Mucosal affairs: glycosylation and expression changes of gill goblet cells and mucins in a fish-polyopisthocotylidan interaction

Enrique Riera-Ferrer; Raquel Del Pozo; Uxue Muñoz-Berruezo; Oswaldo Palenzuela; Ariadna Sitjà-Bobadilla; Itziar Estensoro; M Carla Piazzon

doi:10.3389/fvets.2024.1347707

Mucosal affairs: glycosylation and expression changes of gill goblet cells and mucins in a fish-polyopisthocotylidan interaction

Front Vet Sci. 2024 Apr 9:11:1347707. doi: 10.3389/fvets.2024.1347707. eCollection 2024.

Authors

Enrique Riera-Ferrer¹, Raquel Del Pozo¹, Uxue Muñoz-Berruezo¹, Oswaldo Palenzuela¹, Ariadna Sitjà-Bobadilla¹, Itziar Estensoro¹, M Carla Piazzon¹

Affiliation

¹ Fish Pathology Group, Instituto de Acuicultura Torre de la Sal, Consejo Superior de Investigaciones Científicas (IATS, CSIC), Castellón, Spain.

Abstract

Introduction: Secreted mucins are highly O-glycosylated glycoproteins produced by goblet cells in mucosal epithelia. They constitute the protective viscous gel layer overlying the epithelia and are involved in pathogen recognition, adhesion and expulsion. The gill polyopisthocotylidan ectoparasite Sparicotyle chrysophrii, feeds on gilthead seabream (Sparus aurata) blood eliciting severe anemia.

Methods: Control unexposed and recipient (R) gill samples of gilthead seabream experimentally infected with S. chrysophrii were obtained at six consecutive times (0, 11, 20, 32, 41, and 61 days post-exposure (dpe)). In histological samples, goblet cell numbers and their intensity of lectin labelling was registered. Expression of nine mucin genes (muc2, muc2a, muc2b, muc5a/c, muc4, muc13, muc18, muc19, imuc) and three regulatory factors involved in goblet cell differentiation (hes1, elf3, agr2) was studied by qPCR. In addition, differential expression of glycosyltransferases and glycosidases was analyzed in silico from previously obtained RNAseq datasets of S. chrysophrii-infected gilthead seabream gills with two different infection intensities.

Results and discussion: Increased goblet cell differentiation (up-regulated elf3 and agr2) leading to neutral goblet cell hyperplasia on gill lamellae of R fish gills was found from 32 dpe on, when adult parasite stages were first detected. At this time point, acute increased expression of both secreted (muc2a, muc2b, muc5a/c) and membrane-bound mucins (imuc, muc4, muc18) occurred in R gills. Mucins did not acidify during the course of infection, but their glycosylation pattern varied towards more complex glycoconjugates with sialylated, fucosylated and branched structures, according to lectin labelling and the shift of glycosyltransferase expression patterns. Gilthead seabream gill mucosal response against S. chrysophrii involved neutral mucus hypersecretion, which could contribute to worm expulsion and facilitate gas exchange to counterbalance parasite-induced hypoxia. Stress induced by the sparicotylosis condition seems to lead to changes in glycosylation characteristic of more structurally complex mucins.

Keywords: Sparicotyle chrysophrii; Sparus aurata; aquaculture; glycosyltransferase; lectin; mucin sequence; parasite; transcriptomics.

Grants and funding

The author(s) declare that financial support was received for the research, authorship, and/or publication of this article. This study was supported by the Spanish Ministry of Science and Innovation (MCIN/AEI/10.13039/501100011033) through the projects SpariControl (RTI2018-098664-B-I00), with AEI/FEDER, UE funding, and Mucosal Frontier (PID2020-115070RA-I00); the ThinkInAzul Programme supported by MICIN with funding from NextGeneration EU (PRTR-C17.I1), the Generalitat Valenciana (THINKINAZUL/2021/022), and the Generatitat Valenciana AICO2023 funding (CIAICO/2022/144). ER-F was supported by the FPI contract PRE2019-087409. MP was supported by the Ramón y Cajal fellowship (RYC2018-024049-I and ACOND/2022 Generalitat Valenciana), both funded by MICIN (MCIN/AEI/10.13039/501100011033) and co-funded by the European Social Fund (ESF), and UM-B was supported by the JAE Intro ICU grant from CSIC (JAEICU-21-IATS-07).