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原位揭示荧光曼氏血吸虫寄生虫以破解豆螺黑箱。

Breaking Biomphalaria black box by in situ revelation of fluorescent Schistosoma mansoni parasites.

机构信息

IHPE, Université de Perpignan Via Domitia, CNRS, Ifremer, Université de Montpellier, 58 avenue Paul Alduy, 66860, Perpignan, France.

Institut de Génomique Fonctionnelle, Université de Montpellier, CNRS, INSERM, 141 rue de la Cardonille, 34091, Montpellier, France.

出版信息

Fish Shellfish Immunol. 2024 Oct;153:109800. doi: 10.1016/j.fsi.2024.109800. Epub 2024 Aug 2.

DOI:10.1016/j.fsi.2024.109800
PMID:39096981
Abstract

Tissue clearing is an old-fashioned method developed in the 1900's and used to turn an opaque biological object into a 3D visualizable transparent structure. Developed and diversified over the last decade, this method is most of the time applied to mammals' tissues, and especially mouse and human tissues for cytological, histological and pathophysiological studies. Through autofluorescence, immunofluorescence, in situ hybridization, intercalating agents, fluorescent transfection markers or fluorescent particle uptake, optically cleared samples can be monitored to discover new biological structures and cellular interactions through 3D-visualization, which can be more challenging in some extend through classical histological methods. Most of the tissue clearing procedures have been developed for specific applications like endogenous fluorescence visualization, immunolabeling or for revealing specific organs. Thus, choosing the adapted protocol may be empirical for non-model species, especially for mollusks for which very little related literature is available. Herein, we suggest an effective optical tissue clearing procedure for the freshwater snail Biomphalaria glabrata, known as the intermediate host of the human parasite Schistosoma mansoni. This clearing procedure involves solvents with a minimal toxicity, preserves the endogenous fluorescence of labeled parasites inside snail tissues and is compatible with an immunolabeling procedure.

摘要

组织透明化是一种 20 世纪发展起来的古老方法,用于将不透明的生物物体转化为可 3D 可视化的透明结构。该方法在过去十年中得到了发展和多样化,主要应用于哺乳动物的组织,特别是用于细胞学、组织学和病理生理学研究的小鼠和人类组织。通过自发荧光、免疫荧光、原位杂交、嵌入剂、荧光转染标记物或荧光颗粒摄取,可对光学透明化样本进行监测,以通过 3D 可视化发现新的生物结构和细胞相互作用,这在某种程度上比经典的组织学方法更具挑战性。大多数组织透明化程序都是为特定的应用而开发的,例如内源性荧光可视化、免疫标记或用于显示特定器官。因此,对于非模式物种,特别是对于相关文献很少的软体动物,选择合适的方案可能是经验性的。在此,我们提出了一种针对淡水蜗牛生物玻利瓦尔(Biomphalaria glabrata)的有效光学组织透明化程序,该蜗牛是人类寄生虫曼氏血吸虫(Schistosoma mansoni)的中间宿主。该透明化程序涉及毒性最小的溶剂,可保留蜗牛组织内标记寄生虫的内源性荧光,并与免疫标记程序兼容。

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