球囊损伤血管内皮后血管紧张素ⅡAT_1受体mRNA的变化

目的 研究球囊损伤血管内皮后内膜增生的过程及血管紧张素ⅡAT1受体mRNA的变化。方法 建立球囊剥脱大鼠主动脉内皮模型 ,将大鼠随机分为对照组 (n =2 4)和手术组 (n =2 4) ,各组分别在内皮损伤后 3、7、14和 2 8d取主动脉组织 ,通过组织学方法及逆转录聚合酶链反应 (RT -PCR)技术检测主动脉内膜增生的过程及AT1受体mRNA的水平。结果 (1)AT1受体mRNA于术后 3d已明显增加 ,并于术后 14d达高峰 ,术后 2 8d恢复至对照组水平。 (2 )内皮损伤后 3d已有增殖的血管平滑肌细胞 (VSMC)移行至内膜层 ;损伤后 7d内膜开始增生 ;损伤后 14dVSMC的增殖及内膜的增生更加明显 ;损伤后2 8dVSMC的增殖明显减弱 ,但细胞外基质成份增加 ,内膜继续增生。结论 血管内皮损伤后内膜增生的过程中AT1受体mR NA表达增加。

Insulin-like growth factor-1 mRNA isoforms and insulinlike growth factor-1 receptor mRNA expression in chronic hepatitis C

AIM: to evaluate the expression of different insulinlike growth factor(IGF)-1 mRNA isoforms and IGF-1 receptor(IGF-1R) mRNA in hepatitis C virus(HCV)-infected livers. METHODS: Thirty-four liver biopsy specimens from chronic hepatitis C(CH-C) patients were obtained before anti-viral therapy. Inflammatory activity(grading) and advancement of fibrosis(staging) were evaluated using a modified point scale of METAVIR. The samples were analyzed using quantitative real-time PCR technique. From fragments of liver biopsies and control liver that were divided and ground in liquid nitrogen, RNA was isolated using RNeasy Fibrous Tissue Mini Kit according to the manufacturer's instruction. Expression levels of IGF-1 mRNA isoforms(IGF-1A, IGF-1B, IGF-1C, P1, and P2) and IGF-1R mRNA were determined through normalization of copy numbers in samples as related to reference genes: glyceraldehyde-3-phosphate dehydrogenase and hydroxymethylbilane synthase. Results on liver expression of the IGF-1 mRNA isoforms and IGF-1R transcript were compared to histological alterations in liver biopsies and with selected clinical data in the patients. Statistical analysis was performed using Statistica PL v. 9 software. RESULTS: The study showed differences in quantitative expression of IGF-1 mRNA variants in HCV-infected livers, as compared to the control. Higher relative expression of total IGF-1 mRNA and of IGF-1 mRNAs isoforms(P1, A, and C) in HCV-infected livers as compared to the control were detected. Within both groups, expression of the IGF-1A mRNA isoform significantly prevailed over expressions of B and C isoforms. Expression of P1 mRNA was higher than that of P2 only in CH-C. Very high positive correlations were detected between reciprocal expressions of IGF-1 mRNA isoforms P1 and P2(r = 0.876). Expression of P1 and P2 mRNA correlated with IGF-1A mRNA(r = 0.891; r = 0.821, respectively), with IGF-1B mRNA(r = 0.854; r = 0.813, respectively), and with IGF-1C mRNA(r = 0.839; r = 0.741, respectively). Expression of IGF-1A mRNA significantly correlated with isoform B and C mRNA(r = 0.956; r = 0.869, respectively), and B with C isoforms(r = 0.868)(P < 0.05 in all cases). Lower expression of IGF-1A and B transcripts was noted in the more advanced liver grading(G2) as compared to G1. Multiple negative correlations were detected between expression of various IGF-1 transcripts and clinical data(e.g., alpha fetoprotein, HCV RNA, steatosis, grading, and staging). Expression of IGF-1R mRNA manifested positive correlation with grading and HCV-RNA. CONCLUSION: Differences in quantitative expression of IGF-1 mRNA isoforms in HCV-infected livers, as compared to the control, suggest that HCV may induce alteration of IGF-1 splicing profile.

The Effect of Dehydroepiandrosterone on the Expression of AT_1 receptor and TNF-induced ICAM-1 in Vascular Smooth Muscle Cells

Objectives To further invest- igate the molecular mechanism of vasoprotective role of dehydroepiandrosterone (DHEA), we examined DHEA on AT1 receptor and ICAM-1 gene expression in vascular smooth muscle cells (VSMCs). Methods RT-PCR and Western Blot was used to determine the change of the expressions of mRNA and protein of AT1 and ICAM- 1 when given various concentration dehydroepian- drosterone. Results 1.AT1 was abundant under the basal condition. The expression of AT1 mRNA and protein decreased after stimulated by DHEA (at 10- 10mol/L , 10-8 mol/L, 10-6 mol/L) , and the effects of DHEA on AT1 protein was dose-dependent. ER inhibitor Tamoxifen and AR inhibitor Flutamide enhanced AT1 protein expression, but did not influence the mRNA expression. 2. The exp-ression of ICAM-1 gene was low under the basal condition.It increased when induced by TNF-α,but decreased when induced by DHEA (at 10-10 mol/L, 10-8 mol/L, 10-6 mol/L) , and the effects of DHEA on ICAM-1 gene expression were dose-dependent. Conclusions These findings suggest that DHEA modulates AT1 and inflammatory factor induced ICAM-1 gene expression in VSMC, but further studies are necessary in the mecha-nism of DHEA action.

转换酶抑制剂及AT_1受体拮抗剂对血管紧张素Ⅱ(AngⅡ)受体的作用

目的：本文探讨转换酶抑制剂及ＡＴ_１受体拮抗剂对血管紧张素 Ⅱ（ＡｎｇⅡ）受体的作用方法：ＳＨＲ与ＷＫＹ大鼠服用两种不同药物（ｂｅｎａｘｅｐｒｉｌ和ｌｏｓａｒｔａｎ），检测动物肾皮质ＡＴ_１ｍＲＮＡ表达情况和ＡＴ_１受体密度。原发性高血压患者服用ｂｅｎａｘｅｐｒｉｌ或ｌｏｓａｒｔａｎ后检测血小板ＡＴ_１ｍＲＮＡ的表达情况。结果：ＳＨＲ喂用ｂｅｎａｚｅｐｒｉｌ后肾脏ＡＴ_１ｍＲＮＡ和ＡＴ_１受体密度均无明显变化，而喂用ｌｏｓａｒｔａｎ后肾脏ＡＴ_１ｍＲＮＡ及ＡＴ_１受体密度则明显降低。ＳＨＲ肾ＡＴ_１受体密度在ｂｅｎａｚｅｐｒｉｌ组无明显变化，而在ｌｏｓａｒｔａｎ组明显降低。相应的高血压患者服用 ｂｅｎａｘｅｅｒｉｌ后血小板 ＡＴ_１ ｍＲＮＡ无明显变化，而 ｌｏｓａｒｔａｎ组ｂｅｎａｘｅｐｒｉｌ后血小板ＡＴ_１ｍＲＮＡ的表达明显降低。结论：ＡＴ_１ＲＡ能下调ＡｎｇⅡ受体密度而 ＡＣＥＩ则无此作用，ＡＣＥＩ和ＡＴ_１ＲＡ对肾皮质ＲＡＳ系统作用机制是不同的。测定人血小板的ＡＴ_１ｍＲＮＡ是反映ＡＴ_１受体状况的有用指标。

大鼠骨髓细胞PPARγ和Cbf α1mRNA表达的增龄变化及相关性研究

目的观察大鼠骨髓细胞中过氧化物酶体增殖物激活受体(peroxisome proliferator-activated receptor γ,PPARγ)与核结合因子α1(cote binding factoralpha l,Cbfα1)表达的增龄性变化,分析二者变化的相关性,探讨老年性骨衰退发生的可能分子机制。方法取1、3、7、12、16、18和 20月龄的SD大鼠,每组雌雄各5只,无菌获得腰椎骨髓细胞,用RT-PCR方法检测骨髓细胞中 PPARγ与Cbfα 1mRNA的表达水平;并采用SPSS11．0统计软件进行差异单因素方差分析和相关分析。结果 PPARγ mRNA的表达水平在3月龄前变化不大,7月龄时下降,约为3月龄的34％ (P<0．01),之后逐渐上调,18月龄约为7月龄的8．8倍(P<0．001);Cbfα1 mRNA表达水平在3 月龄为最高,为1月龄的3倍(P<0．001),随后逐渐下调, 18月龄为最低,约为3月龄的6％ (P<0．001)．PPARγ与Cbfα 1mRNA的表达水平从3月龄开始呈负相关(r=0．5967,P<0．01), 相关系数随月龄增加而增加,16～20月龄期间二者变化的相关性最大。结论 PPARγ mRNA在老年大鼠骨髓细胞中高表达,且与Cbfα 1mRNA的表达呈负相关,提示骨髓细胞PPARγ高表达可能参与老年性成骨细胞前体减少和骨衰退的过程。

应用RT-PCR技术检测银屑病皮损中IGF-1受体mRNA

为了了解银屑病皮损中ＩＧＦ１受体ｍＲＮＡ的表达，采用ＲＴＰＣＲ对２０例银屑病和正常人皮肤组织块进行检测，结果证实银屑病患者表皮中ＩＧＦ１受体ｍＲＮＡ表达显著高于对照（Ｐ＜００１），真皮中未有ＰＧＦ１受体ｍＲＮＡ表达。提示ＩＧＦ１受体与银屑病角质形成细胞在转录水平与其增殖、分化有关。ＩＧＦ１通过旁分泌机制作用于角质形成细胞上受体。

内皮素受体拮抗剂对肝硬变门静脉高压症大鼠门静脉压及ET-1 mRNA表达的影响

目的 :探讨内皮素受体拮抗剂在肝硬变门静脉高压症大鼠降压中的作用。方法 :32只雄性SD大鼠 ,随机分成 4组 ,每组 8只。其中模型对照组、BQ 12 3组、BQ 788组制备CCl4诱导的肝硬变模型 ,后 2组于造模成功后每d 2次分别皮下注射BQ 12 3(12 .5 μg/kg)和BQ 788(15 μg/kg) ;正常对照组 (NL) ,普通饲养 ,不做任何处理。采用生理八导仪测定门静脉压力 (PVP) ;RT PCR测定大鼠肝组织ET 1mRNA表达水平。结果 :BQ 12 3组 ,BQ 788组的PVP及肝组织ET 1mRNA表达量均较模型对照组显著降低 (P均 <0 .0 5 ) ,与正常对照组比较差异无统计学意义 ;模型对照组、BQ 12 3组、BQ 788组PVP与其ET 1mRNA的表达水平明显相关 (r分别 0 .94 4 ,0 .837和 0 .85 5 ;P均 <0 .0 5 )。结论 :应用内皮素受体拮抗剂能显著降低肝硬变门静脉高压症大鼠的PVP。

局灶性脑缺血及再灌注大鼠大脑皮质IL-1 RⅠ蛋白和mRNA的表达

①目的 探讨脑缺血白细胞介素 1Ⅰ型受体 (IL 1RⅠ )蛋白和mRNA表达及其在缺血性脑损伤中的作用。②方法 应用免疫组化和原位杂交方法 ,检测栓线法阻塞大脑中动脉制备的局灶性脑缺血及再灌注模型大鼠脑内IL 1RⅠ蛋白和mRNA的表达。③结果 正常及假手术大鼠IL 1RⅠ蛋白免疫阳性细胞主要在皮质表达 ;缺血后IL 1RⅠ蛋白免疫阳性细胞在缺血侧皮质、海马及纹状体表达明显增加 ,在皮质再灌注后 12h达高峰 ,随后逐渐降低。原位杂交结果显示 ,正常及假手术大鼠IL 1RⅠmRNA阳性细胞主要在皮质表达 ,海马区偶见阳性细胞 ;脑缺血大鼠IL 1RⅠmRNA阳性细胞在缺血再灌注后 2h表达增加 ,再灌注后 6h达高峰 ,随后逐渐降至正常水平。④结论 脑缺血后IL 1RⅠ上调竞争结合IL 1β 。

七氟醚对新生大鼠海马神经元NMDA受体1亚基和2B亚基mRNA的影响

目的观察七氟醚对新生大鼠海马组织NMDA受体1亚基和2B亚基mRNA的表达水平及大鼠在学习、记忆能力方面的影响。方法将48只出生后7 d的SD乳鼠,体质量10～15 g,雌雄不限,随机分为两组,即七氟醚吸入组(S组):吸入2.3%七氟醚4 h;对照组(D组):吸入氧气4 h,各24只。麻醉结束后,立即随机取S组8只(S1组)、D组8只(D1组)断头取脑,分离海马组织,进行实时荧光定量PCR检测NMDA受体l亚基和2B亚基mRNA的表达情况。剩余的S组和D组乳鼠各16只,在空气条件下饲养7 d后,随机各取8只分为S2组和D2组,取大脑海马组织重复实时荧光定量PCR检测NMDA受体l亚基和2B亚基mRNA的表达情况。最后存活的乳鼠各8只,即S3组和D3组,进行跳台试验。结果与对照组(D1组和D2组)比较,吸入七氟醚的实验组(S1组和S2组),乳鼠的大脑海马组织的NMDA受体1亚基、2B亚基mRNA表达降低,与对照组(D3组)比较,吸入七氟醚的实验组(S3组)乳鼠学习成绩、记忆成绩显著降低,差异均有统计学意义(P<0.05)。结论持续暴露于七氟醚中可降低未成熟SD大鼠学习、记忆能力,其原因可能与NMDA受体l亚基、2B亚基mRNA的表达降低有关。

罗格列酮对鼠血管平滑肌细胞血管紧张素Ⅱ1型受体mRNA表达的影响

目的探讨罗格列酮对血管紧张素Ⅱ（AngⅡ）诱导鼠血管平滑肌细胞（VSMC）血管紧张素Ⅱ1型受体（AT1R）mRNA表达的影响。方法选6～10代处于对数生长期的鼠血管平滑肌细胞，用终浓度为1μmol·L^-1 AngⅡ预先培养2h后分成A、B和C组，分别加入终浓度为20、30、50μmol·L^-1罗格列酮培养12h；另外，取预先用终浓度为1μmol·L^-1 AngⅡ培养6h的鼠血管平滑肌细胞，加入终浓度为30μmol·L^-1的罗格列酮分别再培养0、6、12、24h。提取总RNA，采用逆转录聚合酶链反应（RT-PCR）检测平滑肌细胞AT1RmRNA的表达。结果与空白对照组（23．82±4．68）相比，AngⅡ组AT1RmRNA的表达显著升高（P〈0．01）；与AngⅡ组（61．04±12．20）比较，罗格列酮干预组（A、B和C组）AT1RmRNA的表达（45．22±7．17、39．82±6．34、34．70±6．69）呈浓度依赖性降低，差异均有显著性（P〈0．01）。30μmol·L^-1的罗格列酮干预组呈时间依赖性抑制AngⅡ诱导的VSMC AT1RmRNA的高表达（57．37±8．04、46．99±4．81、39．82±6．34、35．7l±6．13），差异均有显著性（P〈0．01）。结论一定浓度范围内，罗格列酮可呈浓度和时间依赖性地下调AngⅡ诱导的鼠VSMC AT1RmRNA的表达，这可能是其抗炎、抗动脉粥样硬化（AS）作用的重要机制之一。

1,25-二羟维生素D_3对其D_3受体mRNA表达的细胞特异性调节

目的:以人原始巨核白血病细胞系（HIMeg）和人骨肉瘤细胞系（HOS－8603）为细胞模型，研究1，25一二羟维生素D3[1，25（OH）2D3]对维生素D3受体（VDR）mRNA表达的调节作用。方法：VDRmRNA的检测采用定量逆转录．聚合酶链反应（RT－PCR）。结果：HOS－8603细胞经1，25（OH）2D3处理0～24h后，VDRZRNA表达水平无明显变化；但是1，25（OH）2D3却可以使HIMeg细胞VDRmRNA水平明显降低，且具有时间依赖性，24h后达到最低水平，仅为对照组的15％。结论：1，25（OH）2D3对VDRmRNA表达的调节作用具有组织细胞特异性。

N-苯基-1H-吡咯取代的双苯并咪唑类衍生物的合成及其AT_1受体拮抗活性研究

目的:寻找活性强、作用时间长的新型非肽类AT1受体拮抗剂。方法:以替米沙坦(telmisartan)为原型物,根据分子-受体结合模型的研究结果对其进行结构优化:运用生物电子等排原理,用苯基吡咯代替联苯结构,在此基础上将羧基与四氮唑两种酸性基团的作用进行比较;改变苯并咪唑2-位亲脂性侧链的长度;在苯基吡咯5-位引入吸电子取代基,共设计了3类结构新颖的N-苯基-1H-吡咯取代的双苯并咪唑类衍生物,并完成了12个目标化合物的合成。通过测定目标化合物抑制AⅡ诱导的兔胸主动脉环收缩的能力评价了其对AT1受体的拮抗活性。结果:目标化合物均未见文献报道,其结构经MS、IR1、H NMR和元素分析确证,其中化合物Ⅰd的AT1受体拮抗活性大于先导物替米沙坦。结论:Ⅰd具有进一步的研究价值。

短暂性前脑缺血后大鼠海马各区NMDA受体亚单位1mRNA的表达变化

目的 观察短暂性前脑缺血后大鼠海马各区N 甲基 D 天门冬氨酸受体 (NR) 1mRNA的表达变化。方法 采用大鼠前脑缺血 15min再灌注 0 5h～ 7d动物模型和原位杂交、图像分析等技术。 结果 缺血后 ,海马CA1区NR1mRNA的表达呈明显上升趋势 ,至 2 4h达高峰 ;然后表达开始回落 ,至缺血后 7d降至低谷。在CA3区 ,NR1mRNA的表达变化与CA1区类似 ,但变化幅度明显减小。在齿状回 ,缺血后 0 5h～ 72h ,NR1mRNA的表达未见显著性变化 ;缺血后 7d ,表达亦显著降低。 结论 短暂性前脑缺血后 ,大鼠海马各区RN1mRNA的表达变化不同 ,这种不同可能与海马的选择性易损现象和迟发性细胞死亡有关。

电针对APP/PS1转基因小鼠海马低密度脂蛋白受体相关蛋白-1及其mRNA表达的影响

目的:研究电针是否是通过影响LRP1mRNA水平、提高LRP1的表达,从而促进脑内Aβ清除。方法:将4月龄APP/PS1转基因鼠,随机分为模型组、电针治疗组,以同窝同背景转基因阴性小鼠为正常对照组。电针干预"涌泉"、"百会"0.1 m A,15 min/次,隔日1次,治疗6周。治疗后,以免疫组化法观察脑组织LRP1阳性表达,以Western blotting法检测海马LRP1表达,以Real-time PCR法检测海马LRP1mRNA表达。结果:LRP1表达于脑微血管内皮细胞、胶质细胞、神经元等处。模型组海马LRP1蛋白、LRP1mRNA相对表达量低于正常对照组(P<0.05),电针治疗组海马LRP1及LRP1mRNA比模型组有上升趋势,但差异无统计学意义(P>0.05)。结论:电针干预可能影响5月龄APP/PS1转基因小鼠海马内所有细胞LRP1及LRP1mRNA表达,可能是电针干预AD发病的潜在靶点,但实验方案还需进一步完善。

β_1受体mRNA在心功能不全发生机制中的作用

采用ＲＴ－ＰＣＲ技术对２０例健康对照者和５８例不同心功能状态心脏病患者进行外周血淋巴细胞β１受体ｍＲＮＡ水平测定。结果发现心功能Ⅱ级患者的β１受体ｍＲＮＡ已开始下降，心功能Ⅳ级患者下降５０％以上，下降程度和心脏受损的严重程度呈正相关。

口腔黏膜下纤维化组织中内皮素受体mRNA表达的研究

目的:通过研究内皮素A型受体(endothelin receptor A,ETA)和内皮素B型受体(endothelin receptor B,ETB)在口腔黏膜下纤维化中mRNA的表达,探讨ETA、ETB与口腔黏膜下纤维化(oral submucous fibrosis,OSF)病变发生发展的关系。方法:选取30例OSF患者,其中早、中、晚期组各10例,5例健康志愿者作为对照组,每例研究对象取其口腔颊黏膜,运用逆转录聚合酶链反应(RT-PCR)研究ETA、ETB在OSF中mRNA的表达水平。结果:ETA mRNA和ETB mRNA在OSF各期中的表达均较正常口腔黏膜高(P<0.05);ETA mRNA在OSF早期的表达明显低于中、晚期(P<0.05),其中期的表达与晚期相比差异无显著性(P>0.05);ETB mRNA在OSF各组之间的表达差异无显著性(P>0.05)。结论:咀嚼槟榔等理化因素导致的ETA、ETB在基因转录水平的高表达以及由此所介导的缩血管效应可能是OSF微血管病变发生发展的始动因素。

mTOR及Tfr1 mRNA在腮腺黏液表皮样癌组织中的表达及与预后的关系

目的:探讨雷帕霉素靶蛋白(rapamycin target protein,mTOR)mRNA、转铁蛋白受体1(transferrin receptor 1,Tfr1) mRNA在腮腺黏液表皮样癌中的表达及与预后的关系.方法:选取2013年6月-2015年7月唐山市工人医院口腔科收治的35例腮腺黏液表皮样癌患者为研究对象,检测腮腺组织mTOR及Tfr1 mRNA的相对表达量,分析mTOR及Tfr1 mRNA与腮腺黏液表皮样癌患者临床病理及预后的关系.采用SPSS 19.0软件包对数据进行统计学处理.结果:腮腺黏液表皮样癌组织mTOR及Tfr1 mRNA相对表达量显著高于癌旁组织(P<0.05).mTOR及Tfr1 mRNA相对表达量与肿瘤浸润深度、肿瘤级别、临床分期及淋巴结转移相关(P<0.05).预后良好组患者,mTOR及Tfr1mRNA相对表达量显著低于预后不良组患者(P<0.05).mTOR mRNA评估患者预后不良的AUC为0.815,高于Tfr1mRNA的AUC(0.813),两者联合检测评估患者预后不良的AUC为0.922,高于两者单独检测.Cox单因素及多因素分析显示,分化程度、TNM分期、mTOR mRNA、Tfr1 mRNA与腮腺黏液表皮样癌患者预后不良关系密切.结论:腮腺黏液表皮样癌患者mTOR mRNA、Tfr1 mRNA相对表达量是否显著升高,可用于评估患者预后.

TLR4 mRNA和HO-1水平在ICVD病情及预后评估中的价值

目的探讨Toll样受体(TLR)4 mRNA和血红素氧合酶-1(HO-1)在缺血性脑血管病(ICVD)病情及预后评估中的价值。方法选取ICVD患者324例(ICVD组)、体检健康者324名(正常对照组)。分别检测HO-1水平及外周血TLR4 mRNA相对表达量。根据美国国立卫生研究院卒中量表(NIHSS)评分将ICVD患者分为轻度损伤组、中度损伤组和重度损伤组。根据头颅多普勒超声检查结果将ICVD患者分为轻度狭窄组、中度狭窄组和重度狭窄组。对ICVD患者随访6个月,根据随访结果分为预后较好组和预后不良组。采用Pearson相关分析评估HO-1及TLR4mRNA与NIHSS评分的相关性,采用Spearman相关分析评估HO-1及TLR4mRNA与颅内动脉狭窄程度的相关性。采用受试者工作特征(ROC)曲线评估HO-1及TLR4 mRNA判断ICVD预后的价值。结果 ICVD组HO-1水平及TLR4 mRNA相对表达量均高于正常对照组(P=0.000)。轻度狭窄组、中度狭窄组、重度狭窄组之间以及轻度损伤组、中度损伤组、重度损伤组之间HO-1水平及TLR4 mRNA相对表达量均依次升高,各组间差异均有统计学意义(P<0.05)。预后较好组HO-1水平及TLR4 mRNA相对表达量均低于预后不良组(P<0.05)。ICVD组HO-1水平及TLR4 mRNA相对表达量与颅动脉狭窄程度、NIHSS评分均呈正相关(P<0.05)。ROC曲线分析结果显示,HO-1、TLR4 mRNA判断ICVD预后不良的最佳临界值分别为4.364 ng/mL、0.989,曲线下面积分别为0.800、0.815,敏感性分别为81.4%、85.1%,特异性分别为72.4%、73.5%。结论 HO-1及TLR4或可作为ICVD患者病情评估及预后判断的有效指标。

宫颈组织HPV E6/E7 mRNA Atg-12 Tie-1表达情况与鳞状上皮内病变病理分级的相关性

目的探讨宫颈组织人类乳头瘤病毒(HPV)E6/E7 mRNA、自噬相关蛋白-12(Atg-12)、酪氨酸激酶受体-1(Tie-1)表达情况与鳞状上皮内病变(SIL)病理分级的相关性。方法选取2020年5月至2021年10月新乡市中心医院病理科诊断为SIL的患者227例,根据宫颈病变分级分为低级别鳞状上皮内病变(LSIL)组124例和高级别鳞状上皮内病变(HSIL)组103例,另选取子宫肌瘤手术患者80例为对照组。所有患者均采用支链DNA信号扩增法检测HPV E6/E7 mRNA,采用免疫组化法及免疫印迹法检测Atg-12、Tie-1蛋白。分析E6/E7 mRNA、Atg-12、Tie-1与病理分级的相关性,绘制受试者特征(ROC)曲线分析各指标对HSIL与LSIL的鉴别诊断价值。结果HSIL组的HPV E6/E7 mRNA、Tie-1蛋白阳性检出率高于LSIL组和对照组(P<0.05),HSIL组的Atg-12蛋白阳性检出率低于LSIL组和对照组(P<0.05),HSIL组的HPV E6/E7 mRNA拷贝数、Tie-1蛋白表达量高于LSIL组和对照组(P<0.05),HSIL组的Atg-12蛋白表达量低于LSIL组和对照组(P<0.05)。HPV E6/E7 mRNA、Tie-1蛋白表达量与SIL病理分级呈正相关(r=0.514,0.488),Atg-12蛋白表达量与SIL病理分级呈负相关(r=-0.433)。HPV E6/E7 mRNA、Atg-12、Tie-1鉴别诊断HSIL与LSIL的灵敏度为88.57%、74.29%、82.86%,特异度为57.14%、66.67%、64.29%。3项指标联合诊断的灵敏度为77.14%,特异度为85.71%(AUC=0.854)。结论HSIL患者HPV E6/E7 mRNA、Tie-1表达较高,Atg-12表达较低。HPV E6/E7 mRNA、Atg-12、Tie-1表达与SIL病理分级有一定相关性,联合诊断可为HSIL与LSIL的鉴别诊断提供参考。

Controlling N-methyl-D-aspartate receptor subunit 1 with calcitonin gene related peptide after cerebral ischemic injury

BACKGROUND: Activation of N-methyl-D-aspartate receptor (NMDAR) is a key link of exitotoxicity at the phase of cerebral ischemic injury. Because NMDAR is a main way to mediate internal flow of Ca2+ among glutamic acid receptors, over-excitation can cause neuronal apoptosis. Calcitonin gene related peptide has a strongly biological activity. On one hand, it can protect ischemic neurons through inhibiting the expression of NMDAR1 mRNA; on the other hand, it can play the protective effect through down-regulating the expression of NMDAR1 mRNA by exogenous calcitonin gene related peptide. OBJECTIVE: To observe the expression of NMDAR1 and the regulatory effect of calcitonin gene related peptide on the expression of NMDAR1 mRNA and protein in the cerebral cortex of rats with focal cerebral ischemia/reperfusion (I/R). DESIGN: Randomized controlled animal study. SETTING: China Medical University. MATERIALS: A total of 216 healthy male Wistar rats, general grade, weighing 250-280 g, were selected in this study. Twelve rats were randomly selected to regard as control group; meanwhile, other 204 rats were used to establish middle cerebral artery occlusion/reperfusion (MACO) models. The main reagents were detailed as follows: calcitonin gene related peptide (Sigma Company); calcitonin gene related peptide kit (Boster Company); antibody Ⅰ, Ⅱ and antibody β-actin Ⅰ, Ⅱ of NMDAR1 mRNA and chemiluminescence reagent (Santa Cruz Company, USA). METHODS: The experiment was carried out in the Laboratory of Neurobiology of China Medical University from August 2005 to June 2006. ① Right MCAO models of rats were established to cause focal ischemia and scored based on Zea Longa five-grade scale. If the scores were 1, 2 and 3 after wakefulness, the MACO models were established successfully and involved in the experiment. A total of 120 rats with successful modeling were randomly divided into I/R group and administration group with 60 in each group. All rats in the both groups were observed at five time points, including 6, 12, 24, 48 and 72 hours after reperfusion and after 2-hour ischemia, with 12 experimental animals at each time point. Six rats were prepared for detection of hybridization in situ, and the other 6 were used for Western blotting histochemical detection. Rats in the control group were opened their skin to separate common carotid artery and not treated with line and drugs. In addition, rats in the I/R group were treated with 1 mL saline at 2 hours after focal cerebral ischemia, and then, rats in the administration group were treated with 1 mL (1 g/L) calcitonin gene related peptide at 2 hours after focal cerebral ischemia. ② The expression of NMDAR1 mRNA was detected with hybridization in situ at various time points; moreover, the expression of NMDAR1 protein was measured with Western blotting method at various time points. The results were analyzed with Metamoph imaging analytical system. MAIN OUTCOME MEASURES: The expression of NMDAR1 mRNA and its protein in cortical neurons of rats at various time points. RESULTS: A total of 84 rats were excluded because of non-symptoms, exanimation or death; and then, 132 rats were involved in the final analysis. The expression of NMDAR1 mRNA and its protein in cortical neurons of rats in the control group was 0.205±0.001 and 0.184±0.001, respectively; after I/R, expression of NMDAR1 mRNA and its protein was up-regulated, especially, expression of mRNA at 6, 12, 24, 48 and 72 hours was 0.245±0.003, 0.287±0.004, 0.354±0.008, 0.284±0.002 and 0.217±0.006, respectively; moreover, expression of protein at 6, 12, 24, 48 and 72 hours was 0.222±0.003, 0.261±0.028, 0.311±0.004, 0.259±0.013 and 0.210±0.008, respectively. There was significant difference between the two groups (0.205±0.001, P < 0.01). The expression was up-related in the former 24 hours, reached peak at 24 hours, down-regulated, and decreased to the level of control group at 72 hours. Except 72 hours, the expression of NMDAR1 mRNA and its protein was lower in administration group than that in I/R group at other four time points. In addition, the expression of mRNA at 6, 12, 24, 48 and 72 hours was 0.223±0.005, 0.243±0.001, 0.292±0.002, 0.250±0.003 and 0.213±0.003, respectively; moreover, the expression of protein at 6, 12, 24, 48 and 72 hours was 0.216±0.006, 0.245±0.025, 0.276±0.003, 0.241±0.045 and 0.202±0.013, respectively. There was significant difference at various time points (P < 0.05). CONCLUSION: The expressions of NMDAR1 mRNA and its protein of peripheral cortical neurons are up-related in ischemic area after focal cerebral I/R. Meanwhile, exogenous calcitonin gene related peptide can protect cortical neurons through inhibiting expression of NMDAR1 mRNA and its protein after focal cerebral I/R.