Lonicera japonica-induced inhibition of interleukin-1 beta thermogenesis and E-type prostaglandin receptor-3 expression in the preoptic area of rabbits

BACKGROUND： It has been shown that interleukin-1β（IL-1β） can induce fever by activating vascular endothelial cells and macrophages of the supraoptic crest to generate prostaglandin E2, which binds with receptors of the thermo-sensitive hypothalamic neurons. Lonicera japonica is one of the medicinal plants used widely in Asia for its antipyretic properties. However, these mechanisms have not yet been intensively studied. OBJECTIVE： To investigate the antipyretic effect and mechanisms of Lonicera japonica on IL-1β- induced febrile New Zealand rabbits by observing expression changes of E-type prostaglandin receptor-3 （EP3） mRNA in the preoptic anterior hypothalamus （POAH）. DESIGN： A randomized controlled study. SETTING： Electrophysiological Laboratory at the Department of Pathophysiology, Medical College of Jinan University; Department of Orthopaedics, First Hospital Affiliated to Medical College of Jinan University. MATERIALS： The experiment was performed from April to December 2005, using a total of 32 New Zealand white rabbits of both sexes, weighing 1.5 2.0 kg. All the animal experiments were performed according to the internationally accepted ethical guidelines. Lonicera japonica injection was purchased from Huanghe pharmaceutical factory of Xi＇an, China. IL-1βwas purchased from Sigma, USA. METHODS： A total of 32 rabbits were divided randomly into four groups： ① Normal saline （NS） control group;② Lonicerajaponica treatment group; ③ IL-1βtreatment group; and ④Lonicerajaponica plus IL-1βtreatment group. In the first 3 groups, the rabbits were given separate intravenous （i.v.） injections of l mL NS, l mL Lonicera japonica, and 100 ng IL-l β （dissolved in 0.9% NS without pyrogen）. In the Lonicerajaponica plus IL-1βgroup each rabbit was given i.v. injections of l mL NS and, 30 minutes later, 100 ng IL-1 β. MAIN OUTCOME MEASURES： Colonic temperature of each rabbit was measured at 0, 10, 20, 30, 40, 50, 60, and 70 minutes after injection and the maximum temperature rise （ A T） and the temperature response index after l hour （TRII） was calculated. Subsequently, in situ hybridization （ISH） was done with an ISH kit, EP3 mRNA expression in the POAH of all groups was measured （number of positive cells and average gray scale value）. RESULTS： A total of 32 rabbits were included in the result analysis, without any loss, （i） A T and TRII： there was no significant difference between the Lonicera japonica group and NS group （P 〉 0.05）. The IL-1β group was significantly greater compared to NS group （P 〈 0.01）. The Lonicera japonica plus IL-1β group was significantly less than the IL-1β group （P 〈 0.05）. ② In the NS and Lonicera japonica groups, the EP3 mRNA expression was negative （no coloration） or only weakly positive （only a few brown yellow particles in the cytoplasm cells could not be identified）. The number of positive cells and the average gray scale value were not significantly different between the two groups （P 〉 0.05）. In the IL-1β group, the number of positive cells was remarkably higher and the average gray scale value was lower than the NS group （P 〈 0.0 l）. In the Lonicera japonica plus IL-1β group, the number of positive cells was significantly less than the IL-1β group （P 〈 0.05）. However, the average gray scale value was greater than the IL-1β group （P 〈 0.05）. CONCLUSION： Lonicera japonica has obvious antipyretic effects on IL-1β-induced febrile rabbits and acts by inhibiting expression of EP3 mRNA in the POAH.

Cyclooxygenase-2 expression is associated with initiation of hepatocellular carcinoma, while prostaglandin receptor-1 expression predicts survival

AIM to determine whether cyclooxygenase-2(COX-2) and prostaglandin E1 receptor(EP1) contribute to disease and whether they help predict prognosis.METHODS We retrospectively reviewed the records of 116 patients with hepatocellular carcinoma(HCC) who underwent surgery between 2008 and 2011 at our hospital. Expression of COX-2 and EP1 receptor was examined by immunohistochemistry of formalin-fixed, paraffinembedded tissues using polyclonal antibodies. Possible associations between immunohistochemical scores and survival were determined.RESULTS Factors associated with poor overall survival(OS) were alpha-fetoprotein > 400 ng/m L, tumor size ≥ 5 cm, and high EP1 receptor expression, but not high COX-2 expression. Disease-free survival was not significantly different between patients with low or high levels of COX-2 or EP1. COX-2 immunoreactivity was significantly higher in well-differentiated HCC tissues(Edmondson grade Ⅰ-Ⅱ) than in poorly differentiated tissues(Edmondson grade Ⅲ-Ⅳ)(P = 0.003). EP1 receptor immunoreactivity was significantly higher in poorly differentiated tissue than in well-differentiated tissue(P = 0.001).CONCLUSION COX-2 expression appears to be linked to early HCC events(initiation), while EP1 receptor expression may participate in tumor progression and predict survival.

Expression and localization of prostaglandin receptors and stromal factors in human cervix—Variations in pregnant and non-pregnant states

Prostaglandins (PGs) mediate cervical ripening leading to parturition. PGs are used successfully to induce cervical ripening. However, the cell type specific expression of PG receptor subtypes and various stromal factors important for cervical ripening in human cervix is not known. Our objective was to investigate the expression and localization of PG receptors EP1-4 and FP and localization of stromal factors CTGF (connective tissue growth factor), furin, calgranulin ?B, ALOX12 (arachidonate 12-lipooxy-genase) and ALOX15 in human cervical tissue from pregnant and non-pregnant women. Cervical biopsies were obtained from non-pregnant (NP), term pregnant (TP) and post-partum (PP) women. The mRNA expression was determined with real-time PCR, protein expression and localization with immunohistochemistry. Our results show that the EP2 mRNA level was higher in the PP group as compared to TP, whereas the EP4 mRNA level was lower in the TP group as compared to NP. Concomitantly stromal EP2 and epithelial EP3 immunoreactivity was higher in the TP as compared to the NP group, while the EP4 immunostaining in glands was lower in the TP as compared to the PP group. Immunostaining of endothelial CTGF, smooth muscle furin and ALOX12, were all lower in the TP group as compared to NP, for CTGF also the PP group was lower than NP. Endothelial calgranulin B immunoreactivity was higher in the PP group than the NP group. PG receptors and stromal factors exhibit differential expression in the cervix from women in non-pregnant and pregnant states, implying their involvement in the process of cervical ripening.

Aldo-keto reductase family member C3(AKR1C3)promotes hepatocellular carcinoma cell growth by producing prostaglandin F2α

Hepatocellular carcinoma(HCC)is a leading cause of death worldwide.Current therapies are effective for HCC patients with early disease,but many patients suffer recurrence after surgery and have a poor response to chemotherapy.Therefore,new therapeutic targets are needed.We analyzed gene expression profiles between HCC tissues and normal adjacent tissues from public databases and found that the expression of genes involved in lipid metabolism was significantly different.The analysis showed that AKR1C3 was upregulated in tumors,and high AKR1C3 expression was associated with a poorer prognosis in HCC patients.In vitro,assays demonstrated that the knockdown of AKR1C3 or the addition of the AKR1C3 inhibitor indomethacin suppressed the growth and colony formation of HCC cell lines.Knockdown of AKR1C3 in Huh7 cells reduced tumor growth in vivo.To explore the mechanism,we performed pathway enrichment analysis,and the results linked the expression of AKR1C3 with prostaglandin F2 alpha(PGF2a)downstream target genes.Suppression of AKR1C3 activity reduced the production of PGF2a,and supplementation with PGF2a restored the growth of indomethacin-treated Huh7 cells.Knockdown of the PGF receptor(PTGFR)and treatment with a PTGFR inhibitor significantly reduced HCC growth.We showed that indomethacin potentiated the sensitivity of Huh7 cells to sorafenib.In summary,our results indicate that AKR1C3 upregulation may promote HCC growth by promoting the production of PGF2α,and suppression of PTGFR limited HCC growth.Therefore,targeting the AKR1C3-PGF2a-PTGFR axis may be a new strategy for the treatment of HCC.

Expression of prostaglandin E_2 receptors in rat hippocampus

BACKGROUND: Prostaglandin E2 (PGE2) can directly regulate toxic injury of hippocampal neurons through participation by its receptor. Increase of excitability of hippocampal membrane and long-term synaptic elasticity are closely related to PGE2, PGD2 and PGF2A. This suggests that PGE2 may be a key molecule of neuronal signal passage and regulate the existence of neurons through its receptor. However, which isoforms of PGE2 receptor expressing in hippocampal neurons is still unclear. OBJECTIVE: To research the subtype expression of PGE2 receptor in hippocampus of rats through mRNA transcription and protein interpretation. DESIGN: Animal studies with random, control and operator and designer double-blind methods. SETTING: University of South Carolina, Animal Center. MATERIALS: Sprague-Dawley rats, aged 12 weeks, weighing 200 g, females 48 and males 48, were selected from Animal Center in South Carolina University. Tri ReagentTM kit was provided by Molecular Research Center, USA. METHODS: The experiment was carried out in Animal Center in South Carolina University from January to December 2005. The expression of the PGE2 receptors was profiled and compared in rat hippocampus using real-time RT-PCR and Western-blot techniques. MAIN OUTCOME MEASURES: Expression of PGE2 receptors in various isoforms of hippocampal neurons of rats. RESULTS: mRNAs of all four EP1-4 subtypes were detected in the hippocampus. Western-blot data showed consistently detectable bands at approximately Mr 50 000 of EP1, Mr 40 000 and Mr 52 000 of EP2, Mr 45 000, Mr 57 000 and Mr 105 000 of EP3, and Mr 46 000 of EP4. CONCLUSION: Identifying four subtypes of EPs heterogeneously expresses in the hippocampus.

转录组测序分析黄连总碱抗脑缺血的作用机制

背景:黄连清热燥湿、泻火解毒,黄连及其成分对脑缺血有显著的保护作用,基于网络药理学和转录组测序探究黄连总碱抗脑缺血的作用机制。目的:在明确黄连总碱对脑缺血大鼠保护作用的基础上,基于网络药理学和转录组测序技术探讨黄连总碱干预脑缺血的作用机制。方法:将SD大鼠随机分为假手术组、缺血再灌注组、阳性药物组和黄连总碱组,后3组采用改良线栓法制备大脑中动脉阻塞的缺血再灌注模型,假手术组不插入线栓,其余手术操作相同。通过TTC染色、Longa 5神经功能缺损评分、苏木精-伊红染色、尼氏染色评价黄连总碱对脑缺血再灌注模型大鼠的脑保护作用。对假手术组、缺血再灌注组、黄连总碱组大鼠脑组织进行转录组测序,通过差异表达基因筛选、基因本体论分析、京都基因与基因组百科全书分析以及转录组学与网络药理学关联分析,阐明黄连总碱干预脑缺血的作用特点,最后通过ELISA检测及免疫荧光染色对黄连总碱干预脑缺血的关键靶点进行验证。结果与结论:①黄连总碱可降低缺血再灌注模型大鼠Longa 5神经功能缺损评分及脑梗死面积,增加神经元、尼氏小体数目;②黄连总碱治疗后差异表达基因的基因本体论功能富集分析包括炎症反应、分裂原活化蛋白激酶级联的正调控等生物学过程;京都基因与基因组百科全书通路富集分析主要涉及白细胞介素17信号通路、神经活性配体-受体相互作用、环磷腺苷信号通路等通路;③转录组分析发现黄连总碱主要调控的基因有前列腺素内过氧化物合酶2、脑源性神经营养因子、瞬间受体电位A1等;④采用网络药理学分析发现,黄连总碱中9个成分可能通过87个成分靶点关联到过氧化物合酶2、脑源性神经营养因子及瞬间受体电位A1而发挥作用;⑤ELISA检测及免疫荧光染色结果进一步证实,黄连总碱调控脑缺血再灌注模型大鼠过氧化物合酶2、脑源性神经营养因子和瞬间受体电位A1的表达;⑥提示黄连总碱能明显改善脑缺血再灌注模型大鼠损伤,可能通过调控过氧化物合酶2、脑源性神经营养因子和瞬间受体电位A1而发挥作用。

The oral commensal Streptococcus mitis activates the aryl hydrocarbon receptor in human oral epithelial cells

Streptococcus mitis （S. mitis） is a pioneer commensal bacterial species colonizing many of the surfaces of the oral cavity in healthy individuals. Yet, not much information is available regarding its interaction with the host. We used examination of its transcriptional regulation in oral keratinocytes to elucidate some of its potential roles in the oral cavity. Transcription factor analysis of oral keratinocytes predicted S. mitis.mediated activation of aryl hydrocarbon receptor （AhR）, Activation and functionality of AhR was confirmed through nuclear translocation determined by immunofluorescence microscopy and real-time polymerase chain reaction with reverse transcription analysis of CYPIA1, the hallmark gene for AhR activation. Addition of Streptococcus mutans or Streptococcus gordonfi did not induce CYPIA1 transcription in the keratinocyte cultures. Introduction of an AhR-specific inhibitor revealed that S. mitis-mediated transcription of CXCL2 and CXCL8 was regulated by AhR. Elevated levels of pmstaglandin E2 （enzyme-linked immunosorbent assay） in supernatants from S. mitis-treated oral epithelial cells were also attenuated by inhibition of AhR activity. The observed AhR-regulated activities point to a contribution of S. mitis in the regulation of inflammatory responses and thereby to wound healing in the oral cavity. The concept that the oral commensal microbiota can induce AhR activation is important, also in view of the role that AhR has in modulation of T-cell differentiation and as an anti-inflammatory factor in macrophaees.

肺腺癌组织中前列腺素内过氧化物合酶2表达水平与表皮生长因子受体基因突变的相关性分析

目的 分析肺腺癌组织中前列腺素内过氧化物合酶2(PTGS2)表达水平与表皮生长因子受体(EGFR)基因突变的相关性。方法 选取57例肺腺癌患者为研究对象,收集肺腺癌组织及其相应癌旁组织。采用实时荧光定量PCR(RT-PCR)法检测癌组织及癌旁组织中PTGS2 mRNA表达水平;采用免疫组织化学法分析PTGS2蛋白表达;采用RT-PCR法检测癌组织及癌旁组织EGFR基因突变情况。分析肺腺癌患者临床病理参数与PTGS2 mRNA水平、EGFR基因突变情况的关系。采用Spearman秩相关分析探讨肺腺癌患者EGFR基因突变情况与PTGS2 mRNA水平的相关性。结果 57例肺腺癌患者中,5例癌旁组织EGFR基因突变型患者,其对应癌组织也均发生突变,且为同一突变类型。26例(45.61%)癌组织EGFR基因突变型患者,未发现双重突变,其中19外显子突变17例(29.82%),均为缺失突变;21外显子突变9例(15.79%),均为L858R点突变。癌组织中PTGS2mRNA表达水平、PTGS2蛋白阳性率及EGFR基因突变型比例高于癌旁组织,EGFR基因野生型比例低于癌旁组织(P<0.01)。肺腺癌患者性别、TNM分期、吸烟与PTGS2 mRNA表达水平、EGFR基因突变情况有关(P<0.05或0.01)。EGFR基因突变型PTGS2 mRNA表达水平高于EGFR基因野生型(P<0.01)。肺腺癌患者EGFR基因突变与PTGS2 mRNA表达水平呈正相关(r=0.512,P<0.01)。结论 肺腺癌患者癌组织中PTGS2mRNA表达水平及PTGS2蛋白阳性率升高,且与EGFR基因突变关系密切,二者可能共同影响疾病进程。

Differential Mechanisms of the Effect of Peroxisome Proliferator-Activated Receptor Gamma Agonists on Bleomycin-Induced Lung Fibrosis

Background and Objectives: Peroxisome proliferator-activated receptor-g (PPAR-g) is a nuclear receptor whose activation regulates inflammation and fibrosis in various organs. We aimed to investigate the effect of two PPAR-g ligands, telmisartan and rosiglitazone, on lung injury and fibrosis induced by intratracheal bleomycin (BLM). Methods: Lung injury and fibrosis was induced in female C57Bl/6 mice by intratracheal instillation of 1.0 mg/kg of BLM. Some of the animals received rosiglitazone intraperitoneally or telmisartan in drinking water. Bronchoalveolar lavage (BAL) was performed 2, 7, 14 or 21 days after BLM instillation for cell counting and measurement of mediators in the lung. In a separate series, the lungs were sampled for collagen assay and histopathological evaluation. Results: Treatment with rosiglitazone or telmisartan significantly attenuated the BLM-induced increases in lung collagen content, pathological score, and inflammatory cells in BAL fluid. Rosiglitazone significantly suppressed BLM-induced elevation of TGF-b1, MCP-1, and IL-6 levels in the lung. In contrast, telmisartan made no changes in these cytokines, whereas it mitigated the BLM-induced increase in prostaglandin F2a in the lung. Higher concentrations of rosiglitazone and telmisartan attenuated proliferation of lung fibroblasts in vitro. Conclusions: Two PPAR-g ligands, rosiglitazone and telmisartan, exert protective effects on BLM-induced lung fibrosis through the suppression of different profibrotic mediators.

PGE2抑制TDO2表达和活性调控巨噬细胞功能变化的机制

目的探究色氨酸-2,3-双加氧酶(TDO2)在胶原诱导型关节炎(CIA)小鼠中的表达以及前列腺素E2(PGE2)抑制TDO2表达和活性调控巨噬细胞功能的机制。方法Ⅱ型胶原诱导DBA/1J小鼠制备CIA模型。X射线检测CIA小鼠踝关节损伤变化;免疫组化检测小鼠踝关节、脾脏中TDO2表达;qPCR和免疫荧光检测小鼠腹腔巨噬细胞中TDO2表达变化。通过在RAW264.7细胞中分别小干扰TDO2、给予TDO2抑制剂680C91、给予不同浓度PGE2(0.1、1、10μmol/L)刺激和给予前列腺素受体4(EP4)激动剂CAY10598后,qPCR和Western blot检测TDO2表达;流式细胞术检测巨噬细胞吞噬和极化功能;比色法检测TDO2活性。结果与正常组小鼠比较,CIA小鼠踝关节软组织肿胀变大,关节滑膜、脾脏及腹腔巨噬细胞中TDO2表达增加。在RAW264.7细胞中分别小干扰TDO2、给予TDO2抑制剂680C91、给予PGE2刺激、给予EP4受体激动剂CAY10598后TDO2表达明显被抑制,巨噬细胞吞噬功能下降,M1/M2比值下降(P<0.05);比色法结果显示RAW264.7细胞中分别给予PGE2刺激以及EP4激动剂CAY10598后TDO2的活性被抑制(P<0.05)。结论巨噬细胞TDO2表达升高可能促进了CIA小鼠关节滑膜损伤,PGE2通过激活EP4受体抑制TDO2表达和活性从而调节巨噬细胞功能。

血清KYNA、EP4在老年急性心肌梗死患者中表达水平及其与心肌损伤预后的相关性

目的探讨老年急性心肌梗死(AMI)患者血清犬尿喹啉酸(KYNA)、E-前列腺素受体4(EP4)表达与心肌损伤预后的相关性。方法选取长江大学附属仙桃市第一人民医院收治的87例老年AMI患者作为试验组,同时选择80例老年健康体检者作为对照组,试验组依据预后情况分为预后良好组(75例)及预后不良组(12例)。检测血清KYNA、EP4及心肌酶指标cTnI、CK-MB、CK表达水平;血清KYNA、EP4与心肌酶指标的相关性采用Pearson相关性分析;KYNA、EP4水平与老年AMI患者预后的关系采用Kaplan-Meier生存曲线分析;老年AMI患者预后不良的影响因素采用多因素COX回归分析。结果试验组TG、LDL-C及TC高于对照组(P<0.05),试验组患者血清KYNA及心肌酶指标cTnI、CK-MB及CK的表达水平升高,EP4表达水平降低(P<0.05);相关性分析显示,血清KYNA与心肌酶指标呈正相关,EP4与心肌酶指标呈负相关;血清KYNA低表达患者3年生存率高于高表达患者,EP4高表达患者3年生存率高于低表达患者。预后不良组cTnI、CK-MB、CK及KYNA水平高于预后良好组,EP4水平低于预后良好组(P<0.05),KYNA、EP4是AMI预后不良的影响因素(P<0.05)。结论老年AMI患者血清KYNA表达水平升高,血清EP4表达水平降低,二者与患者心肌损伤的预后相关。

初步构建与评估递送柚皮素的RGD外泌体

目的:本研究旨在制备生物合成纳米载体递送柚皮素(naringenin,Ng),并研究其对乳腺癌的体外抑瘤效果。方法:使用精氨酸甘氨酸天冬氨酸前列腺素F2受体阴性调节因子绿色荧光蛋白(Arg-Gly-Asp-prostaglandin F2 receptor negative regulator-green fluorescent protein,RGD-P-G)质粒进行转染,构建分泌RGD-P-G外泌体(RGD-P-G-Exosomes,RGD-P-G-Exo)的293F细胞。通过超速离心收集293F细胞上清液中的RGD-P-G-Exo,加入Ng,并通过水浴超声促使RGD-P-G-Exo包封Ng,形成RGD-P-G-Exo@Ng。使用荧光显微镜对转染RGD-P-G的293F细胞进行鉴定。通过透射电子显微镜、纳米颗粒跟踪分析技术、蛋白质免疫印迹等方法对RGD-P-G-Exo@Ng的形貌、粒径、标志物和绿色荧光蛋白(GFP)表达情况进行表征。采用紫外分光光度法评估包封率和载药量。通过细胞摄取实验评估纳米药物被吞噬摄取的效果。通过CCK-8法检测Exo@Ng和RGD-P-G-Exo@Ng对乳腺癌MDA-MB-231细胞的杀伤能力。结果:电镜结果显示RGD-P-G-Exo@Ng呈茶托状结构,纳米颗粒追踪分析技术显示RGD-P-G-Exo@Ng粒径主要分布在147.0 nm。蛋白免疫印迹结果表明RGD-P-G-Exo@Ng表达CD9、CD63等外泌体标志物和GFP,证明RGD-P-G-Exo的构建成功。RGD-P-G-Exo@Ng纳米药物的包封率为(28.1±0.6)%,载药量为(6.0±0.1)%。在高浓度下,Exo及RGD-P-G-Exo对MDA-MB-231细胞的存活率无显著影响,具有良好的生物相容性。在细胞摄取实验中,与Exo@Ng相比,RGD-P-G-Exo@Ng具有更强的细胞摄取效果(P<0.05)。药效实验中,Exo@Ng和RGD-P-G-Exo@Ng均表现出浓度依赖性的MDA-MB-231细胞毒性,其中RGD-P-G-Exo@Ng比相同浓度的Exo@Ng具有更强的细胞杀伤能力(P<0.05)。结论:本研究初步合成了一种用于靶向递送Ng的纳米药物,为开发生物纳米靶向肿瘤药物递送系统提供了新的策略。

羊膜间充质干细胞经PGE2/EP2途径调节类风湿关节炎患者T细胞免疫

目的探讨人羊膜间充质干细胞(AMSCs)调节类风湿性关节炎(RA)患者T细胞免疫的作用与涉及PGE2/EP2途径的机制。方法含RA患者自体血浆的培养基非接触共培养AMSCs与RA患者外周血来源T细胞,实验分为T细胞组、AMSCs组、共培养组和EP2组,流式细胞术检测T细胞亚群和炎症因子,ELISA法检测PGE2和IL-6,Western blot检测PI3K、Akt及其磷酸化蛋白水平。结果AMSCs降低RA患者T细胞增殖数量和Th17细胞比例,增高Treg细胞比例和Treg/Th17比值,减少共培养上清液IL-17含量,这些效应可被40 nmol/L的EP2受体拮抗剂AH6809所阻断。与AMSC组相比,共培养组细胞培养上清液中IL-1β、IL-6和IL-8的含量明显降低,EP2受体拮抗剂组与共培养组比较无明显差异。AMSCs增加T细胞p-PI3K蛋白水平,降低p-AKT蛋白水平,EP2受体拮抗剂只逆转AMSCs对p-AKT蛋白的下调。结论AMSCs抑制RA患者T细胞增殖、上调Treg/Th17和下调IL-17分泌的作用机制涉及激活PGE2/EP2途径。

前列腺素家族中的PGB2、15-keto-PGE2、8-iso-PGF2α在非酒精性脂肪性肝病中的作用

目的探讨前列腺素家族(prostaglandins,PGs)成员对非酒精性脂肪肝(non-alcoholic fatty liver disease,NAFLD)的影响。方法以人肝癌细胞系HepG2细胞为研究对象。试验设为对照组(Ctrl)、脂肪变组(FFA)、前列腺素B2(PGB2、10μg/mL)处理组、15-酮基-前列腺素E2(15-keto-PGE2、10μg/mL)处理组、8-异前列腺素F2a(8-iso-PGF2α、10μg/mL)处理组。采用噻唑蓝(MTT)试验检测细胞活性,油红O染色检测脂质沉积,实时荧光定量PCR(qRT-PCR)检测炎性因子基因的表达情况,Western blot检测磷酸化胰岛素受体底物(p-IRS)蛋白的表达水平。另取15只SPF级雄性C57BL/6J小鼠,随机分为基础组(CD组,n=5,10%低脂饲料喂养16周)、高脂组(HFD组,n=5,60%高脂饲料喂养16周,建模NAFLD)、PGB2组(n=5,60%高脂饲料喂养16周后,每天给予尾静脉注射PGB220μg/kg,持续2周)。采用小鼠葡萄糖耐量试验(IPGTT)检测小鼠的糖耐量水平,HE染色验证小鼠肝脏脂肪变程度。结果油红O染色结果显示,PGs对NAFLD的脂质沉积没有显著影响,但PGs能够缓解NAFLD伴随产生的炎症。qRT-PCR结果显示,FFA组IL-1β水平[(2.274±0.550)倍]与对照组相比显著升高(P=0.0028),而在50μg/mL PGB2、10μg/mL 15-keto-PGE2和10μg/mL 8-iso-PGF2α的作用下,IL-1β分别降低至[(0.720±0.036)倍,P=0.0031、(0.857±0.225)倍,P=0.0064和(1.767±0.725)倍,P=0.0297]。Western blot结果显示,经过PGs处理,p-IRS蛋白的表达水平增加。CD组小鼠体重为(28.560±2.028)g,HFD组小鼠体重升高至(49.300±0.667)g,而PGB2组显著降低至(40.840±4.043)g,各组间差异有统计学意义(P=0.0017);此外,PGB2组葡萄糖耐量结果优于HFD组。HE染色结果显示,与HFD组比较,PGB2组肝脏脂肪变的程度降低。结论PGs中的PGB2、15-keto-PGE2、8-iso-PGF2α可通过缓解IL-1β介导的炎症,上调p-IRS表达,促进胰岛素信号传导,减轻胰岛素抵抗,缓解NAFLD的发生、发展。

前列腺素EP_3受体激动剂诱导发热及其机制初探

目的 :研究前列腺素EP3 受体激动剂对大鼠体温的影响并初步探讨其作用机制。方法 :观察脑室注射前列腺素EP3 受体激动剂sulprostone对大鼠体温的影响 ,并与同当量PGE2 比较 ;利用PI-PLC及CaMKⅡ特异性抑制剂初步分析PGE2 和sulprostone诱导发热的机理。结果 :脑室注射sulprostone可剂量依赖性升高大鼠体温 ,较之同当量PGE2 发热峰值更高、持续时间更长 ;同时给予PI-PLC、CaMKⅡ抑制剂可以明显抑制PGE2 和sulprostone诱导的体温升高。结论 :前列腺素E2 可能主要通过EP3 受体诱导大鼠发热 ,其胞内环节可能与PI -PLC -IP3 -Ca2 + /CaM -CaMKⅡ通路有关。

金银花对发热新西兰兔解热作用机制的研究

目的探讨金银花解热作用的中枢机制,为其在临床应用提供实验依据。方法用白细胞介素-1β(IL-1β)复制新西兰兔发热模型,在观察金银花解热作用的基础上,应用免疫组化技术检测静脉注射金银花对IL-1β作用下新西兰兔视前区-下丘脑前部(preoptic anterior hypothalamus,POAH)组织中前列腺素受体EP3(E-type prostaglandin receptorEP3)表达的影响。结果金银花静脉注射后对正常新西兰兔结肠温度没有明显影响,与生理盐水组相比,最大体温上升高度(△T)及1 h体温反应指数(TRI1)两组间无统计学意义(P>0.05);IL-1β组在静脉注射IL-1β后,结肠温度逐渐升高,△T及TRI1与生理盐水组比较,有统计学意义(P<0.01);而金银花+IL-1β组结肠温度上升峰值明显低于IL-1β组,两组△T及TRI1有显著性差异(P<0.05)。新西兰兔POAHEP3在生理状态下仅有少量表达;静脉注射IL-1β诱导实验动物发热时,EP3表达明显增强(P<0.01);而金银花能减少IL-1β引起的EP3表达(P<0.05)。结论金银花对IL-1β性发热新西兰兔的解热作用机制可能与其抑制视前区-下丘脑前部EP3的表达有关。

兰索拉唑对乙醇诱导大鼠胃黏膜损伤的保护作用及其机制

目的 研究兰索拉唑 (LP)对乙醇诱导大鼠胃黏膜损伤的保护作用 ,探讨胃泌素受体和环氧化酶 2 (COX 2 )表达在此过程中的作用。方法 大鼠ig给予LP 0 5、5、5 0mg·kg-1·d-1,或ig联合给予LP 5 0mg·kg-1·d-1和胃泌素受体拮抗剂AG 0 4 1R 3、10、30mg·kg-1·d-1,对照组ig给予羧甲基纤维素 (CMC) 2 5mg·kg-1·d-1,连续 14d。末次给药后 8h各组大鼠ig给予无水乙醇 1ml,观察胃损伤指数 (LI)及光镜下的胃黏膜病理学改变。酶免疫方法测定胃黏膜前列腺素E2 (PGE2 )水平 ,WesternBlot和免疫组化检测胃黏膜COX 2表达。评价特异性COX 2抑制剂NS 398对LP诱导的PGE2 合成及胃黏膜保护作用的影响。结果 在 0 5、5、5 0mg·kg-1LP组 ,LI分别为 (2 5 3± 0 33) %、(1 84±0 2 9) %和 (0 83± 0 12 ) % ,小于对照组 (3 6 5± 0 19) % (P<0 0 5 ) ;胃黏膜PGE2 含量分别为 (42 7± 32 ) ,(483± 12 1)和 (6 14± 82 ) pg·g-1wwt ,高于对照组 (2 6 6± 81) pg·g-1wwt(P <0 0 5 )。LP剂量依赖性地增加大鼠胃黏膜COX 2表达。然而 ,同时给予AG 0 4 1R阻断了LP诱导的胃黏膜保护作用、COX 2表达和PGE2 合成。NS 398抑制LP诱导的PGE2 合成及胃黏膜保护作用。

前列腺素F_(2α)受体与子宫腺肌病痛经的相关性研究

目的研究前列腺素F2α受体(prostaglandin F2αreceptor,PTGFR)在子宫腺肌病(adenomyosis,AM)患者子宫不同部位的表达与分布特征,探讨其与子宫腺肌病痛经的相关性。方法采用免疫组化SP法检测2013年10月-2014年6月就诊于我院的30例AM患者在位内膜组织及异位内膜组织PTGFR的表达,并和同期因子宫肌瘤行全子宫切除术且无痛经的30例患者正常子宫内膜组织作对照。通过视觉模拟评分法(visual analogue scale/score,VAS)对AM患者痛经程度进行评分,并分析其与PTGFR的相关性。结果 PTGFR在AM在位内膜、异位内膜和对照组的正常子宫内膜的阳性表达率及表达强度差异均有统计学意义(P<0.05);PTGFR在不同的月经周期表达差异无统计学意义(P>0.05);AM在位内膜组及异位内膜组痛经程度与PTGFR的表达强度之间均存在正相关,相关系数分别为0.753 6(P<0.01)和0.619 3(P<0.01)。结论 AM患者不同组织部位PTGFR的表达不同,痛经程度与在位内膜及异位内膜PTGFR的表达强度有关,PTGFR表达越强,痛经程度越严重。

Toll样受体、前列腺素受体EP2在溃疡性结肠炎组织的表达与炎症细胞因子的关系

目的探讨溃疡性结肠炎(UC)组织中Toll样受体、前列腺素受体EP2的表达变化及与组织中炎性细胞因子表达的关系。方法选取我院2016年1月至2017年1月收治的100例UC组织(UC组)、50例正常结肠黏膜组织(对照组),采用免疫组化染色检测两组标本中的Toll样受体2(TLR2)、Toll样受体4(TLR4)、前列腺素受体EP2蛋白的表达水平,采用酶联免疫吸附法(ELISA)检测两组标本中的白细胞介素-17(IL-17)、白细胞介素-10(IL-10),并分析TLR2、TLR4、前列腺素受体EP2与IL-17、IL-10的关系。结果 UC组中TLR2、TLR4、前列腺素受体EP2蛋白阳性表达率59. 00%、61. 00%、69. 00%均高于对照组的26. 00%、18. 00%、26. 00%,差异有统计学意义(P<0. 05);活动期、Ⅲ级UC组中TLR2、TLR4、前列腺素受体EP2蛋白阳性表达均显著的高于非活动期、Ⅰ级+Ⅱ级的UC患者,差异有统计学意义(P <0. 05); TLR2、TLR4、前列腺素受体EP2蛋白阳性的UC组织中的IL-17水平高于阴性表达的患者,IL-10表达水平则低于阴性表达的UC组织,差异有统计学意义(P<0. 05)。结论 Toll样受体、前列腺素受体EP2在UC组织表达上调,并且与UC病情进展及炎症反应程度加重有关。

骨碎补总黄酮对去卵巢骨质疏松模型大鼠血清中瘦素、白细胞介素6、前列腺素E_2及骨组织中β_2-肾上腺素受体的影响

目的:观察骨碎补总黄酮对去卵巢骨质疏松(OP)模型大鼠血清中瘦素(LEP)、白细胞介素6(IL-6)、前列腺素E_2(PGE_2)及骨组织中β_2-肾上腺素受体(ADRB2)的影响。方法:采用双侧卵巢切除法复制OP大鼠模型;造模12周后以双能X线法检测骨矿物质密度(BMD),确定OP模型是否复制成功;用药12周后应用酶联免疫法检测血清中LEP、IL-6和PGE_2的浓度,免疫组化法检测大鼠骨组织中ADRB2的表达。结果:造模12周后,模型组与假手术组相比,多个部位BMD显著下降(P<0.01),提示OP模型复制成功。用药12周后模型组LEP、IL-6和PGE_2较假手术组均有显著增高(P<0.05);骨碎补总黄酮组LEP和IL-6较模型组有明显降低(P<0.01),PGE_2无显著差异(P>0.05);模型组ADRB2表达与假手术组和给药组间比较有显著差异(P<0.05),假手术组和给药组间比较无显著差异(P>0.05)。结论:去卵巢OP大鼠血清LEP、IL-6、PGE_2和骨组织ADRB2表达升高;而骨碎补总黄酮能降低去卵巢OP大鼠血清中LEP、IL-6水平和骨组织ADRB2表达,抑制骨吸收,这可能是骨碎补总黄酮防治OP的作用机制之一。