类固醇受体辅助活化因子-1和核受体辅阻遏子在子宫腺肌病中的表达

目的:通过检测子宫腺肌病组织芯片中雌激素受体(ER)、孕激素受体(PR)、类固醇受体辅助活化因子-1(SRC-1)和核受体辅阻遏子(NCoR)的表达,观察SRC-1、NCoR与ER、PR之间的关系,探讨其在子宫腺肌病发生、发展中的作用。方法:用组织芯片技术和免疫组化方法检测42例子宫腺肌病患者异位子宫内膜组织(异位内膜组)和15例因子宫肌瘤行子宫切除术患者非瘤区对照子宫内膜组织(对照内膜组)中ER、PR、SRC-1和NCoR的阳性细胞的平均光密度值(IOD),及两组子宫内膜组织的增殖期和分泌期的IOD值,并进行比较。结果:ER、PR在异位内膜组中的IOD值显著低于对照内膜组(P<0.05);SRC-1在异位内膜组中IOD值明显高于对照内膜组(P<0.05);NCoR在异位内膜组中IOD值明显低于对照内膜组(P<0.05);异位内膜组中SRC-1、NCoR、ER和PR的IOD值增殖期和分泌期的比较,差异无统计学意义(P>0.05);对照内膜组中SRC-1、NCoR、ER和PR的IOD值增殖期高于分泌期(P<0.05)。结论:低表达的ER存在时,SRC-1在异位内膜组织中表达增高,低表达的PR可能降低NCoR的表达,SRC和NCoR可能导致子宫腺肌病异位内膜组织增生活性增高,可能与子宫腺肌病的种植和侵袭有关。

miR-762通过靶向调控NCOR1表达对人舌鳞状细胞癌细胞增殖和凋亡的影响

目的:探讨miR-762与核受体辅助抑制因子1(NCOR1)的靶向关系及其对人舌鳞状细胞癌(TSCC)细胞增殖和凋亡的影响,为TSCC临床诊断和治疗提供新的分子标志物和靶点。方法:采用实时荧光定量PCR(RT-qPCR)法检测48例TSCC患者癌组织及其癌旁正常组织中miR-762和NCOR1 mRNA表达水平,并通过Pearson相关分析法分析两者表达的相关性。采用RT-qPCR法和Westernblotting法检测人正常舌上皮细胞Hacat及人TSCC细胞(Tca-8113、CAL-27、SCC-15和SCC-9)中miR-762和NCOR1 mRNA及蛋白表达水平。将miR-762 inhibitor或si-NCOR1分别或同时转染至CAL-27细胞中,实验分为空白对照组、inhibitor-NC组、miR-762 inhibitor组、si-NC组、si-NCOR1组和miR-762 inhibitor+si-NCOR1组,采用RT-qPCR法检测CAL-27细胞中miR-762和NCOR1 mRNA表达水平,MTT法检测各组细胞增殖活性,EdU法检测各组EdU染色阳性细胞率,流式细胞术检测各组细胞凋亡率,Westernblotting法检测各组细胞中NCOR1、活化半胱氨酸天冬氨酸蛋白酶3(cleaved-Caspase-3)、B细胞淋巴瘤2(Bcl-2)和Bcl-2相关X蛋白(Bax)表达水平,荧光素酶报告实验验证miR-762与NCOR1的靶向调控关系。结果:与癌旁正常组织和正常上皮细胞Hacat比较,TSCC组织和TSCC细胞中miR-762表达水平明显升高(P<0.01),而NCOR1 mRNA表达水平明显降低(P<0.01),且在TSCC组织中miR-762与NCOR1 mRNA表达水平呈负相关关系(r=-0.711,P=0.003)。荧光素酶报告实验证实NCOR1是miR-762的靶基因。与空白对照组和inhibitor-NC组比较,miR-762 inhibitor组细胞增殖活性、EdU阳性细胞率和细胞中Bcl-2蛋白表达水平明显降低(P<0.01),细胞凋亡率和细胞中cleaved-Caspase-3及Bax蛋白表达水平明显升高(P<0.01);与miR-762 inhibitor组比较,miR-762 inhibitor+si-NCOR1组细胞增殖活性、EdU阳性细胞率和细胞中Bcl-2蛋白表达水平明显升高(P<0.01),细胞凋亡率和细胞中cleaved-Caspase-3及Bax蛋白表达水平明显降低(P<0.01)。结论:抑制miR-762表达能通过靶向上调NCOR1表达抑制TSCC细胞的增殖,并促进细胞凋亡。

大豆苷原对成骨细胞MC3T3-E1甾体激素受体辅激活因子1表达的调节作用及其机制

目的:研究大豆苷原对成骨细胞MC3T3-E1甾体激素受体辅激活因子1(steroid receptorcoactivator-1,SRC-1)和核受体辅抑制因子(nuclear receptor corepressor,NcoR)表达的调节作用及其机制。方法:体外培养MC3T3-E1细胞于含2%胎牛血清(fetal bovine serum,FBS)的α最低必须培养基(α-minimal essential medium,α-MEM)中,给予不同浓度大豆苷原或10^(-8)mol/L的雌二醇作用3 d后收获细胞,采用蛋白质印迹法观察SRC-1和NcoR蛋白的表达水平。分别应用雌激素受体(estrogen receptor,ER)拮抗剂ICI182780(Faslodex,ICI,10^(-7) mol/L)和雌激素受体α(estrogen receptorα,ERα)特异性拮抗剂(methyl-piperidino-pyrazole,MPP,10^(-6) mol/L)干预,观察大豆苷原对细胞SRC-1和NcoR蛋白表达水平的影响。结果:大豆苷原可上调MC3T3-E1细胞SRC-1的表达,10^(-7)mol/L和10^(-5)mol/L大豆苷原组SRC-1的蛋白水平分别增加至对照组的2.5倍(P<0.05)和2倍(P<0.05)。各剂量组NcoR表达水平与对照组比较差异无统计学意义。雌二醇组SRC-1水平与对照组比较未见明显变化,而其NcoR表达水平较对照组下调35%(P<0.05)。ICI182780可拮抗大豆苷原对SRC-1的上调作用。在ICI182780作用下,各剂量组SRC-1蛋白水平与对照组比较差异无统计学意义;MPP干预下,10^(-7)mol/L和10^(-5) mol/L大豆苷原组SRC-1的蛋白水平分别为对照组的1.8倍(P<0.05)和2.4倍(P<0.05)。结论:大豆苷原可增加成骨细胞SRC-1的蛋白表达水平,提高细胞SRC-1/NcoR比值。ERβ参与了大豆苷原对SRC-1的调节过程。成骨细胞内SRC-1蛋白的增加和SRC-1/NcoR比值的提高是大豆苷原促进成骨细胞分化的机制之一。

宫颈癌组织中CHI3L1、NRIP1蛋白及LCoR的表达与临床病理特征、预后的相关性

目的探讨几丁质酶-3样蛋白-1(CHI3L1)、核受体相互作用蛋白1(NRIP1)、配体依赖性辅助抑制因子(LCoR)在宫颈癌组织内的表达意义及其与临床病理特征、预后的关系。方法选取72例宫颈癌患者为研究对象,于术中取其癌组织与癌旁组织(距肿瘤组织边缘≥5 cm)。采用免疫组织化学法检测两者的CHI3L1、NRIP1、LCoR表达情况,探究CHI3L1、NRIP1、LCoR阳性表达与宫颈癌患者临床病理特征以及预后的联系。结果癌组织中CHI3L1、NRIP1、LCoR阳性表达率[79.17%(57/72)、69.44%(50/72)、80.56%(58/72)]均高于癌旁组织[34.72%(25/72)、29.17%(21/72)、36.11%(26/72)],有统计学差异(P<0.05)。宫颈癌组织内CHI3L1、NRIP1、LCoR表达水平与年龄、病理类型无关(P>0.05),与国际妇产科联盟(FIGO)分期、肿瘤浸润深度、肿瘤最大直径、淋巴结转移有关(P<0.05);Kaplan-Meier结果显示:CHI3L1、NRIP1、LCoR阳性表达患者的3年生存率均低于阴性表达,有统计学差异(P<0.05)。结论宫颈癌组织内CHI3L1、NRIP1、LCoR阳性表达率处于较高水平,与患者的FIGO分期、肿瘤浸润深度等密切相关,且阳性表达患者预后更差,临床需予以积极的重视。

Nuclear corepressor 1 expression predicts response to first-line endocrine therapy for breast cancer patients on relapse

Background Estrogen receptor alpha （ER α） is the most important endocrine therapy responsiveness predictor for women with breast cancer. The accuracy of the prediction of the response to endocrine therapy was thought to be affected by involving the estrogen receptor coregulatory proteins and cross-talk between ER and other growth factor-signaling networks. Nuclear corepressor 1 （NCOR1） is one of the ER a transcription repressor. The objective of the study is to investigate the expression of NCOR1 at the protein level and pursue its predictive value for breast cancer endocrine therapy. Methods In the present study, the level of expression of NCOR1 protein has been assessed by immunohistochemistry in 104 cases of invasive carcinoma of the breast. Associations between NCOR1 protein expression and different clinicopathological factors and survival were sought. Results It was found that NCOR1 was expressed at significantly higher levels in responsive patients treated with endocrine therapy as first-line treatment on relapse. Responsive patients also had a significantly longer post-relapse survival and overall survival. No NCOR1 expression difference was found between patient by age, tumor size, lymph node status, different histological grade groups and human epidermal growth factor receptor 2 （HER2） status. Multivariate analysis showed that NCOR1 is an independent prognostic factor for over-all survival. Conclusions In breast cancer, NCOR1 protein expression level predicts response to endocrine therapy as first-line treatment for breast cancer patients on relapse and NCOR1 protein level assay may increase the accuracy in the endocrine treatment determination and, therefore, improving the patients survival.

ghrelin对海马神经干细胞糖氧剥夺性损伤的影响及机制

目的观察ghrelin对糖氧剥夺诱导海马神经干细胞损伤的影响,并探讨核受体辅阻遏子1(N-CoR1)/磷脂酰肌醇3-激酶(PI3K)通路在该影响中的作用。方法将细胞随机分为正常对照组、损伤模型组、ghrelin治疗组、GHRP组、LY294002组、siRNA空白对照组、N-CoR1 siRNA组。正常对照组在正常糖含量的培养基、正常氧含量混合气体的普通培养箱中培养24 h,其余各组细胞行糖氧剥夺处理,处理后培养条件同正常对照组。siRNA空白对照组、N-CoR1 siRNA组行糖氧剥夺处理前1 h,培养液更换为含等量转染溶剂Lipofectamine2000或N-CoR siRNA脂质体的培养液,持续转染至糖氧剥夺之后的24 h。ghrelin治疗组在糖氧剥夺处理结束后,将培养液更换为含ghrelin的培养基继续培养24 h。GHRP-6组、LY294002组在糖氧剥夺处理结束后,预先给予ghrelin受体拮抗剂D-Lys ^3-GHRP-6或PI3K抑制剂LY294002处理1 h,再同时给予ghrelin处理,继续培养24 h。收集各组细胞,采用CCK-8法检测海马神经干细胞增殖活力,Western blotting法检测N-CoR1、PI3K、增殖标志蛋白增殖细胞核抗原(PCNA)及凋亡标志蛋白Bax、Bcl-2。CCK-8实验中ghrelin治疗组ghrelin浓度分别为4、20、100 nmol/L,其余实验中ghrelin浓度均为100 nmol/L。结果与正常对照组比较,损伤模型组海马神经干细胞增殖活力降低,细胞PCNA表达减少、Bax/Bcl-2增大,N-CoR表达明显增多、PI3K表达减少(P均<0.01);与损伤模型组比较,ghrelin治疗组随ghrelin作用浓度增高细胞增殖活力增高(P均<0.01),细胞PCNA表达增多、Bax/Bcl-2减小,N-CoR表达减少、PI3K表达增多(P均<0.01);与ghrelin治疗组(100 nmol/L)比较,GHRP组、LY29400组神经干细胞增殖活力降低,PCNA表达减少、Bax/Bcl-2增大,N-CoR表达明显增多、PI3K表达减少(P均<0.01)。与siRNA空白对照组比较,N-CoR siRNA组神经干细胞增殖活力增高,N-CoR siRNA组PCNA表达增多、Bax/Bcl-2减小,N-CoR siRNA组N-CoR表达减少、PI3K表达增多(P均<0.01)。结论ghrelin可抑制糖氧剥夺诱导的海马神经干细胞损伤,其机制与调节N-CoR/PI3K信号通路有关。

Exchange of a nuclear corepressor between NF-kB and CREB mediates inhibition of phosphoenolpyruvate carboxykinase transcription by NF-kB

Background NF-KB p65 was shown to inhibit transcription of phosphoenolpyruvate carboxykinase （PEPCK）, a rate-limiting enzyme in gluconeogenesis in the liver. To understand the mechanism of action of NF-KB p65, we investigated the nuclear receptor corepressor in the regulation of PEPCK transcription. Methods Rat H411E cells, human hepatoma HepG2 cells and human embryo kidney （HEK） 293 cells were used in this study. The transcriptional activity of a rat PEPCK gene promoter （-490/＋100） was analyzed in HepG2 cells, a HepG2 super suppressor IkBa （sslkBa） stable cell line, and HEK 293 cells. The effects of p65 and sslkBa on a rat PEPCK gene promoter were observed using the PEPCK luciferase reporter system. The interaction of the cAMP-response- element-binding （CREB） protein, histone deacetylase 3 （HDAC3） and silencing mediator for retinoic and thyroid hormone receptors （SMRT） with the PEPCK gene promoter were investigated using the chromatin immunoprecipitation （CHIP） assay, p65 cotransfection and RNAi-mediated gene knockdown were used to determine the corepressor involved in the inhibition of PEPCK by NF-KB p65 and the transcriptional regulation of CREB by NF-KB p65. Results NF-KB p65 inhibited PEPCK expression and the inhibition was blocked by sslkBa. The inhibitory effect of p65 was completely blocked in a HepG2 stable cell line in which sslkBa was expressed. HDAC3 or SMRT knockdown led to a significant up-regulation of PEPCK reporter activity in the presence of p65 cotransfection. In the ChIP assay the interaction of HDAC3 and SMRT with the PEPCK gene promoter was induced by p65 activation, but the CREB signal was reduced. Transcriptional activity of CREB was inhibited by NF-kB p65 cotransfection. The inhibitory effect of NF-kB p65 was blocked by HDAC3 RNAi or SMRT RNAi. Conculsions The study showed that the inhibition of PEPCK by NF-kB p65 was dependent on HDAC3 and SMRT, which form a nuclear corepressor complex for transcriptional inhibition. The transcription factors NF-kB p65 and CREB share the same corepressor HDAC3-SMRT, and the corepressor exchange leads to inhibition of PEPCK gene transcription by NF-kB p65.

PR、ER、NCOR及SRC-1在高强度聚焦超声治疗外阴营养不良中的表达

目的探讨妇女外阴营养不良(增生型)在高强度聚焦超声(HIFU)治疗后上皮组织中孕激素受体(PR)、雌激素受体(ER)、核受体辅阻遏子(NCOR)及类固醇受体辅助活化因子-1(SRC-1)的表达及意义。方法应用免疫组织方法,检测并比较正常妇女外阴上皮组织、外阴营养不良上皮组织及外阴营养不良HIFU治疗后上皮组织中PR、ER、NCOR和SRC-1的阳性细胞平均光密度值(IOD)。结果 PR、ER、NCOR和SRC-1在外阴营养不良病变组织中的IOD值明显低于外阴正常上皮组织中的PR、ER、NCOR和SRC-1的IOD值(P<0.05);PR、ER、NCOR和SRC-1在外阴白斑病变治疗后的IOD值明显高于其在外阴白斑病变组织中的IOD值(P<0.05)。结论 PR、ER、NCOR和SRC-1在外阴营养不良病变组织中表达显著降低,这可能与外阴营养不良发病有关;HIFU治疗后,PR、ER、NCOR和SRC-1在外阴营养不良病变组织中的表达升高,可作为判断高强度聚焦超声疗效的指标。

心肌细胞来源NCoR1对小鼠心肌梗死损伤的保护作用

目的探究心肌细胞来源的核受体辅抑制因子1(NCoR1)对小鼠心肌梗死损伤发挥的作用。方法构建心肌细胞NCoR1特异性敲除小鼠并根据不同手术处理分为假手术野生型组、假手术基因敲除组、心肌梗死野生型组和心肌梗死基因敲除组,每组各50只小鼠。统计各组小鼠在心肌梗死28 d的生存率和心功能水平;通过病理染色判断梗死面积与纤维化程度;测定小鼠血清心肌酶[磷酸肌酸激酶(CK-MB)、乳酸脱氢酶(LDH)]及炎症指标[肿瘤坏死因子α(TNF-α)、白介素6(IL-6)]水平。结果与野生型小鼠相比,基因敲除组小鼠存活率更低,左心室射血分数[(30.39±5.13)%vs.(9.46±2.10)%]和左心室缩短分数[(14.62±2.69)%vs.(4.26±0.96)%]均明显下降,而左室容积[(101.50±14.07)μL vs.(197.50±22.41)μL]明显升高(均P<0.05);小动物PET/CT提示心肌梗死后野生型小鼠对^(18)F-FDG的摄取量更高[(2.74±0.06)MBq vs.(1.60±0.03)MBq],梗死程度[(36.22±0.86)%vs.(47.17±1.27)%]和纤维化程度[(32.70±0.85)%vs.(46.38±1.31)%]更低(均P<0.05);血清学指标显示敲除小鼠心肌损伤更重且炎症水平更高(均P<0.05)。结论心肌细胞中NCoR1在小鼠心肌梗死中发挥重要的保护作用。

核受体辅抑制因子1对缺血再灌注损伤小鼠的心肌保护作用

目的探讨心肌细胞来源的核受体辅抑制因子1(nuclear receptor corepressor 1, NCoR1)对心肌缺血再灌注损伤(myocardial ischemia/reperfusion injury, MI/RI)小鼠心肌的保护作用及可能机制。方法心肌细胞NCoR1基因特异性敲除小鼠44只,随机分为假手术基因敲除组和MI/RI基因敲除组各22只;具有心脏特异性aMHC-Cre标签的野生型小鼠44只,随机分为假手术野生型组和MI/RI野生型组各22只。MI/RI基因敲除组、MI/RI野生型组结扎左冠状动脉30 min后恢复灌注血流制备MI/RI模型;假手术基因敲除组、假手术野生型组仅穿线不结扎左冠状动脉。造模成功后24 h,各组分别取12只小鼠测定左室射血分数(left ventricular ejection fraction, LVEF)和左心室短轴缩短分数(left ventricular fractional shortening, LVFS),然后处死小鼠取心脏,采用TTC染色法评估心肌梗死面积百分比;各组分别取1只小鼠行MRI检查,评估小鼠心肌收缩情况和水肿程度。造模成功后3 h,各组分别取4只小鼠处死后取心脏组织,行DHE染色观察活性氧(reactive oxygen species, ROS)含量,行免疫组织化学染色观察还原型烟酰胺腺嘌呤二核苷酸磷酸(nacotinamide adenine dinucleotide phosphate, NADPH)、3-硝基酪氨酸(3-nitrotyrosine, 3-NT)阳性细胞;各组分别再取5只小鼠,采用ELISA法检测心肌组织中NADPH、3-NT水平。结果造模后24 h, LVEF、LVFS在MI/RI基因敲除组[(34.16±1.61)%、(16.08±0.87)%]、MI/RI野生型组[(40.61±1.07)%、(19.61±0.60)%]均低于假手术基因敲除组[(58.47±2.12)%、(29.59±1.64)%]、假手术野生型组[(58.23±2.13)%、(30.35±1.47)%](P<0.05),心肌梗死面积百分比在MI/RI基因敲除组[(38.71±2.63)%]大于MI/RI野生型组[(18.34±2.16)%](P<0.05),MI/RI基因敲除组LVEF、LVFS均低于MI/RI野生型组(P<0.05);MI/RI基因敲除组心肌收缩、水肿程度均较MI/RI野生型组严重。ROS含量及NADPH、3-NT水平在MI/RI基因敲除组[(1.61±0.08)%、(3.26±0.19)μg/L、(15.50±1.07)μg/L]、MI/RI野生型组[(0.58±0.03)%、(2.39±0.17)μg/L、(9.96±0.70)μg/L]均高于假手术野生型组[0、(1.12±0.09)μg/L、(3.12±0.14)μg/L]、假手术基因敲除组[0、(0.95±0.04)μg/L、(3.25±0.28)μg/L](P<0.05),MI/RI基因敲除组高于MI/RI野生型组(P<0.05),假手术野生型组与假手术基因敲除组比较差异无统计学意义(P>0.05)。结论心肌细胞来源NCoR1对MI/RI小鼠的心肌具有保护作用,其机制可能缓解MI/RI损伤诱发的氧化应激损伤。