Transfection of the Human Sodium/Iodide Symporter(NIS) Gene with Liposomes and the Expression of the NIS Protein in Human Lung A549 Cancer Cells

OBJECTIVE To examine the possibility of human sodium iodide symporter （hNIS） protein expression in lung cancer cells. METHODS Human lung A549 cancer cells were thawed and cultured in vitro. The cells were divided into an experimental group transfected with a recombinant pcDNA3-hNIS plasmid and a control group transfected only with a pcDNA3 plasmid. The recombinant plasmid vector encoding the hNIS gene （pcDNA3-hNIS） was amplified, purified and identified. The hNIS gene was followed by DNA sequencing. A Western blot and an immunohistochemical assay were applied to detect the hNIS protein expression in the transfected human lung A549 cancer cells. RESULTS Restriction enzyme digestion and DNA sequencing results showed the size and direction of the inserted gene in the recombinant pcD- NA3-hNIS plasmid was correct. The Western blot method and immunohistochemical analysis showed a positive NIS protein expression in the experimental group. The NIS protein was detected mainly in the cell membranes showing a positive rate up to 70.6% with no expression of the NIS protein in the control group. There was a significant difference between two groups （P=0.000）. CONCLUSION The hNIS gene was transfected effectively into human lung A549 cancer cells mediated by Lipofectamine 2000, and was expressed with its protein in vitro.

Radioiodine therapy for castration-resistant prostate cancer following prostate-specific membrane antigen promoter-mediated transfer of the human sodium iodide symporter

Radioiodine therapy, the most effective form of systemic radiotherapy available, is currently useful only for thyroid cancer because of the thyroid-specific expression of the human sodium iodide symporter （hNIS）. Here, we explore the efficacy of a novel form of gene therapy using prostate-specific membrane antigen （PSMA） promoter-mediated hNIS gene transfer followed by radioiodine administration for the treatment of castration-resistant prostate cancer （CRPC）. The androgen-dependent C33 LNCaP cell line and the androgen-independent C81 LNCaP cell line were transfected by adenovirus. PSMA promoter-hNIS （Ad.PSMApro-hNIS） or adenovirus.cytomegalovirus-hNIS containing the cytomegalovirus promoter （Ad.CMM-hNIS） or a control virus. The iodide uptake was measured in vitro. The in vivo iodide uptake by C81 cell xenografts in nude mice injected with an adenovirus carrying the hNIS gene linked to PSMA and the corresponding tumor volume fluctuation were assessed. Iodide accumulation was shown in different LNCaP cell lines after Ad.PSMApro-hNIS and Ad.CMV-hNIS infection, but not in different LNCaP cell lines after adenovirus.cytomegalovirus （Ad.CMV） infection. At each time point, higher iodide uptake was shown in the C81 cells infected with Ad.PSMApro-hNIS than in the C33 cells （P 〈 0.05）. An in vivo animal model showed a significant difference in 1311 radioiodine uptake in the tumors infected with Ad.PSMApro-hNIS, Ad.CMV-hNIS and control virus （P 〈 0.05） and a maximum reduction of tumor volume in mice infected with Ad.PSMApro-hNIS. These results show prostate-specific expression of the hNIS gene delivered by the PSMA promoter and effective radioiodine therapy of CRPC by the PSMA promoter-driven hNIS transfection.

Human sodium/iodide symporter gene induced iodine uptake in human lung adenocarcinoma via baculovirus

To investigate human sodium/iodide symporter (hNIS) induced iodine uptake in human lung adenocarcinoma via baculovirus, a recombinant baculovirus encoding hNIS gene was constructed under the control of CMV promoter (Bac-CMV-hNIS). In vitro, baculovirus infected A549 cells accumulated about 27 times more 125I than that of noninfected cells. The 125I uptake was maximal after 30-min incubation of the cells, and efflux of the radioactivity was rapid, with 50% lost during the first 2 min after 125I-containing medium had been replaced by nonradioactive medium. Competition experiments in the presence of sodium perchlorate revealed a dose-dependent decrease of 125I uptake. Bac-CMV-hNIS infected tumor cells were selectively killed by exposure to 131I, as revealed by clonogenic assays. In nude mice, Bac-CMV-hNIS infected A549 cells accumulated more 131I than that of the control monitored by 1-h scintigraphy after 131I administration. The transduction of hNIS gene through baculovirus is sufficient to induce iodine transporting in A549 cells in vitro and in vivo, outlining the potential of this novel tumor gene imaging approach. But a rapid efflux of radioactivity from the tumor was shown in vivo and the in vivo therapy test showed no sign of effect.

Radiofrequency induction on sodium/iodide symporter expression of thyroid cancer

Objective; The aim of this study was to investigate the effects of radiofrequency treatment on sodium/iodide symporter expression of thyroid cancer ceils. Methods： In 29 thyroid cancer patients with low or no expression of soda ／ iodide symporter, the radio frequency combined 1311 therapy was used, the whole-body scintigraphy and serum Ig were detected before and after the radiofrequency treatment. Results： The whole-body scintigraphy showed that 4 cases （4/29） before radiofrequenc_y treatment had positive iodine uptake, 19 cases （19/29） two weeks after radiofrequency treatment had the positive iodine uptake, 12 cases （12/29） four weeks after radiofrequency treatment had the positive iodine uptake. Four weeks after radiofrequency treatment, 5 cases had increased serum Ig levels, 17 cases had decreased serum Ig levels, 7 cases showed no change. 25 cases （25/29） were effective, 15 cases （15/29） were cured. Conclusion： The radiofrequency induced the non-expressed the sodium/iodide symporter of thyroid cancer cells regain the iodine intake ability, it improved the clinical efficacy of 131I therapy in dedifferentiated thyroid cancer.

Correlation analysis between serum β2-MG and sodium/iodide symporter in patients with thyroid carcinoma

Objective： The aim of our study was to investigate the correlation between the expression of sodium/iodide symporter, serum levels of β2-MG and prognosis of thyroid carcinoma patients. Methods： Ninty-five cases with thyroid carcinoma, using enzyme-linked immunosorbent assay with double-antibody sandwich to detect the serum β2-MG levels and immunehistochemistry to detect NIS expression of thyroid cancer tissue. Results： Thirty-seven cases showed positive expression of sodium/iodide symporter （38.9%） and 30 cases showed positive expression of β2-MG （31.57%）. There were significant differences of NIS expression （X2 = 8.207, P = 0.017） and β2-MG expression （X2 = 10.121, P = 0.006） between different pathological types of thyroid carcinoma, but there was no correlation between the positive rate of the two research groups （r = -0.546, P = 0.633）. The significant differences was observed in expression of sodium/iodide symporter （X2 = 9.272, P=0.002） and expression of β2-MG （X2 = 4.441, P = 0.035） between the group with neck lymph node metastasis and the group without neck lymph node metastasis and both positive rate was significantly negatively correlated （r = -1.000, P = 0.000）. The significant differences was observed in expression of sodium/iodide symporter （X2 = 9.272, P = 0.002） and expression of β2-MG （X2 = 3.867, P = 0.043） between the group with distant organ metastasis and the group without distant organ metastasis （X2 = 11.985, P = 0.001） and both positive rate was significantly negatively correlated （r = -1.000, P = 0.000）. Conclusion： There are significantly negatively correlated between neck lymph node metastasis, distant organ metastasis and expression of sodium/iodide symporter and expression of β2-MG. Thyroid cancer lymph node and distant organ metastasis, the tumor tissue NIS expression and serum levels of β2-MG is significantly negatively correlated. The detection of serum β2-MG provides clinical reference value for the effects on radionuclide therapy and prognosis assessment of thyroid carcinoma. Serum β2-MG levels is negatively correlated with prognosis in thyroid cancer patients.

Adenovirus-mediated and tumor-specific transgene expression of the sodium-iodide symporter from the human telomerase reverse transcriptase promoter enhances killing of lung cancer cell line in vitro

Background The sodium-iodide symporter （NIS） protein can mediate the active radioiodine uptake.The human telomerase reverse transcriptase （hTERT） promoter is known to be selectively reactivated in majority of tumors and hence could be used for tumor targeting.We constructed a recombinant adenovirus containing the human sodium iodide symporter （hNIS） gene directed by the hTERT promoter, characterized the ability of infected cells in uptaking iodide, and explored the therapeutic efficacy of 131I in a lung cancer cell line in vitro.Methods The hTERT promoter was amplified by PCR from DNA isolated from log-phase HepG2 cells, subcloned into lineralized FL＊-hNIS/pcDNA3, and then the hTERT-hNIS sequence was subcloned into the shuttle plasmid pAdTrack.The recombinant adenovirus Ad-hTERT-hNIS was constructed by AdEasy system.A positive control adenovirusAd-CMV-hNIS and a negative control adenovirus Ad-CMV were created similarly.A549 cells were transduced with recombinant adenoviruses.125I uptake studies and sodium perchlorate suppression studies were used to confirm hNIS expression and function.Toxic effects of 131I on tumor cells were studied by in vitro clonogenic assay.Results We first successfully constructed an adenovirus mediated transgene expression system of the hNIS under the control of hTERT promoter.When infected with recombinant adenovirus constructs expressing hNIS directed by hTERTand CMV-promoters （Ad-hTERT-hNIS and Ad-CMV-hNIS, respectively）, the lung cancer cell line A549 had increased ability to uptake radioiodide up to 23- and 30- fold compared to the control parental cells, respectively.The radioiodide uptake ability of both the Ad-CMV-hNIS and Ad-hTERT-hNIS transduced cell lines were repressed 11-fold by sodium perchlorate （NaCIO4）.The subsequent in vitro clonogenic assay of the infected A549 cell line was further repressed to 23% （Ad-CMV-hNIS） and 30% （Ad-hTERT-hNIS） of the control group after receiving radioiodide for 7 hours （P 〈0.001）.Conclusion Our preliminary study indicates that an adenovirus mediated transgene expression system of the hNIS under the control of hTERT promoter has the potential to become an effective wide-spectrum yet highly specific anti-cancer strategy.

甲状腺癌碘-131治疗抵抗发生的分子机制研究进展

甲状腺癌是内分泌系统最常见的恶性肿瘤,其中分化型甲状腺癌(differentiated thyroid carcinoma,DTC)占90%以上。多数DTC患者经过系统治疗后预后良好,但少数患者肿瘤原发灶或转移灶出现失分化现象,进展为放射性碘难治性DTC(radioiodine-refractory DTC,RAIR-DTC),预后明显变差,是甲状腺癌致死的主要原因。钠碘转运体(sodium iodide symporter,NIS)的表达和功能异常,是导致甲状腺癌碘-131治疗抵抗的主要原因,其发生受遗传学改变、表观遗传学改变、肿瘤微环境作用、自噬作用等多因素影响。遗传学改变如BRAF基因的V600E位点突变、RET/PTC基因重排等导致致癌信号通路的激活,直接或间接地影响NIS的表达及其在细胞膜上的正常定位。表观遗传学调控特定基因的表达模式,调节NIS的表达水平,进而影响甲状腺细胞的碘摄取功能。肿瘤微环境中的免疫细胞、细胞因子和细胞外基质等成分也可能通过降低NIS的表达水平和/或干扰其在细胞膜上的正常功能导致细胞碘摄取障碍。此外,自噬作为一种细胞内部的代谢调节机制,也可以调节NIS的表达及其在细胞内的分布,从而影响碘的摄取和碘-131治疗的敏感性。通过综述以上因素在甲状腺癌失分化中的作用机制,可以更全面地理解RAIR-DTC的发生和发展过程,有助于探寻新的治疗靶点,改善预后,并为患者提供更有效的个体化治疗策略。

The effects of thyroid-stimulating hormone,estradiol and prolactin on sodium/iodide symporter mRNA expression in mouse lactating mammary gland cells under different iodine levels

Objective The present study investigated the sodium/iodide symporter mRNA expression in mouse lactating mammary gland cells under different iodine levels and the effects of thyroid-stimulating hormone(TSH),estradiol(E2)and prolactin(PRL)on NIS mRNA expression in mouse lactating mammary gland cells.

溴结构域蛋白4经PTEN/PI3K/AKT通路对甲状腺乳头状癌细胞摄碘相关指标影响的研究

目的研究溴结构域蛋白4(BRD4)在甲状腺乳头状癌(PCT)中的表达水平及其抑制剂JQ1对PCT细胞增殖、迁移能力的影响,进一步探索影响摄碘能力的调控机制。方法采用实时荧光定量聚合酶链反应(qRT-PCR)技术及蛋白质印迹法分别检测BRD4在正常甲状腺细胞Nthy-ori 3-1及人PCT细胞TPC-1、K1的表达水平。采用CCK-8及划痕实验分别检测JQ1对TPC-1、K1细胞增殖及迁移能力的影响。采用高内涵细胞成像与分析系统观察TPC-1、K1细胞在JQ1作用下的形态及数目变化。采用qRT-PCR技术检测影响PCT摄碘能力相关基因的表达。结果BRD4在PCT细胞及癌组织中高表达。JQ1对TPC-1、K1细胞增殖能力呈时间及浓度依赖性抑制。TPC-1、K1细胞的48 h半抑制浓度分别为(9.045±0.772)、(14.169±1.406)μmol/L。JQ1可以抑制TPC-1、K1细胞的迁移,且具有统计学意义(P<0.05)。JQ1分别作用于TPC-1、K1细胞48 h后,实验组BRD4、磷脂酰肌醇3激酶(PI3K)和蛋白激酶B(AKT)的mRNA表达水平降低。第10号染色体同源缺失性磷酸酶-张力蛋白基因(PTEN)、钠-碘转运蛋白的mRNA表达升高。结论BRD4在PCT中呈现高表达状态。JQ1可有效抑制BRD4的表达,并影响PTEN/PI3K/AKT通路从而抑制PCT细胞的增殖及迁移,使得其摄碘能力增加。

逆转钠碘转运蛋白在治疗放射性碘难治性分化型甲状腺癌中的研究进展

分化型甲状腺癌(differentiated thyroid carcinoma,DTC)的常规治疗手段包括手术、放射性碘治疗和促甲状腺激素抑制性治疗,大部分DTC患者在治疗后效果较好,但部分DTC去分化影响钠碘转运蛋白(sodium iodide symporter,NIS)的表达,无法进行放射性碘治疗,总体预后较差。因此,逆转NIS在DTC中的表达进而提高碘摄取能力成为近年来的研究热点。本文就NIS的调控、抑制NIS表达的分子机制以及放射性碘难治性DTC再分化治疗进行综述。

携带人NIS基因的重组腺病毒的构建

利用RT-PCR技术从Graves甲亢病人的甲状腺组织中扩增得到甲状腺钠/碘同向转运体(NIS)可编码区片段,并克隆到T载体,测序后亚克隆到腺病毒载体穿梭质粒pAdTrack-CMV上,再与含有骨架质粒pAdEasy-1的大肠杆菌BJ5183同源重组,经293细胞包装并扩增得到重组腺病毒AdNIS。结果显示重组腺病毒质粒经PmeI酶切鉴定,电泳中出现了诊断性片段;感染的293细胞出现了明显的细胞病变效应;PCR产物电泳证实了重组病毒的存在。病毒滴度为2.5～3×109efu/ml。表明成功构建了携带人NIS基因的重组腺病毒,这为基因转移NIS介导131I治疗非甲状腺肿瘤提供实验研究基础。

碘对大鼠体内及体外甲状腺钠碘转运体mRNA表达的调节

目的探讨碘过量对体内、体外甲状腺钠碘转运体(NIS)mRNA表达的影响。方法Wistar大鼠,随机分为低碘组(LI)、适碘组(NI)、5倍高碘组(5HI)、10倍高碘组(10HI)、50倍高碘组(50HI)、100倍高碘组(100HI),检测尿碘、甲状腺NISmRNA表达水平。FRTL细胞分别在含有10-6～10-3mol/L碘化钾的培养基中培养24、48h,检测NISmRNA水平的变化。结果LI组尿碘显著低于NI组,而甲状腺NISmRNA表达水平明显高于NI组(P<0.01);各高碘组尿碘与NI组比较呈成倍升高,NISmRNA水平与NI组相比逐渐下降。FRTL细胞在分别含有10-6～10-3mol/L碘化钾的培养基中培养24、48h,NISmRNA的表达水平与对照组差异无统计学意义(P>0.05)。结论碘对体内、体外甲状腺NISmRNA表达的影响存在不同的机制,长期、慢性处于高碘摄入的大鼠主要通过转录水平影响甲状腺NISmRNA的表达,而体外急性实验表明,高碘则可能通过转录后水平而起作用。

维甲酸诱导甲状腺癌细胞摄碘的实验研究

目的 探讨全反式维甲酸(ATRA)诱导甲状腺癌细胞系的钠碘同向转运体(NIS)表达及其碘摄取。方法 通过ATRA诱导甲状腺癌细胞系滤泡状甲状腺癌细胞株(FTC 133)、乳头状甲状腺癌细胞株(W3)及未分化甲状腺癌细胞株( 85 0 5C)后,经逆转录 聚合酶链反应(RT PCR)及Westernblot检测甲状腺癌细胞系的NISmRNA及其蛋白质表达,并测定甲状腺癌细胞系诱导后的摄碘变化。结果 ATRA诱导甲状腺癌细胞系4 8h后,FTC 133和W3的NISmRNA及蛋白质表达增高,85 0 5C未见变化;ATRA诱导甲状腺癌细胞系2周后,FTC 133和W3的摄碘增高。结论 ATRA能诱导分化型甲状腺癌细胞摄碘增高。

甲状腺癌NIS和TSHR表达的矛盾性及非相关性

目的研究钠/碘转运蛋白(sodium/iodide symporter,NIS)和促甲状腺激素受体(thyroid stim-ulating hormone receptor,TSHR)在甲状腺癌中的表达和相关性。方法收集正常甲状腺组织18例、甲状腺癌23例,通过荧光定量分析和免疫组织化学SP法对NIS和TSHR的表达进行研究。结果甲状腺癌NIS和TSHR mRNA的表达显著低于正常甲状腺组织(P<0.005),正常甲状腺组织NIS和TSHR的表达呈显著正相关(r=0.667,P=0.000),而在甲状腺癌中无相关性(r=0.222,P=0.376)。免疫组织化学结果表明甲状腺癌NIS阳性产物主要定位于细胞质,TSHR阳性产物定位于细胞质和细胞膜,甲状腺癌NIS及TSHR蛋白阳性表达率显著高于正常组(P<0.05);甲状腺癌NIS mRNA表达下降同时伴有细胞质NIS蛋白表达升高的有17例(74%)。结论甲状腺癌NIS和TSHR表达具有非相关性以及在转录和翻译水平上具有矛盾性,NIS蛋白非功能定位于细胞质,因而不能发挥正常的运输及聚碘功能,我们推测这可能是造成甲状腺癌患者放射性碘治疗失败的重要原因。

hNIS转基因介导^(131)碘对鼻咽癌细胞增殖和凋亡的影响

目的:克隆人的甲状腺钠/碘同向转运体(hNIS)基因,研究其转导在鼻咽癌细胞内的功能,以及131碘对鼻咽癌细胞增殖和凋亡的影响。方法:利用逆转录和聚合酶链反应(RT-PCR)从毒性弥漫性甲状腺肿(Graves病)病人的甲状腺组织中扩增得到hNIS的可编码区基因,并克隆到pcDNA3.1(+)-FLAG载体,获得重组真核表达质粒pcDNA3.1(+)-hNIS-FLAG。采用脂质体转染的方法,将pcDNA3.1(+)-hNIS-FLAG质粒导入到鼻咽癌细胞株CNE2,G418筛选得到稳定表达hNIS鼻咽癌细胞系CNE2-hNIS,体外培养条件下检测其对放射性碘的摄取和外流情况。CCK8试剂盒检测131碘对鼻咽癌细胞增殖的作用,AnnexinⅤ-FITC/PI双标记流式细胞技术(FCM)检测131碘作用后鼻咽癌细胞凋亡情况。结果:成功克隆hNIS基因,并建立能稳定表达hNIS的鼻咽癌细胞系CNE2-hNIS。CNE2-hNIS对125碘的吸收量比CNE2高约15倍,但在无碘的环境中,细胞内滞留的碘外流迅速,有效半衰期约8min。131碘在72 h后对CNE2-hNIS的增殖产生抑制作用,细胞早期凋亡率增加,并随着131碘浓度的增加,作用逐渐增强(P<0.01)。结论:从Graves病人的甲状腺组织中克隆的hNIS基因转染鼻咽癌细胞后,能使鼻咽癌细胞发挥高水平吸碘功能,131碘能够抑制转染hNIS的鼻咽癌细胞的增殖,促进细胞凋亡。

杆状病毒介导NIS基因放射治疗甲状腺癌的实验研究

目的探讨重组钠碘同向转运体(NIS)基因杆状病毒介导甲状腺癌细胞放射性碘治疗的可行性。方法构建杆状病毒载体质粒(pFBNIS)并制备重组NIS杆状病毒(BacNIS),体外感染甲状腺癌细胞,通过免疫荧光检测NIS蛋白的表达,通过动态摄碘及NaClO4摄碘抑制实验观察表达蛋白的功能和特性;进行131I杀伤细胞的克隆形成实验。结果成功构建了重组NIS杆状病毒,受巨细胞病毒(CMV)极早期基因启动子调控;BacNIS体外感染的甲状腺癌细胞表达的NIS蛋白具有摄碘功能和NaClO4抑制的特性;BacNIS感染的肿瘤细胞可被131I有效杀伤。结论BacNIS是介导肿瘤细胞摄碘的有效方法,为杆状病毒介导NIS基因治疗失分化甲状腺癌转移灶提供依据。

裸鼠模型的人钠/碘转运体基因转染人大细胞肺癌介导放射性核素显像

目的在动物体内实验观察人钠/碘转运体(hNIS)基因转染人大细胞肺癌介导放射性核素显像是否可行。方法①利用重组质粒以脂质体转染法将hNIS基因转染入人大细胞肺癌H460细胞系中,获得稳定表达hNIS的细胞株(hNIS-H460)。②用hNIS-H460细胞株建立大细胞肺癌荷瘤裸鼠模型,进行放射性核素99mTcO4-显像和131I显像。结果①体外实验表明hNIS-H460细胞株可以摄取碘。②裸鼠大细胞肺癌(hNIS-H460)移植瘤的99mTcO4-和131I显像结果较清晰。结论转染后的hNIS-H460细胞具有一定的摄碘能力。裸鼠大细胞肺癌(hNIS-H460)移植瘤可以进行99mTcO4-和131I显像;99mTcO4-显像的质量优于131I显像。

重组pDC316-MCMV/hNIS真核表达质粒的构建及在肿瘤细胞的功能

【目的】克隆人的钠/碘同向转运体(hNIS)基因可编码序列,并研究其在非甲状腺肿瘤细胞内的功能表达。【方法】利用逆转录和聚合酶链反应(RT-PCR)从毒性弥漫性甲状腺肿(又称Graves病)病人的甲状腺组织中扩增得到NIS的可编码区基因,并克隆到T载体,测序后亚克隆到腺病毒载体穿梭质粒pDC316载体上,获得重组真核表达质粒载体pDC316-MCMV/hNIS。采用脂质体转染的方法,把pDC316-MCMV/hNIS重组质粒(实验组)或pDC316空质粒(对照组)分别导入到胰腺癌细胞株CAPAN-Ⅱ细胞、PANC-1细胞和卵巢癌细胞株SK-OV-3细胞,转染后48h采用RT-PCR方法检测转染细胞内的hNIS mRNA水平,转染后第2、3、4天分别检测肿瘤细胞对125I的吸收功能。【结果】序列分析结果证实克隆片段与文献报道的hNIS基因cDNA序列完全一致。实验组转染后48h,在CAPAN-Ⅱ细胞、PANC-1细胞及SK-OV-3细胞内均能检测到hNIS mRNA高水平表达,对照组基本无hNIS mRNA表达。转染后第3天细胞吸碘达到高峰,实验组CAPAN-Ⅱ细胞、PANC-1细胞和SK-OV-3细胞对125I的吸收量分别比对照组高24倍、17倍和13倍。【结论】从Graves病人的甲状腺组织中克隆的hNIS基因转染肿瘤细胞后,能使肿瘤细胞发挥高水平吸碘功能,为进一步运用放射性核素体内靶向治疗非甲状腺肿瘤奠定了基础。

二甲双胍对甲状腺功能减退大鼠甲状腺激素的影响

目的探讨二甲双胍对甲状腺功能减退大鼠甲状腺激素水平的影响及其机制。方法取3个月龄雄性SD大鼠36只,随机分为正常对照(NC)组、甲状腺功能减退(HT)组、二甲双胍(Met)组。HT组和Met组以含0.01%氨基三唑的饮用水喂养大鼠4周制备甲状腺功能减退大鼠模型,NC组大鼠喂养普通饮用水。造模成功后,Met组用200 mg/kg二甲双胍灌胃,HT组和NC组用等体积0.05%羟甲基纤维素钠(CMC-Na)灌胃。于灌胃第8周时对3组大鼠甲状腺组织行H-E染色,采用q PCR检测下丘脑促甲状腺激素释放激素前体(pro TRH)mRNA的表达;于灌胃第8、12周时采用电化学发光法检测3组大鼠血清T3、T4水平,采用q PCR和蛋白质印迹法检测甲状腺组织钠碘同向转运体(NIS)mRNA和蛋白表达。结果在灌胃8、12周时,HT组大鼠血清T3、T4水平均低于NC组,而Met组T3、T4水平均高于HT组(P<0.05)。灌胃8周时,H-E染色结果显示NC组滤泡大小不等,内见大量胶质及吸收空泡;HT组大鼠甲状腺滤泡缩小,滤泡上皮成柱状,滤泡周围吸收空泡减少;Met组滤泡上皮增生较HT组稍改善。灌胃8周时,q PCR结果显示HT组大鼠下丘脑pro TRH和甲状腺组织NIS mRNA表达均高于NC组,而Met组均低于HT组(P<0.05);蛋白质印迹法检测结果显示Met组NIS蛋白表达低于HT组(P<0.05),而HT组和NC组NIS蛋白表达差异无统计学意义(P>0.05)。灌胃12周时,HT组和Met组甲状腺组织NIS mRNA表达差异无统计学意义(P>0.05),Met组NIS蛋白表达高于HT组(P<0.05)。结论二甲双胍能升高甲状腺功能减退大鼠的甲状腺激素水平,但短期内并不是由甲状腺NIS表达升高所致。

EGCG对甲状腺癌细胞增殖和摄碘能力的影响

目的:观察表没食子儿茶素没食子酸酯(epigallocatechin-3-gallate,EGCG)对甲状腺癌细胞增殖和摄碘能力的影响。方法:用不同浓度的EGCG处理甲状腺癌W3细胞株48 h后,用3-(4,5-二甲基噻唑-2)-2,5-二苯基四氮唑溴盐(MTT)法检测W3细胞增殖能力,流式细胞术、免疫荧光法检测钠-碘转运体(sodium iodide symporter,NIS)的变化,摄碘能力实验检测W3细胞摄碘能力。结果:与对照组比较,随着EGCG浓度的增加,W3细胞的增殖能力逐渐降低(P<0.01),NIS的表达逐渐增加(P<0.01),呈浓度依赖性。摄碘实验显示,在一定浓度范围内,EGCG明显促进W3细胞对碘的吸收能力(P<0.01)。结论:EGCG能抑制甲状腺癌细胞的增殖能力,通过上调NIS的表达促进甲状腺癌细胞株的摄碘能力。