Optimization of BeWo model to investigate placental responses to Plasmodium falciparum infected erythrocytes.

MalariaWorld journal Pub Date : 2017-03-18 eCollection Date: 2017-01-01 DOI:10.5281/zenodo.10757455
Winifrida Kidima, Naveen Bobbili, Diane W Taylor
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Abstract

Background: Establishment of an in vitro model to study placental malaria is essential for understanding the biology and pathogenesis of placental malaria. We defined experimental variables for obtaining responses of BeWo cells to placental binding Plasmodium falciparum infected erythrocytes (IE, CS2 parasites).

Materials and methods: Experimental variables included i) concentration of forskolin, a cyclic adenosine monophosphate inducer important in the induction of syncytialisation of BeWo, ii) suitable period of incubating BeWo with forskolin, and iii) ratio of IE to BeWo cells and length of incubation to induce physiological changes in BeWo cells, including the vasculogenic factors vascular endothelial growth factor A (VEGFA), endoglin, and angiopoietin-2; an anti-angiogenic factor (inhibin A); a regulator of cell growth, mammalian target of rapamycin (mTOR); a chemokine (IL-8); and the cytokine macrophage inhibition factor. The human hormone, chorionic gonadotrophin was used as a marker for syncytialisation.

Results: We showed that 72 hrs incubation of BeWo with 10 μm forskolin resulted in higher levels of syncytialisation and hCG secretion. Overall, the best condition was to co-culture syncytialised BeWo with a 10:1 ratio of IE for 48 hours. Under these conditions, when co-cultured with IE, BeWo produced increased amounts of IL-8 (p=0.0001), VEGF (p=0.001) and endoglin (p=0.001).

Conclusion: The model can be used to evaluate the impact of IE, inflammatory cytokines and other factors associated with placental malaria on syncytiotrophoblast function.

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优化 BeWo 模型,研究胎盘对恶性疟原虫感染红细胞的反应。
背景:建立研究胎盘疟疾的体外模型对于了解胎盘疟疾的生物学和发病机制至关重要。我们定义了获得 BeWo 细胞对胎盘结合恶性疟原虫感染红细胞(IE,CS2 寄生虫)反应的实验变量:实验变量包括:i) 福斯可林的浓度,福斯可林是一种环磷酸腺苷诱导剂,对诱导 BeWo 细胞的合胞化很重要;ii) BeWo 细胞与福斯可林的合适孵育期;iii) IE 与 BeWo 细胞的比例和孵育时间,以诱导 BeWo 细胞发生生理变化,包括血管内皮生长因子 A(VEGFA)、内皮素和血管生成素-2;抗血管生成因子(抑制素 A)、细胞生长调节因子哺乳动物雷帕霉素靶标(mTOR)、趋化因子(IL-8)和细胞因子巨噬细胞抑制因子。人类激素绒毛膜促性腺激素被用作合胞化的标记物:结果:我们发现,BeWo 与 10 μm 福斯克林孵育 72 小时会导致更高水平的合胞化和 hCG 分泌。总体而言,最佳条件是将合胞化的 BeWo 与 10:1 比例的 IE 共同培养 48 小时。在这些条件下,当与 IE 共同培养时,BeWo 产生的 IL-8 (p=0.0001)、VEGF (p=0.001) 和 endoglin (p=0.001) 的数量均有所增加:该模型可用于评估 IE、炎症细胞因子和其他与胎盘疟疾相关的因素对合胞滋养细胞功能的影响。
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