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细胞表面RNA表达调节肺泡上皮功能。

Cell Surface RNA Expression Modulates Alveolar Epithelial Function.

作者信息

Abledu Jubilant Kwame, Herbst Christopher J, Brandt Raphael, Kocak Alen, Ghosh Pritam, López Jacob L Gorenflos, Diestelhorst Kevin, Block Stephan, Hackenberger Christian, Seitz Oliver, Lopez-Rodriguez Elena, Gökeri Cengiz, Witzenrath Martin, Ochs Matthias, Kuebler Wolfgang M

机构信息

Institute of Physiology.

Department of Infectious Diseases, Respiratory Medicine, and Critical Care, Charité - Universitätsmedizin Berlin, Berlin, Germany.

出版信息

Am J Respir Cell Mol Biol. 2025 Sep;73(3):466-478. doi: 10.1165/rcmb.2024-0284OC.

DOI:10.1165/rcmb.2024-0284OC
PMID:40042871
Abstract

Glycosylated RNA (glycoRNA) has recently emerged as a novel constituent of the glycocalyx on cell surfaces, yet its biological functions remain largely unexplored. In this report, we present the first analysis of glycoRNA expression and functionality in alveolar epithelial cells. To this end, we optimized new techniques for the detection of glycoRNA on living cell surfaces and in cell membrane-associated RNA samples through in-gel imaging after labeling with fluorescent dye conjugates. Specifically, we used conjugation of Cy5-hydrazide after mild oxidation with sodium periodate for detection of total cell surface sialoglycoRNA. Conjugation of dibenzocyclooctyne-sulfo-Cy5 in cells fed with tetraacetylated -azidoacetyl-mannosamine or 6-azido-L-fucose detected -formed sialoglycoRNA or fucoglycoRNA, respectively. Finally, biotinylated lectins in combination with infrared dye-conjugated streptavidin were used to differentiate between specific glycosidic linkages. Comparisons across primary alveolar epithelial cells and different alveolar epithelial-like cell lines revealed a cell-type-specific variation in glycoRNA abundance. Treatment of primary alveolar epithelial cells with an RNase cocktail reduced epithelial surface glycoRNA and was associated with a reduction in transepithelial electrical resistance and influenza A viral particle abundance. As such, the present work identifies glycoRNA as a novel component of the alveolar epithelial glycocalyx with potential relevance in epithelial barrier regulation and viral infection.

摘要

糖基化RNA(glycoRNA)最近已成为细胞表面糖萼的一种新型成分,但其生物学功能在很大程度上仍未得到探索。在本报告中,我们首次分析了肺泡上皮细胞中glycoRNA的表达和功能。为此,我们优化了新技术,通过用荧光染料共轭物标记后进行凝胶成像,来检测活细胞表面和细胞膜相关RNA样本中的glycoRNA。具体而言,我们在用高碘酸钠轻度氧化后使用Cy5-酰肼共轭来检测总细胞表面唾液酸糖基化RNA。在用四乙酰化叠氮乙酰甘露糖胺或6-叠氮基-L-岩藻糖喂养的细胞中,二苯并环辛炔-磺基-Cy5共轭分别检测到唾液酸糖基化RNA或岩藻糖糖基化RNA。最后,生物素化凝集素与红外染料共轭链霉亲和素结合使用,以区分特定的糖苷键。对原代肺泡上皮细胞和不同肺泡上皮样细胞系的比较揭示了glycoRNA丰度的细胞类型特异性差异。用核糖核酸酶混合物处理原代肺泡上皮细胞可降低上皮表面glycoRNA,并与跨上皮电阻和甲型流感病毒颗粒丰度的降低有关。因此,本研究确定glycoRNA是肺泡上皮糖萼的一种新成分,在调节上皮屏障和病毒感染方面具有潜在意义。

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引用本文的文献

1
GlycoRNA-L and glycoRNA-S mediate human monocyte adhesion via binding to Siglec-5.糖基化RNA-L和糖基化RNA-S通过与唾液酸结合免疫球蛋白样凝集素-5结合介导人类单核细胞黏附。
Biochim Biophys Acta Mol Cell Res. 2025 Jul 1;1872(7):120017. doi: 10.1016/j.bbamcr.2025.120017.