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卵黄囊组织三维培养的初步表征

Initial Characterization of 3D Culture of Yolk Sac Tissue.

作者信息

Pereira Vitória Mattos, Pinto Priscila Avelino Ferreira, Motta Lina Castelo Branco, Almeida Matheus F, de Andrade André Furugen Cesar, Pavaneli Ana Paula Pinoti, Ambrósio Carlos Eduardo

机构信息

Department of Veterinary Medicine, Faculty of Animal Science and Food Engineering (FZEA), University of São Paulo (USP), Pirassununga 13635-900, SP, Brazil.

School of Pharmacy, University of Wyoming, Laramie, WY 82072, USA.

出版信息

Animals (Basel). 2023 Apr 22;13(9):1435. doi: 10.3390/ani13091435.

Abstract

The role of the yolk sac (YS) in miscarriage is not yet clear, largely due to ethical reasons that make in vivo studies difficult to conduct. However, 3D cultures could provide a solution to this problem by enabling cells to be arranged in a way that more closely mimics the structure of the YS as it exists in vivo. In this study, three domestic species (porcine, canine, and bovine) were chosen as models to standardize 3D culture techniques for the YS. Two techniques of 3D culture were chosen: the Matrigel and Hanging-Drop techniques, and the 2D culture technique was used as a standardized method. The formed structures were initially characterized using scanning electron microscopy (SEM), immunohistochemistry (IHC), and quantitative real-time PCR (RT-qPCR). In general, the 3D culture samples showed better organization of the YS cells compared to 2D cultures. The formed structures from both 3D methods assemble the mesothelial layer of YS tissue. Regarding the IHC assay, all in vitro models were able to express zinc and cholesterol transport markers, although only 3D culture techniques were able to generate structures with different markers pattern, indicating a cell differentiation process when compared to 2D cultures. Regarding mRNA expression, the 3D models had a greater gene expression pattern on the Hemoglobin subunit zeta-like () gene related to the YS tissue, although no significant expression was found in Alpha-fetoprotein (), indicating a lack of endodermal differentiation in our 3D model. With the initial technique and characterization established, the next step is to maintain the cultures and characterize the diversity of cell populations, stemness, functions, and genetic stability of each 3D in vitro model.

摘要

卵黄囊(YS)在流产中的作用尚不清楚,这主要是由于伦理原因使得体内研究难以开展。然而,三维(3D)培养可为解决这一问题提供一种方法,它能使细胞以更接近体内存在的YS结构的方式排列。在本研究中,选择了三种家畜物种(猪、犬和牛)作为模型,以标准化YS的3D培养技术。选择了两种3D培养技术:基质胶和悬滴技术,并将二维(2D)培养技术用作标准化方法。最初使用扫描电子显微镜(SEM)、免疫组织化学(IHC)和定量实时聚合酶链反应(RT-qPCR)对形成的结构进行表征。总体而言,与2D培养相比,3D培养样本显示出YS细胞的组织性更好。两种3D方法形成的结构都组装了YS组织的间皮层。关于IHC分析,所有体外模型都能够表达锌和胆固醇转运标记物,尽管只有3D培养技术能够生成具有不同标记物模式的结构,这表明与2D培养相比存在细胞分化过程。关于mRNA表达,3D模型在与YS组织相关的血红蛋白亚基ζ样()基因上具有更大的基因表达模式,尽管在甲胎蛋白()中未发现显著表达,这表明我们的3D模型中缺乏内胚层分化。随着初始技术和表征的建立,下一步是维持培养并表征每个3D体外模型的细胞群体多样性、干性、功能和遗传稳定性。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/2f3a/10177165/772be459fd07/animals-13-01435-g001.jpg

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