Increased expression of human calcium-activated chloride channel 1 is correlated with mucus overproduction in the airways of Chinese patients with chronic obstructive pulmonary disease

Background Chronic obstructive pulmonary disease （COPD） is usually complicated with mucus overproduction in airway. Recently the increased expression of the human calcium-activated chloride channel 1 （CaCC1） was found to play an important role in mucus overproduction in the asthmatic airways. To investigate the relationship of CaCC1 and mucus overproduction in the airway of Chinese patients with COPD, the expressions of CaCC1, MUC5AC and mucus in bronchial tissues were examined. Methods Bronchial tissues were obtained from fiberoptic bronchoscopy and bronchial biopsy in West China Hospital from April to July in 2004. Twenty-five patients were diagnosed as the patients with COPD overproduction, and other 20 were the control subjects. The expressions of CaCC1, MUC5AC and mucin in bronchial tissues were detected by reverse transcriptase-polymerase chain reaction （RT-PCR）, in situ hybridization with digoxigenin （DIG）-Iabeled RNA probe, immunohistochemical and alcian blue-periodic acid Schiff （AB-PAS） staining, respectively. Results Compared with the control group, the stronger expressions of CaCC1 were further detected throughout the bronchial tissues from patients with COPD （P〈0.01）. Furthermore, the stronger expressions of the CaCC1 mRNA were related to the severity of airflow obstruction. Samples from COPD showed a stronger staining for MUC5AC than those in control subjects （P〈0.01） and AB-PAS staining revealed more mucins in COPD patients＇ submucosal gland comparing with that in control subjects （P〈0.01）. Expression levels of the CaCC1 mRNA were respectively negatively correlated with the patients＇ forced expiratory volume in one second （FEV~） / forced vital capacity （FVC） data, FEV1% predicted data, V50% predicted data, V25% predicted data （r=-0.43, r=-0.43, r=-0.35, r=-0.36, P〈0.01, P〈0.01, P〈0.05, P〈0.05）. While the expression levels of the CaCC1 mRNA were well correlated with the expression levels of the MUC5AC mRNA of airway epithelium and the PAS-AB stained area of submucosal glands （r=0.39, r=0.46, P〈0.05, P〈0.01）. Expression levels of the MUC5AC mRNA were negatively correlated with the patients＇ FEV1/FVC data （P=0.01）, FEV1% pred data （P=-0.01）, V50% predicted data, V25% predicted data（r=-0.53, r=-0.53, r=-0.48, r=-0.43, P〈0.01, P〈0.01, P〈0.01, P〈0.01）. While the expression levels of the MUC5AC mRNA were well correlated with the positively PAS-AB stained area of submucosal gland （P〈0.05）, and the correlation coefficients were 0.43. Conclusion These results suggest that the stronger gene expression of CaCC1 exists, complicated with mucus overproduction in the airwav of Chinese patients with COPD.

Chloride intracellular channel 1 regulates colon cancer cell migration and invasion through ROS/ERK pathway

AIM: To investigate the mechanisms of chloride intracellular channel 1 (CLIC1) in the metastasis of colon cancer under hypoxia-reoxygenation (H-R) conditions.

Function of chloride intracellular channel 1 in gastric cancer cells

AIM:To investigate the effect of chloride intracellular channel 1(CLIC1) on the cell proliferation,apoptosis,migration and invasion of gastric cancer cells.METHODS:CLIC1 expression was evaluated in human gastric cancer cell lines SGC-7901 and MGC-803 by real time polymerase chain reaction(RT-PCR).Four segments of small interference RNA(siRNA) targeting CLIC1 mRNA and a no-sense control segment were designed by bioinformatics technology.CLIC1 siRNA was selected using Lipofectamine 2000 and transfected transiently into human gastric cancer SGC-7901 and MGC-803 cells.The transfected efficiency was observed under fluorescence microscope.After transfection,mRNA expression of CLIC1 was detected with RT-PCR and Western blotting was used to detect the protein expression.Proliferation was examined by methyl thiazolyl tetrazolium and apoptosis was detected with flow cytometry.Polycarbonate membrane transwell chamber and Matrigel were used for the detection of the changes of invasion and migration of the two cell lines.RESULTS:In gastric cancer cell lines SGC-7901 and MGC-803,CLIC1 was obviously expressed and CLIC1 siRNA could effectively suppress the expression of CLIC1 protein and mRNA.Proliferation of cells transfected with CLIC1 siRNA3 was enhanced notably,and the highest proliferation rate was 23.3%(P = 0.002) in SGC-7901 and 35.55%(P = 0.001) in MGC-803 cells at 48 h.The G2/M phase proportion increased,while G0/G1 and S phase proportions decreased.The apoptotic rate of the CLIC1 siRNA3 group obviously decreased in both SGC-7901 cells(62.24%,P = 0.000) and MGC-803 cells(52.67%,P = 0.004).Down-regulation of CLIC1 led to the inhibition of invasion and migration by 54.31%(P = 0.000) and 33.62%(P = 0.001) in SGC-7901 and 40.74%(P = 0.000) and 29.26%(P = 0.002) in MGC-803.However,there was no significant difference between the mock group cells and the negative control group cells.

Identification of Herbal Compound Imperatorin with Adverse Effects on ANO1 and CFTR Chloride Channels

Calcium-activated chloride channels（CaCCs） are the crucial regulators of transepithelial fluid secretion, smooth muscle contraction and sensory transduction. Recently, compelling evidence has indicated that TMEM16A（ANO1 or anoctamin-1） is a bona fide calcium-acvtivated chloride channel. A few small molecule CaCCs regulators are available for functional and therapeutic studies. We screened 126 natural compounds from Chinese herbs. Screening was performed with an iodide influx assay in Fischer rat thyroid epithelial cells to coexpress ANO1 and an iodide-sensitive fluorescent indicator（EYFP-H148Q/I152L）. Imperatorin, a coumarin compound, was identified to inhibit ANO1-mediated chloride transport activated by multiple calcium-elevating agonists. The inhibitory effect is dose-dependent with IC50～14.63 μmol/L. Interestingly, imperatorin activated CFTR chloride channel with EC50～35.52 μmol/L. The adverse effects of imperatorin on CaCC and CFTR chloride channels will make it useful in pharmacological dissection of chloride transport in airway and intestinal epithelium. Further studies are required to evaluate the therapeutic effects of imperatorin on hypertension, asthma and certain tumors.

Chloride channel blocker 4,4-diisothiocyanatostilbene-2,2'-disulfonic acid inhibits nitric oxide-induced apoptosis in cultured rat hippocampal neurons

Apoptosis in cultured rat hippocampal neurons was induced using the nitric oxide donor 3-morpholinosydnonimine, and cells were treated with the chloride channel blocker, 4,4- diisothiocyanatostilbene-2,2＇-disulfonic acid. Results showed that the survival rate of neurons was significantly increased after treatment with 4,4-diisothiocyanatostilbene-2,2＇-disulfonic acid, and the rate of apoptosis decreased. In addition, the expression of the apoptosis-related proteins poly（adenosine diphosphate-ribose）polymerase-1 and apoptosis-inducing factor were significantly reduced. Our experimental findings indicate that the chloride channel blocker 4,4- diisothiocyanatostilbene-2,2＇-disulfonic acid can antagonize apoptotic cell death of hippocampal neurons by inhibiting the expression of the apoptosis-related proteins poly（adenosine diphosphate-ribose）polymerase-1 and apoptosis-inducing factor.

Effect of electroacupuncture on calcium-activated chloride channel currents in interstitial cells of Cajal in rats with diabetic gastroparesis

Objective:To investigate the mechanisms of electroacupuncture(EA)at Zusanli(ST 36),Liangmen(ST 21)and Sanyinjiao(SP 6)in intervening diabetic gastroparesis(DGP)based on calcium-activated chloride channel.Methods:Forty Sprague-Dawley rats were randomly divided into four groups,including a normal control group(group A),a model group(group B),an EA group(group C)and a metoclopramide group(group D),with 10 rats in each group.A single intraperitoneal injection of 2%streptozotocin(STZ)combined with 8-week high-glucose high-fat diet was used to establish a DGP rat model.After intervention,gastrointestinal propulsive rate was observed;the expression level of transmembrane protein 16A(TMEM16A)was examined by immunohistochemistry;the Ca2+concentration in interstitial cells of Cajal(ICCs)was detected by immunofluorescence;and whole-cell patch-clamp technique was applied to detect the current intensity of calcium-activated chloride channel(ICaCC)in ICCs in gastric antrum.Results:After modeling,the blood glucose levels in group B,group C and group D were significantly increased compared with group A(all P<0.01);after intervention,compared with group B,the blood glucose levels in group C and group D were significantly decreased(P<0.05,P<0.01);the intra-group comparison of blood glucose level between after modeling and after intervention found significant difference only in group C(P<0.01).The gastrointestinal propulsive rates in group B,group C and group D were significantly different from that in group A(P<0.01 or P<0.05);the gastrointestinal propulsive rates were markedly higher in group C and group D than in group B(P<0.01,P<0.01).The expressions of TMEM16A in group B and group C were decreased compared with group A(P<0.01,P<0.05);the expressions of TMEM16A in group C and group D were increased compared with group B(P<0.01,P<0.05).The fluorescence intensity of Ca2+was significantly lower in group B than in group A(P<0.01);the fluorescence intensity of Ca2+was significantly higher in group C and group D than in group B(P<0.01,P<0.05).ICaCC in ICCs in group B was significantly decreased compared with group A;ICaCC in group C and group D were increased compared with group B.Conclusion:EA at Zusanli(ST 36),Liangmen(ST 21)and Sanyinjiao(SP 6)can significantly improve gastrointestinal motility in DGP rats by up-regulating the ICaCC in ICCs.

Murine calcium-activated chloride channel family member 3 induces asthmatic airway inflammation independently of allergen exposure

Background Expression of murine calcium-activated chloride channel family member 3 （mCLCA3） has been reported to be increased in the airway epithelium of asthmatic mice challenged with ovalbumin （OVA）. However, its role in asthmatic airway inflammation under no OVA exposure has not yet been clarified. Methods mCLCA3 plasmids were transfected into the airways of normal BALB/c mice. mCLCA3 expression and airway inflammation in mouse lung tissue were evaluated. Cell differentials and cytokines in bronchoalveolar lavage fluid （BALF） were analyzed. The expression of mCLCA3 protein and mucus protein mucin-5 subtype AC （MUC5AC） were analyzed by Western blotting. The mRNA levels of mCLCA3, MUC5AC and interleukin-13 （IL-13） were determined quantitatively. Results mCLCA3 expression was not detected in the control group while strong immunoreactivity was detected in the OVA and mCLCA3 plasmid groups, and was strictly localized to the airway epithelium. The numbers of inflammatory cells in lung tissue and BALF were increased in both mCLCA3 plasmid and OVA groups. The protein and mRNA levels of mCLCA3 and MUC5AC in the lung tissue were significantly increased in the mCLCA3 plasmid and OVA groups compared to the control group. The level of IL-13, but not IL-4, IL-5, IFN-y, CCL2, CCL5 or CCL11, was significantly increased compared with control group in BALF in the mCLCA3 plasmid and OVA groups. The level of IL-13 in the BALF in the mCLCA3 plasmid group was much higher than that in the OVA group （P 〈0.05）. The level of mCLCA3 mRNA in lung tissue was positively correlated with the levels of MUC5AC mRNA in lung tissue, IL-13 mRNA in lung tissue, the number of eosinophils in BALF, and the content of IL-13 protein in BALE The level of IL-13 mRNA in lung tissue was positively correlated with the number of eosinophils in BALF and the level of MUC5AC mRNA in lung tissue. Conclusion These findings suggest that increased expression of a single-gene, mCLCA3, could simulate an asthma attack, and its mechanism may involve mCLCA3 overexpression up-regulating IL-13 expression.

钙激活氯通道ANO1在小鼠心肌细胞的表达及其功能鉴定

目的:探讨钙激活氯通道蛋白anoctamin 1(ANO1)在小鼠原代培养心肌细胞中的表达及其功能特性。方法:采用胰酶与胶原酶共同消化,联合2次差速贴壁法获得C57BL/6小鼠原代心肌细胞;并用免疫荧光染色法检测α-横纹肌肌动蛋白,以鉴定心肌细胞纯度;应用RT-PCR检测小鼠心肌细胞ANO1 mRNA的表达;免疫印迹检测ANO1蛋白在小鼠心肌细胞的表达情况;应用荧光淬灭动力学实验检测ANO1钙激活氯通道的功能特性。结果:RT-PCR结果表明原代培养的小鼠心肌细胞表达ANO1 mRNA。免疫印迹实验结果显示原代培养的小鼠心肌细胞表达ANO1蛋白。荧光淬灭动力学实验证实表达于小鼠心肌细胞的ANO1具有钙激活氯通道典型的阴离子转运功能特性。结论:ANO1在小鼠心肌细胞中有明确表达,并具有钙激活氯离子通道特性,提示ANO1是钙激活氯通道的分子基础。

低渗诱导高分化鼻咽癌细胞CNE-1容积激活性氯电流

目的:研究细胞外低渗诱导的高分化鼻咽癌细胞CNE-1的容积激活性氯电流。方法:全细胞膜片钳记录氯电流,通过应用氯通道阻断剂、离子置换和改变细胞容积方法研究该电流的特性。结果:当细胞在等渗环境中背景电流微弱且稳定,细胞外给予47%低渗刺激后电流迅速增大,呈外向优势,对阴离子通透性的大小为:I->Br->Cl->葡萄糖酸。氯通道阻断剂ATP和NPPB可逆性地抑制此电流,ATP的抑制作用在外向电流显著强于内向电流。此电流对细胞容积改变敏感,细胞肿胀时被激活,细胞发生皱缩时则被抑制。结论:细胞外低渗诱导CNE-1细胞产生氯电流,此电流对细胞容积的改变敏感,在CNE-1细胞容积调节中起重要作用。

内皮素-1对牛脑血管平滑肌细胞ClC-3通道表达的影响

目的 研究内皮素 1(ET 1)对牛脑血管平滑肌细胞(CSMC)内源性ClC 3表达的影响。方法 采用培养的CSMC ,用免疫印迹 (westernblot)方法分析CSMCClC 3通道表达。结果 ①牛脑基底动脉、大脑中动脉、微动脉均有ClC 3蛋白表达 ,分子量约 10 5ku ,以微动脉表达最丰富 ,基底动脉表达最少 ;②培养的CSMC有内源性ClC 3蛋白表达 ,分子量约 95ku ;③ET 1能增加CSMCClC 3蛋白表达 ;④nifedipine、SK&F96 36 5能减少ET 1作用 ,环匹阿尼酸(cyclopiazonicacid ,CPA)浓度依赖性促进ClC 3蛋白表达 ,并能增强ET 1作用。结论 脑血管平滑肌细胞存在内源性ClC 3,ET 1可增强ClC 3表达 ,减少或增加胞浆内Ca2 + 浓度均可影响ET

CLIC-1 mRNA及蛋白在结肠癌的表达及临床意义

目的探讨氯离子通道-1(chloride intracellular channel 1,CLIC-1)mRNA及蛋白在结肠癌中的表达及其临床意义。方法采用RT-PCR和免疫组化检测2011年1-6月本院手术切除的54例结肠癌和相应癌旁组织中CLIC-1mRNA及蛋白的表达,分析其与临床病理特征的关系。结果结肠癌组织中的CLIC-1 mRNA表达水平高于癌旁组织[(0.658±0.043)vs(0.281±0.027),P<0.05],CLIC-1蛋白表达与浸润程度、有无淋巴结转移和TNM分期比较差异有统计学意义(P<0.05,P<0.01),而与患者的年龄、性别、肿瘤直径、原发部位、分化程度方面比较差异无统计学意义(P>0.05)。结论 CLIC-1在结肠癌中的表达明显升高,在结肠癌的进展中可能有一定作用。

细胞外氯离子浓度对大鼠ClC-1通道去激活动力学特性的影响

为探讨ClC 1通道的门控机制 ,实验应用爪蟾卵母细胞异源性表达大鼠野生型ClC 1(WTrClC 1)通道基因 ,并使用双电极电压钳法记录通道电流。通过改变细胞外氯离子浓度 ,采用双指数拟合的方法分析通道去激活电流 ,对其去激活门控动力学特性进行了研究。结果表明 ,降低细胞外氯离子浓度可增加快速去激活电流成分 ,减少慢速去激活成分 ;同时 ,慢速去激活和快速去激活电流的时间常数都显著减小 ,说明细胞外氯离子浓度的改变可影响通道去激活动力学参数 ,从而改变通道的门控过程。

氯离子通道-3反义寡核苷酸对内皮素-1促增殖体外培养的牛角膜内皮细胞的抑制作用

目的观察氯离子通道-3(chloride channel3,ClC-3)反义寡核苷酸(antisense oli-gonucleotides,AS-ODN)对内皮素1(endothelin-1,ET-1)促增殖体外培养的牛角膜内皮细胞(bovine corneal endothelial cells,BCECs)的抑制作用。方法 BCECs细胞悬液接种培养12h后,通过脂质体介导转染不同浓度的ClC-3寡核苷酸。体外培养BCECs24h后加入200pmol.L-1ET-1,继续培养48h。通过倒置荧光显微镜观察BCECs寡核苷酸的摄取。采用逆转录聚合酶链反应、免疫印迹法检测ClC-3mRNA和蛋白的表达。采用MTT法观察BCECs增殖状况,计算细胞存活率,同时应用流式细胞仪检测细胞周期时相的变化,计算细胞增殖指数。结果寡核苷酸可被培养的BCECs摄取。ClC-3mRNA与蛋白的表达变化呈平行关系。与不加时相比,ClC-3AS-ODN浓度依赖性地减少BCECsClC-3mRNA和蛋白的表达,同样也浓度依赖性地降低BCECs MTT吸光度值(OD值)和细胞存活率。经100mg·mL-1ClC-3AS-ODN处理后,与对照组相比,细胞G0/G1期细胞比例明显增高,S期及G2期细胞比例则明显降低,出现明显的凋亡峰,增殖指数明显下降。结论 ClC-3AS-ODN可能通过减少ClC-3mRNA和蛋白的表达,浓度依赖性抑制ET-1对体外培养BCECs的增殖作用,并使细胞周期停滞在G1期。

DIDS对SIN-1诱导大鼠海马神经元凋亡及PARP-1/AIF表达的影响

目的观察氯通道阻断剂4,4'-二异硫氰基芪-2,2'-二磺酸(DIDS)对NO诱导的大鼠离体海马神经元凋亡的保护作用。方法离体培养12 d的SD大鼠海马神经元,随机分为正常对照组、3-吗啡斯德酮亚胺(3-morpholinosyndnomine,SIN-1)处理组、SIN-1+DIDS组。对各组神经元分别在相应的时间点用MTT法测定细胞生存率、Hoechst 33258测定凋亡百分数、免疫化学荧光分析检测凋亡信号蛋白PARP-1/AIF的变化、Western blot分析凋亡蛋白Caspase-3的变化。结果 DIDS呈剂量依赖性地抑制SIN-1诱导的神经元损伤,减少凋亡发生数目,并能抑制损伤所引起的Caspase-3的激活、削弱PARP-1/AIF的表达。结论氯通道可能参与了NO诱导的海马神经元损伤,氯通道阻断剂DIDS的保护作用可能与削弱PARP-1/AIF的表达有关。

氯离子通道1过表达对小鼠肝癌细胞株Hca-P生物学行为的影响

背景与目的:氯离子通道l(chloride intracellular channel l,CLICl)是CLIC家族中的一员,研究表明CLIC1与肿瘤转移相关。本研究旨在探讨CLICl过表达在体外对小鼠肝癌低淋巴道转移细胞株Hca-P生长、体外迁移和侵袭能力的影响。方法:构建CLIC1过表达真核载体pcDNA3.1(+)-CLIC1表达质粒,将重组的pcDNA3.1(+)-CLIC1基因和空载体pcDNA3.1(+)转染Hca-P母系细胞,通过G418筛选获得稳定表达CLIC1基因的pcDNA3.1(+)-CLIC1-Hca-P细胞株和转染空载体的pcDNA3.1(+)-Hca-P细胞株,RT-PCR和ELISA鉴定CLIC1过表达水平,CCK-8法检测细胞活力和分裂增殖能力,Transwell实验检测细胞的体外迁移能力和侵袭能力。结果:成功建立了稳定表达CLIC1基因的细胞株pcDNA3.1(+)-CLIC1-Hca-P,与空载体对照组相比,pcDNA3.1(+)-CLIC1质粒转染入Hca-P细胞后CLIC1基因表达水平显著升高。pcDNA3.1(+)-CLIC1-Hca-P细胞增殖明显高于Hca-P母系细胞组和空载体对照组,差异有统计学意义(P<0.05),且细胞增殖主要集中在72～96 h;Transwell检测各组肿瘤细胞迁移能力结果显示,pcDNA3.1(+)-CLIC1-Hca-P、pcDNA3.1(+)-Hca-P和Hca-P细胞株迁移到膜下和小室下室的平均细胞数分别为205.43±22.87、132.72±20.45和121.35±19.64。pcDNA3.1(+)-CLIC1-Hca-P与Hca-P、pcDNA3.1(+)-Hca-P细胞株比较差异有统计学意义(P<0.05);Transwell检测各组肿瘤细胞侵袭能力结果显示,pcDNA3.1(+)-CLIC1-Hca-P细胞穿过基膜的细胞数为(76.2±4.62)个,明显多于pcDNA3.1(+)-Hca-P的穿膜细胞数(48.34±3.45)个和Hca-P细胞的穿膜细胞数(49.8±5.51)个,差异有统计学意义(P<0.05)。结论:CLIC1过表达可以显著促进Hca-P细胞增殖、增强其侵袭能力。CLIC1有望成为临床治疗肝癌的基因治疗靶点之一。

子宫内膜样腺癌中CLIC1蛋白的表达及临床意义

目的探讨细胞内氯离子通道蛋白1(CLIC1)在子宫内膜样腺癌中的表达及其与临床病理特征的关系。方法采用免疫组化SP法检测100例子宫内膜样腺癌组织和50例正常子宫内膜组织中CLIC1蛋白的表达,并分析其表达与子宫内膜样腺癌临床病理特征的关系。结果 CLIC1蛋白在子宫内膜样腺癌组织中的阳性表达率为63.0%,高于其在正常子宫内膜组织中的22.0%(P<0.05);CLIC1蛋白在子宫内膜样腺癌中的表达与病理分期及淋巴结转移有关(P<0.05),而与年龄、是否绝经、浸润深度和组织学分级无关(P>0.05)。结论 CLIC1蛋白过表达可能促进了子宫内膜样腺癌的发生、发展。

血管紧张素-(1-7)通过抑制ClC-3通道减轻高糖引起的心肌细胞损伤

目的探讨血管紧张素-(1-7)[Ang-(1-7)]能否通过调控ClC-3通道保护心肌细胞对抗高糖引起的损伤。方法应用35 mmol/L葡萄糖处理H9c2心肌细胞24 h建立损伤模型。Ang-(1-7)或氯通道抑制剂与心肌细胞共处理24 h观察对高糖诱发的心肌细胞损伤的影响。应用细胞计数试剂盒8检测细胞存活率;Hoechst33258染色荧光显微镜照相术检测凋亡细胞的形态学改变;双氯荧光素染色荧光显微镜照相术测定细胞内活性氧水平;超氧化物歧化酶试剂盒测定活性;罗丹明123染色荧光显微镜照相术检测线粒体膜电位;Western blot法测定心肌细胞ClC-3通道蛋白的表达水平。结果 35 mmol/L葡萄糖处理H9c2心肌细胞24 h明显地增加ClC-3通道蛋白的表达水平(P<0.01);1μmol/LAng-(1-7)与葡萄糖共处理心肌细胞24 h显著地抑制葡萄糖对ClC-3通道蛋白表达的上调作用(P<0.01);1μmol/LAng-(1-7)或100μmol/L氯通道抑制剂氯通道抑制剂与葡萄糖共处理心肌细胞24 h减轻葡萄糖引起的损伤作用,表现为增加细胞存活率和超氧化物歧化酶活性,减小细胞凋亡数量,胞内活性氧水平及线粒体膜电位丢失(P<0.01)。结论 ClC-3通道参与葡萄糖引起的心肌细胞损伤;Ang-(1-7)通过抑制ClC-3通道保护心肌细胞对抗葡萄糖引起的损伤。

氯通道蛋白-3和水通道蛋白-1在大鼠半乳糖性白内障晶状体中表达水平的变化

目的研究大鼠半乳糖性白内障晶状体中氯离子通道蛋白-3(CLC-3)和水通道蛋白-1(AQP-1)表达水平的变化,探讨CLC-3和AQP-1与白内障发病的关系。方法健康清洁级Wistar大鼠88只随机分为空白对照组(8只)、生理盐水组(40只)和半乳糖性白内障模型组(Gal组)(40只)。生理盐水组和Gal组根据处理时间不同各亚分为5个亚组,每个亚组8只大鼠。Gal组单侧眼球后注射D-半乳糖生理盐水注射液,生理盐水组同期单侧眼球后注射等体积无菌生理盐水,每日裂隙灯下观察大鼠晶状体混浊的动态变化,并参照Kador等的分级标准分期记录。分别于第1次给药后第3、7、14、21、30天在全身麻醉下处死各组实验大鼠,摘出晶状体,应用实时荧光定量PCR法检测各组晶状体中CLC-3mRNA和AQP-1mRNA含量的变化。结果透明晶状体和半乳糖性白内障晶状体中均有CLC-3mRNA和AQP-1mRNA的表达;生理盐水组各时间点CLC-3mRNA和AQP-1mRNA的表达差异无统计学意义(P>0.05);Gal组于3、7、14d时CLC-3mRNA表达逐渐增高,均高于同期生理盐水组,到14d时约达正常水平的7倍,21d、30d时又有所下降,均低于同期生理盐水组(P<0.01);各时间点晶状体CLC-3mRNA含量两两比较,差异均有统计学意义(P<0.01);模型组于3d时AQP-1mRNA表达已下降,与同期生理盐水组比较差异有统计学意义(P<0.05),且随着白内障的进一步发展,AQP-1mRNA含量逐渐降低,均低于同期生理盐水组(P<0.01);各时间点晶状体AQP-1mRNA含量两两比较,差异均有统计学意义(P<0.01)。结论晶状体中CLC-3和AQP-1表达的变化可能与白内障的发生发展有着密切的联系。

氯离子通道蛋白1调控放射抵抗食管鳞癌细胞放射敏感性的机制

目的:探讨氯离子通道蛋白1(chloride intracellular ion channel 1,CLIC1)对食管鳞癌细胞获得性放射抵抗特性的影响及作用机制。方法:采用蛋白印记法及逆转录聚合酶链式反应法检测Eca109R50Gy细胞中CLIC1的表达水平。采用CLIC1小分子特异抑制剂IAA-94(indanyloxyacetic acid-94,IAA-94)抑制Eca109R50Gy细胞中CLIC1功能,通过克隆形成试验、流式细胞仪分析对比CLIC1功能抑制前后的细胞存活分数(SF)、细胞凋亡比率及细胞周期分布。结果:Eca109R50Gy细胞中CLIC1在转录水平及蛋白水平均呈现显著高表达(P<0.001);CLIC1功能抑制组Eca109R50Gy细胞克隆形成能力明显受抑(SF_(IAA-94vs) SF_(Control),P<0.001),而细胞凋亡比率显著增高(P<0.01)。CLIC1功能抑制组Eca109R50Gy细胞G2/M期细胞比例显著增加(P<0.01)。结论:CLIC1在放射抵抗的食管鳞癌细胞中高表达并与其获得性放射抵抗特性有关,抑制CLIC1功能可增强放射抵抗的食管癌细胞对放射线的敏感性,其增敏机制与影响细胞周期分布有关。

呋喃苯胺酸对白细胞介素-1β促骨髓基质细胞增殖的抑制作用

目的：观察Ｃｌ－ 通道阻断剂呋喃苯胺酸对重组人白细胞介素－１β（ｉｎｔｅｒｌｅｕｋｉｎ－ １β，ＩＬ－ １β）诱导的小鼠骨髓基质细胞（ＢＭＳＣ） 增殖作用的影响。方法：ＭＴＴ法测定原代培养的小鼠ＢＭＳＣ增殖活性。结果：ＩＬ－１β（２００～１ ０００ｋＵ·Ｌ－１） 对ＢＭＳＣ具显著的促增殖作用。呋喃苯胺酸（２０ ～５００μｍｏｌ·Ｌ－１）特异性地抑制ＩＬ－ １β的促增殖作用，效应呈浓度依赖性。结论：Ｃｌ－ 通道与ＩＬ－ １β促ＢＭＳＣ增殖作用有关，Ｃｌ－