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验证阴道微生物组替代物在模拟乳杆菌主导的阴道培养的体外实验中的有效性。

Validation of vaginal microbiome proxies for in vitro experiments that biomimic Lactobacillus-dominant vaginal cultures.

机构信息

School of Medicine, The University of Texas Medical Branch at Galveston, Galveston, Texas, USA.

Division of Basic Science and Translational Research, Department of Obstetrics and Gynecology, The University of Texas Medical Branch at Galveston, Galveston, Texas, USA.

出版信息

Am J Reprod Immunol. 2023 Dec;90(6):e13797. doi: 10.1111/aji.13797.

Abstract

The vaginal microbiome includes diverse microbiota dominated by Lactobacillus [L.] spp. that protect against infections, modulate inflammation, and regulate vaginal homeostasis. Because it is challenging to incorporate vaginal microbiota into in vitro models, including organ-on-a-chip systems, we assessed microbial metabolites as reliable proxies in addition to traditional vaginal epithelial cultures (VECs). Human immortalized VECs cultured on transwells with an air-liquid interface generated stratified cell layers colonized by transplanted healthy microbiomes (L. jensenii- or L. crispatus-dominant) or a community representing bacterial vaginosis (BV). After 48-h, a qPCR array confirmed the expected donor community profiles. Pooled apical and basal supernatants were subjected to metabolomic analysis (untargeted mass spectrometry) followed by ingenuity pathways analysis (IPA). To determine the bacterial metabolites' ability to recreate the vaginal microenvironment in vitro, pooled bacteria-free metabolites were added to traditional VEC cultures. Cell morphology, viability, and cytokine production were assessed. IPA analysis of metabolites from colonized samples contained fatty acids, nucleic acids, and sugar acids that were associated with signaling networks that contribute to secondary metabolism, anti-fungal, and anti-inflammatory functions indicative of a healthy vaginal microbiome compared to sterile VEC transwell metabolites. Pooled metabolites did not affect cell morphology or induce cell death (∼5.5%) of VEC cultures (n = 3) after 72-h. However, metabolites created an anti-inflammatory milieu by increasing IL-10 production (p = .06, T-test) and significantly suppressing pro-inflammatory IL-6 (p = .0001), IL-8 (p = .009), and TNFα (p = .0007) compared to naïve VEC cultures. BV VEC conditioned-medium did not affect cell morphology nor viability; however, it induced a pro-inflammatory environment by elevating levels of IL-6 (p = .023), IL-8 (p = .031), and TNFα (p = .021) when compared to L.-dominate microbiome-conditioned medium. VEC transwells provide a suitable ex vivo system to support the production of bacterial metabolites consistent with the vaginal milieu allowing subsequent in vitro studies with enhanced accuracy and utility.

摘要

阴道微生物组包括以乳杆菌属[L.] spp.为主的多样化微生物群,可预防感染、调节炎症和维持阴道稳态。由于将阴道微生物组纳入体外模型(包括器官芯片系统)具有挑战性,因此我们评估了微生物代谢产物作为传统阴道上皮培养物(VEC)的可靠替代物。在具有气液界面的 Transwell 上培养的人永生化 VEC 可形成分层细胞层,这些细胞层被移植的健康微生物组(以 L. jensenii 或 L. crispatus 为主)或代表细菌性阴道病(BV)的群落定植。48 小时后,qPCR 阵列确认了预期的供体群落谱。将混合的顶端和基底上清液进行代谢组学分析(非靶向质谱),然后进行 IPA 分析。为了确定细菌代谢产物在体外重现阴道微环境的能力,将无细菌的混合代谢产物添加到传统的 VEC 培养物中。评估细胞形态、活力和细胞因子产生。对定植样本的代谢产物进行 IPA 分析,其中包含与次级代谢、抗真菌和抗炎功能相关的信号网络有关的脂肪酸、核酸和糖酸,这表明与无菌 VEC Transwell 代谢物相比,阴道微生物组更健康。混合代谢产物在 72 小时后不会影响 VEC 培养物(n=3)的细胞形态或诱导细胞死亡(约 5.5%)。然而,代谢产物通过增加 IL-10 的产生(p=0.06,T 检验)并显著抑制促炎细胞因子 IL-6(p=0.0001)、IL-8(p=0.009)和 TNFα(p=0.0007),从而创造了抗炎环境与未成熟的 VEC 培养物相比。BV VEC 条件培养基不会影响细胞形态或活力;然而,与 L. 主导的微生物组条件培养基相比,它通过升高 IL-6(p=0.023)、IL-8(p=0.031)和 TNFα(p=0.021)的水平,诱导了促炎环境。VEC Transwell 为支持与阴道环境一致的细菌代谢产物的产生提供了一个合适的离体系统,从而允许随后的体外研究具有更高的准确性和实用性。

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