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首页> 外文期刊>Stem Cell Research & Therapy >Fluorescence-based tracing of transplanted intestinal epithelial cells using confocal laser endomicroscopy
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Fluorescence-based tracing of transplanted intestinal epithelial cells using confocal laser endomicroscopy

机译:共聚焦激光内镜检查基于荧光的移植肠上皮细胞示踪

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Intestinal stem cell transplantation has been shown to promote mucosal healing and to engender fully functional epithelium in experimental colitis. Hence, stem cell therapies may provide an innovative approach to accomplish mucosal healing in patients with debilitating conditions such as inflammatory bowel disease. However, an approach to label and trace transplanted cells, in order to assess engraftment efficiency and to monitor wound healing, is a key hurdle to overcome prior to initiating human studies. Genetic engineering is commonly employed in animal studies, but may be problematic in humans due to potential off-target and long-term adverse effects. We investigated the applicability of a panel of fluorescent dyes and nanoparticles to label intestinal organoids for visualization using the clinically approved imaging modality, confocal laser endomicroscopy (CLE). Staining homogeneity, durability, cell viability, differentiation capacity, and organoid forming efficiency were evaluated, together with visualization of labeled organoids in vitro and ex vivo using CLE. 5-Chloromethylfluorescein diacetate (CMFDA) proved to be suitable as it efficiently stained all organoids without transfer to unstained organoids in co-cultures. No noticeable adverse effects on viability, organoid growth, or stem cell differentiation capacity were observed, although single-cell reseeding revealed a dose-dependent reduction in organoid forming efficiency. Labeled organoids were easily identified in vitro using CLE for a duration of at least 3?days and could additionally be detected ex vivo following transplantation into murine experimental colitis. It is highly feasible to use fluorescent dye-based labeling in combination with CLE to trace intestinal organoids following transplantation to confirm implantation at the intestinal target site.
机译:肠干细胞移植已显示出可促进粘膜愈合并在实验性结肠炎中产生功能全面的上皮细胞。因此,干细胞疗法可以为患有诸如炎症性肠病之类的衰弱性疾病的患者提供粘膜愈合的创新方法。然而,标记和追踪移植细胞以评估植入效率和监测伤口愈合的方法是在开始人类研究之前要克服的关键障碍。基因工程通常用于动物研究中,但由于潜在的脱靶和长期不良影响,在人类中可能会出现问题。我们调查了一组荧光染料和纳米粒子在使用临床认可的成像方式,共聚焦激光内窥镜检查(CLE)进行可视化标记肠类器官的过程中的适用性。评估染色的均质性,耐久性,细胞活力,分化能力和类器官形成效率,以及使用CLE在体外和离体显示可视化的类器官。 5-氯甲基荧光素二乙酸酯(CMFDA)被证明是合适的,因为它可以有效地染色所有类器官,而不会在共培养物中转移到未染色的类器官。没有观察到对存活率,类器官生长或干细胞分化能力的明显不利影响,尽管单细胞再接种显示出类器官形成效率的剂量依赖性降低。标记的类器官很容易在体外使用CLE鉴定,持续时间至少3天,并且可以在移植到鼠类实验性结肠炎中后进行离体检测。在移植后使用基于荧光染料的标记与CLE结合以追踪肠道类器官是非常可行的,以确认在肠道目标部位的植入。

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