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Giantin mediates Golgi localization of Gal3-O-sulfotransferases and affects salivary mucin sulfation in patients with Sjögren’s disease
Matilde Nuñez, … , María-Julieta González, Isabel Castro
Matilde Nuñez, … , María-Julieta González, Isabel Castro
Published October 10, 2024
Citation Information: JCI Insight. 2024;9(22):e171585. https://doi.org/10.1172/jci.insight.171585.
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Research Article Cell biology

Giantin mediates Golgi localization of Gal3-O-sulfotransferases and affects salivary mucin sulfation in patients with Sjögren’s disease

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Abstract

Sjögren’s disease is a chronic autoimmune disease characterized by symptoms of oral and ocular dryness and extraglandular manifestations. Mouth dryness is not only due to reduced saliva volume, but also to alterations in the quality of salivary mucins in patients with Sjögren’s disease. Mucins play a leading role in mucosa hydration and protection, where sulfated and sialylated oligosaccharides retain water molecules at the epithelial surface. The correct localization of glycosyltransferases and sulfotransferases within the Golgi apparatus determines adequate O-glycosylation and sulfation of mucins, which depends on specific golgins that tether enzyme-bearing vesicles. Here, we show that a golgin called Giantin was mislocalized in salivary glands from patients with Sjögren’s disease and formed protein complexes with Gal3-O-sulfotransferases (Gal3STs), which changed their localization in Giantin-knockout and -knockdown cells. Our results suggest that Giantin could tether Gal3ST-bearing vesicles and that its altered localization could affect Gal3ST activity, explaining the decreased sulfation of MUC5B observed in salivary glands from patients with Sjögren’s disease.

Authors

Matilde Nuñez, Patricia Carvajal, Sergio Aguilera, María-José Barrera, Soledad Matus, Alicia Couto, Malena Landoni, Gaelle Boncompain, Sergio González, Claudio Molina, Karina Pino, Sebastián Indo, Lourdes Figueroa, María-Julieta González, Isabel Castro

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Figure 8

Altered Gal3ST-4 localization in TNF-α–stimulated HSG cells.

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Altered Gal3ST-4 localization in TNF-α–stimulated HSG cells.
Representat...
Representative micrographs of (A–D) nontreated (NT) HSG cells or (E–H) HSG cells stimulated with 10 ng/mL TNF-α for 24 hours. (A and E) The merged RGB channels of the double staining of Giantin (green) and GM130 (red). (B and F) The green channel of the double staining of Gal3ST-4 (green) and GMAP210 (red). (C and G) The merged RGB channels. (D and H) The merged RGB channels of the double staining of GRP78 (green) and GM130 (red). Hoechst 33342 (blue) was used for nuclear staining. Scale bars: 10 μm. (I) Box plot showing the quantification of Gal3ST-4 staining. Boxes represent the 25th–75th percentiles; the lines within the boxes represent the median; and the whiskers represent the minimum and maximum. *P < 0.05 was considered significant using the Mann-Whitney test.

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