细胞分裂周期蛋白73基因缺失抑制粟酒裂殖酵母细胞的有性生殖和有丝分裂

cdc73基因编码粟酒裂殖酵母(Schizosaccharomyces Pombe)RNA聚合酶Ⅱ辅助因子Cdc73,参与G_(2)期检查点激活并调控细胞周期。但cdc73基因缺失对细胞有丝分裂动力学的调控尚不清楚。本研究采用活细胞成像、荧光蛋白标记技术探究粟酒裂殖酵母cdc73基因缺失后对细胞有性生殖和细胞有丝分裂中微管、肌动蛋白、线粒体和组蛋白动力学的影响。结果表明:在有性生殖中,cdc73基因缺失会导致子囊孢子长度增加14.23%,产4个孢子数量的细胞减少64.08%;活细胞成像结果分析发现,在有丝分裂中,分裂后期微管伸长的长度缩短11.21%,伸长时间减少17.39%;肌动蛋白环形成和收缩速率分别降低33.33%和26.09%,形成和收缩时间分别延长58.00%和40.38%;同时,肌动蛋白环、线粒体和组蛋白表达量都增加。本研究揭示了cdc73基因缺失可抑制有丝分裂中纺锤体的伸长,延缓肌动蛋白环的形成与收缩,为进一步探寻Cdc73蛋白在细胞分裂中参与调控微管和肌动蛋白动力学功能提供了一定的科学依据。

Identification of circulating CD90^+ CD73^+ cells in cirrhosis of liver

AIM:To identify circulating CD90 + CD73 + CD45 cells and evaluate their in vitro proliferating abilities.METHODS:Patients with cirrhosis(n=43),and healthy volunteers(n=40)were recruited to the study.Mononuclear cells were isolated and cultured from the peripheral blood of controls and cirrhosis patients.Fibroblast-like cells that appeared in cultures were analyzed for morphological features,enumerated by flow cytometry and confirmed by immunocytochemistry(ICC).Colony forming efficiency(CFE)of these cells was assessed and expressed as a percentage.RESULTS:In comparison to healthy volunteers,cells obtained from cirrhotic patients showed a significantincrease(P<0.001)in the percentage of CD90+CD73+ CD45 cells in culture.Cultured cells also showed 10 fold increases in CFE.Flow cytometry and ICC confirmed that the proliferating cells expressed CD90 + CD73 + in the cultures from cirrhosis patients.CONCLUSION:These results indicate the presence of circulating CD90 + CD73 + CD45 cells in patients with liver cirrhosis that have the potential to proliferate at a higher rate.

Effect of GP73 silencing on proliferation and apoptosis in hepatocellular cancer

AIM: To investigate the roles of Golgi protein(GP) 73 in the regulation of cell proliferation and apoptosis. METHODS: Stealth RNAi targeting GP73 gene sequence was used to silence its expression in Hep G2 cells and Bel7402 cells. Stealth RNAi effects were assessed by reverse transcriptase polymerase chain reaction and ELISA. Cell proliferation assay and cell cycle analysis were assessed by MTT assay and flow cytometry. Apoptosis was assessed by flow cytometry andtransmission electron microscopy. Apoptosis-related proteins were assessed by western immunoblot analysis.RESULTS: Stealth RNAi targeting GP73 gene sequence markedly reduced the expression of GP73 gene. The reduction of GP73 in Hep G2 cells and Bel7402 cells inhibited cell proliferation and induced apoptosis, however, terminal apoptosis occurred in Hep G2 cells, but early apoptosis occurred in Bel7402 cells. Reduced expression of GP73 gene might lead to a reduction in Bcl-2/Bax ratio, an increase in cytochrome c, but a reduction in capase-3.CONCLUSION: GP73 might play an important role in proliferation and apoptosis in hepatocellular carcinoma cells.

载脂蛋白E通过降低高尔基体膜蛋白73表达抑制小鼠肝癌细胞系增殖

目的探究载脂蛋白E(APOE)与高尔基体膜蛋白73(GP73)之间的调控关系,并明确其对肝癌细胞增殖的影响。方法分析在线网站肝癌数据库中APOE与GP73的相关性;小鼠分为对照及Apoe缺失组、对照及Gp73缺失组;细胞分为Gp73敲低组、Apoe敲低组(转染小干扰RNA或感染慢病毒)及相应对照;GP73过表达组、APOE过表达组(转染过表达质粒)及相应对照;GP73低表达组(转染小干扰RNA或雷帕霉素处理)及对照组。Western blot检测APOE和GP73的蛋白表达;CCK8法检测细胞增殖。结果在肝癌中GP73与APOE的表达负相关(P<0.001);在小鼠肝脏、肾脏组织中,Gp73缺失不影响APOE表达,而Apoe缺失导致GP73表达上调(P<0.001);在肝癌细胞系中,GP73改变不影响APOE表达,而APOE过表达或敲低引起GP73相应下调或上升(P<0.01);降低APOE促进肝癌细胞系增殖(P<0.01);下调GP73抑制Apoe敲低促进的小鼠肝癌细胞系增殖(P<0.001)。结论APOE负调控GP73。而通过降低GP73表达,从而抑制APOE下调介导的小鼠肝癌细胞系增殖。这种调控关系可能是肝癌的一个病理机制和潜在治疗靶点。

RNA干扰技术沉默GP73对人肝癌HepG2细胞迁移和侵袭的影响

目的·探讨RNA干扰技术(RNAi)沉默人肝癌HepG2细胞中高尔基体蛋白73(GP73)基因表达后,对细胞迁移和侵袭能力的影响。方法·应用阳离子脂质体法将设计合成的GP73小干扰RNA(siRNA)瞬时转染HepG2细胞。HepG2细胞分为空白对照组、阴性对照组和GP73 siRNA干扰组。各组培养48 h后,采用实时定量PCR(qRT-PCR)和ELISA法检测转染后HepG2细胞中GP73 mRNA和蛋白表达水平变化,Transwell迁移实验、划痕愈合实验及侵袭实验分别观察迁移和侵袭能力改变,qRTPCR和Western blotting法检测基质金属蛋白酶2(MMP-2)和MMP-9的表达情况。结果·GP73 siRNA能显著降低HepG2细胞中GP73 mRNA和蛋白的表达,转染后细胞的迁移和侵袭能力明显下降,其MMP-2和MMP-9 mRNA和蛋白表达水平均明显降低。结论·siRNA干扰介导GP73基因沉默可抑制人肝癌HepG2细胞的迁移和侵袭,其机制可能与下调MMP-2和MMP-9的表达水平有关。

三七总皂甙对肝癌细胞株、甲胎蛋白异质体及高尔基体糖蛋白-73表达的影响

目的:研究三七总皂甙(panax notoginsenosides,P N S)对不同肝癌细胞株、甲胎蛋白异质体(alpha-fetoprotein-L3,AFP-L3)分泌及高尔基体糖蛋白-73(Golgi glucoprotein 73,GP-73)的影响.方法:以肝癌细胞HepG2两种细胞株SMMC-7721和Bel-7402作为研究对象,分为空白对照组、5-氟尿嘧啶(5-fluorouracil,5-Fu)组和不同浓度梯度(10-400μg/mL)的PNS组,共培养120 h,利用MTT比色测定法检测细胞活性,ELISA及细胞分化法检测AFP-L3及GP-73活性.结果:PNS在>200μg/mL时可表现出对两种肝癌细胞株增殖的抑制,高浓度PNS(400μg/mL)对细胞活性影响较大,抑制率与5-Fu(40μg/mL)的作用相似.PNS组200、400μg/mL剂量均明显抑制肝癌两种细胞株GP-73活性,且剂量400μg/mL的抑制作用与5-Fu组比较有显著差异(P<0.05).PNS组剂量达400μg/mL时才能有效抑制肝癌两种细胞株AFP-L3活性,与对照组比较差异显著(P<0.01);且400 ng/mL剂量的抑制作用与5-Fu组没有显著差异.结论:PNS具有抑制肝癌细胞株的生长,降低AFP-L3与GP-73活性,肝癌细胞基因分化,诱导其在体外向正常肝细胞分化,且效果与剂量-时间呈正相关.

高尔基体蛋白73单克隆抗体的制备和鉴定

目的探讨高尔基体蛋白73(GP73)鼠源单克隆抗体的制备方法并进行鉴定。方法用GP73重组抗原蛋白免疫5只小鼠获得血清抗体,免疫小鼠脾细胞与sp2/0骨髓瘤细胞融合,经过筛选后选择GP73抗体阳性杂交瘤细胞进行克隆化培养,通过腹水制备获得高特异性和高效价的GP73单克隆抗体(单抗)。结果成功筛选出11株能稳定分泌特异性GP73单抗的杂交瘤细胞株,经多次复苏传代仍能稳定分泌特异性强、效价高的抗体。11株单抗均能结合天然状态下的GP73蛋白,与无关蛋白均无交叉反应,提示有较强的特异性。应用筛选出的配对GP73单抗可检测出浓度为1ng/ml的GP73基因工程表达抗原。结论制备的GP73杂交瘤细胞株分泌的抗体对GP73蛋白具有特异亲和性,并且有较高效价,为GP73蛋白诊断试剂的研制提供了关键技术基础。

基因重组人HSP73抗体的制备及对肿瘤细胞在温热作用后HSP70表达的检测

目的 用基因工程方法表达、提纯人热休克类似蛋白 73(HSP73) ,制备抗体 ,检测吐温 80协同 41℃温热对肿瘤细胞HSP70表达的影响。方法 用人HSP73基因构建原核细胞表达载体 pETHSP73,在大肠杆菌BL2 1中用半乳糖苷 (IPTG)诱导表达 ,经电泳法和ATP亲和层析法提取HSP73并作检测。用提纯蛋白免疫新西兰兔 ,制备抗HSP70多克隆抗体 ,测定其活性 ,用此抗体作免疫组化法观察 41℃温热和吐温 80协同时BGC 82 3胃癌细胞及B16黑色素瘤细胞的热休克蛋白 70 (HSP70 )表达情况。结果 人基因重组构建的pETHSP73能很好地在大肠杆菌中表达出分子量为73kD的蛋白。两种提纯方法均能有效提取表达蛋白 ,用 3a3单抗作Westrnblot检测证明该蛋白具有人HSP70的抗原活性 ,所得蛋白氨基酸测定和N端测序的结果与有关报道一致。以此蛋白制成的抗体活性可达 1∶80 0 0以上。并可检测出吐温 80合并温热有明显抑制肿瘤细胞SHP70表达的作用。结论 2 .1kb的基因片段构建的高表达载体能很好表达人HSP73活性蛋白。该蛋白免疫新西兰兔所得多克隆抗体具有很高抗人和鼠HSP70活性。用该抗体免疫组化法检测表明吐温 80协同 41℃温热可明显抑制肿瘤细胞HSP70的表达和耐热性的产生。

CD_(73)在皮肤鳞状细胞癌、基底细胞癌中的表达

目的探讨CD_(73)在皮肤鳞状细胞癌及基底细胞癌中的表达及意义。方法免疫组化方法检测10例人体正常皮肤、30例皮肤鳞状细胞癌及30例皮肤基底细胞癌皮损石蜡包埋标本中CD_(73)的表达情况。结果 CD_(73)在30例鳞状细胞癌中阳性表达率为100%,30例基底细胞癌中阳性表达率为60%,人体正常皮肤中阳性表达率为10%,CD_(73)在人体正常皮肤中阳性表达率明显低于鳞状细胞癌及基底细胞癌组(P值均<0.001)。CD_(73)在鳞状细胞癌中的表达强度高于基底细胞癌(P<0.001),CD_(73)在基底细胞癌中表达强度与人体正常表皮无差异(P>0.0167)。鳞状细胞癌中CD_(73)表达强度与肿瘤分化程度无统计学意义(P>0.05)。结论 CD_(73)在鳞状细胞癌中的表达显著升高,CD_(73)在基底细胞癌及鳞状细胞癌中表达存在差异。

GP73通过p53信号通路调节乳腺癌细胞MCF-7的增殖和凋亡

目的探讨高尔基蛋白73(GP73)对乳腺癌细胞MCF-7的增殖、凋亡的影响及相关机制。方法利用干扰及过表达GP73质粒转染乳腺癌细胞MCF-7,并利用CCK-8检测处理后细胞的增殖能力,利用流式细胞术方法检测处理组细胞的凋亡水平,利用qRT-PCR和Western印迹法测定GP73和p53 mRNA和蛋白的表达。采用qRT-PCR测定20例临床乳腺癌和癌旁组织中GP73和p53的mRNA水平,并分析乳腺癌组织中GP73和p53的mRNA水平的相关性。结果过表达GP73后MCF-7较对照组增殖能力上升(P<0.05),凋亡水平下降(P<0.05);干扰GP73后MCF-7增殖能力下降(P<0.05),凋亡率升高。同时过表达GP73和p53的乳腺癌细胞较单独过表达GP73的MCF-7细胞的增殖能力下降,凋亡水平上升。乳腺癌组织中GP73和p53 mRNA表达也呈负相关(r=-0.528,P<0.01)。结论 GP73可能通过p53信号通路调节乳腺癌细胞MCF-7的增殖和凋亡。

P^(73)基因在喉鳞癌中的表达及相关性研究

目的:探讨P73基因的表达与喉鳞癌LSCC的关系。方法:用免疫组化方法检测30例喉鳞癌组织和30例声带息肉中P73的表达。结果:P73阳性表达除2例定位于胞浆,1例定位于核膜外,其余均定位于细胞核。P73阳性表达率在喉癌组织和声带息肉中分别为:66.7%(20/30),50.0%(15/30)(P>0.05),P73与喉鳞癌的临床分型、分期无相关性。结论:P73基因可能并非喉癌癌变过程中的靶基因,在喉癌的发生发展中可能不发挥重要作用。

5型腺病毒E1A基因通过调控GP73的表达抑制肝癌细胞增殖的初步研究

目的:研究5型腺病毒(Ad5)E1A基因通过调控高尔基蛋白73(GP73)的表达水平,抑制肝癌细胞HepG2的增殖。方法:以腺病毒为模板、pcDNA-flag-Vector为载体,构建真核表达载体pcDNA3-Flag-Ad5E1A;免疫印迹实验鉴定重组蛋白Ad5E1A的表达;免疫印迹实验验证Ad5E1A对GP73表达水平的影响;将Ad5E1A基因转染HepG2细胞,用CCK-8试剂盒检测HepG2细胞的增殖情况。结果:免疫印迹实验结果证实,真核表达载体pcDNA3-Flag-Ad5E1A在HEK293细胞中得到表达;Ad5E1A可明显抑制GP73的表达。酶标仪检测发现,与转染Flag-GP73组相比,Ad5E1A组的抑制率为17.5%,差异无统计学意义(P>0.05);而与转染Flag-GP73组比,共转Ad5E1A和GP73组的抑制率为37.8%,差异有统计学意义(P<0.05)。结论:Ad5E1A基因通过调控GP73的表达抑制了肝癌细胞HepG2的增殖。为研究肝癌发生机制,开发新型治疗方案提供了实验基础。

Bone-derived MSCs encapsulated in alginate hydrogel prevent collagen-induced arthritis in mice through the activation of adenosine A_(2A/2B)receptors in tolerogenic dendritic cells

Tolerogenic dendritic cells(tol DCs)facilitate the suppression of autoimmune responses by differentiating regulatory T cells(Treg).The dysfunction of immunotolerance results in the development of autoimmune diseases,such as rheumatoid arthritis(RA).As multipotent progenitor cells,mesenchymal stem cells(MSCs),can regulate dendritic cells(DCs)to restore their immunosuppressive function and prevent disease development.However,the underlying mechanisms of MSCs in regulating DCs still need to be better defined.Simultaneously,the delivery system for MSCs also influences their function.Herein,MSCs are encapsulated in alginate hydrogel to improve cell survival and retention in situ,maximizing efficacy in vivo.The three-dimensional co-culture of encapsulated MSCs with DCs demonstrates that MSCs can inhibit the maturation of DCs and the secretion of pro-inflammatory cytokines.In the collagen-induced arthritis(CIA)mice model,alginate hydrogel encapsulated MSCs induce a significantly higher expression of CD39^(+)CD73^(+)on MSCs.These enzymes hydrolyze ATP to adenosine and activate A_(2A/2B)receptors on immature DCs,further promoting the phenotypic transformation of DCs to tol DCs and regulating naive T cells to Tregs.Therefore,encapsulated MSCs obviously alleviate the inflammatory response and prevent CIA progression.This finding clarifies the mechanism of MSCs-DCs crosstalk in eliciting the immunosuppression effect and provides insights into hydrogel-promoted stem cell therapy for autoimmune diseases.

血管靶向药联合化疗治疗中晚期肝癌的临床效果

目的探究血管靶向药联合化疗治疗中晚期肝癌的临床效果。方法选取2019年4月至2021年1月136例中晚期肝癌患者作为研究对象,随机将其分为对照组和观察组,各68例。对照组采用化疗治疗,观察组在对照组的基础上联合血管靶向药治疗。比较两组的治疗效果。结果治疗前,两组的甲胎蛋白(AFP)、甲胎蛋白异质体(AFP-L3)、高尔基体蛋白73(GP73)水平比较,差异无统计学意义(P>0.05);治疗后3个月,两组的AFP、AFP-L3、GP73水平均低于治疗前,且观察组低于对照组,差异具有统计学意义(P<0.05)。治疗前,两组的白细胞介素-2(IL-2)、肿瘤坏死因子-α(TNF-α)、白细胞介素-4(IL-4)、白细胞介素-6(IL-6)及白细胞介素-10(IL-10)水平比较,差异无统计学意义(P>0.05);治疗后3个月,两组的IL-2、TNF-α、IL-6水平低于治疗前,IL-4、IL-10水平高于治疗前,且观察组优于对照组,差异具有统计学意义(P<0.05)。两组的毒副反应总发生率比较,差异无统计学意义(P>0.05)。结论血管靶向药物联合化疗治疗中晚期肝癌患者的安全性较高,可降低肿瘤标志物水平,改善辅助性T细胞1(Th1)、辅助性T细胞2(Th2)因子水平,调节机体免疫功能,巩固化疗效果,值得临床推广与应用。

Hepatoprotective effects of Nigella sativa seed extract against acetaminophen-induced oxidative stress

Objective:To investigate the protective effects of Nigella sativa seed extract(NSSE) against acetaminophen(APAP)-induced hepaloloxicity in TIB-73 cells and rats.Methods:Toxicity in TIB-73 cells was induced with 10 μmol/L APAP and the protective effects of NSSE were evaluated at 25.50.75,100 μg/mL.For in rim examination,a total of 30 rals were equally divided into five experimental groups:normal control(vehicle),APAP(800 mg/kg body weight single IP injection) as a hepatotoxic control,and three APAP and NS pretreated(2 weeks) groups(APAP+NSSE 100 mg:APAP+NSSE 300 mg and APAP+NSSK 900 mg/kg).Results:TIB-73 cell viability was drastically decreased by(49.0±l.9)%after the 10 μmol/L APAP treatment,which also increased reactive oxygen species production.Co-treatment with NSSE at 25.50.75,and 100 μg/mL significantly improved cell viability and suppressed reactive oxygen species generation.In viro the APAP induced alterations in blood lactate levels,pH,anionic gap,and ion levels(HCO_3^-,Mg^(2+) and K^+),which tended to normalize with the NSSE pretreatment.The NSSE also significantly decreased elevated serum levels of alanine aminotransferase,aspartate aminotransferase,lactate dehydrogenase,and alkaline phosphatase induced by APAP,which correlated with decreased levels of hepatic lipid peroxidation(nialondialdehyde),increased superoxide dismutase levels,and reduced glutathione concentrations.Improved hepatic histology was also found in the treatment groups other than APAP group.Conclusions:The in vitro and in vim findings of this study demonstrated that the NSSE has protective effects against APAP-induced hepalotoxicity and metabolic disturbances by improving antioxidant activities and suppressing both lipid peroxidation and ROS generation.

神经祖细胞不对称分裂中纺锤体取向与细胞皮层极性的偶联机制

神经祖细胞的不对称分裂是神经发生的必要环节。近年来关于不对称分裂的研究,为果蝇及哺乳动物中枢神经系统发育期间神经祖细胞的分化机制提供了新的理解。在这一分裂模式中,纺锤体作为细胞结构的支架,受到细胞皮层极性信号的引导而改变取向,保证底部细胞命运决定子(cell fate determinants)的不对称分配。G蛋白亚基、各种接头蛋白及微管相关蛋白组成极性蛋白复合体,在纺锤体取向改变中发挥了有序的调节作用。现在细胞和分子水平探讨不对称分裂纺锤体与细胞皮层极性偶联这一标志性事件。

靶向CD73/PD-L1双特异性抗体的制备及其体外抗肿瘤功能评价

目的制备同时靶向胞外5'-核苷酸酶(cluster of differentiation 73,CD73)与程序性细胞死亡配体1(programmed cell death-ligand 1,PD-L1)的双特异性抗体,并对其体外结合能力和杀伤能力进行评价。方法采用基因工程方法,将PD-L1单链抗体(single-chain fragment variable,scFv)插入至CD73单抗铰链区中,构建抗CD73/PD-L1双特异性抗体(BS-21),通过CHO GS表达系统进行筛选,获得高表达量细胞株,经Protein A及分子筛纯化后,采用分子排阻高效液相色谱法(size exclusion chromatography-high performance liquid chromatography,SEC-HPLC)检测抗体纯度;流式细胞术检测抗体体外结合能力;通过外周血单个核细胞(peripheral blood mononuclear cell,PBMC)体外杀伤人肺癌细胞Calu 1检测抗体体外杀伤能力。结果经加压筛选获得了高产的细胞株;经纯化获得纯度为99.6%的双特异性抗体BS-21,该抗体能同时结合CD73和PD-L1分子;与anti CD73和anti PD-L1组相比,BS-21组显著提高免疫细胞对Calu 1肿瘤细胞的杀伤率(F均为30.36,P均<0.001)。结论双特异性抗体BS-21能同时降低CD73和PD-L1对免疫细胞的免疫抑制作用,具有较好的抗肿瘤功能。

舌鳞状细胞癌中p73、p63和p53基因的表达

目的 研究p 73、p 63和p 5 3基因蛋白在舌鳞状细胞癌中的表达及其意义。方法 用免疫组织化学S-P法检测 64例舌鳞状细胞癌组织标本p 73、p 63和p 5 3基因蛋白表达。结果 舌鳞癌中p 73、p 63和p 5 3基因蛋白阳性率分别为 61%、92 %和 5 0 %。p 73蛋白表达与T分类 (r =0 .3 44,P =0 .0 5 7)、区域淋巴结转移 (r =0 .3 3 4,p =0 .0 0 7)、肿瘤侵袭方式 (r =0 .3 40 ,P =0 .0 60 )和不良预后 (r =-0 .473 ,P =0 .0 0 0 )相关。p 63与所有临床病理特征和预后无关。p 5 3与区域淋巴结转移 (r=0 .2 63 ,P =0 .0 3 6)和不良预后 (r =-0 .3 42 ,P =0 .0 13 )相关。结论 p 73和p 5 3表达有助于判断舌鳞癌的生物学行为和预后。p

p73和GADD45α蛋白在邻苯二甲酸单(2-乙基己基)酯致人正常肝细胞L02和人肝癌细胞Hep3B周期阻滞中的作用

目的研究抑癌基因p73和生长抑制及DNA损伤诱导基因45α(GADD45α)蛋白对邻苯二甲酸单(2-乙基己基)酯[di(2-ethylhexyl)phthalate,MEHP]染毒人正常肝细胞L02和人肝癌细胞Hep3B周期的影响。方法将处于对数生长期的L02细胞和Hep3B细胞分别暴露于终浓度为0(溶剂对照,DMSO终浓度<1‰)、6.25、12.502、5.00、50.00、100.00μmol/L的MEHP溶液染毒细胞12 h。采用四甲基氮唑蓝(methylthiazoletetrazolium,MTT)比色法检测细胞增值率,采用流式细胞仪检测细胞的周期时相,采用Western blot法检测细胞周期调控蛋白p53、p73和GADD45α的表达量。结果与溶剂对照组相比,仅50μmol/L MEHP染毒L02细胞的增殖率升高(P<0.05),各浓度MEHP染毒Hep3B细胞的增殖率均下降(P<0.01),差异有统计学意义。与溶剂对照组相比,仅100μmol/L MEHP染毒L02细胞的G1期和G2期细胞构成比下降,S期细胞构成比上升,差异均有统计学意义(P<0.05);而100μmol/L MEHP染毒Hep3B细胞的G1期和25.00、50.00、100.00μmol/L MEHP染毒Hep3B细胞的S期细胞构成比下降,50.00和100.00μmol/L MEHP染毒Hep3B细胞的G2期细胞构成比上升,差异均有统计学意义(P<0.01)。与溶剂对照组相比,各浓度MEHP染毒L02细胞均未见p53p、73和GADD45α蛋白表达量明显增加,差异无统计学意义;而各浓度MEHP染毒Hep3B细胞p73蛋白表达量和50.00、100.00μmol/L MEHP染毒Hep3B细胞GADD45α蛋白表达量均升高,差异有统计学意义(P<0.05,P<0.01)。结论一定浓度MEHP(50μmol/L和100μmol/L)可能通过独立于p53途径诱导p73和GADD45α蛋白表达增加而导致p53基因缺失的Hep3B细胞阻滞在G2期。

p53 functional loss,stemness and hepatocellular carcinoma

The tumor suppressor p53 is a key player in the control of genomic integrity and homeostasis in connection with p63 and p73,the two other members of the p53 family.Loss of functional p53 leads to the proliferation and survival of mature cells and progenitor or stem cells that accumulate genetic alterations,thus favoring tumorigenesis.p53 loss of function,observed in a wide variety of human tumor types,is frequently caused by missense mutations more frequently found in the DNA binding domain,but can also be due to the expression of a plethora of viral and cellular negative regulators.Human hepatocellular carcinoma(HCC)represents a specific situation,first because the TP53 gene mutations pattern exhibits a“hot spot”rarely found in other tumor types that is linked to Aflatoxin B1 exposure and,second,because many HCCs do not exhibit any TP53 mutation.Here,we provide an overview of the current knowledge about the inhibition of p53 functions by the N-terminal(ΔN)truncated forms of the family,and their role in the emergence and maintenance of pre-malignant cells with stem cell characteristics and in HCC development.We focus in particular on the Nanog-IGF1R-ΔNp73 axis that is associated with stem-like features in HCC cells and that may provide an attractive new therapeutic target and help to develop new biomarkers for HCC risk stratification,as well as preventive strategies.