Effects of Hyperosmolality on Expression of Urea Transporter A2 and Aquaporin 2 in Mouse Medullary Collecting Duct Cells

In this study,the effects of hyperosmolality on the expression of urea transporter A2 (UTA2) and aquaporin 2 (AQP2) were investigated in transfected immortalized mouse medullary collecting duct (mIMCD3) cell line.AQP2-GFP-pCMV6 and UTA2-GFP-pCMV6 plasmids were stably transfected into mIMCD3 cells respectively.Transfected mIMCD3 and control cells were cultured in different hy-pertonic media,which were made by NaCl alone,urea alone,or an equiosmolar mixture of NaCl and urea.The mRNA and protein expression of AQP2 was elevated by the stimulation of NaCl alone,urea alone and NaCl plus urea in AQP2-mIMCD3 cells;whereas NaCl alone and NaCl plus urea rather than urea alone increased the mRNA and protein expression of UTA2 in UTA2-mIMCD3 cells,and all the expression presented an osmolality-dependent manner.Moreover,the mRNA and protein expression of UTA2 rather than AQP2 was found to be synergistically up-regulated by a combination of NaCl and urea in mIMCD3 cells.It is concluded that NaCl and urea synergistically induce the expression of UTA2 rather than AQP2 in mIMCD3 cells,and hyperosmolality probably mediates the expression of AQP2 and UTA2 through different mechanisms.

充血性心力衰竭水潴留的机制——Aquaporin2水通道蛋白的作用

水潴留是充血性心力衰竭的重要病理生理表现。长期以来人们对心力衰竭时水重吸收增加的肾脏机制所知甚少。Aquaporin水通道 (AQP)家族的发现是水通道生物学研究的一个新的里程碑。研究发现充血性心力衰竭时肾脏AQP2水通道基因mRNA和蛋白的表达明显上调 ;AQP2的上调主要由血管加压素所介导 ,V2受体拮抗剂可显著降低此上调 ;在充血性心力衰竭时肾脏AQP2表达的改变是选择性的 ,不伴有肾脏AQP1和AQP3蛋白表达的增加。证实AQP2水通道是充血性心力衰竭时调节水潴留的关键性蛋白质 。

高心排心力衰竭大白鼠肾脏Aquaporin2水通道蛋白基因的表达

目的 :研究高心排心力衰竭大白鼠 Aquaporin2基因的表达及精氨酸血管加压素 ( AVP)受体拮抗剂的治疗作用。方法 :SD大白鼠分别行腹腔动脉 -下腔静脉分流术 ,建立高心排心力衰竭动物模型。术后随机分为 A- C分流对照组、A- C分流及 V1受体拮抗剂治疗组、A- C分流及 V2受体拮抗剂组 ,和 A- C分流及 V1/ V2受体拮抗剂治疗组。每周测定尿量 ,尿渗透压 ,4周后测定 AVP浓度 ,同时做 AQP2基因蛋白表达的检测。结果 :A- C分流大白鼠 4周后出现 AVP水平升高 ( P <0 .0 1) ,同时伴有 AQP2基因蛋白表达增加 ;AVPV2受体拮抗剂能抑制 A- C分流过程中 AVP的升高及 AQP2基因蛋白的过度表达。结论 :A- C分流大白鼠 AQP2基因蛋白表达增加 ,其与AVP水平相关 ;AVP V2受体拮抗剂能够改善心力衰竭时的水钠潴留 ,为开发 AVP V2受体拮抗剂这类新型利尿药物提供了理论基础。

Influence of Sanao Tang on urine volume and expression of aquaporin 2 in rats with respiratory function impairment induced by passive smoking and lipopolysaccharide

OBJECTIVE: To investigate the effect of Sanao Tang(SAT) on urine volume and the expression of aquaporin-2(AQP2) in rats with lung dysfunction induced by passive smoking and lipopolysaccharide.METHODS: Totally 45 healthy Specific pathogen Free Wistar Rats were randomized into 3 groups:normal control group, model group and SAT group.A rat model of respiratory dysfunction induced by exposure to cigarette smoking and lipopolysaccharide(LPS). Lavage of decoction of the Chinese medicine was performed for rats in the SAT group. Anires 2005 System was used to analyze the pulmonary function. Urine of rats was collected through metabolism cage method. Enzyme-linked immunosorbent assay(ELISA) was used to determine content of antidiuretic hormone(ADH), angiotensin Ⅱ(AngⅡ), atrial natriuretic factor(ANP), endothelin 1(ET-1), nitric oxide(NO) and prostaglandin E2(PGE2) in serum, lung and kidney. The expression of AQP2 in rat renal tissue was determined with real-time fluorescence quantitative PCR(RT-PCR).RESULTS:(a) In comparison with the normal control, It was found that enforced vital capacity(FVC),1-second forced expiratory volume/forced vital capacity%(FEV1/FVC%), 24 h urine volume content of NO and PGE2 were decreased, while AQP2 m RNA level and content of ADH, Agn Ⅱ, ANP and ET-1were increased in the model group with statistical significance(P < 0.05).(b) In comparison with the model group, It was found that FVC, FEV1, FEV1/FVC%, 24 h urine volume, content of PGE2 and NO decreased, while AQP2 m RNA level, content of ANP,ADH and AngⅡ decreased in the SAT group with statistical significance(P < 0.05).CONCLUSION: SAT might effectively regulate the urine volume in the modeled rats; ADH, Ang Ⅱ,ANP, ET-1, NO and PGE2 might play an important role in the regulation on urine volume by lungs.This might be the mechanisms underpinning the function of lung governing water passage in terms of the theory of Traditional Chinese Medicine.

Effect of Micardis on the Expression of Renal Medulla Aquaporin-2 in Diabetic Mice

In current study, the effect of angiotensin receptor blocker Micardis on the localization and expression of aquaporin-2 （AQP2） was investigated in the renal medullary collecting duct of mice with diabetic nephropathy （DN）. Mice were divided into three groups： normal group, DN group and Micardis-treated group. Six weeks after establishment of STZ-induced DN model in mice, the expression of AQP2 in renal medulla was detected measured by semiquantitative immunofluorescence histochemistry and Western blot techniques, and the localization of AQP2 by confocal immunofluorescence laser scanning microscopy. The results showed that the urinary osmolality was decreased in DN group as compared with normal group （2.39±0.11 vs 3.16±0.16, P〈0.05）. Although the localization of AQP2 on the renal medulla was unchanged, the expression of AQP2 was increased significantly in DN group as compared with normal group. Micardis could partly attenuate above changes. It was concluded that treatment with Micardis could partly rectify the abnormal expression of AQP2 in renal medulla of DN mice, which suggested that rennin-angiotensin system （RAS） is implicated in the pathogenesis of DN by regulating the expression of AQP2.

Tolvaptan regulates aquaporin-2 and fecal water in cirrhotic rats with ascites

AIM: To investigate the role of tolvaptan in regulating aquaporin(AQP)-2 expression and fecal water content in cirrhotic rats with ascites.METHODS: Cirrhosis with ascites was induced in rats by repetitive dorsal injection of CCl4 for 14 wk. In total, 84 cirrhotic rats with ascites divided into three groups(vehicle, 3 mg/kg and 5 mg/kg tolvaptan), and then further divided into five subgroups(days 1, 2, 3, 4, and 5). Blood samples were obtained to measure vasopressin and sodium concentrations. Rats were killed and colonic mucosa was scraped for analysis of protein expression and AQP-2 transcriptional level. The whole layer was fixed for hematoxylin&eosin(HE) staining and feces were collected for determination of fecal water content. CONCLUSION: Compared with vehicle, vasopressin decreased significantly in the tolvaptan groups from day 2 to a similar level in each treatment group. AQP-2 showed significant upregulation in cirrhotic rats with ascites compared with an untreated control group(100% ± 22.9% vs 22.2% ± 10.23%, P < 0.01). After administration of tolvaptan, AQP-2 expression began to decrease significantly from day 2 in each treatment group, but no significant difference was finally found between the treatment groups. Fecal water content inthe distal colon was increased by 5 mg/kg tolvaptan on day 1(66.8% ± 9.3% vs 41.4% ± 6.3%, in the vehicle group, P < 0.05). Fecal water content returned to baseline at day 4 at the latest in both treatment groups, and did not correspond to the change in AQP-2 expression. HE staining of the colonic mucosa showed no mucosal damage related to tolvaptan.CONCLUSION: Upregulation of AQP-2 in the distal colon is found in cirrhotic rats with ascites. Tolvaptan inhibits its expression and may decrease water reabsorption and induce diarrhea.

Downregulation of Aquaporin 4 Expression through Extracellular Signal-regulated Kinases1/2 Activation in Cultured Astrocytes Following Scratch-injury

Objective To investigate the role of extracellular signal-regulated kinase1/2（ERK1/2） pathway in the regulation of aquaporin 4（AQP4） expression in cultured astrocytes after scratch-injury. Methods The scratch-injury model was produced in cultured astrocytes of rat by a 10-μL plastic pipette tip. The morphological changes of astrocytes and lactate dehydrogenase（LDH） leakages were observed to assess the degree of scratch-injury. AQP4 expression was detected by immunofluorescence staining and Western blot, and phosphorylated-ERK1/2（p-ERK1/2） expression was determined by Western blot. To explore the effect of ERK1/2 pathway on AQP4 expression in scratch-injured astrocytes, 10 μmol/L U0126（ERK1/2 inhibitor） was incubated in the medium at 30 min before the scratch-injury in some groups. Results Increases in LDH leakage were observed at 1, 12, and 24 h after scratch-injury, and AQP4 expression was reduced simultaneously. Decrease in AQP4 expression was associated with a significant increase in ERK1/2 activation. Furthermore, pretreatment with U0126 blocked both ERK1/2 activation and decrease in AQP4 expression induced by scratch-injury. Conclusion These results indicate that ERK1/2 pathway down-regulates AQP4 expression in scratch-injured astrocytes, and ERK1/2 pathway might be a novel therapeutic target in reversing the effects of astrocytes that contribute to traumatic brain edema.

葡萄籽原花青素提取物对心肌梗死大鼠肾素-血管紧张素系统及AQP2蛋白表达的影响

目的:探讨葡萄籽原花青素提取物(GSPE)对心肌梗死大鼠肾素血管紧张素-系统及水通道蛋白2(AQP2)表达的影响。方法:将55只无特定病原体(SPF)级Sprague-Dawley(SD)大鼠按照随机数字表法分为健康组、模型组、辛伐他汀组、GSPE低剂量组及GSPE高剂量组,每组11只。除健康组外其余大鼠均采用冠状动脉结扎法制备心肌梗死模型,建模成功后,GSPE低剂量组、高剂量组大鼠分别灌胃100 mg/kg、400 mg/kg葡萄籽原花青素溶液,辛伐他汀组灌胃40 mg辛伐他汀溶液。苏木精-伊红(HE)染色后观察心肌组织形态;末端脱氧核苷酸转移酶介导的原位缺口末端转移酶标记法(TUNEL)检测心肌细胞凋亡;超声心动图监测心功能;放射免疫法检测血管紧张素Ⅱ(AngⅡ)、血浆肾素活性(PRA)、醛固酮水平;免疫印迹法检测心肌组织中AQP2、B细胞淋巴瘤/白血病2号基因(Bcl-2)及半胱天冬氨酸蛋白酶-3(Caspase-3)蛋白水平。结果:与健康组比较,模型组大鼠左心室收缩末期内径(LVESD)、左心室舒张末期内径(LVEDD)升高,左心室射血分数(LVEF)和左心室短轴缩短分数(LVFS)降低(P<0.05);与模型组比较,GSPE低剂量组、GSPE高剂量组及辛伐他汀组LVEDD、LVESD降低,LVEF、LVFS升高(P<0.05),GSPE低剂量组、GSPE高剂量组间比较差异有统计学意义,而GSPE高剂量组与辛伐他汀组比较差异无统计学意义(P>0.05)。与健康组比较,模型组大鼠AngⅡ、PRA、醛固酮升高(P<0.05);与模型组比较,GSPE低剂量组、GSPE高剂量组及辛伐他汀组AngⅡ、PRA、醛固酮降低(P<0.05)。健康组、模型组、GSPE低剂量组、GSPE高剂量组及辛伐他汀组的心肌细胞凋亡率分别为(5.11±0.33)%、(46.22±3.97)%、(28.46±3.77)%、(15.42±2.33)%及(16.34±2.57)%,各组比较差异有统计学意义(P<0.05)。与健康组比较,模型组大鼠心肌组织中AQP2、Caspase-3蛋白水平升高,Bcl-2蛋白水平降低(P<0.05);与模型组比较,GSPE低剂量组、GSPE高剂量组、辛代他汀组大鼠心肌组织中AQP2、Caspase-3蛋白水平降低,Bcl-2蛋白水平升高(P<0.05)。结论:GSPE对心肌梗死有保护作用,可改善心功能水平,减少心肌细胞凋亡,其作用机制可能与调控AQP2蛋白表达有关。

2型糖尿病阴虚证与尿AQP2、AQP7表达的相关性研究

目的观察2型糖尿病阴虚证临床特征,明确患者尿中水通道蛋白-2(aquaporin-2,AQP2)、水通道蛋白-7(aquaporin-7,AQP7)表达特点及相关因素对其的影响,以利于进一步探索2型糖尿病阴虚证病证结合证候特点。方法制定2型糖尿病临床观察表、2型糖尿病阴虚证辨证标准量表以及中医证候诊断标准量表,将2021年3月—2021年12月北京中医药大学东直门医院肾病内分泌科住院部34例2型糖尿病患者分为阴虚证组(观察组)和阳虚证组(对照组)。采集两组患者血生化标本及清晨第一次全部尿液并采用酶联免疫吸附法(enzyme linked immunosorbent assay,ELISA)检测尿AQP2、AQP7的表达水平。对病例的性别、年龄、病程等多因素进行校正,分析两组尿AQP2、AQP7的差异。结果经校正后,2型糖尿病阴虚证患者尿AQP2水平明显低于阳虚证患者,MD(95%CI)为-64.23(-93.59,-34.87)(P<0.01),而尿AQP7水平低于阳虚证患者,MD(95%CI)为-3.98(-9.77,1.80)(P>0.05)。结论该研究所纳入2型糖尿病阴虚证患者尿AQP2指标表达低于阳虚证患者,提示AQP2可能是2型糖尿病阴虚证特异性生物标志物。

基于AVP-V2R-AQP2通路探讨益气活血方干预慢性心力衰竭水潴留的实验研究

[目的]观察益气活血方对慢性心力衰竭(CHF)大鼠心脏及肾脏结构的影响,并从水的重吸收角度开展机制研究。[方法]对Sprague-Dawley(SD)大鼠进行麻醉处理后,通过左侧冠状动脉前降支结扎方法建立CHF模型。造模4周后,对大鼠进行分组,随机分为假手术组、模型组、卡托普利组及益气活血方低、中、高剂量组。卡托普利组给予卡托普利片13.5 mg/(kg·d),益气活血方各剂量组分别给予益气活血颗粒剂2.5、5、10 g/(kg·d),假手术组及模型组给予等量蒸馏水灌胃,持续灌胃8周。干预结束后采用小动物彩色多普勒超声分析大鼠心脏结构及功能;采集血清检测氨基末端脑利钠肽前体(NT-proBNP)表达水平;采用苏木精-伊红(HE)染色观察大鼠的心肌纤维化水平及肾脏上皮细胞形态;染色后对大鼠肾小管上皮细胞进行分析;通过免疫组织化学方法分析大鼠肾脏水通道蛋白2(AQP2)、pS256-AQP2分布和表达水平;通过酶联免疫吸附(ELISA)法检测血清精氨酸加压素(AVP)水平;通过蛋白免疫印迹(Western Blot)法检测肾脏AQP2、pS256-AQP2、抗利尿激素V2型受体(V2R)表达水平。[结果]与假手术组比较,模型组大鼠射血分数(EF)降低(P<0.01),血清NT-proBNP水平上升(P<0.01);模型组大鼠的心肌形态不规则,出现明显的炎性浸润,肾小管管腔狭窄,模型组AQP2、pS256-AQP2阳性面积高于假手术组,AQP2、AVP、V2R表达上升(P<0.01)。益气活血方各剂量组大鼠EF高于模型组(P<0.01),血清NT-proBNP水平较模型组降低(P<0.01);心肌组织基本保持规则,对应的坏死和凋亡不明显;各给药组大鼠肾小管未见明显异常,肾细胞轻微水肿。卡托普利组、益气活血方中、高剂量组中AQP2、pS256-AQP2阳性表达面积降低(P<0.01或P<0.05),各给药组均能不同程度下调AQP2、pS256-AQP2、AVP、V2R蛋白表达水平。[结论]益气活血方能够通过改善肾脏调节机制,进而调控肾脏对水的重吸收效应,改善心脏结构及功能,延缓CHF进程,其机制可能与调节AVP-V2R-AQP2信号通路的相关因子表达相关。

血清及尿β_(2)微球蛋白、视黄醇结合蛋白、水通道蛋白-2与肾盂输尿管连接部梗阻致小儿肾积水严重程度的关系研究

目的探讨血清及尿β_(2)微球蛋白(β_(2)-MG)、视黄醇结合蛋白(RBP)、水通道蛋白-2(AQP2)与肾盂输尿管连接部梗阻(UPJO)致小儿肾积水严重程度的关系。方法选取南宁市第六人民医院泌尿外科接受肾盂输尿管梗阻手术治疗的60例肾积水患儿为肾积水组,根据肾积水严重程度分为轻度组(n=13)、中度组(n=22)和重度组(n=25),另外选取同期该院接受体检的60例健康儿童为对照组。比较对照组和肾积水组不同严重程度患儿血清及尿β_(2)-MG、RBP、AQP2水平;分析β_(2)-MG、RBP、AQP2水平与超声参数[肾盂前后径(APD)、肾实质厚度(PT)]的相关性;采用受试者工作特征(ROC)曲线分析血清及尿β_(2)-MG、RBP、AQP2对中重度肾积水的诊断效能。结果肾积水组血清及尿β_(2)-MG、RBP水平均高于对照组,血清及尿AQP2水平均低于对照组,差异有统计学意义(P<0.05)。肾积水患儿血清β_(2)-MG、尿β_(2)-MG、尿RBP水平和APD水平由低到高为轻度组、中度组、重度组,尿AQP2水平和PT由高到低为轻度组、中度组、重度组,差异均有统计学意义(P<0.05)。轻度组血清RBP水平低于中度组和重度组,差异有统计学意义(P<0.05)。肾积水患儿血清β_(2)-MG、尿β_(2)-MG、尿RBP水平与APD均呈正相关,与PT均呈负相关(P<0.05);尿AQP2水平与APD呈负相关,与PT呈正相关(P<0.05)。ROC曲线分析结果显示,血清β_(2)-MG、尿β_(2)-MG、尿RBP、尿AQP2检测对中重度肾积水均具有一定诊断价值,曲线下面积(AUC)分别为0.652、0.688、0.859、0.680,尿RBP诊断中重度肾积水的AUC显著大于其余指标(P<0.05)。结论血清β_(2)-MG、尿β_(2)-MG、尿RBP、尿AQP2与UPJO致小儿肾积水严重程度相关,尿RBP对中重度肾积水的诊断效能优于其他指标。

大黄对大鼠肾脏水通道蛋白2、4表达的影响

目的探讨大黄对大鼠肾脏水通道蛋白2、4(AQP2、AQP4)表达的影响。方法32只SD大鼠随机分为正常对照组,大黄低、中、高剂量组,分别给予生理盐水不同剂量的大黄提取物(大黄总蒽醌)灌胃,测定大鼠6 h及24 h尿量,运用免疫组化、Western blot和RT-PCR法检测肾脏AQP2、AQP4蛋白及mRNA表达变化。结果与正常对照组比较,大黄高、中剂量组大鼠尿量明显增加,肾脏AQP2、AQP4蛋白表达及mR- NA表达明显下降,差异有统计学意义(均P<0.01);与正常对照组比较,大黄低剂量组大鼠尿量及肾脏AQP2、AQP4蛋白及mRNA表达变化不明显,差异无统计学意义。结论大黄能抑制大鼠肾脏AQP2、AQP4蛋白及mRNA表达水平,这可能是其利尿功效的机制之一。

大黄素对LoVo细胞水通道蛋白2表达的调节效应

目的探讨大黄素对体外培养LoVo细胞水通道蛋白2(aquaporin 2,AQP2)表达的调节效应。方法体外培养LoVo细胞并予不同质量浓度大黄素含药培养液24 h处理及大黄素含药培养液(20 mg/L)不同时间处理,采用免疫细胞化学方法观察LoVo细胞AQP2蛋白表达位置并初步观察AQP2蛋白表达的变化趋势,采用Western blotting及半定量RT-PCR检测AQP2蛋白及mRNA的表达。结果AQP2表达于LoVo细胞的细胞膜,且与大黄素用药浓度及用药时间存在着相关性。进一步的Western blotting证实,不同质量浓度大黄素含药培养液均可抑制AQP2蛋白的表达,药物质量浓度愈大,AQP2蛋白的表达愈低,其中大黄素20 mg/L组及40 mg/L组AQP2蛋白表达显著性降低;大黄素作用3、6 h组,AQP2蛋白表达上升,但与对照组比较,无显著差异;作用12、24、48 h组,AQP2蛋白表达呈进行性下降趋势。半定量RT-PCR结果显示,随着大黄素质量浓度的增加,AQP2 mRNA表达呈进行性下降趋势;在时间-效应方面,随着用药时间的延长,AQP2 mRNA表达呈进行性下降趋势。结论大黄素可抑制LoVo细胞AQP2基因转录与翻译,这提示大黄素对AQP2表达的调节效应可能与大黄的泻下作用有关。

大黄总蒽醌对大鼠远端结肠AQP2表达的调节效应

目的:探讨大黄总蒽醌对大鼠远端结肠水通道蛋白2(aquaporin2,AQP2)表达的调节作用。方法:32只SD大鼠随机分为正常组,大黄总蒽醌低、中、高剂量组(0.14,2.5,4.5 g·kg^(-1)·d^(-1),灌胃),正常组给予生理盐水灌胃。大鼠5 d后麻醉处死,取全段结肠内粪便,干燥后检测粪便含水量;留取远端结肠,运用免疫组织化学、Western Not及RT-PCR检测远端结肠AQP2表达的变化。结果:低剂量组大鼠没有出现泻下现象,其远端结肠AQP2表达无显著差异;中剂量组(2.5 g·kg^(-1)·d^(-1))大鼠出现软便及稀便,高剂量组(4.5 g·kg^(-1)·d^(-1))大鼠出现稀便和水样便,粪便含水量显著性增加,其远端结肠AQP2表达亦显著降低(P<0.01)。结论:大黄总蒽醌能抑制大鼠远端结肠AQP2的转录与翻译、增加粪便的含水量,这可能是其泻下效应产生的机制之一。

加减猪苓汤治疗糖尿病肾病Ⅳ期的临床观察及对尿AQP2的影响

目的探讨加减猪苓汤治疗糖尿病肾病(diabetic kidney disease,DKD)Ⅳ期的临床疗效及对尿水通道蛋白2(Aquaporin2,AQP2)的影响。方法临床采用辨证属阴虚水肿型DKDⅣ期样本50例,随机分为治疗组25例和对照组25例,所有病例均进行常规降糖药控制血糖、低盐、优质低蛋白、低脂饮食、控制血压和运动指导等一般治疗。对照组口服厄贝沙坦片150 mg/d,治疗组在上述治疗基础上,加用加减猪苓汤,6周后比较治疗前后两组24尿蛋白定量、肝肾功能、糖化血红蛋白、血糖、中医症候积分情况等,同时分别在第1、3、6周末检测两组尿AQP2表达。结果治疗6周后,两组中医症候积分、24 h尿蛋白定量、血浆白蛋白、血肌酐及均较治疗前有所改善,差异有统计学意义(P<0.05),且治疗组优于对照组(P<0.05),治疗组尿AQP2在第3周及第6周均表达高于第1周(P<0.05),且高于对照组(P<0.05)。结论猪苓汤猪苓汤治疗DKDⅣ期的患者可减少尿蛋白、改善肾功能及减少中医症候积分,同时提高尿中AQP2表达,延缓DKD的进展。

轻度肾积水儿童肾脏水通道蛋白2、3和4的表达

目的探讨水通道蛋白2、3、4（AQP2～4）在儿童轻度积水肾脏（HnK）的表达。方法收集6例来自肾母细胞瘤周围的正常肾脏组织标本为对照组（男2例,女4例;平均60.33个月）,12例轻度肾积水患儿（男5例,女7例;平均14.58个月）的HnK标本为积水组（B超示集合系统分离均〈3.5cm,肾实质轻度变薄）。采用免疫组织化学法检测AQP2～4在正常肾脏和HnK中的定位及其表达情况。结果正常肾脏AQP2阳性着色主要分布于肾脏集合管上皮细胞胞膜和胞质,AQP3阳性着色主要分布于肾脏集合管主细胞的基底侧,AQP4阳性着色主要分布于肾内髓集合管上皮细胞基底侧。HnK中AQP2～4的表达阳性率均明显低于对照组（Pa〈0.05）。结论AQP2～4在儿童HnK组织中表达明显降低,提示AQP2～4的表达降低可能是引起HnK形态功能改变的早期因素之一。

糖尿病大鼠肾脏水通道蛋白-2mRNA的表达及黄芪的调节作用

目的观察黄芪注射液(astragalus membranaceus,AM)对链脲佐菌素(streptozotocin,STZ)诱导糖尿病(diabetes mellitus,DM)大鼠肾脏髓质水通道蛋白-2(aquaporin-2,AQP-2)基因表达的影响,以探讨黄芪治疗糖尿病的分子生物学机制。方法实验大鼠分为4组:正常组、糖尿病模型组、AM小剂量组和AM大剂量组,后两组应用AM5、10g·kg-1·d-1腹腔注射6周,测定各组大鼠血糖、血清胰岛素及C肽水平,用代谢笼法测定各组大鼠24h尿量,RT-PCR方法测定各组大鼠肾AQP-2 mRNA的表达。结果糖尿病大鼠血糖水平明显增高,血清胰岛素及C肽水平明显下降,单用黄芪注射液治疗对血糖、血清胰岛素和C肽水平无明显影响,但黄芪治疗可使糖尿病大鼠尿量明显增加。RT-PCR检测发现糖尿病大鼠肾髓质AQP-2 mRNA的表达明显上调,黄芪治疗可使其表达下降。结论黄芪治疗糖尿病利水消肿、改善水平衡代谢紊乱的作用可能与其降低肾髓质AQP-2 mRNA的表达有关。

尿液中水孔蛋白-2的检测及其与肾组织中表达的相关性

目的：研究尿液 Ａ Ｑ Ｐ２ 水孔蛋白检测的方法及其与肾脏 Ａ Ｑ Ｐ２ 水孔蛋白表达量之间的相关性，为应用尿液 Ａ Ｑ Ｐ２ 蛋白监测机体的水重吸收状况提供理论依据。 方法：用 Ｗｅｓｔｅｒｎ 印迹分析法测定自由进水和禁水２４ｈ 大鼠肾脏 Ａ Ｑ Ｐ２ 的表达量及尿液 Ａ Ｑ Ｐ２ 的含量，并分析两者之间的相关性。 结果： Ａ Ｑ Ｐ２ 蛋白可在尿液中检测到。尿液 Ａ Ｑ Ｐ２ 与肾脏 Ａ Ｑ Ｐ２ 呈正相关（ ｒ ＝ ０７９９） 。 结论：尿液 Ａ Ｑ Ｐ２ 水平可以反映肾脏集合管 Ａ Ｑ Ｐ２ 蛋白的表达量，是较好的监测机体水重吸收状况的方法。

肾脏水通道蛋白2的短时调控机制研究进展

肾脏集合管细胞通过水通道蛋白2(aquaporin-2,AQP2)调控水的重吸收进而调控机体的水代谢平衡。AQP2主要分布于集合管主细胞的管腔侧质膜及细胞内囊泡内,精氨酸加压素(arginine vasopressin,AVP)可刺激其由囊泡转移至质膜,这种AQP2的再分布过程被称为AQP2的短时调控,也被称作囊泡穿梭机制。其过程涉及多种分子机制,包括AQP2的磷酸化、激酶锚定蛋白、磷酸二酯酶、细胞骨架、钙离子、细胞膜的锚定以及胞吞作用等。本文就AQP2囊泡穿梭机制的研究进展作一综述。

利尿剂对大鼠肾脏水通道蛋白-2基因表达和尿液水通道蛋白2的影响

目的探讨临床常用利尿剂呋塞米、双氢克尿噻及安体舒通对正常大鼠肾脏水通道蛋白-2(AQP2)基因表达及尿液水通道蛋白-2浓度的影响。方法40只健康SD大鼠随机分成4组:对照组、呋塞米组、安体舒通组、双氢克尿噻组。观测尿量、血钠及尿渗量,应用RT-PCR半定量检测肾内髓质AQP2和血管加压素-2型受体(V2-R) mRNA水平,Western blotting检测肾髓质AQP2蛋白含量,酶联免疫吸附测定法(ELISA法)检测尿液AQP2浓度。结果①与对照组比较,利尿剂组大鼠尿量均显著增多(P<0.05),尿液中AQP2浓度明显增加(P<0.05)。但呋塞米组尿渗量低于对照组(P<0.05),而双氢克尿噻组和安体舒通组尿渗量高于对照组(P<0.05)。②呋塞米组肾脏AQP2 mRNA、V2-RmRNA和AQP2蛋白表达较对照组明显增加(P<0.05),而双氢克尿噻组较对照组明显降低(P<0.05),安体舒通组有所减少但无统计学差异。结论三类利尿剂均可显著增加正常大鼠尿液AQP2蛋白的排出。但对正常大鼠肾脏水通道蛋白2基因表达的影响并不相同,双氢克尿噻可以抑制正常大鼠肾内髓质AQP2 mRNA和蛋白的表达,呋塞米能增加正常大鼠肾内髓质AQP2 mRNA和蛋白的表达。