Low exposition to lithium prevents nephrogenic diabetes insipidus but not microcystic dilations of the collecting ducts in long‐term rat model

Author:

Tabibzadeh Nahid12ORCID,Klein Mathieu3ORCID,Try Mélanie12,Poupon Joël4,Houillier Pascal125,Klein Christophe6,Cheval Lydie12,Crambert Gilles12,Lasaad Samia12ORCID,Chevillard Lucie3,Megarbane Bruno37ORCID

Affiliation:

1. Laboratoire de Physiologie Rénale et Tubulopathies, Centre de Recherche des Cordeliers, INSERM Sorbonne Université, Université Paris Cité Paris France

2. EMR 8228 Unité Métabolisme et Physiologie Rénale, CNRS Paris France

3. Inserm UMRS‐1144 Université Paris Cité Paris France

4. Department of Biological Toxicology, AP‐HP, Lariboisière Hospital University Paris VII Paris France

5. Assistance Publique‐Hôpitaux de Paris, Hôpital Européen Georges Pompidou, Service de Physiologie Paris France

6. Centre d'Histologie, d'Imagerie et de Cytométrie (CHIC), Centre de Recherche des Cordeliers, INSERM Sorbonne Université, Université de Paris Paris France

7. Department of Medical and Toxicological Critical Care Lariboisière Hospital, Federation of Toxicology, APHP Paris France

Abstract

AbstractLithium induces nephrogenic diabetes insipidus (NDI) and microcystic chronic kidney disease (CKD). As previous clinical studies suggest that NDI is dose‐dependent and CKD is time‐dependent, we investigated the effect of low exposition to lithium in a long‐term experimental rat model. Rats were fed with a normal diet (control group), with the addition of lithium (Li+ group), or with lithium and amiloride (Li+/Ami group) for 6 months, allowing obtaining low plasma lithium concentrations (0.25 ± 0.06 and 0.43 ± 0.16 mmol/L, respectively). Exposition to low concentrations of plasma lithium levels prevented NDI but not microcystic dilations of kidney tubules, which were identified as collecting ducts (CDs) on immunofluorescent staining. Both hypertrophy, characterized by an increase in the ratio of nuclei per tubular area, and microcystic dilations were observed. The ratio between principal cells and intercalated cells was higher in microcystic than in hypertrophied tubules. There was no correlation between AQP2 messenger RNA levels and cellular remodeling of the CD. Additional amiloride treatment in the Li+/Ami group did not allow consistent morphometric and cellular composition changes compared to the Li+ group. Low exposition to lithium prevented overt NDI but not microcystic dilations of the CD, with differential cellular composition in hypertrophied and microcystic CDs, suggesting different underlying cellular mechanisms.

Funder

Agence Nationale de la Recherche

Publisher

Wiley

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