IDO1影响外阴阴道念珠菌病小鼠阴道组织中巨噬细胞功能变化的研究

doi:10.35541/cjd.20240163

中华皮肤科杂志 ›› 2024, Vol. 57 ›› Issue (10): 931-939.doi: 10.35541/cjd.20240163

IDO1影响外阴阴道念珠菌病小鼠阴道组织中巨噬细胞功能变化的研究

唐诗琴¹ 郝瑞英¹ 贺慧娜¹ 田亚楠¹ 徐艳艳^2，3 李小静^3，4 景婷婷^2，3

¹河北工程大学临床医学院，邯郸 056002；²河北工程大学附属医院皮肤科，邯郸 056002；³河北省免疫性皮肤病实验室，邯郸 056002；4河北工程大学，邯郸 056038

收稿日期:2024-03-27 修回日期:2024-08-06 发布日期:2024-09-29
通讯作者: 李小静 E-mail:zlmdsh@126.com; xuyanyan0308@163.com
基金资助:
河北省自然科学基金（H2021402009）；河北省临床医学优秀人才培养项目（ZF2023222、ZF2024205）

Effect of IDO1 on functional changes in macrophages in vaginal tissues from mouse models of vulvovaginal candidiasis

Tang Shiqin¹, Hao Ruiying¹, He Huina¹, Tian Yanan¹, Xu Yanyan^2,3, Li Xiaojing^3,4, Jing Tingting^2,3

¹School of Clinical Medicine, Hebei University of Engineering, Handan 056002, Hebei, China; ²Department of Dermatology, Affiliated Hospital of Hebei University of Engineering, Handan 056002, Hebei, China; ³Hebei Immunological Dermatology Laboratory, Handan 056002, Hebei, China; 4Hebei University of Engineering, Handan 056038, Hebei, China

Received:2024-03-27 Revised:2024-08-06 Published:2024-09-29
Contact: Li Xiaojing; Xu Yanyan E-mail:zlmdsh@126.com; xuyanyan0308@163.com
Supported by:
Natural Science Foundation of Hebei Province （H2021402009）; Hebei Province Excellent Talent Training Project （ZF2023222, ZF2024205）

摘要/Abstract

摘要： 【摘要】目的通过调控吲哚胺2，3-双加氧酶（IDO1）观察外阴阴道念珠菌病（VVC）小鼠模型中巨噬细胞功能的变化。方法 40只无特定病原级雌性ICR小鼠按完全随机法分为4组：空白组、VVC模型组、VVC模型 + 1-甲基色氨酸组（简称1-MT组）、VVC模型 + γ干扰素组（简称IFN-γ组），每组10只。除空白组外，在造模前6 d，每隔1天予小鼠腹部皮下注射苯甲酸雌二醇油剂诱导假发情；发情成功后开始建模，继续皮下注射苯甲酸雌二醇油剂，予小鼠阴道接种2 × 109 CFU/ml白念珠菌菌悬液，每天1次，连续5 d；1-MT组和IFN-γ组分别在接种菌悬液前1 d予1-MT或IFN-γ预处理，之后每天1次，连续干预6 d；空白组和VVC模型组给予相应的生理氯化钠溶液。在造模第5天时，观察小鼠阴道情况，并进行阴道症状评分；收集阴道灌洗液涂片镜检和真菌载荷计数；随后处死小鼠，收集阴道组织，分别进行苏木精-伊红（HE）染色及过碘酸希夫（PAS）染色，免疫荧光法检测组织中IDO1和巨噬细胞表面标志物F4/80的表达；实时荧光定量PCR（qPCR）检测组织中IDO1、诱导型一氧化氮合酶（iNOS）、精氨酸酶1（Arg-1）mRNA表达水平，Western印迹检测组织中IDO1蛋白表达。采用单因素方差分析检验组间各指标的差异，Tukey检验进行两两多重比较。结果造模第5天，小鼠阴道灌洗液涂片镜检，VVC模型组中菌丝细长，见少量孢子；1-MT组大量细长菌丝聚集成团，周围可见孢子；IFN-γ组见少量细短菌丝，孢子较多。小鼠阴道灌洗液载菌量计数显示，与VVC模型组载菌量（360.0 ± 15.9）相比，1-MT组较高（523.7 ± 67.7，P = 0.002），而IFN-γ组较低（258.3 ± 27.6，P = 0.026）。HE染色和PAS染色显示，VVC模型组表皮局灶可见小脓肿形成，表皮及真皮全层见以中性粒细胞为主的炎症细胞浸润，且存在大量孢子，伴少量菌丝；1-MT组表皮增生、增厚，真皮可见大量以中性粒细胞为主的炎症细胞弥漫性浸润，表皮及真皮全层大量菌丝和孢子聚集成团，以菌丝为主；IFN-γ组表皮聚集孢子，未见明显菌丝，真皮见少量以中性粒细胞为主的炎症细胞浸润。免疫荧光检测显示，IFN-γ组IDO1相对荧光强度最高，而1-MT组F4/80相对荧光强度最高。Western印迹结果显示，VVC模型组IDO1蛋白表达显著高于空白组（P＜0.001）和1-MT组（P＜0.05），低于IFN-γ组（P＜0.05）。qPCR检测显示，VVC模型组iNOS mRNA表达高于空白组（P＜0.01），IFN-γ组高于空白组、VVC模型组和1-MT组（均P＜0.001）；VVC模型组Arg-1 mRNA表达显著高于空白组（P＜0.001）及IFN-γ组（P＜0.01），1-MT组显著高于空白组、VVC模型组和IFN-γ组（均P＜0.001）。结论在VVC小鼠模型中上调IDO1可能引起巨噬细胞向M1极化，抑制IDO1引起巨噬细胞募集增多，炎症反应加剧。

关键词: 白色念珠菌, 念珠菌病, 外阴阴道, 巨噬细胞, 吲哚胺2, 3-双加氧酶, 宿主免疫

Abstract: 【Abstract】 Objective To analyze functional changes in macrophages in mouse models of vulvovaginal candidiasis （VVC） by modulating indoleamine 2,3-dioxygenase 1 （IDO1）. Methods Forty specific-pathogen-free female ICR mice were randomly divided into 4 groups using a complete randomization method: a blank group, a VVC model group, a VVC model + 1-methyltryptophan （1-MT） group （referred to as the 1-MT group）, a VVC model + interferon-γ （IFN-γ） group （referred to as the IFN-γ group）, with 10 mice in each group. Except for the blank group, all the mice were injected subcutaneously with estradiol benzoate oil solution in the abdomen every other day for 6 days prior to modeling to induce pseudoestrus; after successful induction of pseudoestrus, the mice were inoculated vaginally with Candida albicans suspensions at a concentration of 2 × 109 CFU/ml once a day for 5 days to establish VVC mouse models, and subcutaneous injections of estradiol benzoate oil solution were continued simultaneously to maintain the pseudoestrus state; 1 day before inoculation with fungal suspensions, mice in the 1-MT group and IFN-γ group were pretreated with 1-MT and IFN-γ respectively, followed by once-daily same intervention for 6 consecutive days; mice in the blank group and VVC model group were intraperitoneally injected with physiological saline solution once a day for 6 consecutive days. On the 5th day of modeling, vaginal conditions in mice were observed and vaginal symptoms were scored; the vaginal lavage fluid was collected for smear microscopy and fungal colony counting; then, the mice were sacrificed, the vaginal tissues were collected and subjected to hematoxylin-eosin （HE） staining and periodic acid-Schiff （PAS） staining, and the expression of IDO1 and the macrophage surface marker F4/80 was determined in the vaginal tissues by an immunofluorescence method; real-time fluorescence-based quantitative PCR （qPCR） was performed to determine mRNA expression levels of IDO1, inducible nitric oxide synthase （iNOS）, and arginase 1 （Arg-1） in the vaginal tissues, and Western blot analysis to determine the IDO1 protein expression in the vaginal tissues. One-way analysis of variance was used to analyze the differences in indices among groups, and Tukey test was used for multiple comparisons. Results Smear microscopic examination of the vaginal lavage fluid on the 5th day of modeling showed elongated hyphae with a few spores in the VVC model group, a large number of elongated hyphae aggregating in clusters with surrounding spores in the 1-MT group, and a few thin and short hyphae with a large number of spores in the IFN-γ group. Compared with the VVC model group （360.0 ± 15.9）, the fungal colony counts in the vaginal lavage fluid significantly increased in the 1-MT group （523.7 ± 67.7, P = 0.002）, but significantly decreased in the IFN-γ group （258.3 ± 27.57, P = 0.026）. HE staining and PAS staining showed small abscess formation in the epidermis and predominant infiltration of neutrophils throughout the epidermal and dermal layers with a large number of spores and a few hyphae in the VVC model group; thickened epidermis and diffuse inflammatory infiltration predominated by neutrophils in the dermis were seen in the 1-MT group, with a large number of hyphae and spores aggregating into clusters, which were predominated by hyphae; in the IFN-γ group, spores aggregated in the epidermis without obvious hyphae, and a small amount of inflammatory cells predominated by neutrophils infiltrated the dermis. Immunofluorescence assay revealed that the relative fluorescence intensities of IDO1 and F4/80 were highest in the IFN-γ group and the 1-MT group, respectively. Western blot analysis revealed that the IDO1 protein expression in the VVC model group was significantly higher than that in the blank group （P < 0.001） and the 1-MT group （P < 0.05）, but significantly lower than that in the IFN-γ group （P < 0.05）. qPCR showed that iNOS mRNA expression significantly increased in the VVC model group compared with the blank group （P < 0.01）, and increased in the IFN-γ group compared with the blank group, VVC model group and 1-MT group （all P < 0.001）; Arg-1 mRNA expression significantly increased in the VVC model group compared with the blank group （P < 0.001） and IFN-γ group （P < 0.01）, and increased in the 1-MT group compared with the blank group, VVC model group, and IFN-γ group （all P < 0.001）. Conclusion In the VVC mouse models, upregulation of IDO1 may cause macrophage polarization toward the M1 phenotype, and inhibition of IDO1 may cause increased macrophage recruitment and exacerbate the inflammatory response.

Key words: Candida albicans, Candidiasis, vulvovaginal, Macrophages, IDO1, Host immunity

唐诗琴郝瑞英贺慧娜田亚楠徐艳艳李小静景婷婷. IDO1影响外阴阴道念珠菌病小鼠阴道组织中巨噬细胞功能变化的研究[J]. 中华皮肤科杂志, 2024,57(10):931-939. doi:10.35541/cjd.20240163

Tang Shiqin, Hao Ruiying, He Huina, Tian Yanan, Xu Yanyan, Li Xiaojing, Jing Tingting, . Effect of IDO1 on functional changes in macrophages in vaginal tissues from mouse models of vulvovaginal candidiasis[J]. Chinese Journal of Dermatology, 2024, 57(10): 931-939.doi:10.35541/cjd.20240163

参考文献 45

［1］	Senthilganesh J, Ravichandran S, Durairajan R, et al. Metal sulfide nanoparticles based phytolectin scaffolds inhibit vulvovaginal candidiasis causing Candida albicans［J］. J Clust Sci, 2021,33（4）:1361⁃1372. doi: 10.1007/s10876⁃021⁃02061⁃0.
［2］	Willems H, Ahmed SS, Liu J, et al. Vulvovaginal candidiasis: a current understanding and burning questions［J］. J Fungi （Basel）, 2020,6（1）:27. doi: 10.3390/jof6010027.
［3］	段志敏, 杜蕾蕾, 刘彩霞, 等. Dectin⁃1介导人急性单核细胞白血病细胞巨噬细胞样细胞吞噬白念珠菌的作用研究［J］. 中华皮肤科杂志, 2018,51（6）:425⁃428. doi: 10.3760/cma.j.issn. 0412⁃4030.2018.06.006.
［4］	König A, Hube B, Kasper L. The dual function of the fungal toxin candidalysin during Candida albicans⁃macrophage interaction and virulence［J］. Toxins （Basel）, 2020,12（8）:469. doi: 10.3390/toxins12080469.
［5］	Domingues N, Gonçalves T, Girao H. Phagolysosomal remodeling to confine Candida albicans in the macrophage［J］. Trends Microbiol, 2022,30（6）:519⁃523. doi: 10.1016/j.tim.2022.03.004.
［6］	Zhang Y, Tang C, Zhang Z, et al. Deletion of the ATP2 gene in Candida albicans blocks its escape from macrophage clearance［J］. Front Cell Infect Microbiol, 2021,11:643121. doi: 10.3389/fcimb.2021.643121.
［7］	Wang Y, Lin Q, Zhang H, et al. M2 macrophage⁃derived exosomes promote diabetic fracture healing by acting as an immunomodulator［J］. Bioact Mater, 2023,28:273⁃283. doi: 10. 1016/j.bioactmat.2023.05.018.
［8］	Cervenka I, Agudelo LZ, Ruas JL. Kynurenines: tryptophan's metabolites in exercise, inflammation, and mental health［J］. Science, 2017,357（6349）:eaaf9794. doi: 10.1126/science.aaf 9794.
［9］	Sorgdrager F, Naudé P, Kema IP, et al. Tryptophan metabolism in inflammaging: from biomarker to therapeutic target［J］. Front Immunol, 2019,10:2565. doi: 10.3389/fimmu.2019.02565.
［10］	Munn DH, Mellor AL. Indoleamine 2,3 dioxygenase and metabolic control of immune responses［J］. Trends Immunol, 2013,34（3）:137⁃143. doi: 10.1016/j.it.2012.10.001.
［11］	Lashgari NA, Roudsari NM, Shayan M, et al. IDO/kynurenine; novel insight for treatment of inflammatory diseases［J］. Cytokine, 2023,166:156206. doi: 10.1016/j.cyto.2023.156206.
［12］	Mellor AL, Munn DH. Tryptophan catabolism and T⁃cell tolerance: immunosuppression by starvation?［J］. Immunol Today, 1999,20（10）:469⁃473. doi: 10.1016/s0167⁃5699（99）01520⁃0.
［13］	Fallarino F, Grohmann U, You S, et al. The combined effects of tryptophan starvation and tryptophan catabolites down⁃regulate T cell receptor zeta⁃chain and induce a regulatory phenotype in naive T cells［J］. J Immunol, 2006,176（11）:6752⁃6761. doi: 10.4049/jimmunol.176.11.6752.
［14］	Bozza S, Fallarino F, Pitzurra L, et al. A crucial role for tryptophan catabolism at the host/Candida albicans interface［J］. J Immunol, 2005,174（5）:2910⁃2918. doi: 10.4049/jimmunol. 174.5.2910.
［15］	De Luca A, Carvalho A, Cunha C, et al. IL⁃22 and IDO1 affect immunity and tolerance to murine and human vaginal candidiasis［J］. PLoS Pathog, 2013,9（7）:e1003486. doi: 10.1371/journal.ppat.1003486.
［16］	Deng W, Su Z, Liang P, et al. Single⁃cell immune checkpoint landscape of PBMCs stimulated with Candida albicans［J］. Emerg Microbes Infect, 2021,10（1）:1272⁃1283. doi: 10.1080/22221751.2021.1942228.
［17］	Li H, Yuan Y, Chen H, et al. Indoleamine 2,3⁃dioxygenase mediates the therapeutic effects of adipose⁃derived stromal/stem cells in experimental periodontitis by modulating macrophages through the kynurenine⁃AhR⁃NRF2 pathway［J］. Mol Metab, 2022,66:101617. doi: 10.1016/j.molmet.2022.101617.
［18］	Ji R, Ma L, Chen X, et al. Characterizing the distributions of IDO⁃1 expressing macrophages/microglia in human and murine brains and evaluating the immunological and physiological roles of IDO⁃1 in RAW264.7/BV⁃2 cells［J］. PLoS One, 2021,16（11）:e0258204. doi: 10.1371/journal.pone.0258204.
［19］	Yeung AW, Terentis AC, King NJ, et al. Role of indoleamine 2,3⁃dioxygenase in health and disease［J］. Clin Sci （Lond）, 2015,129（7）:601⁃672. doi: 10.1042/CS20140392.
［20］	Ravishankar B, Liu H, Shinde R, et al. The amino acid sensor GCN2 inhibits inflammatory responses to apoptotic cells promoting tolerance and suppressing systemic autoimmunity［J］. Proc Natl Acad Sci U S A, 2015,112（34）:10774⁃10779. doi: 10.1073/pnas.1504276112.
［21］	Cady SG, Sono M. 1⁃Methyl⁃DL⁃tryptophan, beta⁃（3⁃benzofuranyl）⁃DL⁃alanine （the oxygen analog of tryptophan）, and beta⁃［3⁃benzo（b）thienyl］⁃DL⁃alanine （the sulfur analog of tryptophan） are competitive inhibitors for indoleamine 2,3⁃dioxygenase［J］. Arch Biochem Biophys, 1991,291（2）:326⁃333. doi: 10.1016/0003⁃9861（91）90142⁃6.
［22］	Knutson KL, Disis ML. Tumor antigen⁃specific T helper cells in cancer immunity and immunotherapy［J］. Cancer Immunol Immunother, 2005,54（8）:721⁃728. doi: 10.1007/s00262⁃004⁃0653⁃2.
［23］	Dang M, Zeng X, Chen B, et al. Interferon⁃γ mediates the protective effects of soluble receptor for advanced glycation end⁃product in myocardial ischemia/reperfusion［J］. Lab Invest, 2019,99（3）:358⁃370. doi: 10.1038/s41374⁃018⁃0102⁃z.
［24］	孔小锋, 陈琢. 昆明小鼠白色念珠菌性阴道炎模型构建条件的摸索［J］. 中西医结合研究, 2009,1（5）:236⁃240. doi: 10. 3870/j.issn.1674⁃4616.2009.05.004.
［25］	Curti A, Trabanelli S, Salvestrini V, et al. The role of indoleamine 2,3⁃dioxygenase in the induction of immune tolerance: focus on hematology［J］. Blood, 2009,113（11）:2394⁃2401. doi: 10.1182/blood⁃2008⁃07⁃144485.
［26］	Mándi Y, Stone TW, Guillemin GJ, et al. Editorial: multiple implications of the kynurenine pathway in inflammatory diseases: diagnostic and therapeutic applications［J］. Front Immunol, 2022,13:860867. doi: 10.3389/fimmu.2022.860867.
［27］	Lee SM, Park HY, Suh YS, et al. Inhibition of acute lethal pulmonary inflammation by the IDO⁃AhR pathway［J］. Proc Natl Acad Sci U S A, 2017,114（29）:E5881⁃E5890. doi: 10.1073/pnas.1615280114.
［28］	Romani L, Zelante T, De Luca A, et al. Indoleamine 2,3⁃dioxygenase （IDO） in inflammation and allergy to Aspergillus［J］. Med Mycol, 2009,47（Suppl 1）:S154⁃161. doi: 10.1080/13693780802139867.
［29］	Zelante T, Pieraccini G, Scaringi L, et al. Learning from other diseases: protection and pathology in chronic fungal infections［J］. Semin Immunopathol, 2016,38（2）:239⁃248. doi: 10.1007/s00281⁃015⁃0523⁃3.
［30］	Choera T, Zelante T, Romani L, et al. A multifaceted role of tryptophan metabolism and indoleamine 2,3⁃dioxygenase activity in Aspergillus fumigatus⁃host interactions［J］. Front Immunol, 2017,8:1996. doi: 10.3389/fimmu.2017.01996.
［31］	Fidel PL Jr, Sobel JD. Immunopathogenesis of recurrent vulvovaginal candidiasis［J］. Clin Microbiol Rev, 1996,9（3）:335⁃348. doi: 10.1128/CMR.9.3.335.
［32］	Yano J, Peters BM, Noverr MC, et al. Novel mechanism behind the immunopathogenesis of vulvovaginal candidiasis: "neutrophil anergy"［J］. Infect Immun, 2018,86（3）:e00684⁃00617. doi: 10. 1128/IAI.00684⁃17.
［33］	Silva MT. Macrophage phagocytosis of neutrophils at inflammatory/infectious foci: a cooperative mechanism in the control of infection and infectious inflammation［J］. J Leukoc Biol, 2011,89（5）:675⁃683. doi: 10.1189/jlb.0910536.
［34］	Patin EC, Thompson A, Orr SJ. Pattern recognition receptors in fungal immunity［J］. Semin Cell Dev Biol, 2019,89:24⁃33. doi: 10.1016/j.semcdb.2018.03.003.
［35］	Wu MY, Lu JH. Autophagy and macrophage functions: inflammatory response and phagocytosis［J］. Cells, 2019,9（1）:70. doi: 10.3390/cells9010070.
［36］	Wang Y, Li H, Xu Z, et al. Exosomes released by Brucella⁃infected macrophages inhibit the intracellular survival of Brucella by promoting the polarization of M1 macrophages［J］. Microb Biotechnol, 2023,16（7）:1524⁃1535. doi: 10.1111/1751⁃7915.14274.
［37］	Zhang L, Zhang K, Li H, et al. Cryptococcus neoformans⁃infected macrophages release proinflammatory extracellular vesicles: insight into their components by multi⁃omics［J］. mBio, 2021,12（2）:e00279⁃00221. doi: 10.1128/mBio.00279⁃21.
［38］	Brauer VS, Pessoni AM, Bitencourt TA, et al. Extracellular vesicles from Aspergillus flavus induce M1 polarization in vitro［J］. mSphere, 2020,5（3）:e00190⁃00120. doi: 10.1128/mSphere. 00190⁃20.
［39］	Yu F, Jiang W, Zhang L, et al. IDO regulates macrophage functions by inhibiting the CCL2/CCR2 signaling pathway in fungal keratitis［J］. Cornea, 2023,42（8）:1005⁃1015. doi: 10. 1097/ICO.0000000000003309.
［40］	Lin L, Wang M, Zeng J, et al. Sequence variation of Candida albicans Sap2 enhances fungal pathogenicity via complement evasion and macrophage M2⁃like phenotype induction［J］. Adv Sci （Weinh）, 2023,10（20）:e2206713. doi: 10.1002/advs.2022 06713.
［41］	Wang XF, Wang HS, Wang H, et al. The role of indoleamine 2,3⁃dioxygenase （IDO） in immune tolerance: focus on macrophage polarization of THP⁃1 cells［J］. Cell Immunol, 2014,289（1⁃2）:42⁃48. doi: 10.1016/j.cellimm.2014.02.005.
［42］	Lee S, Zhang QZ, Karabucak B, et al. DPSCs from inflamed pulp modulate macrophage function via the TNF⁃α/IDO axis［J］. J Dent Res, 2016,95（11）:1274⁃1281. doi: 10.1177/002203451 6657817.
［43］	Jiang N, Zhao GQ, Lin J, et al. Expression of indoleamine 2,3⁃dioxygenase in a murine model of Aspergillus fumigatus keratitis［J］. Int J Ophthalmol, 2016,9（4）:491⁃496. doi: 10.18240/ijo. 2016.04.03.
［44］	Hill M, Tanguy⁃Royer S, Royer P, et al. IDO expands human CD4+CD25high regulatory T cells by promoting maturation of LPS⁃treated dendritic cells［J］. Eur J Immunol, 2007,37（11）:3054⁃3062. doi: 10.1002/eji.200636704.
［45］	Bracho⁃Sanchez E, Rocha FG, Bedingfield SK, et al. Suppression of local inflammation via galectin⁃anchored indoleamine 2,3⁃dioxygenase［J］. Nat Biomed Eng, 2023,7（9）:1156⁃1169. doi: 10.1038/s41551⁃023⁃01025⁃1.

[1]	李硕孙袁媛郝瑞英徐艳艳刘钊景婷婷李小静张秀娟. 巨噬细胞来源外泌体对白念珠菌形态转换的影响[J]. 中华皮肤科杂志, 2024, 57(6): 539-546.
[2]	赵莹杨勇王焱魏琴王烨涛. 巨噬细胞在瘢痕疙瘩发病机制及治疗中的研究进展[J]. 中华皮肤科杂志, 2024, 0(3): 20240090-e20240090.
[3]	杨璐段志敏何艳艳王嘉宁陈青, 陈旭, 李岷, . 白念珠菌诱导小鼠骨髓来源巨噬细胞焦亡的初步研究[J]. 中华皮肤科杂志, 2023, 56(4): 301-308.
[4]	张瑞珺苏小睿李婷何肖杨元文康玉英. 山西省某三甲医院黏膜念珠菌病病原菌和耐药性分析[J]. 中华皮肤科杂志, 2023, 56(1): 56-58.
[5]	王晓雯李若瑜. 白细胞介素17相关生物制剂治疗银屑病过程中浅部真菌感染的发生及应对策略[J]. 中华皮肤科杂志, 2022, 55(3): 272-275.
[6]	杨璐段志敏李岷. 白念珠菌对棘白菌素类药物耐药机制的研究进展[J]. 中华皮肤科杂志, 2022, 55(12): 1114-1117.
[7]	杨璐段志敏徐松陈旭李岷. 烟曲霉对小鼠巨噬细胞自噬流的影响初步研究[J]. 中华皮肤科杂志, 2022, 55(11): 962-968.
[8]	丁甜甜崔宝红米淑宏张杨郑海林石继海刘维达. 浅部与深部感染来源白念珠菌氟康唑耐药株药物敏感性及耐药基因突变比较[J]. 中华皮肤科杂志, 2022, 55(10): 874-878.
[9]	杨瑞孔庆涛许洁张晨桑红. 复发性念珠菌颈部淋巴结炎1例易感基因筛查及免疫学研究[J]. 中华皮肤科杂志, 2022, 55(1): 50-54.
[10]	张海妮寇彩霞刘进权张瑞华马印尼张瑞丽王千秋. 梅毒螺旋体对巨噬细胞极化的诱导作用[J]. 中华皮肤科杂志, 2021, 54(8): 688-695.
[11]	林泽杭段志敏徐松陈旭李岷. 白念珠菌菌丝调控小鼠巨噬细胞自噬关键分子微管相关蛋白1轻链3的实验研究[J]. 中华皮肤科杂志, 2021, 54(3): 189-195.
[12]	王若珺李若瑜. 白细胞介素17A及其受体拮抗剂治疗银屑病的不良反应[J]. 中华皮肤科杂志, 2021, 54(2): 170-173.
[13]	王昊珏房灵崔成军施启丰陆胜陆显义高利增. Fe3O4纳米酶对白念珠菌的体外抑制实验研究[J]. 中华皮肤科杂志, 2020, 53(7): 554-556.
[14]	吕妍张艳丽张展鹏赵亚婧张艺山李水秀张宏. ATP1通过调节氧化应激促进白念珠菌逃逸巨噬细胞杀伤的研究[J]. 中华皮肤科杂志, 2020, 53(7): 519-524.
[15]	郑国霞刘如锦齐燕王小波闫玉涛谭晓华杨磊. 病毒巨噬细胞炎症蛋白Ⅱ对293T细胞APOBEC3G表达的影响[J]. 中华皮肤科杂志, 2019, 52(9): 624-630.

IDO1影响外阴阴道念珠菌病小鼠阴道组织中巨噬细胞功能变化的研究

Effect of IDO1 on functional changes in macrophages in vaginal tissues from mouse models of vulvovaginal candidiasis

PDF

可视化

摘要/Abstract

引用本文

使用本文

参考文献 45

相关文章 15

Metrics

本文评价

推荐阅读 10