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活功能测定揭示了肾类器官中跨上皮运输的纵向成熟。

Live functional assays reveal longitudinal maturation of transepithelial transport in kidney organoids.

作者信息

Rizki-Safitri Astia, Gupta Navin, Hiratsuka Ken, Kobayashi Kenichi, Zhang Chengcheng, Ida Kazumi, Satlin Lisa M, Morizane Ryuji

机构信息

Nephrology Division, Massachusetts General Hospital, Boston, MA, United States.

Department of Medicine, Harvard Medical School, Boston, MA, United States.

出版信息

Front Cell Dev Biol. 2022 Aug 15;10:978888. doi: 10.3389/fcell.2022.978888. eCollection 2022.

Abstract

Kidney organoids derived from hPSCs have opened new opportunities to develop kidney models for preclinical studies and immunocompatible kidney tissues for regeneration. Organoids resemble native nephrons that consist of filtration units and tubules, yet little is known about the functional capacity of these organoid structures. Transcriptomic analyses provide insight into maturation and transporter activities that represent kidney functions. However, functional assays in organoids are necessary to demonstrate the activity of these transport proteins in live tissues. The three-dimensional (3D) architecture adds complexity to real-time assays in kidney organoids. Here, we develop a functional assay using live imaging to assess transepithelial transport of rhodamine 123 (Rh123), a fluorescent substrate of P-glycoprotein (P-gp), in organoids affixed to coverslip culture plates for accurate real-time observation. The identity of organoid structures was probed using Lotus Tetragonolobus Lectin (LTL), which binds to glycoproteins present on the surface of proximal tubules. Within 20 min of the addition of Rh123 to culture media, Rh123 accumulated in the tubular lumen of organoids. Basolateral-to-apical accumulation of the dye/marker was reduced by pharmacologic inhibition of MDR1 or OCT2, and OCT2 inhibition reduced the Rh123 uptake. The magnitude of Rh123 transport was maturation-dependent, consistent with MDR1 expression levels assessed by RNA-seq and immunohistochemistry. Specifically, organoids on day 21 exhibit less accumulation of Rh123 in the lumen unlike later-stage organoids from day 30 of differentiation. Our work establishes a live functional assessment in 3D kidney organoids, enabling the functional phenotyping of organoids in health and disease.

摘要

源自人多能干细胞的肾类器官为开发用于临床前研究的肾脏模型以及用于再生的免疫相容性肾脏组织带来了新机遇。类器官类似于由过滤单元和肾小管组成的天然肾单位,但对这些类器官结构的功能能力了解甚少。转录组分析有助于深入了解代表肾脏功能的成熟和转运体活性。然而,类器官中的功能测定对于证明这些转运蛋白在活组织中的活性是必要的。三维(3D)结构增加了肾类器官实时测定的复杂性。在这里,我们开发了一种功能测定方法,使用活细胞成像来评估罗丹明123(Rh123)的跨上皮转运,Rh123是P-糖蛋白(P-gp)的荧光底物,在固定于盖玻片培养板上的类器官中进行准确的实时观察。使用莲四棱豆凝集素(LTL)探测类器官结构的特征,LTL与近端小管表面存在的糖蛋白结合。在向培养基中添加Rh123后20分钟内,Rh123在类器官的肾小管腔中积累。通过对MDR1或OCT2的药理抑制,染料/标记物从基底外侧到顶端的积累减少,并且OCT2抑制降低了Rh123的摄取。Rh123转运的程度取决于成熟度,这与通过RNA测序和免疫组织化学评估的MDR1表达水平一致。具体而言,与分化第30天的后期类器官不同,第21天的类器官在管腔中Rh123的积累较少。我们的工作建立了3D肾类器官的活功能评估,能够对健康和疾病状态下的类器官进行功能表型分析。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/1aa9/9420851/b9e8e1509b0e/fcell-10-978888-g001.jpg

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