芪榔合剂对功能性便秘小鼠结肠AQP4和AQP8含量的影响研究

目的观察芪榔合剂对功能性便秘模型小鼠结肠组织中水通道蛋白4(AQP4)和水通道蛋白8(AQP8)表达的影响,探讨芪榔合剂治疗功能性便秘的作用机制。方法将40只健康昆明种小鼠按性别、体质量随机分为阴性对照组、便秘组、大剂量中药组、小剂量中药组,每组10只。阴性对照组给予50 mg/kg蒸馏水灌胃,其余组均予以50 mg/kg复方地芬诺酯灌胃20 d制作便秘模型。造模成功后第2天,阴性对照组、便秘组给予蒸馏水0.002mL/g灌胃7 d;大剂量中药组、小剂量中药组给予0.025 mL/g相应量中药(分别含生药2.9 g/mL和1.45 g/mL,相当于成人体质量30倍和15倍)灌胃7d。采用免疫组化法检测各组小鼠结肠组织中AQP4、AQP8表达情况。结果便秘组小鼠结肠组织中AQP4、AQP8含量均明显高于阴性对照组(P均<0.05);大剂量中药组、小剂量中药组小鼠结肠组织中AQP4、AQP8含量均明显低于便秘组,且小剂量中药组AQP8含量明显低于大剂量中药组(P<0.05)。结论便秘小鼠结肠组织中AQP4、AQP8含量明显升高,芪榔合剂对功能性便秘小鼠结肠组织中AQP4、AQP8含量具有一定的调节作用。

复方地芬诺酯建立便秘模型与AQP8的相关性研究

目的:通过复方地芬诺酯法建立大鼠慢传输型便秘模型,探索一种简便易行的大鼠便秘造模方法,并探讨大鼠便秘造模过程中对结肠AQP8表达的影响。方法:SD大鼠30只随机分为空白组和便秘模型组。空白组大鼠用生理盐水灌胃,便秘模型组用复方地芬诺酯灌胃,观察两组大鼠大便粒数及大便湿重。大鼠便秘模型建立后。将大鼠集体处死,取大鼠近端结肠标本,用免疫组织化学的方法检测两组大鼠结肠AQP8的表达情况。使用彩色病理图像分析系统对阳性表达的平均光密度值进行半定量分析。结果:建立便秘模型末次给药后,便秘组24 h大便粒数、大便湿重均低于空白对照组(P<0.05),差异有统计学意义,表明大鼠慢传输型便秘模型成功建立;免疫组化结果显示:便秘组结肠AQP8的MD值大于空白对照组(P<0.05),差异有统计学意义。结论:复方地芬诺酯灌胃法成功建立大鼠便秘模型,便秘模型的建立与大鼠结肠AQP8的表达增高相关。

低渗状态下星形胶质细胞AQP8的表达变化

目的探讨低渗透压作用下,星形胶质细胞水通道蛋白8(aquaporin8,AQP8)的表达变化规律。方法原代培养大鼠星形胶质细胞,随机分为对照组(常规培养液)和低渗组(268、254、240mmol/L),每组分别作用1、3、6、12、24h,共5个时间点。通过MTT比色法检测细胞活力,免疫细胞化学、免疫荧光、Realtime-PCR研究AQP8及其mRNA的表达变化。结果对照组星形胶质细胞的细胞形态、细胞活性、AQP8及其mRNA的表达在各时间点均无明显变化(P>0.05)。低渗组中,星形胶质细胞水肿,细胞活性下降;AQP8及其mRNA的表达水平随低渗程度的下调和低渗作用时间的延长而增强。低渗液(268、254、240mmol/L)作用后,免疫细胞化学显示星形胶质细胞的AQP8表达从低渗作用1h的(0.2583±0.0098,0.2800±0.0109,0.2817±0.0075)到低渗作用24h的(0.3850±0.0109,0.4067±0.0070,0.4250±0.0104)(P<0.05);RealtimePCR显示:AQP8与beta-actin的mRNA水平比从低渗作用1h的(0.1275±0.0118,0.1344±0.0324,0.1675±0.0078)上升到(3.2780±0.1212,5.4104±0.1041,8.3510±0.2880)。结论低渗作用下,AQP8介导的水分子运输可导致星形胶质细胞肿胀,继而引发细胞结构、功能的损伤;AQP8的表达上调可能是导致星形胶质细胞水肿形成和发展的重要分子机制之一。

水通道蛋白8在人胎盘和胎膜中的表达

目的:探讨水通道蛋白8(aquaporin 8,AQP8)在正常人胎膜及胎盘中的表达情况。方法:采集6例正常足月剖宫产的胎膜和胎盘组织,采用逆转录聚合酶链反应(RT-PCR)技术检测AQP8mRNA在胎膜、胎盘中的表达,用免疫组织化学的方法检测AQP8蛋白在胎膜、胎盘中的定位表达。结果:AQP8mRNA在羊膜、绒毛膜和胎盘均有表达,AQP8蛋白主要表达于羊膜上皮细胞、绒毛膜滋养细胞和胎盘合体滋养细胞的胞浆和胞膜中。结论:AQP8在羊水平衡的调节和母儿液体交换过程中可能起重要作用。

大黄素对脓毒症大鼠肝细胞线粒体水通道蛋白8表达的影响

目的 探讨大黄素对脓毒症大鼠肝细胞线粒体水通道蛋白8(AQP-8)表达的影响。方法 成年雄性SD大鼠96只,分为4组:对照组、脓毒症组、预处理组、治疗组,每组24只,采用盲肠结扎穿孔法构建脓毒症大鼠模型,对照组探查盲肠后回纳腹腔。预处理组、治疗组采用大黄素悬浊液连续喂养5d,治疗组大鼠建模2h后腹腔内注射大黄素。18h后随机每组处死12只大鼠,采集标本,剩余12只大鼠观察生存时间。生化分析仪测定外周血ALT、AST、m-AST含量;ELISA法测定外周血IL-1β、IL-6、TNF-α、HMGB-1、NO含量;肝组织行ATP含量测定,肝细胞线粒体膜Na^(+)-K^(+)-ATP酶、Mg^(+)-ATP酶、Ca2+-ATP酶、Ca^(2+)-Mg^(2+)-ATP酶的活性测定;RT-PCR法测定线粒体内膜AQP-8mRNA含量,蛋白免疫印迹法测定AQP-8蛋白水平。结果 对照组、预处理组和治疗组大鼠存活时间较脓毒症组长(P<0.01);与对照组相比,脓毒症组血清ALT、AST和m-AST水平显著升高,肝细胞ATP含量显著降低,肝细胞线粒体膜ATP酶活性、肝细胞线粒体AQP8 mRNA和AQP8蛋白表达量明显下降(P<0.01)。与脓毒症组相比,预处理组和治疗组血清ALT、AST和m-AST水平显著升高,肝细胞ATP含量显著降低,肝细胞线粒体膜ATP酶活性、肝细胞线粒体AQP8 mRNA和AQP8蛋白表达量明显上升(P<0.01),预处理组和治疗组间无差异(P>0.05);与对照组相比,脓毒症组血清IL-1β、IL-6、TNF-α、HMGB-1、NO含量明显上升(P<0.01);与脓毒症组相比,预处理组和治疗组血清IL-1β、IL-6、TNF、HMGB-1、NO含量明显下降(P<0.01),预处理组和治疗组间无差异(P>0.05)。结论 脓毒症可以导致肝细胞线粒体膜AQP8 mRNA和蛋白表达下降。大黄素可以上调脓毒症大鼠肝细胞线粒体膜AQP8 mRNA和蛋白的表达,延缓大鼠CLP手术后出现脓毒症症状的时间,延长脓毒症大鼠的生存时间。

痛泻要方对腹泻型肠易激综合征模型大鼠结肠水通道蛋白8表达影响的机制研究

目的:探讨痛泻要方治疗腹泻型肠易激综合征(D-IBS)模型大鼠的作用机制。方法:健康雄性Wistar大鼠40只随机分为正常组、模型组、中药组、药抗组,采用应激与束缚的方法18 d复制肠易激综合征模型,造模成功后中药组和药抗组大鼠给予中药23.6 g.kg-1,ig 1次/d,连续7 d,药抗组第4天开始给予血管活性肠肽(VIP)受体拮抗剂35μg.kg-1,iv 1次/d,连续4 d。检测大鼠粪便含水量,采用RT-PCR法和SABC免疫组化法检测结肠组织水通道蛋白8(aquaporin 8,AQP8)的表达。结果:①大鼠粪便含水量:与正常组比较,模型组粪便含水量升高(P<0.01);与模型组比较,中药组粪便含水量降低(P<0.01);药抗组粪便含水量与模型组差异无统计学意义。②结肠组织AQP8:与正常组比较,模型组AQP8表达下调(P<0.01);与模型组比较,中药组AQP8表达上调(P<0.01);药抗组AQP8表达与模型组差异没有统计学意义。结论:痛泻要方治疗D-IBS的药理学机制可能通过VIP途径调节AQP8的表达实现。

Expression of aquaporin 8 and its relationship with melanosis coli

Background The relationship between melanosis coli （MC） and aquaporin 8 （AQP8） has not yet been elucidated. The aim of this research was to investigate the relationship between the expression of AQP8 and the pathological mechanism of MC.Methods Expression of AQP8 was detected by immunohistochemistry and reverse transcription-polymerase chain reaction （RT-PCR） in 37 MC colon tissues and 13 control colon tissues. Global gene expression analysis was also used to identify differently expressed genes. Its relationship with MC was analyzed by SPSS 11.5 statistical software.Results The positive rate of AQP8 expression detected by immunohistochemistry in the MC group was 24.3% （9/37）,significantly lower than the 69.2% （9/13） in the control group （P 〈0.05）. The relative expression level of AQP8 in MC group was 0.639±0.160, lower than 0.921±0.148 of controls （P 〈0.05）. Global gene expression analysis showed that AQP8 mRNA expression was downregulated in MC patients.Conclusions The decreased AQP8 expression in MC patients indicates that chronic use of laxatives containing anthraquinone may cause reduced water absorption. The expression of AQP8 may be related to MC.

Expression of aquaporin 8 in colonic epithelium with diarrhoeapredominant irritable bowel syndrome

Background We analysed and compared the aquaporin 8 （AQP8） expression in ascending and descending colon mucosa between patients with diarrhoea-predominant irritable bowel syndrome （D-IBS） and healthy volunteers, in order to study the relationship between the clinical feature of IBS, the expression of AQP8 and the pathological mechanism of D-IBS. Methods Specimens were taken from the proximal ascending colon or distal descending colon of D-IBS patients （n=-26） and healthy volunteers （n=30）, and AQP8 mRNA expression of each specimen was determined by fluorescent quantitative reverse transcription polymerase chain reaction （FQ-RT-PCR）. In patients with D-IBS, the relationship was analysed between AQP8 expression in both ascending and descending colons and clinical features including gender, age of onset, duration of illness, frequency of defecation, and stool characteristics. Results Although AQP8 was present in the epithelium of the ascending and descending colons in healthy persons and D-IBS patients, the AQP8 level of the D-IBS patients was significantly lower than that of the healthy persons （P〈0.01 in the ascending colon, P〈0.05 in the descending colon）. AQP8 expression was not correlated with the age of patients with D-IBS （P〉0.05 both in the ascending and descending colons） or the age at the onset （P〉0.05 both in the ascending and descending colons）, but closely with the duration of illness （P〈0.05 in the ascending colon, P〈0.01 in the descending colon）, frequency of defecation （P〈0.01 in the ascending colon, P〈0.05 in the descending colon） and stool characteristics （P〈0.01 in the ascending colon, P〉0.05 in the descending colon）. Conclusions The decreased AQP8 expression in D-IBS patients indicates that dysfunction of colonic absorption may cause reduced water absorption, loose stool and diarrhoea. The expression of AQP8 may be related to D-IBS.

Aquaporin 8 expression is reduced and regulated by microRNAs in patients with ulcerative colitis

Background Ulcerative colitis （UC） is associated with differential expression of genes involved in inflammation and tissue remodeling. MicroRNA （miRNA） plays an important role in the pathogenesis of UC by regulating the gene expression at the post-transcriptional level and control crucial physiological processes. This study aimed to identify aquaporin 8 （AQP8） expression and its relationship with miRNA in UC patients. Methods Human colon samples, in this study, were obtained from 20 patients with UC and 16 healthy subjects undergoing diagnostic colonoscopy at the Chinese People＇s Liberation Army General Hospital between December 2009 and June 2010. We screened different genes from UC tissues and healthy subjects using genome-wide microarray, quantitative reverse transcription-polymerase chain reaction （qRT-PCR） and Western blotting. Regulation of gene expression by miRNAs was assessed by luciferase reporter construct assays and transfection of specific miRNA mimics and inhibitor. Results We identified that 1596 genes were increased and 1301 genes were decreased in UC patients compared to healthy subjects. Among them, we focused on the analysis of AQP8 which was decreased three folds in UC tissues （P 〈0.01）. The expression of AQP8 mRNA and protein were decreased in UC tissue and tumor necrosis factor （TNF）-α treated HT29 cells compared with controls （P 〈0.05）. We searched candidate target miRNAs of AQP8 through bioformatics and the luciferase report assay analysis indicated that miR-424, miR-195, miR-330, miR-612, and miR-16 which has complementary site in the 3-untranslated region （3＇UTR） of AQP8 could decrease the relative luciferase activities by 10%-45%. Conclusion AQP8 and its relationship with miRNAs may be involved in the pathogenesis of UC.