Expression of indoleamine 2,3-dioxygenase in a murine model of Aspergillus fumigatus keratitis

AIM： To observe the presence and expression of indoleamine 2,3-dioxygenase（IDO） during the corneal immunity to Aspergillus fumigatus（A. fumigatus） in the murine models.·METHODS： The murine model of fungal keratitis was established by smearing with colonies of A. fumigatus after scraping central epithelium of cornea and covering with contact lenses in C57BL/6 mice. The mice were randomly divided into control group, sham group and A.fumigatus keratitis group. The cornea was monitored daily using a slit lamp and recorded disease score after infection. Corneal lesion was detected by immunofluorescence staining. IDO m RNA and protein were also detected by quantitative reverse transcription-polymerase chain reaction（q RT-PCR） and Western blot.· RESULTS： The disease score and slit lamp photography indicated that disease severity was consistent with corneal inflammation in the murine models, and the disease scores in A. fumigatus keratitis group were obviously higher than those in the sham group. By immunofluorescence staining, IDO was mainly localized in corneal epithelium and stroma in the murine corneal tissues with A. fumigatus keratitis. Compared with the sham group, IDO m RNA expression was significantly enhanced in corneal epithelium infected by A. fumigatus. Furthermore, IDO protein expression detected by Western blot was in accord with transcript levels of IDO m RNA measured by q RT-PCR. IDO protein expression was enhanced after A. fumigatus infection compared with the sham group.·CONCLUSION： IDO is detected in corneal epithelium and stroma locally, which indicates IDO takes part in the pathogenesis of A. fumigatus keratitis and plays a key role in immune regulation at the early stage.

Relationship of Abortion and the Expression of Indoleamine 2,3- dioxygenase (IDO) in Villus and Syncytiotrophoblasts

Objective To study the relationship of abortion and the expression of indoleamine 2, 3- dioxygenase （IDO） in villus and syncytiotrophoblast in vitro. Methods RT-PCR was applied to analyze the mRNA transcription of lDO in villus of normal pregnancy and inevitable abortion and JAR cells as well. Immunohistochemistry was applied to analyze the expression of IDO protein in villus. Western blot was applied to determinate the expression of IDO protein on cultured syncytiotrophoblast. Highperformance liquid chromatography was applied to determinate whether there was kynurenine in cell culture medium of syncytiotrophoblast. Results The expression of IDO mRNA and protein in villus of inevitable abortion was lower than that of normal pregnancy; IDO mRNA did not express in JAR cells. IDO protein expressed on cultured syncytiotrophoblast, and there was kynurenine in cell culture medium of syncytiotrophoblast. Conclusion Appropriate expression of IDO in villus is necessary.for maintenance of normal pregnancy and an active IDO protein expresses in syncytiotrophoblast.

Molecular Cloning and Characterization of Porcine Indoleamine 2,3-Dioxygenase and Its Expression in Various Tissues

In order to confirm the existence of indoleamine 2,3-dioxygenase(IDO) gene in swine,and to clone the novel gene followed by the molecule structure properties and expression pattern analysis,the porcine mRNA sequences homologous to human IDO were obtained from GenBank database by bioinformatics method.By using RT-PCR,the IDO gene was cloned from porcine endothelial cell line and the accuracy of the nucleic acid sequence was confirmed,and the expression pattern of the gene was detected.The three-dimensional structure model of porcine IDO was built referring to the tertiary structure of human IDO using biological sequence analysis software and database.The results showed that the porcine IDO was identified by sequencing.The nucleotide sequences were confirmed as a novel gene after submitted to Genbank.Porcine IDO was expressed in the lung,thymus,epididymis and anterior chamber with a basic level,however in peripheral blood mononuclear cells(PBMCs) the IDO gene was highly expressed.The three-dimensional structure model of porcine IDO was similar to that of human IDO.It was suggested that identification of the structure information of porcine IDO is essential to further investigate the immunologic function of the gene.Study of IDO on NK cells-mediated xenograft rejection will be a novel therapeutic target for the development of xenotransplantation.

Indoleamine 2,3-dioxygenase in tumor induced tolerance

Objective To review the recent studies about the role of indoleamine 2,3-dioxygenase （IDO） in tumor induced tolerance. Data sources Published articles （1978-2009） on IDO and tumor induced tolerance were selected from Medline. Study selection Articles selected were relevant to development of IDO in tumor induced tolerance. Of all originally identified articles, 50 specially addressed the stated purpose. Results Recent work has revealed IDO at high levels in tumors and in tumor-draining lymph nodes and a close relationship between IDO activity and the regulatory T cells. Conclusion Up-regulation of IDO is proven to be a mechanism of acquired tolerance in tumors, in which the closely coupled positive feedback system between IDO and reclulatorv T cells may be considered to play an important role.

Indoleamine-2,3-dioxygenase 1/cyclooxygenase 2 expression prediction for adverse prognosis in colorectal cancer

AIM To evaluate indoleamine-2,3-dioxygenase 1/cyclooxygenase 2(IDO1/COX2) expression as an independent prognostic biomarker for colorectal cancer(CRC) patients.METHODS We retrospectively studied the medical records of 95 patients who received surgical resection from August 2008 to January 2010. All patients were randomly assigned to adjuvant treatment with or without celecoxib groups after surgery. We performed standard immunohistochemistry to assess the expression levels of IDO1/COX2 and evaluated the correlation of IDO1/COX2 with clinicopathological factors and overall survival(OS) outcomes.RESULTS The expression of nuclear IDO1 was significantly correlated with body mass index(P < 0.001), and IDO1 expression displayed no association with sex, age, tumor differentiation, T stage, N stage, carcinoembryonic antigen, cancer antigen 19-9, CD3+ and CD8+ tumor infiltrating lymphocytes, and COX2. In univariate analysis, we found that nuclear IDO1(P = 0.039), nuclear/cytoplasmic IDO1 [hazard ratio(HR) = 2.044, 95% confidence interval(CI): 0.871-4.798, P = 0.039], nuclear IDO1/COX2(HR = 3.048, 95%CI: 0.868-10.7, P = 0.0049) and cytoplasmic IDO1/COX2(HR = 2.109, 95%CI: 0.976-4.558, P = 0.022) all yielded significantly poor OS outcomes. Nuclear IDO1(P = 0.041), nuclear/cytoplasmic IDO1(HR = 3.023, 95%CI: 0.585-15.61, P = 0.041) and cytoplasmic IDO1/COX2(HR = 2.740, 95%CI: 0.764-9.831, P = 0.038) have significantly poor OS outcomes for the CRC celecoxib subgroup. In our multivariate Cox model, high coexpression of cytoplasmic IDO1/COX2 was found to be an independent predictor of poor outcome in CRC(HR = 2.218, 95%CI: 1.011-4.48, P = 0.047) and celecoxib subgroup patients(HR = 3.210, 95%CI: 1.074-9.590, P = 0.037).CONCLUSION Our results showed that cytoplasmic IDO1/COX2 coexpression could be used as an independent poor predictor for OS in CRC.

吲哚胺2,3-双加氧酶1在肝癌中的表达及其作用的初步研究

目的:探讨吲哚胺2,3–双加氧酶1(IDO1)在肝癌与癌旁组织中的表达情况及其作用。方法:应用公共数据库获取IDO1在泛癌和肝癌中的表达数据。应用免疫荧光染色法对82例肝癌和配对癌旁组织以及14例无配对的肝癌组织中IDO1的表达情况进行检测。皮下接种人源肝癌细胞SK–HEP1建立裸鼠皮下移植瘤模型,并予以IDO1抑制剂干预,通过苏木精–伊红(HE)病理染色和增殖细胞核抗原(PCNA)免疫组化染色评价IDO1抑制剂对肝癌细胞在体内生长速度的影响,免疫荧光染色检测瘤体组织中簇分化抗原(CD)4^(+)T细胞和CD8^(+)T细胞的浸润情况。结果:IDO1在多种癌组织中高表达。与癌旁组织相比,肝癌组织中IDO1的表达水平明显升高。病理染色结果示,抑制IDO1的表达可以明显降低肝癌移植瘤组织中PCNA的表达水平,增加CD4^(+)T细胞和CD8^(+)T细胞的浸润。结论:IDO1在肝癌组织中高表达,下调IDO1的表达可抑制肝癌细胞在体内增殖,延缓皮下瘤体的生长速率,增强免疫细胞对肿瘤细胞的应答。

吲哚胺2,3-双加氧酶1在胃癌中的研究进展

胃癌(Gastric Cancer,GC)是全球第五大最常见的恶性肿瘤,也是第四大癌症死亡相关原因。胃癌异质性明显,肿瘤微环境复杂,免疫检查点抑制剂虽然在晚期胃癌中展现出一定抗肿瘤疗效,但获益人群仍在少数。吲哚胺2,3-双加氧酶1(Indoleamine 2,3-Dioxygenase 1,IDO1)是色氨酸沿犬尿氨酸途径代谢中的关键酶,对肿瘤免疫逃逸起到了关键作用。目前已有多项研究表明IDO1在胃癌发生发展及幽门螺杆菌感染和EB病毒感染中发挥重要作用,所以靶向IDO1有望成为胃癌免疫治疗的新策略。本文就IDO1作用机制、IDO1在胃癌及相关疾病中的研究进展及IDO1抑制剂在胃癌中的应用前景进行综述。

吲哚胺2,3-双加氧酶1对急性放射性肠道损伤的保护作用

目的:探讨吲哚胺2,3-双加氧酶1(IDO1)对急性放射性肠道损伤的作用。方法:使用TCGA和GTEX数据集中结肠癌、直肠癌组织和正常对照组织的测序结果,分析IDO1基因在肠癌组织及正常肠道组织中的表达情况。使用CRISPR/Cas9技术敲除鼠正常肠上皮IEC-6细胞中IDO1基因的部分第2、3外显子序列,建立鼠IEC-6的IDO1 KO(IDO1^(-/-))细胞系,并给予两个细胞系(野生型和IDO1^(-/-))放射处理。C57BL/6野生型小鼠和IDO1基因敲除(IDO1^(-/-))小鼠也给予腹部X射线照射以建立细胞和动物急性放射性肠道损伤模型。使用蛋白质印记法(Western blot)检测野生型和IDO1^(-/-)的IEC-6细胞及小鼠肠道组织中上皮紧密连接蛋白在放射前、后的蛋白表达水平。结果:Western blot证实IDO1在鼠IEC-6细胞、肠道组织中均有表达。对TCGA和GTEX数据集分析后也同样看到IDO1基因在结肠癌、直肠癌、正常肠道组织中均有表达,但癌组织中IDO1水平较正常肠道组织高(P<0.05)。体内外的放射照射后,IDO1、Claudin 1、Occludin、ZO-1等出现明显变化:与放射前比,放射后的细胞和小鼠组织中的IDO1的表达水平升高(P<0.05),而紧密连接蛋白Claudin 1、Occludin、ZO-1则下降(P<0.05);与野生型IEC-6细胞和小鼠相比,在IDO1^(-/-)IEC-6细胞和小鼠肠组织中,Claudin 1、Occludin、ZO-1下降更显著(P<0.05)。结论:IDO1在急性放射性肠道损伤中起保护作用,其保护作用可能是通过保护肠上皮细胞间紧密连接功能而实现的。

基于虚拟筛选的新型吲哚胺2,3-双加氧酶抑制剂的发现及活性评价

目的应用药效团模型及分子对接的综合虚拟筛选策略,对Specs及Chembridge数据库进行筛选并进行生物学活性评价,以期发现新型吲哚胺2,3-双加氧酶(IDO1)抑制剂。方法基于已报道IDO1抑制剂,利用Discovery Studio 2019软件的Pharmacophores(Hiphop)模块构建药效团模型。通过最优药效团模型初步筛选了Specs及Chembridge数据库,后采用LibDock及CDOCKER程序靶向IDO1活性位点进行层级分子对接,最终保留了40个苗头化合物,并在100μmol/L浓度下进行了细胞水平IDO1酶抑制活性初筛。选取初筛抑制率大于50%的11个化合物进行细胞水平及生化水平抑酶活性的进一步测定。采用SPR及分子对接模型进一步确证及阐明化合物与IDO1酶之间的相互作用方式。结果发现羟基嘧啶类化合物29在细胞水平及生化水平上均呈现了IDO1酶抑制活性,EC50和IC50分别为(53.93±1.22)μmol/L和(179±8.12)μmol/L。SPR研究进一步确证了化合物29与IDO1之间的直接结合(KD=65.92μmol/L)。分子对接模型研究显示羟基嘧啶基团与IDO1的卟啉环之间存在较为丰富的相互作用,是靶向识别的关键基团。结论羟基嘧啶类化合物29是一类新型IDO1抑制剂,可作为IDO1酶抑制剂的先导物,通过进一步结构改造及优化,有望获得高效、结构新颖的IDO1抑制剂及新型肿瘤免疫治疗药物。

不同棘球蚴抗原诱导树突状细胞表达吲哚胺2,3-双加氧酶的实验研究

目的检测不同的棘球蚴抗原体外诱导树突状细胞(DCs)表达吲哚胺2,3-双加氧酶(IDO)的情况。方法从C57BL/6小鼠股骨中分离出骨髓细胞,用小鼠重组巨噬细胞集落刺激因子(rmGM-CSF)诱导后,获得小鼠骨髓源树突状细胞(BMDCs)。分别用重组抗原B(rAgB,15μg/ml)、小鼠细粒棘球蚴囊液(MHF,5 mg/ml)、γ干扰素(IFN-γ,1 000 U/ml,为阳性对照)和RPMI 1640完全培养液(阴性对照)刺激DCs,于18、24和48 h后收集细胞和细胞上清。采用流式细胞术检测各组DCs的表面标志物CD40、CD80、CD86和I-A/I-E的阳性表达情况,并利用实时荧光定量PCR(FQ-RT-PCR)检测各组的IDO mRNA相对转录水平。利用高效液相色谱法(HPLC)检测各组细胞上清中的色氨酸(Try)浓度。结果流式细胞术检测结果显示,DCs受rAgB和MHF刺激后,其表面标志物CD40、CD80、CD86和I-A/I-E的阳性表达率均降低。刺激24 h后,rAgB组的CD40、CD86和I-A/I-E阳性表达率分别为(22.60±2.69)%、(35.50±4.38)%和(57.30±4.38)%,与MHF组[(38.00±3.54)%、(53.00±3.39)%和(77.10±1.70)%]和阴性对照[(37.95±3.61)%、(19.55±1.06)%和(85.45±1.63)%]的差异均有统计学意义(P<0.05)。FQ-RT-PCR结果显示,刺激18、24和48 h后,rAgB组的IDO mRNA水平[(9.20±0.01)、(29.44±0.02)和(16.48±0.04)]和MHF组的[(9.67±0.02)、(17.52±0.01)和(16.81±0.01)]均高于阴性对照组[(2.46±0.01)、(7.77±0.01)和(10.56±0.01)](P<0.01),rAgB组和MHF组IDO mRNA水平的差异均有统计学意义(P<0.05)。HPLC结果显示,刺激18、24和48 h后,rAgB组DCs上清中的色氨酸浓度[(23.65±0.64)、(13.95±1.06)和(19.05±0.64)μmol/L]均较其他3组低,刺激24 h后的色氨酸浓度与阴性对照组(22.90±0.14)和MHF组(20.65±0.35)的差异均有统计学意义(P<0.05)。结论在体外实验条件下,rAgB、MHF均可上调DCs表面IDO的表达,作用24 h后,rAgB上调IDO的能力强于MHF。

急性髓细胞白血病细胞的吲哚胺2,3-双加氧酶介导免疫逃逸的实验研究

为了探讨急性髓细胞白血病细胞的吲哚胺2,3-双加氧酶(IDO)参与肿瘤免疫逃逸的机制,从23例急性髓性白血病患者获取骨髓细胞,采用免疫组织化学染色法和RT-PCR法检测白血病细胞IDO的表达;在有或无1-甲基色氨酸(1-MT)存在下,以白血病细胞为刺激细胞,外周T淋巴细胞为反应细胞建立单向混合淋巴细胞反应体系(MLR),利用MTT法检测T淋巴细胞增殖率,并以反相高效液相色谱法检测相应MLR体系上清液中的IDO活性。结果显示,在23例急性髓细胞白血病患者中17例患者的骨髓白血病细胞上有IDO的表达;白血病细胞上的IDO活性抑制MLR体系中T淋巴细胞的增殖。结论:白血病细胞表达的IDO活性能阻抑外周T淋巴细胞的增殖,它可能参与了肿瘤免疫逃逸。

吲哚胺2,3-双加氧酶-1在宫颈癌中的表达及对增殖及侵袭的影响

目的:研究吲哚胺2,3-双加氧酶-1(IDO1)在宫颈癌组织中的表达及其对宫颈癌细胞增殖、侵袭的影响。方法:免疫组织化学方法检测IDO1蛋白在宫颈癌组织中的原位表达;实时定量PCR检测IDO1信使RNA(mRNA)在宫颈癌细胞系中的表达水平;CCK8方法检测IDO1小干扰RNA(siRNA)及诱导因子干扰素(IFN-γ)对宫颈癌细胞增殖的影响。Transwell检测上述两种处理因素对宫颈癌细胞侵袭的影响。Western blotting实验检测侵袭相关蛋白基质金属蛋白酶9(MMP9)的表达。结果:(1)免疫组化结果显示,IDO1蛋白定位在肿瘤细胞及间质细胞的胞浆中,其阳性表达率(83%)显著高于癌旁组织(55%),差异有统计学意义(P<0.05)。(2)干扰素-γ(IFN-γ)促进HeLa和SiHa细胞IDO1 mRNA表达升高(P<0.01)。(3)siRNA敲减IDO1抑制IFN-γ介导的宫颈癌细胞增殖及侵袭,并且降低MMP9的表达水平。结论:高表达的IDO1受IFN-γ调控,促进宫颈癌细胞的增殖及侵袭。

调节性T细胞与吲哚胺2,3-双加氧酶在乙肝感染者外周血中表达的相关性

目的探讨乙肝病毒(HBV)感染者在不同病程下,吲哚胺-2,3双加氧酶(IDO)表达水平及其与调节性T细胞(Treg)的相关性。方法对142例HBV感染者及28例正常对照者分别采用流式细胞术、实时荧光定量PCR技术和全自动生化分析仪检测受检者外周静脉血IDO mRNA、调节性T细胞及丙氨酸氨基转移酶(ALT)活性;进行各组间检测结果比较及相关性分析。结果 IDO mRNA从高到低依次为肝癌组(HCC)、急性乙型肝炎组(AHB)、慢性乙型肝炎组(CHB)、肝硬化组(LC)、对照组。LC组与对照组均明显低于其余3组(P<0.01),其他各组间两两比较,差异无统计学意义(P>0.05)。Treg计数从高到低依次为HCC组、AHB组、LC组、CHB组和对照组。除CHB组外,各组Treg细胞与对照组比较差异均有统计学意义(均P<0.05),其中HCC组明显高于其他3组(F=10.764,P=0.002)。ALT检测,总体组间比较,除LC组外,各组ALT活性与对照组比较差异均有统计学意义(均P<0.05)。Treg细胞、ALT、IDO mRNA相关性分析显示ALT活性与IDO mRNA表达无相关性(r=0.196,P=0.026),Treg细胞与IDO mRNA表达呈正相关(r=0.912,P<0.01)。结论 HBV感染者IDO表达明显增强,与Treg细胞正相关,即IDO高表达伴随着外周血Treg细胞比例增高,共同影响HBV的免疫耐受。

吲哚胺2,3-双加氧酶及IL-12/IL-10细胞因子平衡与妊娠免疫耐受

目的 :观察妊娠不同时期胎盘来源的单核-巨噬细胞吲哚胺2,3-双加氧酶(indoleamine 2,3-dioxygenase,IDO)的表达及细胞因子白细胞介素(IL)-10、IL-12的分泌情况,探讨其在妊娠免疫耐受中的可能作用。方法:机械分离中期妊娠(21周±3天,19例)及足月妊娠(39周±5天,25例)胎盘中的单核-巨噬细胞,ELISA法检测其分泌IL-10、IL-12的水平;RT-PCR及Western blot法分别检测IDO mRNA及蛋白水平的表达;以CCK-8法检测其激发同种异体T细胞增殖能力的不同。结果:足月妊娠较中期妊娠胎盘来源的单核-巨噬细胞产生更多的IL-12,但IL-10及IDO的表达较之明显减低;并且,足月妊娠较中期妊娠胎盘来源的单核-巨噬细胞刺激同种异体淋巴细胞增殖的能力更强。结论:中期及足月妊娠胎盘来源的单核-巨噬细胞参与维持妊娠免疫耐受及分娩发动可能与其调节IL-12/IL-10细胞因子平衡及影响IDO的表达有关,但IL-12/IL-10细胞因子平衡与单核-巨噬细胞IDO表达的关系还有待进一步研究。

补肾中药对蜕膜巨噬细胞吲哚胺2,3-二氧化酶的影响

目的:探讨补肾中药对人早孕蜕膜巨噬细胞吲哚胺2,3二氧化酶(Indoleamine2,3dioxygenase,IDO)的影响。方法:半定量RTPCR测蜕膜IDOmRNA表达;Westernblot检测蜕膜巨噬细胞IDO蛋白质表达;ELISA测蜕膜巨噬细胞和淋巴细胞共培养上清液中IL10、IFNγ含量,高效液相色谱法测上清色氨酸、犬尿氨酸含量,以二者比值表示IDO活性。结果:正常组蜕膜IDOmRNA表达高于难免流产组;IDO抑制剂使Th细胞因子平衡偏离Th2型;中药血清可提高IDO蛋白质表达及活性,恢复Th细胞因子平衡。结论:蜕膜巨噬细胞IDO正常表达和活性是维持妊娠所必需,补肾中药可提高IDO活性至正常水平。

吲哚胺2，3-二氧化酶对乙肝患者T细胞的免疫抑制作用

目的观察吲哚胺2,3-二氧化酶(IDO)在慢性乙型肝炎(乙肝)病毒感染方面的免疫耐受作用,从而为重建人体主动免疫提供一种新方法。方法采集50例慢性乙肝患者外周静脉血作为乙肝组,检测其乙肝病毒复制水平,T细胞亚群功能,以及IDOmRNA,蛋白定量以及表达活性。统计分析乙肝病毒(HBV)复制水平、T细胞亚群功能以及IDO表达三者之间的关系。采集50例健康体检人群外周静脉血作为正常对照组,以同样方法处理之。结果乙肝患者IDOmRNA、IDO蛋白定量、IDO表达活性均明显高于健康体检人群[mRNA:(2.110±0.615)×103vs(0.143±0.026)×103;蛋白定量:0.22±0.06vs0.02±0.0017;表达活性:26.07±8.12vs4.98±1.65;P<0.05],IDOmRNA与HBV(r=0.502,P<0.001)和ALT(r=0.65,P<0.01)均呈正相关。另外,IDOmRNA、蛋白定量和表达活性均与CD4(+)T细胞(r=-0.622,-0.682,-0.549,P<0.05)、CD8(+)T细胞(r=-0.487,-367,-294,P<0.05)以及CD4/CD8比值(r=-0.426,-0.533,-0.397,P<0.05)呈负相关。结论IDO与HBV密切相关,并且参与HBV的免疫耐受,抑制IDO的功能可以为打破乙肝病毒的免疫耐受提供一个新方法。

吲哚胺2,3双-加氧酶介导肝癌细胞免疫逃逸的实验研究

目的:为了探讨吲哚胺2,3双-加氧酶(IDO)参与肝癌免疫逃逸的机制。方法:混合培养HepG2细胞和T淋巴细胞,在有或无1甲-基色氨酸(1-MT)存在下,用RT-PCR检测细胞中IDOmRNA的表达,流式细胞仪分析混合反应体系中HepG2细胞的凋亡率,MTT检测T淋巴细胞抗HepG2细胞的细胞毒活性。结果:混合反应体系中,HepG2细胞表达IDOmRNA的水平随着1-MT浓度的增高而降低;对照组及实验组(1-MT浓度分别为1.25mmol/L,2.5mmol/L,5mmol/L)中HepG2细胞的早期凋亡率分别为(3.48±0.34)%,(7.82±0.41)%,(18.62±0.42)%,(25.32±0.40)%(P<0.01),T淋巴细胞抗HepG2细胞的细胞毒活性分别为(17.36±1.24)%、(25.48±1.48)%、(32.89±1.73)%、(42.04±2.16)%(P<0.01)。结论:HepG2细胞表达的IDO能抑制外周T淋巴细胞发挥抗肿瘤免疫作用,它可能参与了肝癌的免疫逃逸。

丁酸钠通过下调细胞干扰素调节因子-1抑制鼻咽癌细胞CNE2吲哚胺-吡咯2,3-双加氧酶的表达

目的研究丁酸钠(NaB)抑制鼻咽癌细胞CNE2吲哚胺-吡咯2,3-双加氧酶(IDO)表达从而解除肿瘤免疫耐受的分子机制。方法体外培养人鼻咽癌上皮细胞CNE2,采用NaB和(或)IFN-γ处理CNE2细胞;免疫印迹检测CNE2细胞IDO的表达情况;RT-PCR检测JAK/STAT的细胞因子信号抑制因子1(SOCS1)和SOCS3的转录水平;Real time PCR检测CNE2细胞干扰素调节因子-1(IRF-1)的转录情况。结果在NaB作用下,CNE2细胞内IDO的表达减少,并且IFN-γ诱导的IDO表达也被显著抑制;SOCS1和SOCS3的转录水平未见改变;而IFN-γ诱导的IRF1转录受到NaB的显著抑制。结论 NaB抑制IFN-γ诱导的IDO表达,不是通过增加SOCS1和SOCS3的转录,而可能是通过下调IRF-1,抑制IFN-γ诱导的IDO表达。

中药复方对Lewis肺癌移植鼠肿瘤微环境中吲哚胺2,3-双加氧酶表达的影响

目的:研究中药复方对Lewis肺癌移植鼠肿瘤微环境中吲哚胺2,3-二氧化酶(indoleamine 2,3-dioxygenase,IDO)表达的影响。方法:选用近交系C57BL/6纯系小鼠64只,将Lewis肺癌细胞悬液接种于小鼠右腋皮下建立肺癌模型,接种后小鼠随机分为4组:对照组、化疗组、中药复方组和中药复方加化疗组,通过应用免疫组化法及免疫印迹(Western blot)方法等多种实验技术,分别检测Lewis肺癌移植鼠肿瘤及淋巴组织中IDO表达水平。结果:中药复方及化疗药物顺铂均可在不同程度上影响IDO表达水平。同时中药复方与化疗药物顺铂具有协同作用,两者在不同环节调控调节性T细胞的作用与单一治疗相比存在一定优势。结论:中药复方与化疗在消除肿瘤微环境的局部免疫耐受中具有协同作用。

人绒毛外滋养层细胞HTR-8/SVneo中Toll样受体mRNA的表达及对吲哚胺2,3-双加氧酶mRNA水平的影响

目的系统检测人绒毛外滋养细胞HTR-8/SVneo中Toll样受体(TLR)mRNA的表达情况,定量分析TLRs配体刺激前后吲哚胺2,3双加氧酶(indoleamine 2,3-dioxygenase,IDO)mRNA的表达差异。方法 RT-PCR检测HTR-8/SVneo细胞中TLR 1-10mRNA的表达情况;实时荧光定量RT-PCR检测TLR3、TLR4、TLR7/8、TLR9配体刺激前后IDO mRNA表达水平。结果 HTR-8/SVneo细胞中有IDO及TLR 1-10 mRNA表达;在48 h内IDO mRNA表达随着时间延长,呈升高趋势;IDO mRNA的表达与培养基营养状况相关;TLRs配体刺激后,除TLR-3转录水平表达下调外,TLR-4、7、8、9 mRNA表达均上调;poly(I∶C)刺激后IDO mRNA表达低于正常组,IFN-γ刺激后表达高于正常组(P<0.05)。结论 TLRs mRNA的表达提示该细胞具有抗感染作用;HTR-8/Svneo细胞中IDO mRNA的表达与母胎界面营养状况相关;TLRs配体刺激剂对TLRs及IDO mRNA表达的影响不仅验证了TLRs的功能活性,而且提示了IDO在抗病原体免疫应激中可依赖TLRs途径发挥作用。