Aquaporin-1蛋白在缺血心肌中表达变化及其与心肌水肿的关系

目的在动物心肌梗塞模型中探讨心肌缺血状态下心肌细胞膜水通道蛋白Aquaporin-1的变化趋势及其与心肌水肿的联系。方法采用抗AQP1特异性免疫组化考查AQP1在心肌组织中的分布特点;以Real-timePCR及Westernblotting了解在缺血状态下心肌组织AQP1基因转录及蛋白表达的动态变化趋势;采用Evan’blue定量测定法了解缺血心肌组织中毛细血管通透性的变化及用心肌水含量测定法了解缺血心肌的水肿程度。结果AQP1在心肌中存在着广泛分布,并主要分布于心肌的血管及心肌细胞膜。缺血造成AQP1在心肌的转录及蛋白表达呈现先减后增的趋势;缺血后心肌水肿程度存在着双峰样变化趋势而且AQP1蛋白的表达增加的时间特征上与缺血后的第二个水肿高峰的变化趋势相一致。结论AQP1蛋白在心肌缺血后存在着先减后增的动态变化,AQP1蛋白的表达增加可能与部分地联系到缺血后的心肌水肿的形成。

缺血预适应后心肌水肿与水通道Aquaporin-1蛋白表达变化的关系

目的通过对缺血预适应动物模型与单纯心肌缺血动物模型之间的对照研究,探讨预适应对心肌细胞膜水通道蛋白Aquaporin-1表达的影响及与心肌水肿的关系。方法以Real-time PCR及Western blotting了解在心肌组织AQP1基因转录及蛋白表达的动态变化趋势;采用Evan blue定量测定法了解心肌组织中微血管通透性的变化及用心肌水含量测定法了解缺血心肌的水肿程度。结果与缺血对照组相似,缺血预适应后心肌AQP1基因及其蛋白的表达呈现先减后增的趋势,但增加的程度较对照组为高。预适应后组织血管通透性增高明显受到抑制,但仅伴随着缺血后早期阶段心肌水肿的减轻。与微血管通透性的持续降低形成对比的同时,心肌水肿状态在之后一段时期内保持较高水平与AQP1蛋白表达增高在时间关系上相对应。结论预适应早期心肌水肿的减轻与血管通透性的抑制有关,而AQP1蛋白表达的增加可能是心肌水肿状态维持的因素。

Aquaporin-1在大鼠睾丸输出小管的免疫组织化学定位研究

目的 研究正常大鼠睾丸输出小管上皮细胞上Aquaporin 1(AQP 1)的定位分布以期了解其在水重吸收上的作用机制。方法 对正常Wistar大鼠睾丸输出小管进行常规免疫组织化学方法染色观察。结果 在睾丸输出小管非纤毛上皮细胞的刷状缘及基侧部AQP 1阳性表达强烈 ,核上区的胞内体的质膜上也有阳性表达 ;纤毛上皮细胞的纤毛亦呈阳性反应。结论 Aquaporin 1可能与睾丸输出小管非纤毛上皮细胞水重吸收功能有密切关系。

Aquaporin-1 mRNA在人非小细胞肺癌组织中的表达和意义

目的:探讨Aquaporin-1(AQP1)mRNA在人非小细胞肺癌组织中的表达和意义。方法:以相应患者手术切除的正常肺组织为对照,采用半定量RT-PCR技术检测人非小细胞肺癌(17例鳞癌和18例腺癌)组织中AQP1 mRNA的表达水平。结果:人肺腺癌组织中AQP1 mRNA表达水平为0.419±0.135,高于正常肺组织中的表达水平(0.250±0.124),二者之间差异有统计学意义(P<0.05);人肺鳞癌组织中AQP1 mRNA表达水平为0.341±0.099,与正常肺组织中AQP1 mRNA表达水平(0.264±0.114)之间无统计学差异(P>0.05)。结论:AQP1mRNA在人肺腺癌组织中表达增加,提示AQP1可能与人肺腺癌的发生和发展有关系。

Effect of Dexamethasone and Aquaporin-1 Antisense Oligonucleotides on the Aquaporin-1 Expression in Cultured Human Trabecular Meshwork Cells

The changes in the expression of aquaporin-1 （AQP1） mRNA and protein in cultured human trabecular meshwork （HTM） cells treated with dexamethasone and transfected with antisense oligonucleotides （AS-ODN） were studied, and the implication of AQP1 regulation in corticosteroid-glaucoma and the possibility of AS-ODN inhibiting the AQP1 expression were evaluated. The cultured HTM cells in vitro were treated with different concentrations of dexamethasone and transfected with oligonucleotides for 5 days respectively. Then, total RNA and protein of HTM cells were extracted. The changes of AQP1 mRNA and protein were demonstrated qualitatively and quantitatively by RT-PCR and Western blot. Band intensities were detected by imaging analysis. There was a parallel relationship between the results of RT-PCR and those of Western blot. The expression levels of AQP1 mRNA and protein in dexamethasone-treated groups were increased initially and decreased later as dexamethasone concentration was stepped up. In the 0.04 μg/mL and 0.4 μg/mL groups, the levels of AQP1 were higher than in control group （0 μg/mL）. In the 4 μg/ mL and 40 μg/mL groups, the AQP1 expression levels were lower than in control group. AS-ODN could down-regulate the expression of AQP1 mRNA and protein in a dose-dependent manner. At 5 μg/mL, down-regulation efficiency reached the maximum. There was no statistically significant difference in the expression of AQP1 mRNA and protein between all sense oligonucleotides groups and control group. It was suggested that dexamethasone may induce the changes of the AQP1 expression in HTM cells to be involved in the occurrence of corticosteroid-glaucoma. AS-ODN can down-regulate the AQP1 expression in HTM cells to some extent.

Aquaporin-1 down regulation associated with inhibiting cell viability and inducing apoptosis of human lens epithelial cells

AIM：To investigate the role of Aquaporin-1（AQP-1）in lens epithelial cells（LECs）and its potential target genes.AQP-1 is specifically expressed in LECs of eyes and is significant for lens homeostasis and transparency maintenance.Herein,AQP-1 expression in LECs was investigated to evaluate its influence on cell survival in association with its potential role in cataract formation.·M ETHODS：LECs were transfected with lentivirus carrying AQP-1 small interfering RNA（si RNA）.Real-time polymerase chain reaction（PCR）and Western blotting were conducted to detect AQP-1 expression in LECs from different groups.Meanwhile,cell counting kit-8（CCK-8）assay and flow cytometry were performed to measure LEC proliferation and apoptosis,respectively.·RESULTS：AQP-1 expression was significantly reduced in LECs,both at m RNA and protein levels（〈0.05）,after si RNA treatment.Decreased cell viability was detected by CCK-8 assay in LECs with si RNA interference,compared to control cells（〈0.05）.The apoptosis rate significantly increased in cells after si RNA interference（〈0.05）.·CONCLUSION：The decreased cell viability following AQP-1 down regulation is largely due to its induction of apoptosis of LECs.AQP-1 reduction might lead to changes of physiological functions in LECs,which might be associated with the occurrence and development of cataracts.

Increased aquaporin-1 levels in lens epithelial cells with primary angle-closure glaucoma

AIM： To determine the levels of aquaporin-1（AQP-1） in the lens epithelial cells（LECs） of primary glaucoma and to clarify its correlation with lens thickness.METHODS： This study comprised 64 eyes of 64 patients with primary glaucoma, who were divided into 3 groups： 25 eyes of 25 patients with acute primary angle-closure glaucoma（APACG）, 19 eyes of 19 patients with chronic primary angle-closure glaucoma（CPACG） and 20 eyes of 20 patients with primary open angle glaucoma（POAG）. This study also included 12 eyes of 12 patients with senile cataract as controls. The levels of AQP-1 in LECs were examined by real-time quantitative polymerase chain reaction（RT-q PCR） and immunohistochemistry. The lens thickness was measured by A-scan ultrasonography. RESULTS： The AQP-1 m RNA levels of LECs were 0.84±0.27, 0.69±0.34, 0.44±0.19 and 0.51±0.21 in APACG, CPACG, POAG and senile cataract group, respectively. The levels of AQP-1m RNA were significantly higher in PACG groups compared with those in senile cataract and POAG group（all P〈0.05）. The immunohistochemistry showed the AQP-1 expression were strong-positive in PACG groups, but weak-positive in senile cataract and POAG group. A positive correlation was found between AQP-1 m RNA levels and the lens thickness（r=0.645, P〈0.001）. CONCLUSION： These findings show that the higher expression of AQP-1 in LECs may contribute to increased lens thickness, which might be associated with the occurrence and development of PACG.

Regulatory Effect of Dexamethasone on Aquaporin-1 Expression in Cultured Bovine Trabecular Meshwork Cells

To evaluate the effect of dexamethasone on the expression of aquaporin-1 （AQP-1） in cultured bovine trabeeular meshwork cells, bovine trabeeular meshwork cells were cultured in vitro and reproduced to the third and the fourth generation, then treated with dexamethasone at the concentrations of 5, 25, 50, 250μg/L respectively for 7 days. Immunohistochemical technique-supervision method was employed to measure, and image analysis system to analyze the expression of AQP-1 in normal cultured bovine trahecular meshwork cells and those treated with dexamethasone. In normal bovine trabeeular meshwork cells, the grayseale of AQP-1 positive staining was 167.94± 1.18, while it was 168.92±0.91, 176.72±1.80, 180. 64±1.31, 185.64±1.58 in cells treated with 5, 25, 50, 250μg/L concentrations of dexamethasone. When the concentration of dexamethasone was higher than 25 μg/L, the expression of AQP-1 was significantly inhibited （P〈0.05）. The regulation of AQP-1 expression by dexamethasone in cultured bovine trahecular meshwork cells in vitro may be one of causes that retard the aqueous outflow in glueoeorticoid-induced glaucoma.

Lung injury and aquaporin-1mRNA expression during cardiopulmonary bypass

Objective To testify the lung injury induced by cardiopulmonary bypass(CPB) in canine model and observe the influence of CPB on the aquaporin 1 (AQP1) mRNA expression in canine lung. Methods 8 mongrel dogs were used to perform the cardiopulmonary bypass. The hearts arrested for 90 minutes with mild hypothermia and rebeated for 6 hours. The hemodynamics,the ratio of lung dry weight and wet weight,the plasmic

Aquaporin-1 Expressed in Cultured Human Trabecular Meshwork Cells

Objective:To determine if aquaporin-1 could be detected in cultures of human trabecularshwork cells. Methods: Using primers specific for aquaporin-1, reverse transcription combined withpolymerase chain reaction (RT-PCR) yielded a product and its size with total RNAprepared from the human trabecular meshwork cells. SDS-PAGE and immunoblottingwere also used in this study to detect the specific water channel.Results: The presence of this product and its size (298 base pairs) are consistent withthat of an aquaporin-1 message in these cells. A band of 28 kD in agreement with themolecular size of aquaporin-1 was showed in a film by immunoblotting.Conclusion: The presence of aquaporin-1 in human trabecular meshwork cells, thepredominant cell-type of the primary outflow region of the human eye, suggests that waterchannels may be involved in the movement of aqueous fluid out of the eye. In addition,the existence of aquaporin-1 on cultures of human trabecular meshwork cells provides anin vitro model to study the endogenous expression of aquaporin-1 and its possible role inthe regulation of aqueous outflow.

糖尿病视网膜病变患者SDF-1、HO-1及MDA水平变化及与IL-6、TNF-α、CRP的相关性

目的 分析糖尿病视网膜病变(DR)患者基质细胞衍生因子(SDF-1)、血红素加氧酶-1(HO-1)及丙二醛(MDA)水平变化及与白介素-6(IL-6)、肿瘤坏死因子(TNF-α)、C反应蛋白(CRP)的相关性。方法 选取2020年5月至2023年1月解放军总医院收治的131例DR患者为DR组,另选取同期在本院住院的2型糖尿病患者100例为非DR组。比较两组SDF-1、HO-1、MDA水平;比较两组IL-6、TNF-α、CRP水平;比较不同分期DR患者SDF-1、HO-1、MDA水平;采用Logistic回归分析影响DR发生的相关因素,分析DR组患者SDF-1、HO-1、MDA水平与IL-6、TNF-α、CRP的相关性。结果 DR组SDF-1、HO-1水平比非DR组低,MDA水平比非DR组高,差异有统计学意义(P<0.05);DR组IL-6、TNF-α、CRP水平均比非DR组高,差异有统计学意义(P<0.05);SDF-1、HO-1水平:Ⅰ~Ⅱ期>Ⅲ~Ⅳ期>Ⅴ~Ⅵ期,MDA水平:Ⅰ~Ⅱ期<Ⅲ~Ⅳ期<Ⅴ~Ⅵ期,差异有统计学意义(P<0.05);经Logistic多因素分析显示,性别为女、BMI≥24 km/m2、合并患有高血压、高血脂、IL-6>1.17 mg/mL、TNF-α>30 ng/L、CRP>10 ng/mL、SDF-1>2 ng/mL、HO-1<125 ng/mL、MDA>4.06μmol/mL均是影响DR发生的独立危险因素(P<0.05);血清炎性因子IL-6、TNF-α、CRP与SDF-1、HO-1呈负相关,与MDA呈正相关,且均为中度相关(P<0.05)。结论 SDF-1、HO-1、MDA、IL-6、CRP、TNF-α水平与DR的发生、发展有一定关系,通过检测上述指标水平可为进一步探讨DR的发病机制和治疗方法提供新的思路。

青藤碱可有效抑制白细胞介素1β介导的髓核细胞凋亡

背景:椎间盘退变是导致脊柱退行性疾病的基础,然而目前尚无有效的治疗药物。目的:探讨青藤碱是否可以抑制白细胞介素1β诱导的髓核细胞凋亡及其分子机制。方法:采用胰酶联合Ⅱ型胶原酶消化法体外培养大鼠髓核细胞,并绘制细胞生长曲线,采用CCK-8法筛选合适的青藤碱药物浓度。将髓核细胞分为对照组、青藤碱组、白细胞介素1β组、青藤碱+白细胞介素1β组、锌原卟啉(血红素氧合酶1抑制剂)组、锌原卟啉+青藤碱组、锌原卟啉+白细胞介素1β组、青藤碱+锌原卟啉+白细胞介素1β组。分别检测各组髓核细胞增殖活性、活性氧含量、凋亡率及血红素氧合酶1的表达情况。结果与结论:①体外培养的大鼠髓核细胞呈现多角形、三角形、短楔形等形态,其呈现“S”型曲线生长,接种第1-3天生长缓慢,第4-6天生长迅速,第七八天生长速度缓慢,进入“平台期”,细胞数量不再增加;②当青藤碱的浓度≤80μmol/L时,髓核细胞的增殖活性不会受到显著影响(P>0.05);③白细胞介素1β可以显著降低髓核细胞的增殖活性,增加活性氧含量,导致细胞凋亡(P<0.01);④当采用青藤碱干预后,不仅可以促进血红素氧合酶1的表达(P<0.05),而且可以抑制白细胞介素1β诱导的髓核细胞增殖活性降低、活性氧含量和凋亡率增加(P<0.05),其作用可被锌原卟啉逆转(P<0.01)。

软骨细胞中SIRT1基因敲减后作用状态不明确信号通路及对相关疾病或功能的影响

背景:沉默信息调节因子1以去乙酰化的方式调控软骨细胞中相关蛋白的功能,参与软骨细胞增殖分化,促进软骨缺损修复。目的:利用高通量技术筛选软骨细胞中沉默信息调节因子1基因敲减后作用状态不明确的信号通路以及产生变化的疾病或功能。方法:取处于对数生长期的小鼠ATDC5软骨细胞,分2组转染:对照组转染沉默信息调节因子1基因敲减阴性对照慢病毒,实验组转染沉默信息调节因子1基因敲减慢病毒。转染72 h后,利用小鼠基因表达谱芯片GeneChip®Mouse Genome 4302.0 Array检测mRNA的基因层面变化情况,应用生物信息学技术筛选激活或抑制不明确的信号通路以及这些信号通路相关因子,并分析疾病或功能模块的富集情况。结果与结论:①沉默信息调节因子1基因敲减后,小鼠ATDC5软骨细胞中激活或抑制状态不明确的信号通路有245条;②根据-log(P-value)排序选择排前20的激活或抑制状态不明确信号通路中的因子情况进行报道,包括IGFBP4、TGFBR1、CTGF、COL4A5、LHX2、IL1RL1、KLF6等;③根据-log(P-value)进行排序,细胞生长和增殖、生物体存活和细胞死亡与存活等14个疾病和功能密切相关模块明显变化;根据差异基因数量排序,生物体损伤和异常、癌症和细胞死亡与存活3个疾病和功能密切相关模块明显变化;根据-log(P-value)与差异基因数量综合排序,固有免疫应答这一疾病和功能模块被显著激活。

miR-141-3p对腰椎间盘突出症大鼠背根神经节炎症及下肢疼痛的抑制和改善作用

背景:研究表明,胰岛素样生长因子1/血小板源性生长因子有抑制纤维环细胞凋亡的作用。miR-141-3p微小RNA在骨髓基质细胞中随着年龄的增加而增加,且与炎症信号通路的活化存在一定关系,提示其可能成为腰椎间盘突出症的治疗靶点。目的:探究miR-141-3p通过调控胰岛素样生长因子1/血小板源性生长因子对腰椎间盘突出症大鼠背根神经节炎症及下肢疼痛的影响。方法:选取50只SPF级SD雄性大鼠,随机分为正常组、模型组、miR-NC组、miR-141-3p inhibitor组、miR-141-3p mimics组,每组10只。除正常组外,其余大鼠采用自体髓核移植法进行腰椎间盘突出症建模。建模成功后,对miR-NC组、miR-141-3p inhibitor组和miR-141-3p mimics组大鼠鞘内分别注射10μL 20μmol/L miR-NC,miR-141-3p inhibitor,miR-141-3p mimics,均每天注射1次,连续注射28 d;正常组、模型组同期同位置注射同体积生理盐水。采用热缩足潜伏期阈值评价大鼠下肢疼痛,实时荧光定量PCR检测背根神经节组织miR-141-3p mRNA表达,ELISA法检测背根神经节组织炎症因子,免疫印迹法检测背根神经节组织胰岛素样生长因子1/血小板源性生长因子蛋白表达,并分析miR-141-3p与胰岛素样生长因子1/血小板源性生长因子的相关性。结果与结论:miR-NC组各项指标与模型组比较,差异均无显著性意义。①大鼠热缩足潜伏期阈值:模型组明显低于正常组(P<0.05),miR-141-3p inhibitor组明显低于miR-NC组(P<0.05),miR-141-3p mimics组明显高于miR-141-3p inhibitor组(P<0.05)。②背根神经节组织miR-141-3p mRNA表达:模型组明显低于正常组(P<0.05),miR-141-3p inhibitor组明显低于miR-NC组(P<0.05),miR-141-3p mimics组明显高于miR-141-3p inhibitor组(P<0.05)。③背根神经节组织肿瘤坏死因子α、白细胞介素1β、白细胞介素1含量:模型组明显高于正常组(P<0.05),miR-141-3p inhibitor组明显高于miR-NC组(P<0.05),miR-141-3p mimics组明显低于miR-141-3p inhibitor组(P<0.05)。④背根神经节组织胰岛素样生长因子1、血小板源性生长因子蛋白表达:模型组明显低于正常组(P<0.05),miR-141-3p inhibitor组明显低于miR-NC组(P<0.05),miR-141-3p mimics组明显高于miR-141-3p inhibitor组(P<0.05)。⑤胰岛素样生长因子1与miR-141-3p呈正相关(r=0.904,P<0.001),血小板源性生长因子与miR-141-3p呈正相关(r=0.879,P<0.001)。⑥结论:miR-141-3p可显著改善腰椎间盘突出症大鼠下肢疼痛,抑制背根神经节炎症,其机制可能与促进胰岛素样生长因子1/血小板源性生长因子表达有关。

铁死亡加持PD-1/PD-L1抑制剂杀伤肿瘤细胞综述

恶性肿瘤发生发展的每一环节都与免疫调节息息相关,近年铁死亡及PD-1/PD-L1抑制剂杀伤肿瘤细胞方面的研究是一大热点,因其精准治疗肿瘤的效果被越来越多地应用于临床治疗。但目前尚无将PD-1/PD-L1抑制剂与铁死亡治疗肿瘤细胞结合的研究,本文将对铁死亡的相关机制、铁死亡与肿瘤的关系和PD-1/PD-L1免疫治疗肿瘤等方面进行综述。

疏调气机法联合桂枝茯苓胶囊治疗子宫肌瘤的疗效及其对血清TGF-β_(1)、TSGF的影响

目的:探究疏调气机法联合桂枝茯苓胶囊治疗子宫肌瘤的疗效及其对血清转化生长因子β_(1)(transforming growth factor-β_(1),TGF-β_(1))、肿瘤特异性生长因子(tumor specific growth factor,TSGF)的影响。方法:将135例子宫肌瘤患者采用随机数字表法分为对照A组、对照B组和联合组,每组45例。3组均给予常规西药治疗,在此基础上,对照A组采用疏调气机法治疗,对照B组采用桂枝茯苓胶囊治疗,联合组采用疏调气机法联合桂枝茯苓胶囊治疗。比较3组疗效、不良反应发生率及治疗前后子宫肌瘤体积、子宫体积、子宫内膜厚度、中医证候积分、血清雌激素指标[雌二醇(estradiol,E_(2))、黄体生成素(luteinizing hormone,LH)、催乳素(prolactin,PRL)]、氧化应激指标[晚期氧化蛋白产物(advanced oxidation protein products,AOPP)、丙二醛(malonaldehyde,MDA)、超氧化物歧化酶(superoxide dismutase,SOD)]、TGF-β_(1)、TSGF水平。结果:联合组总有效率为97.78%(44/45),高于对照A组的84.44%(38/45)、对照B组的80.00%(36/45)(P<0.05);治疗后3组患者子宫肌瘤体积、子宫体积均小于治疗前,联合组小于对照A组、对照B组;子宫内膜厚度大于治疗前,联合组大于对照A组、对照B组(P<0.05);与本组治疗前比较,治疗后3组患者月经异常、下腹胀痛、面色晦暗积分均降低,联合组低于对照A组、对照B组(P<0.05);治疗后3组患者血清PRL、LH、E_(2)水平均低于治疗前,联合组低于对照A组、对照B组(P<0.05);治疗后3组患者血清SOD水平均高于治疗前,且联合组高于对照A组、对照B组,血清AOPP、MDA水平均低于治疗前,联合组低于对照A组、对照B组(P<0.05);与本组治疗前比较,治疗后3组患者血清TGF-β_(1)、TSGF水平均降低,联合组低于对照A组、对照B组(P<0.05);联合组不良反应发生率为13.33%(6/45),与对照A组的6.67%(3/45)、对照B组的8.89%(4/45)比较,差异无统计学意义(P>0.05)。结论:疏调气机法联合桂枝茯苓胶囊能提高子宫肌瘤临床疗效,下调血清TGF-β_(1)、TSGF水平,且具有一定安全性。

OGDHL、FHL1在非小细胞肺癌组织中的表达及其临床意义

目的分析OGDHL、4个半LIM结构域蛋白1(FHL1)在非小细胞肺癌组织中的表达水平及其临床意义。方法选取80例非小细胞肺癌患者癌组织标本、癌旁组织标本(距肿瘤边缘4cm处),采用免疫组织化学染色法检测所有标本组织中OGDHL、FHL1表达水平。采用χ^(2)检验分析OGDHL、FHL1表达与患者病理特征的关系,采用Kaplan-Meier生存曲线分析OGDHL、FHL1表达与患者预后的关系,多因素Cox回归模型分析非小细胞肺癌患者预后的影响因素。结果非小细胞肺癌患者癌组织OGDHL高表达率明显低于癌旁组织(35.00%vs 62.50%,P<0.05),FHL1高表达率明显高于癌旁组织(67.50%vs 40.00%,P<0.05)。OGDHL、FHL1表达水平与非小细胞肺癌患者TNM分期、淋巴结转移、分化程度密切相关(P<0.05)。OGDHL高表达患者术后5年总生存率为82.14%,低表达患者术后5年总生存率为36.54%,两者比较差异有统计学意义(P<0.05);FHL1高表达患者术后5年总生存率为40.74%,低表达患者术后5年总生存率为76.92%,两者比较差异有统计学意义(P<0.05)。单因素分析得出,TNM分期、淋巴结转移、分化程度、OGDHL表达、FHL1表达均与非小细胞肺癌患者预后密切相关(P<0.05)。TNMⅢ期、淋巴结转移、低分化、OGDHL低表达、FHL1高表达均为影响非小细胞肺癌患者预后的独立危险因素(P<0.05)。结论非小细胞肺癌患者癌组织中OGDHL蛋白呈低表达,FHL1蛋白呈高表达,两者表达水平与非小细胞肺癌患者的临床病理特征及预后密切相关,能够作为评估患者预后的有效指标。

姜黄素调控转录因子FOXP3影响HIV-1感染辅助受体CCR5的作用机制研究

目的:探讨姜黄素通过调控转录因子FOXP3影响HIV-1感染辅助受体CCR5的作用机制。方法:利用生物信息学方法预测并分析转录因子FOXP3与CCR5启动子的结合位点;采用AutoDock 4.2软件对姜黄素与FOXP3进行柔性对接;MTT法检测姜黄素对Jurkat细胞活性的影响;qRT-PCR和Western blot检测不同浓度姜黄素作用于Jurkat细胞后CCR5和FOXP3 mRNA和蛋白表达水平;构建pcDNA3.1-FOXP3真核表达载体;结合转录因子预测结果,运用Overlap PCR法扩增突变型CCR5基因片段,构建突变型CCR5启动子报告载体pFireRluc-Mt-CCR5;利用双荧光素酶报告基因技术验证转录因子FOXP3与CCR5的启动子结合位点。结果:JASPAR转录因子预测结果显示,CCR5启动子区与转录因子FOXP3存在结合位点;分子对接结果显示,姜黄素能够与FOXP3的酶活区域结合;MTT结果显示,姜黄素作用24 h后对Jurkat细胞活性产生抑制作用,IC50为34.48μmol/L;qRT-PCR和Western bot结果显示,不同浓度姜黄素作用于Jurkat细胞后,CCR5和FOXP3 mRNA和蛋白表达水平均降低,且存在剂量依赖性;双荧光素酶报告基因技术证实FOXP3能够与CCR5启动子结合,且转录因子FOXP3可调控CCR5启动子活性;过表达FOXP3后,姜黄素对CCR5的作用结果显示:当姜黄素浓度为60μmol/L时,作用于共转染pcDNA3.1-FOXP3和pFireRluc-Wt-CCR5的HEK293T细胞CCR5启动子荧光素酶活性相对值明显高于pFireRluc-Wt-CCR5+curcumin-60组(P<0.01)。结论:FOXP3能够调控CCR5启动子活性,其作用机制可能是姜黄素通过作用于FOXP3与CCR5启动子结合位点影响CCR5启动子活性。

岛叶通过GluA1受体和腺苷酸环化酶1参与调控大鼠头痛及相关焦虑行为

目的:通过大鼠模型明确岛叶是否参与偏头痛发病并探索其机制。方法:连续硬膜外注射炎症汤建立慢性偏头痛(chronic migraine,CM)大鼠模型。von Frey纤维丝评估眶周机械阈值。通过旷场和高架十字迷宫实验观察动物焦虑行为。使用免疫印迹实验检测岛叶α-氨基-3-羟基-5-甲基-4-异恶唑丙酸(α-amino-3-hydroxy-5-methyl-4-isoxazolepropionic acid,AMPA)受体亚基1-Glu A1受体及腺苷酸环化酶1(adenylate cyclase 1,AC1)的表达。通过双侧岛叶注射AC1抑制剂探索可能的机制。结果:连续炎症汤刺激硬脑膜可诱导大鼠产生偏头痛样头痛及焦虑行为。与对照组相比,CM组岛叶的c-Fos、Glu A1及其磷酸化(p-Glu A1-S845)和AC1的表达显著增加。岛叶注射AC1抑制剂可缓解大鼠的痛觉过敏和焦虑行为,降低岛叶AC1和Glu A1表达量及p-Glu A1-S845水平。结论:岛叶可能通过Glu A1及AC1参与调控大鼠偏头痛样头痛及焦虑行为。

GLP-1受体激动剂对心血管作用的研究进展

胰高血糖素样肽-1(glucagon-like peptide-1,GLP-1)由肠道内分泌细胞产生。GLP-1受体激动剂(GLP-1 receptor agonists,GLP-1RAs)促进葡萄糖相关的胰岛素分泌和抑制胰高血糖素分泌。GLP-1RAs还能抑制胃排空、食物摄入和限制体质量增加。在过去的十年中,GLP-1RAs对心血管系统影响的研究已经取得重大进展。口服小分子GLP-1RAs具有潜在优势,可以提高该类药物的应用。该文综述了GLP-1RAs在心血管疾病治疗中的多种作用,为GLP-1RAs的心血管获益提供新见解。