盐霉素对乳腺癌MCF-7球囊细胞增殖与上皮间质转化作用的研究

目的探讨盐霉素(Salinomycin)对MCF-7球囊(MCF-7 MS)细胞的增殖与上皮间充质转化(EMT)的作用。方法通过乳腺癌MCF-7细胞无血清悬浮培养富集乳腺癌干细胞(BCSCs)得到MCF-7 MS;CCK-8 assay检测0、10、30、100、300、1 000、3 000及10 000 nmol/L浓度的盐霉素处理24 h对MCF-7 MS细胞存活率的影响,并计算半抑制浓度(IC50)值。Western blot检测30、60 nmol/L终浓度的盐霉素对MCF-7 MS细胞上皮标志物E-钙黏蛋白(E-cadherin)和间质化标志物Snail表达的影响,以等体积DMSO处理的MCF-7 MS细胞作为对照组。BALB/c裸鼠皮下接种MCF-7 MS细胞制备荷瘤鼠模型并分为对照组(等体积生理盐水处理)和盐霉素给药组(5 mg/kg盐霉素处理),免疫组织化学染色检测瘤组织E-cadherin和Snail的表达。结果随着浓度的增加,MCF-7 MS细胞存活率逐渐下降(P<0.05),24 h的IC50值为989 nmol/L。与对照组比较,30和60 nmol/L的盐霉素均可增加E-cadherin的表达,而降低Snail的表达,且后者作用更明显(P<0.05)。与对照组相比,盐霉素给药组荷瘤鼠瘤组织内E-cadherin的表达升高,而Snail的表达下调(P<0.01)。结论盐霉素能够抑制具有BCSCs特性的MCF-7 MS细胞的增殖,且可抑制MCF-7 MS细胞的EMT,是靶向肿瘤干细胞的潜在药物。

靶向ABCG2的RNA干扰逆转乳腺癌球囊细胞化疗耐药的研究

目的通过靶向ABCG2的RNA干扰逆转乳腺癌球囊细胞化疗耐药。方法以ABCG2为靶点,设计ABCG2-siRNA,构建ABCG2干扰慢病毒载体并包装好病毒,稳定转染到筛选好的MCF-7球囊细胞中,Western Blot方法检测ABCG2的表达情况,MTT法检测RNAi沉默ABCG2基因对球囊细胞的增殖抑制作用,同时流式细胞术检测RNAi沉默ABCG2对MCF-7球囊细胞在耐药情况下的细胞周期变化和凋亡状况。结果 ABCG2干扰慢病毒载体成功构建并包装病毒,建立起ABCG2稳定沉默的MCF-7乳腺癌球囊细胞系。Western Blot显示球囊细胞中高表达的ABCG2,在RNAi沉默后表达下降;MTT结果显示,在5-Fu的作用下的MCF-7贴壁细胞抑制率高于MCF-7球囊细胞,而沉默ABCG2的MCF-7球囊细胞其抑制率会随着5-Fu量的增加而增高;流式细胞仪也显示球囊细胞大多处于G0/G1期,加入5-Fu和沉默ABCG2后,处于G0/G1期细胞数会增加,凋亡率会明显增加。结论乳腺癌球囊细胞高表达ABCG2蛋白,其5-Fu耐药性高于亲本MCF-7细胞,沉默ABCG2后能够增加球囊细胞在5-Fu的作用下的细胞抑制率及凋亡率,从而逆转对5-Fu的耐药性。

牛蛙球囊毛细胞电压依赖性钾通道电流的研究

目的 :研究牛蛙球囊毛细胞膜上钾通道的类型。方法 :全细胞膜片钳技术。结果 :1当钳制电位为 - 1 0 0 m V,以 1 0 m V的步距阶跃 ,阶跃从 - 70 m V至 + 2 0 m V,随着膜电位的去极化 ,可记录到一系列快速、瞬时的外向电流 ,4- Ap对其有特异性阻断作用。激活电压为 - 53.85± 7.8m V。2 A型钾通道的数量在牛蛙毛细胞间存在差异。 3当钳制电位为 - 70 m V,以 1 0 m V的步距阶跃去极化 ( - 50 m V～ + 4 0 m V) ,可产生一延迟整流性钾离子流 ,四乙基氯化氨 ( TEA)能使该电流幅度下降 59%± 1 1 %。结论 :牛蛙毛细胞膜上含有 A型钾通道和延迟整流性钾通道。

无血清培养人结肠癌球囊样细胞生物学特性研究

目的采用无血清培养方法从人结肠癌细胞株中分选出富含肿瘤干细胞的球囊样细胞，并分析其增殖和迁移特性。方法人结肠癌细胞株HCTll6、HT29细胞在特殊配制的无血清培养基（SFM）中悬浮培养，观察球囊样细胞的生成。流式细胞仪检测结肠癌干细胞分子标记CDl33表达，利用CCK一8比色法以及Transwell小室法研究结肠癌球囊样细胞的增殖情况和迁移能力。采用成组设计资料的t检验分析检测数据。结果HCTl16、HT29细胞在SFM培养条件下可以获得可稳定传代的球囊样细胞，SFM培养下HCTll6球囊样细胞CDl33阳性细胞占75．44％±11．41％，HT29球囊样细胞CDl33阳性细胞占76．22％±14．23％。与常规含血清培养基（SSM）培养的同系细胞比较，HCTll6及HT29球囊样细胞中结肠癌干细胞分子标记CDl33阳性细胞数明显增多（t：11．43，9．17，P〈0．05），其持续增殖能力和运动迁移能力均增强。结论无血清培养获得的结肠癌球囊样细胞高表达结肠癌干细胞分子标记CDl33，且具有更强的增殖和迁移能力。它可作为进一步研究结肠癌干细胞的良好模型。

Effect of Intravascular Irradiation on Intimal Smooth Muscle Cells Proliferation and Apoptosis in Balloon Injuried Arteries

Objective: To investigate the effect of intravascular in radiation on thearterial wall smooth muscle cells (SMCs) proliferation and apoptosis after iliac artery bollominjury in figs. Methods: Twenty-seven miniature figs were divided into three groups. All pigsunderwent iliac artery balloon over-stretch. An^(192) Ir source through afterloader was positionedat the injuried segments to give 10 Gy in 9 pigs and 20 Gy in the other 9 pigs, and the rest 9 pigswere, used as control group. The pigs were killed on the 3rd, 10th and 28th days respectively forobservation. The injured segments were processed to examine SMCs proliferation by proliferation cellnuclear antigen (PCNA) and apopto-sis by terminal deoxynucleotidyl transferase-mediated dUTPnick-end labeling (TUNEL). Results: PC-NA index analysis has some that SMCs proliferation inneointima was significantly inhibited in irradiation group on the 10th and 28th days. The value forintimal SMCs apoptosis in control vs 10 Gy and 20 Gy irradiation groups were: (1. 185+-0. 49)% vs(2. 27+-0. 49)%(P>0. 05) and (1. 85+-0. 49)% vs (2. 53+-0. 45)%(P<0. 05), at the 10th day; (1.61+-0. 35)% vs (3. 11+-0. 51)%(P<0. 05), and (1.61+-0. 35)% vs (7. 05+-1. 82)% (P<0. 05), on the28th day. In irradiated arteries, the maximal incidence of intimal SMCs apoptosis was (7. 05+--1.82)% in 20 Gy group vs (3. 11+-0. 51)% in 10 Gy group (P<0. 05), on the 28th day. In the same doseirradiation group, the incidence of intimal SMCs apoptosis was higher on the 28th day than that onthe 10th day. Conclusion: Intra-arterial gamma irradiation can inhibit intimal SMCs proliferationand stimulate SMCs apoptosis in balloon-in jured arteries. These may be contributive to preventionof restenosis of arteries after balloon injury.

Adenovirus-mediated gene transfer of TIMP-4 reduces neointimal hyperplasia in balloon-injured rat carotid artery

Objective:To determine the effects of a recombinant replication-deficient adenovirus encoding human tissue inhibitor of metalloproteinase-4(Ad.TIMP-4) on vascular smooth muscle cell(VSMC) function in vitro and neointimal development in the injured rat carotid artery.Methods:Western blotting,gelatin zymography and reverse zymography were used to characterize the expression and functional activity of the TIMP-4 secreted by Ad.TIMP-4-infected VSMCs.The migration and proliferation of VSMCs in vitro were separately detected by using Millicell-PCF invasion chambers and [3H]-thymidine incorporation assay.Immunohistochemistry and morphometric analysis were used to determine the local expression of TIMP-4 and its effect on neointima development in a rat carotid artery balloon injury model.Results:VSMCs infected with Ad.TIMP-4 expressed functionally active human TIMP-4 which increased with the duration of infection.TIMP-4 expression inhibited VSMC migration,but not significantly affect VSMC proliferation.In a balloon-injured rat carotid artery model,a significant 62% reduction in neointimal area was found in Ad.TIMP-4-infected vessels at 14 days after injury.Ad.TIMP-4 infection had no effect on medial area.Conclusion:Our results indicated TIMP-4 over expression can significantly inhibit the migration of cultured VSMCs and prevent neointimal formation after vascular injury.Our findings provide additional evidence that TIMP-4 could play an important role in vascular pathophysiology,and may be an important therapeutic target for future drug development.