入1175例THCA组织和791例正常甲状腺组织样本。CREB3L1 mRNA在THCA组织中呈高表达[SMD=0.11,95%可信区间(95%CI):0.01~0.20],集成SROC曲线下面积为0.62(95%CI:0.57~0.66)。CREB3L1蛋白在THCA组织中高表达患者5年生存率比低表达者低。交叉基因主要富集在细胞周期信号通路上,主要生物学功能为细胞器裂解。细胞分裂周期6蛋白(CDC6)与CREB3L1呈正相关。结论CREB3L1在THCA组织中高表达不利于患者的预后,有可能通过靶向基因CDC6参与了THCA的发生、发展。

TTF-1、CK7、Napsin A联合检验对诊断肺腺癌的价值研究

目的:探究肺腺癌采用甲状腺转录因子-1(TTF-1)、细胞角蛋白7(CK7)、天冬氨酸蛋白酶(Napsin A)进行联合检验的价值。方法:选取2021年1月—2022年11月许昌北海医院收治的非小细胞肺癌患者100例作为研究对象,根据病理诊断结果分为肺鳞癌组、肺腺癌组,各50例。使用免疫组化法,检测患者病理组织中TTF-1、CK7、Napsin A阳性表达率,分析TTF-1、CK7、Napsin A单独检验与联合检验的准确率、敏感性和特异性及有无淋巴结转移患者联合检验阳性、1项阴性情况。结果:肺腺癌组TTF-1、CK7、Napsin A阳性表达率高于鳞癌组,差异有统计学意义(P<0.001);联合检验准确率、敏感度及特异度均高于三项指标单独检验,差异有统计学意义(P<0.05);肺腺癌淋巴结转移患者联合检验阳性率高于未转移患者,差异有统计学意义(P<0.05);淋巴结有转移患者有1项阴性率低于未转移患者,差异有统计学意义(P=0.003)。结论:TTF-1、CK7、NapsinA单项检测,能够帮助患者鉴别肺腺癌,通过联合检测,可获得较高的准确率,同时,肺腺癌患者淋巴结转移者中,阳性表达率较高,可为临床诊断提供参考。