Effects of Low Concentrations of Di-(2-ethylhexyl) and Mono-(2-ethylhexyl) Phthalate on Steroidogenesis Pathways and Apoptosis in the Murine Leydig Tumor Cell Line MLTC-1

The aim of this study was to evaluate the effects of low concentrations of DEHP and MEHP on steroidogenesis in a murine Leydig tumor cell line （MLTC-1） in vitro. The result of flow cytometry analysis revealed that the proportion of apoptotic cells was significantly increased after the exposure to DEHP. All three genes （P450scc, P450c17, and 38HSD） under study showed an increased expression following exposure to DEHP or MEHP, although some insignificant inhibitory effects appeared in the 10μmol/L treatment group as compared with the controls. It was also found that DEHP or MEHP stimulated INSL3 mRNA and protein especially in the 0.001 μmol/L treatment group. Testosterone secretions were stimulated after the exposure to DEHP or MEHP. Alterations of steroidogenic enzymes and INSL3 in MLTC-1 cells might be involved in the biphasic effects of DEHP/MEHP on androgen production.

RADIATION-INDUCED APOPTOSIS OF TWO NASOPHARANGEALCARCINOMA CELL LINES

Objective: To study apoptosis induced by radiation in two nasopharyngeal carcinoma (NPC) cell lines, CNE and CNE-2. Methods: Hoechst 33342 staining, immuno-histochemical staining, RT-PCR, DNA dot blotting and Southern blotting were used to identify apoptosis. Results: A single dose of X-irradiation resulted in apoptosis, the apoptotic index (AI) was time- and dose-dependent. Different apoptotic responses existed in the two cell lines. Immunohistochemical staining showed that bcl-2 protein was strongly positive in CNE but negative in CNE-2. However, RT-PCR revealed p53 mRNA in CNE-2 but not in CNE. P53 and bcl-2 genes were both present in the two cell lines as shown by DNA blotting, but the 2.8 kb fragment of the p53 gene was much lower than the 5.6 kb fragment on CNE which was clearly shown in Southern hybridization, suggestive of partial deletion of p53 gene in CNE. Conclusion: Apoptotic response to radiation is different in two NPC cell lines. CNE is more radioresistant than CNE-2. Overexpression of bcl-2 protein and partial deletion of p53 gene may explain their difference in radiosensitivity.

TIME-AND DOSE-DEPENDENT UP-REGULATION OF TNF-α mRNA AFTER IRRADIATION OF HUMAN NSCLC CELL LINES IN VITRO

Objective： Even though radiotherapy plays a major role in the local treatment of non-small cell lung cancer （NSCLC）, little is known about the molecular effects of irradiation in this tumor. In the present study, we examined two NSCLC cell lines for their endogenous production of TNF-α after irradiation. To investigate the radiation-induced TNF-α production in NSCLC cell lines. Methods： Two human NSCLC cell lines （A549： squamous; NCI-H596： adenosquamous） were investigated for their TNF-α mRNA （real-time RT-PCR） after exposure to different irradiation doses （2, 5, 10, 20, 30, 40 Gy） and time intervals （1, 3, 6, 12, 24, 48 or 72 h）. The TNF-α mRNA expression was quantified by real-time RT-PCR. The clonogenic survival was evaluated after irradiation with 2, 4, 6 and 8 Gy. Results： Non-irradiated NSCLC cells exhibited no or very low TNF-α expression. For the NCI-H596 cell line, TNF-α expression was significantly elevated 1～12 h （maximum 6h： 568fold increase relative to unirradiated cells） in a time-dependent manner. The radiation-induced increase could be observed after irradiation with 2 Gy reaching maximal at 40 Gy, with 83 times higher than normal controls. The clonogenic survival of these cell lines was nearly identical. Conclusion： NCI-H596 cells produce significant quantities of TNF-α following irradiation in a time- and dose-dependent manner. The pro-inflammatory cytokine TNF-α is a key mediator for the pathogenesis of radiation pneumonitis. Radiation-induced endogenous TNF-α expression in NSCLC cells may affect the normal lung adjacent to the tumor and may be associated with an adverse clinical outcome of the patient.

Study of ATP borate ester effects on cell sensitization to radiation emitted by a nuclear reactor

Adenosine triphosphate(ATP)borate ester as a new boron agent for boron neutron capture therapy was tested.It was synthesized via a dehydration reaction induced by heating adenosine triphosphate disodium with boric acid.Next,ATP borate ester pretreatments were assessed to study their effects on cell sensitization from exposure to thermal neutron irradiation emitted by a nuclear reactor.Using cell viability assays(CCK8),survival rates of A549 cells pretreated with or without boroncontaining agents,including ATP borate ester and 4-dihydroxyborylphenylalanine(BPA),were measured.One week after feeding an ATP borate ester solution to tumorbearing nude mice,elemental B content values of tumor muscle and blood were measured using inductively coupled plasma mass spectrometry(ICP-MS).Meanwhile,other tumor tissue samples were placed in a culture medium,subjected to a 3-min neutron irradiation exposure,and then fixed in formalin 24 h later for the terminaldeoxynucleotidyl transferase(TDT)-mediated d UTP nick end labeling(TUNEL)immunohistochemical staining analysis.Results showed that A549 cell irradiation sensitization(irradiation dose of 0.33 Gy)varied with pretreatment.Sensitization values of the ATP borate ester pretreatment group were 1.3–14.1 with boron agent concentrations of 0.3–4.5 mM.Within 1.1–3.4 mM,ATP borate ester showed significantly higher sensitization values than BPA.Meanwhile,TUNEL results demonstrated that apoptosis rates of tumor tissue cells exposed to irradiation after ATP borate ester pretreatment significantly exceeded the corresponding rates for BPA-pretreated cells.In animal experiments,although the distribution ratio of ATP borate ester(tumor tissue/normal muscle,T/N)of 1.2 was not significantly different compared with that of BPA(1.3),the total ATP borate ester concentration in the tumor tissue(0.79±0.05μg/g)significantly exceeded that of BPA(0.58±0.05μg/g).Thus,compared with BPA,the greater enrichment of ATP borate ester in tumor tissues permits preferential targeting toward tumor cells for radiation sensitization.Therefore,ATP borate ester is superior to BPA for use in boron neutron capture therapy.

Specific CEA-producing colorectal carcinoma cell killing with recombinant adenoviral vector containing cytosine deaminase gene

AIM: To kill CEA positive colorectal carcinoma cells specifically using the E coli cytosine deaminase (CD) suicide gene, a new replication-deficient recombinant adenoviral vector was constructed in which CD gene was controlled under CEA promoter and its in vitro cytotoxic effects were evaluated. METHODS: Shuttle plasmid containing CD gene and regulatory sequence of the CEA gene was constructed and recombined with the right arm of adenovirus genome DNA in 293 cell strain. Dot blotting and PCR were used to identify positive plaques. The purification of adenovirus was performed with ultra-concentration in CsCl step gradients and the titration was measured with plaque formation assay. Cytotoxic effects were assayed with MTT method, The fifty percent inhibition concentration (IC(50)) of 5-FC was calculated using a curve-fitting parameter. The human colorectal carcinoma cell line, which was CEA-producing, and the CEA-nonproducing Hela cell line were applied in cytological tests. An established recombinant adenovirus vector AdCMVCD, in which the CD gene was controlled under CMV promoter, was used as virus control. Quantitative results were expressed as the mean +/- SD of the mean. Statistical analysis was performed using ANOVA test. RESULTS: The desired recombinant adenovirus vector was named AdCEACD. The results of dot blotting and PCR showed that the recombinant adenovirus contained CEA promoter and CD gene. Virus titer was about 5.0 X 10(14)pfu/L(-1) after purification. The CEA-producing Lovo cells were sensitive to 5-FC and had the same cytotoxic effect after infection with AdCEACD and AdCMVCD (The IC(50) values of 5-FC in parent Lovo cells, Lovo cells infected with 100 M.O.I AdCEACD and Lovo cells infected with 10 M.O.I AdCMVCD were 】15000, 216.5+/-38.1 and 128.8+/-25.4 micromol.L(-1), P【0.001, respectively), and the cytotoxicity of 5-FC increased accordingly when the m.o.i of adenoviruses were enhanced (The value of IC(50) of 5-FC was reduced to 27.9+/-4.2 micromol.L(-1) in 1000 M.O.I AdCEACD infected Lovo cells and 24.8+/-7.1 micromol.L(-1) in 100 M.O.I AdCMVCD infected Lovo cells, P【0.05, P【0.01, respectively). The CEA-nonproducing Hela cells had no effect after infection with AdCEACD, but Hela cells had the cytotoxic sensitivity to 5-FC after infection with AdCMVCD (The IC(50) of 5-FC in parent Hele cells and Hela cells infected with AdCMVCD at 10 M.O.I was 】15000 and 214.5+/-31.3 micromol.L(-1), P【0.001). AdCEACD/5-FC system also had bystander effect, and the viability was about 30 percent when the proportion of transfected cells was only 10 percent. CONCLUSION: The recombinant adenovirus vector AdCEACD has the character of cell type-specific gene delivery. The AdCEACD/5-FC system may become a new, potent and specific approach for the gene therapy of CEA-positive neoplasms, especially colon carcinoma.

Neutron-induced apoptosis of HR8348 cells in vitro

INTRODUCTIONTo date ,the major therapy for rectal carcinoma is extensive abdomino-perineal resection[1]. Unfortunately ,after resection of rectal carcinoma ,many patients still die of blood-borne metastases ,usually in the liver or lungs ,or local prlvic recurrence[2,3],which is the major cause of morbidity and mortality in patients with rectal carcinoma .Pre-or postoperative radiotherapy can reduce the incidence of local rdcurrence[4-7].

丹皮酚体内外抗人食管癌Eca-109细胞增殖及诱导凋亡的作用

目的研究丹皮酚(paeonol,Pae)在体内外对人食管癌细胞Eca-109的抑瘤作用及其对细胞凋亡的影响。方法采用噻唑蓝(MTT)体外试验法和灌胃给药体内抗肿瘤试验。光镜及电镜观察各组的肿瘤组织的形态学变化。应用末端脱氧核苷酸转移酶介导的缺口末端标记(TUNEL)法测定细胞凋亡指数。结果丹皮酚在体外对Eca-109细胞有明显的细胞毒作用,半数抑制浓度(IC50)为0.342mmol·L-1;体内灌胃给予丹皮酚25、50、100和200mg·kg-1对裸鼠移植人食管癌Eca-109的抑制率分别为10.67%、23.54%、27.91%和34.46%;顺铂5mg·kg-1组抑瘤率为58.71%;丹皮酚在100mg·kg-1剂量下与顺铂5mg·kg-1联合用药抑制率为77.91%。光镜下用药组可见较多凋亡的肿瘤细胞。透射电镜下可见肿瘤细胞核染色质浓缩边聚、胞质浓缩、核碎裂以及凋亡小体形成等典型的凋亡表现。用药组凋亡指数较对照组明显增加。结论丹皮酚在体内外具有抑制人食管癌Eca-109细胞增殖及诱导其凋亡作用。

呋喃二烯的体内外抗肿瘤作用研究

探讨了呋喃二烯的体内外抗肿瘤作用及作用机理.采用MTT法检测呋喃二烯对10种人肿瘤细胞的体外增殖抑制作用,研究发现呋喃二烯对体外培养的多种肿瘤细胞具有很强的抑制和杀伤效应,其IC50在0.98-4.81μg/mL.并对敏感的白血病细胞HL-60进行初步的作用机制研究,其形态学和流式细胞分析试验均表明它能有效诱导细胞调亡.整体动物试验结果可证实呋喃二烯乳注射液能明显延长荷腹水癌S180小鼠的生存期,生命延长率分别为80 mg/kg(91.2%),30 mg/kg(82.4%),10 mg/kg(70.59%).

尖海龙提取物抗癌作用的研究

制备尖海龙提取物 ,再将其分别作用于 Hela、SK- RB- 3细胞系 ,从细胞形态变化、细胞计数、集落形成率、细胞分裂指数变化观察体外药效 .结果表明 ,尖海龙提取物可改变肿瘤细胞的正常生活形态 ,又可显著抑制肿瘤细胞的增殖 ,降低集落形成率 ,减少分裂指数 ,从而证实尖海龙提取物具有抗癌活性 ,其在癌症的治疗与预防方面具有实用价值 .

阿诺宁的抗瘤作用研究

背景与目的:我们先前的研究证明,阿诺宁(anuoning)、bullatacin和squamocin在体外有强抗肿瘤作用,squamocin可诱导HL-60细胞凋亡。本研究目的是进一步研究阿诺宁的细胞毒作用和体内抗瘤作用。方法:体外试验用噻唑蓝还原法(MTT法)检测阿诺宁对体外培养的人结肠癌细胞(HT-29)、人鼻咽癌细胞(SUNE1和CNE2)、人肝癌细胞(bel-7402)、人乳腺癌细胞(MCF-7)和人肺腺癌细胞(GLC-82)的生长抑制作用。建立小鼠移植瘤模型,观察阿诺宁腹腔注射对小鼠肝癌(HepS)和肉瘤S-180的体内抗瘤作用。结果:体外实验表明,阿诺宁对CNE2、bel-7402、HT-29和SUNE1细胞的半数抑制浓度(IC50)依次为0.044μg/ml、0.068μg/ml、0.446μg/ml和1.617μg/ml;对MCF-7和GLC-82细胞的IC50分别为1.857μg/ml和3.481μg/ml。体内试验表明,阿诺宁15、30和60μg/kg,腹腔注射作用10天后,对小鼠肝癌的平均抑瘤率依次为36.9%、51.8%和57.9%,与对照组相比有统计学意义;对小鼠肉瘤S-180的平均抑瘤率依次为43.0%、52.1%和61.0%,与对照组相比有统计学意义。结论:阿诺宁对多种人肿瘤细胞有很强的抑制生长作用,并对小鼠移植瘤具有抗瘤作用。

藤茶总黄酮对人胃癌SGC-7901细胞增殖抑制作用的实验研究

目的探讨藤茶总黄酮的体外抗肿瘤作用。方法采用MTT法、生长曲线法、细胞集落形成法观察藤茶总黄酮对人胃癌SGC-7901细胞抑制作用。结果藤茶总黄酮能明显抑制体外培养的SGC-7901细胞的生长,MTT法IC50为20.71μg.ml-1;细胞生长曲线法提示其对SGC-7901细胞的生长也有明显的抑制作用;集落形成法,当药物浓度在9.90μg.ml-1以上时抑制率为100%,当药物浓度为6.60μg.ml-1时抑制率为69.80%,当药物浓度为4.40μg.ml-1时抑制率为30.23%。结论藤茶总黄酮对体外SGC-7901细胞的生长有明显的抑制作用。

射线诱导的细胞凋亡过程中端粒酶表达及其活性

利用原位端粒酶-凋亡双染色法检测A549细胞和L02细胞hTERT和凋亡双表达,端粒序列扩增检测(TRAP)方法检测群体细胞端粒酶活性,研究γ射线照射人肿瘤细胞和正常细胞后端粒酶的表达变化与凋亡发生的关系。结果表明,1-5Gy照射后24-72h,A549细胞和L02细胞内hTERT表达增强,端粒酶和凋亡双染色阳性细胞随照射剂量的提高而增多;在凋亡发生的过程中,群体细胞端粒酶活性呈剂量依赖性增强,提示放射线诱导人肿瘤和正常细胞凋亡可能不是通过直接抑制端粒酶活性的机制;而辐射诱导端粒酶活性增高可能是细胞修复辐射损伤的机制之一。

BEP2D细胞恶性转化过程中Smad7基因对MAPK信号通路的调控

背景与目的:Smad7基因是转化生长因子(transforminggrouthfactor-茁,TGF-β)信号通路的抑制分子,有研究表明TGF-β通过活化SMAD通路和ras/MEK/ERK通路来诱导某些基因的表达。本研究旨在探讨在人永生化支气管上皮细胞BEP2D经辐射诱发恶性转化过程中,作为SMAD蛋白家族的抑制分子Smad7是否参与TGF-β对MAPK信号通路的调控。方法:将人工合成的Smad7siRNA及Smad7真核表达载体与pTet-Elk,pTet-Jun反式激活载体、报告基因荧光素酶共转染BEP2D细胞,TGF-β刺激,通过报告基因荧光素酶的表达丰度来检测Smad7对MAPK信号通路的调控。结果:永生化BEP2D细胞中,TGF-β刺激之后,Elk和Jun磷酸化活性升高(PElk=0.033,PJun=0.016);Elk或Jun同Smad7真核表达载体共转染之后,Elk磷酸化活性升高,Jun磷酸化活性降低(PElk=0.017,PJun=0.028);Elk或Jun同Smad7-siRNA共转染之后,Elk磷酸化活性降低,Jun磷酸化活性升高(PElk=0.018,PJun=0.005)。恶性化BERP35T2细胞中,TGF-β刺激之后,Elk磷酸化活性增强(P=0.006),Elk同Smad7siRNA共转染之后,Elk磷酸化活性降低(P=0.000);恶性化细胞中几乎检测不到Jun的活性。结论:在BEP2D细胞发生恶性转化过程中,Smad7基因干预MAPK信号通路,使ERK和JNK磷酸化活性的平衡失调,导致促增殖作用强于生长抑制作用,从而有助于细胞向恶性方向发展。

γH2AX对胶质瘤放射敏感性预测效果的实验研究

目的观察高级别胶质瘤细胞系(U87、U251和LN229)γH2AX蛋白表达变化,据此判断胶质瘤对放射线的敏感程度。方法选择胶质瘤细胞系U87、U251和LN229细胞株,通过细胞克隆形成实验,检测经不同剂量(0、2、4、6、8和10 Gy)X线照射后胶质瘤细胞克隆形成率,并绘制细胞存活曲线、测定放射敏感性;采用Western blotting法检测经剂量为2 Gy的X线照射后不同时间点(0 min、30 min、1 h、2 h、6 h、12 h、24 h、36 h和48 h)各胶质瘤细胞系γH2AX蛋白表达变化。结果细胞克隆形成实验显示,随着X线照射剂量的增加,胶质瘤细胞存活分数逐渐降低、细胞克隆形成率减少,放射增敏比自高至低依次为U87、LN229和U251细胞(均P=0.000)。Western blotting法显示,随着X线照射时间的延长,各胶质瘤细胞系γH2AX蛋白表达呈现先上升后下降的时间效应曲线,U87、LN229和U251细胞γH2AX蛋白表达峰值时间依次为2、1和1 h(P=0.000、0.000、0.015);γH2AX蛋白相对衰减速度(r=0.733,P=0.025)和升高程度(r=0.672,P=0.047)均与放射增敏比呈正相关。结论γH2AX蛋白有望成为检测高级别胶质瘤细胞系放射敏感性的一项预测指标。

羟基喜树碱联合放射对人肺腺癌细胞协同杀伤作用的实验研究

目的 研究羟基喜树碱联合放射对人肺腺癌细胞的协同杀伤作用。方法 应用四唑盐比色试验 (MTT)检测细胞抑制百分比 ,DNA琼脂糖电泳检测DNA“Ladder”及流式细胞术检测细胞周期及凋亡峰的比例。结果 羟基喜树碱对该细胞的抑制呈剂量及时间依赖关系 ,且明显阻滞细胞于S期 ,低浓度的羟基喜树碱 (1μg/ml)作用 48小时 ,细胞开始出现凋亡小峰 ,高浓度的羟基喜树碱 (5 0 μg/ml)作用 2 4小时就出现明显的凋亡小峰。单纯放射 (6Gy)后 48小时细胞出现DNA“Ladder”条带 ,单纯羟基喜树碱 (1μg/ml)作用后 2 4～ 72小时 ,细胞出现DNA“Ladder”条带及凋亡小峰 ,细胞经羟基喜树碱联合放射作用后的 0～ 72小时均出现DNA“Ladder”条带及凋亡小峰。

蒲葵根提取物的体外抗肿瘤实验研究

目的:用体外细胞培养法研究蒲葵根提取物对七种肿瘤细胞株生长的抑制作用。方法:采用MTT法、细胞集落形成法、生长曲线法测定蒲葵根提取物对白血病细胞株L1210和P388D1、宫颈癌细胞株Hela、人胃癌细胞株SGC7901、黑色素瘤细胞株B16、神经性肿瘤细胞株NG108-15、人肝癌细胞株Hele 7404生长的抑制情况。结果:MTT法、细胞集落形成法、生长曲线法测定的结果均显示,当蒲葵根提取物浓度在5.0μg/m l以上时,7类肿瘤细胞株的生长均受到明显抑制。结论:蒲葵根提取物在体外具有抗肿瘤作用。

汉防己甲素增加乳腺癌细胞放射敏感性的实验研究

目的:研究汉防己甲素(tetrandrine,Tet)是否增加人乳腺癌细胞对γ射线敏感性,并研究其作用机制及p53基因的作用。方法:采用克隆形成分析法检测Tet和γ射线对人乳腺癌细胞的作用,使用流式细胞术检测细胞在Tet及γ射线作用后各周期的分布情况,Westernblotting检测Tet及γ射线对CyclinB1和Cdc2的影响,应用分裂指数法检测细胞进入有丝分裂期的情况。结果:突变型MCF7ADR细胞在受到γ射线照射后,明显阻滞于G2期;Tet可以降低这种阻滞,显著增加γ射线的杀伤作用,其增敏比为1.51。p53野生型MCF7细胞在γ射线照射后,阻滞于G1期和G2期;加入Tet,阻滞作用降低不明显,增敏比为1.10,表明细胞受照射后诱导的周期阻滞与p53基因功能有密切关系,Tet增加γ射线的杀伤作用与p53基因功能有关;进一步研究显示,细胞在受到γ射线照射后,其CyclinB1与Cdc2蛋白表达水平明显降低,分裂指数也明显降低;在用γ射线处理后,CyclinB1与Cdc2蛋白的表达水平明显增高,分裂指数明显增高。结论:Tet是一种G2期阻滞清除剂,能显著增加γ射线对人乳腺癌细胞的杀伤作用,这种作用与细胞的p53基因功能有关。

Apoptin基因对人胃癌细胞BGC-823的抑制效应及与凋亡信号转导的关系

目的:探讨Apoptin基因对人胃癌细胞BGC-823的抑制作用及其参与胞内细胞信号转导的机制.方法:应用脂质体转染法将重组质粒pVAX1-Apoptin体外转染BGC-823细胞,运用噻唑兰(methylthiazolyltetrazolium,MTT)分析法检测重组质粒对BGC-823肿瘤细胞的抑制作用;通过AO/EB染色法对pVAX1-Apoptin转染的肿瘤细胞进行形态学观察;运用流式细胞术检测细胞线粒体跨膜电位(△Ψm);通过免疫印迹检测细胞色素c(cytochromec,Cytoc)释放;应用底物显色法检测Caspase-3/9活性.结果:pVAX1-Apoptin转染比pVAX1具有更强的抑瘤效应(10μg质粒转染72h后,23.37%vs99.61%,P<0.01),并且肿瘤细胞的死亡方式以凋亡为主.实验结果显示,pVAX1-Apoptin转染导致细胞线粒体跨膜电位下降,与pVAX1转染BGC-823细胞相比有显著差异(46.7%±7.26%vs70.66%±5.98%,P<0.01);同时伴随细胞色素c的释放.另外,pVAX1-Apoptin和pVAX1转染细胞的Caspase-3/9活性具有显著差异(Caspase-9:0.181±0.032vs0.079±0.013,P<0.01;Caspase-3:0.242±0.041vs0.058±0.023,P<0.01).结论:pVAX1-Apoptin转染BGC-823肿瘤细胞导致线粒体跨膜电位下降,并刺激释放细胞色素c,从而激活Caspase-9.经细胞色素c激活的Caspase-9进而活化凋亡通路下游关键作用因子,并对BGC-823肿瘤细胞产生抑制效应.

放射控导的wt-p53蛋白正反馈基因环路对肺腺癌细胞周期、凋亡及放射敏感性的影响

目的研究体外环境放射控导的wt-p53蛋白正反馈基因环路对肺腺癌细胞细胞周期、凋亡率及放射敏感性的影响。方法采用直线加速器8MV-X线,400MU/min、4Gy、源皮距100cm的照射条件照射治疗组pE6R4-p53-EGFP/H1299转染细胞和对照组H1299(p53-/-)、pE6-p53-EGFP/H1299和pR4-p53-EGFP/H1299转染细胞,12h后收集各组细胞,流式细胞仪分析该环路在放射线诱导下对肺腺癌细胞周期和细胞凋亡率的影响;绘制细胞放射剂量-存活曲线,计算平均致死剂量(Do)值及放射增敏比(sensitive enhancement ratio,SER)。结果4Gy8MV-X线照射治疗组和对照组细胞后12h,治疗组细胞在照射后(75.13±1.42)%发生明显G0/G1期阻滞;照射后各组细胞凋亡率均高于照射前,照射后治疗组细胞凋亡率为(23.73±0.21)%,分别是对照组H1299(p53-/-)细胞[(4.17±0.12)%]、pE6-p53-EGFP/H1299细胞[(15.67±0.32)%]、pR4-p53-EGFP/H1299细胞[(9.23±0.15)%]的5.69、1.51倍和2.57倍。治疗组pE6R4-p53-EGFP/H1299细胞和对照组pE6-p53-EGFP/H1299、H1299(p53-/-)细胞Do值分别0.91、1.073、1.413Gy,根据Do值计算SER分别为2.63和1.34。结论放射可诱导wt-p53蛋白正反馈基因环路上调wt-p53蛋白表达,从而调控肺腺癌细胞发生显著G/G1阻滞,使细胞凋亡比例增加,显著提高了肺腺癌细胞放射敏感性。

蒿甲醚对胰腺肿瘤细胞的抑制作用

目的观察蒿甲醚(ART)在体外对人胰腺癌SW-1990细胞的杀伤作用和对细胞增殖和凋亡的影响,以及在体内对荷瘤裸鼠移植瘤的抑制作用。方法采用MTT法检测ART对SW-1990细胞的杀伤作用;采用流式细胞仪检测ART对SW-1990细胞周期和凋亡的影响。建立人胰腺癌裸鼠移植瘤模型,通过测量裸鼠体质量、移植瘤瘤径和瘤质量,计算肿瘤体积和抑瘤率,观察ART在体内的抗肿瘤活性。结果MTT结果显示,ART对SW-1990细胞的杀伤作用与时间-剂量呈正相关(P<0.05);流式细胞仪检测显示,ART使SW-1990细胞阻滞于G0/G1期,并诱导细胞凋亡;荷瘤裸鼠体内实验显示,中、高剂量的ART(4、8 mg)对裸鼠移植瘤的生长抑制效果显著(P<0.05),抑瘤率分别为48.10%和53.51%。结论ART在体外及荷瘤裸鼠体内对SW-1990细胞有明显的抑制作用;其抑制作用与阻滞细胞周期和诱导细胞凋亡有关。