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基于流式细胞术从新生大鼠中分离真皮淋巴管内皮细胞

Flow cytometry-based isolation of dermal lymphatic endothelial cells from newborn rats.

作者信息

Thiele W, Rothley M, Schmaus A, Plaumann D, Sleeman J

出版信息

Lymphology. 2014 Dec;47(4):177-86.

Abstract

The lymphatic system plays a key role in tissue homeostasis, fatty acid transport, and immune surveillance. Pathologically, dysfunction of the lymphatic system results in edema, and increased lymphangiogenesis can contribute to tumor metastasis. Lymphatic vessels are composed of lymphatic endothelial cells (LECs) that can be identified by distinct marker molecules such as Prox-1, podoplanin, VEGFR-3 and LYVE-1. Primary LECs represent a valuable tool for the study of basic functions of the lymphatic system. However, their isolation remains a challenge, particularly if rodent tissues are used as a source. We developed a method for the isolation of rat dermal LECs from the skin of newborn rats based on sequential enzymatic digestion with trypsin and Liberase followed by flow cytometric sorting using LYVE-1 specific antibodies. Cells isolated according to this protocol expressed the lymphatic markers Prox-1, podoplanin, LYVE-1 and VEGFR-3, and displayed an endothelial-like morphology when taken into culture. These primary cells can be used for studying lymphatic biology in rat models, and the protocol we describe here therefore represents an important extension of the experimental repertoire available for rats and for modeling the human lymphatic system.

摘要

淋巴系统在组织稳态、脂肪酸运输和免疫监视中发挥关键作用。在病理情况下,淋巴系统功能障碍会导致水肿,而淋巴管生成增加会促进肿瘤转移。淋巴管由淋巴管内皮细胞(LECs)组成,这些细胞可通过Prox-1、血小板内皮细胞黏附分子-1、血管内皮生长因子受体-3和淋巴管内皮透明质酸受体-1等独特的标记分子来识别。原代LECs是研究淋巴系统基本功能的宝贵工具。然而,它们的分离仍然是一个挑战,特别是当使用啮齿动物组织作为来源时。我们开发了一种从新生大鼠皮肤中分离大鼠真皮LECs的方法,该方法基于用胰蛋白酶和 Liberase 进行顺序酶消化,然后使用淋巴管内皮透明质酸受体-1特异性抗体进行流式细胞术分选。按照该方案分离的细胞表达淋巴标记物Prox-1、血小板内皮细胞黏附分子-1、淋巴管内皮透明质酸受体-1和血管内皮生长因子受体-3,并且在培养时呈现内皮样形态。这些原代细胞可用于研究大鼠模型中的淋巴生物学,因此我们在此描述的方案代表了大鼠可用实验方法的重要扩展以及对人类淋巴系统进行建模的重要扩展。

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