Cathepsin B pH-Dependent Activity Is Involved in Lysosomal Dysregulation in Atrophic Age-Related Macular Degeneration

Author:

Voisin Audrey123ORCID,Monville Christelle45ORCID,Plancheron Alexandra46,Béré Emile17,Gaillard Afsaneh12,Leveziel Nicolas123

Affiliation:

1. University of Poitiers, Laboratoire de Neurosciences Expérimentales et Cliniques, Equipe Thérapie Cellulaire dans les Pathologies Cérébrales, Poitiers F-86073, France

2. INSERM, U1084, Laboratoire de Neurosciences Expérimentales et Cliniques, Equipe Thérapie Cellulaire dans les Pathologies Cérébrales, Poitiers F-86022, France

3. CHU Poitiers, Poitiers F-86021, France

4. INSERM, UMR861, I-Stem, AFM, Genopole Campus 1, Evry F-91030, France

5. UEVE-Paris Saclay, UMR861, I-Stem, AFM, CRCT, Corbeil-Essonnes F-91100, France

6. CECS/I-Stem AFM, CRCT, Corbeil-Essonnes F-91100, France

7. Plateforme ImageUP, 1 Rue Georges Bonnet, F-86022 Poitiers, France

Abstract

Age-related macular degeneration (AMD) is characterized by retinal pigment epithelial (RPE) cell dysfunction beginning at early stages of the disease. The lack of an appropriate in vitro model is a major limitation in understanding the mechanisms leading to the occurrence of AMD. This study compared human-induced pluripotent stem cell- (hiPSC-) RPE cells derived from atrophic AMD patients (77y/o±7) to hiPSC-RPE cells derived from healthy elderly individuals with no drusen or pigmentary alteration (62.5y/o±17.5). Control and AMD hiPSC-RPE cell lines were characterized by immunofluorescence, flow cytometry, and electronic microscopy. The toxicity level of iron after Fe-NTA treatment was evaluated by an MTT test and by the detection of dichloro-dihydro-fluorescein diacetate. Twelve hiPSC-RPE cell lines (6 AMD and 6 controls) were used for the experiment. Under basal conditions, all hiPSC-RPE cells expressed a phenotypic profile of senescent cells with rounded mitochondria at passage 2. However, the treatment with Fe-NTA induced higher reactive oxygen species production and cell death in hiPSC-RPE AMD cells than in hiPSC-RPE Control cells. Interestingly, functional analysis showed differences in lysosomal activity between the two populations. Indeed, Cathepsin B activity was higher in hiPSC-RPE AMD cells compared to hiPSC-RPE Control cells in basal condition and link to a pH more acidic in this cell population. Moreover, oxidative stress exposure leads to an increase of Cathepsin D immature form levels in both populations, but in a higher proportion in hiPSC-RPE AMD cells. These findings could demonstrate that hiPSC-RPE AMD cells have a typical disease phenotype compared to hiPSC-RPE Control cells.

Funder

Region of Nouvelle Aquitaine

Publisher

Hindawi Limited

Subject

Cell Biology,Aging,General Medicine,Biochemistry

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