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Isolation, culture, and characterization of chicken intestinal epithelial cells

免疫荧光 生物 细胞角蛋白 封堵器 细胞生物学 体外 细胞培养 绒毛 波形蛋白 肠粘膜 微生物学 上皮 肠上皮 免疫学 紧密连接 肌动蛋白 抗体 免疫组织化学 生物化学 内科学 医学 遗传学
作者
Federico Ghiselli,Barbara Rossi,Martina Felici,Maria Parigi,Giovanni Tosi,Laura Fiorentini,Paola Massi,Andrea Piva,Ester Grilli
出处
期刊:BMC molecular and cell biology [Springer Nature]
卷期号:22 (1) 被引量:21
标识
DOI:10.1186/s12860-021-00349-7
摘要

Abstract Background Enterocytes exert an absorptive and protective function in the intestine, and they encounter many different challenging factors such as feed, bacteria, and parasites. An intestinal epithelial in vitro model can help to understand how enterocytes are affected by these factors and contribute to the development of strategies against pathogens. Results The present study describes a novel method to culture and maintain primary chicken enterocytes and their characterization by immunofluorescence and biomolecular approaches. Starting from 19-day-old chicken embryos it was possible to isolate viable intestinal cell aggregates that can expand and produce a self-maintaining intestinal epithelial cell population that survives until 12 days in culture. These cells resulted positive in immunofluorescence to Cytokeratin 18, Zonula occludens 1, Villin, and Occludin that are common intestinal epithelial markers, and negative to Vimentin that is expressed by endothelial cells. Cells were cultured also on Transwell® permeable supports and trans-epithelial electrical resistance, was measured. This value gradually increased reaching 64 Ω*cm 2 7 days after seeding and it remained stable until day 12. Conclusions Based on these results it was confirmed that it is possible to isolate and maintain chicken intestinal epithelial cells in culture and that they can be suitable as in vitro intestinal model for further studies.
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