Microencapsulation of cellular aggregates composed of differentiated insulin and glucagon-producing cells from human mesenchymal stem cells derived from adipose tissue

Claudia Jara; Felipe Oyarzun-Ampuero; Flavio Carrión; Esteban González-Echeverría; Claudio Cappelli; Pablo Caviedes

doi:10.1186/s13098-020-00573-9

Diabetology & Metabolic Syndrome (Aug 2020)

Microencapsulation of cellular aggregates composed of differentiated insulin and glucagon-producing cells from human mesenchymal stem cells derived from adipose tissue

Claudia Jara,
Felipe Oyarzun-Ampuero,
Flavio Carrión,
Esteban González-Echeverría,
Claudio Cappelli,
Pablo Caviedes

Affiliations

Claudia Jara: Programa de Farmacología Molecular y Clínica, ICBM, Facultad de Medicina, Universidad de Chile
Felipe Oyarzun-Ampuero: Advanced Center of Chronic Diseases (ACCDiS), Universidad de Chile
Flavio Carrión: Programa de Inmunología Traslacional, Facultad de Medicina, Clínica Alemana Universidad del Desarrollo
Esteban González-Echeverría: Programa de Farmacología Molecular y Clínica, ICBM, Facultad de Medicina, Universidad de Chile
Claudio Cappelli: Laboratorio de Patología Molecular, Instituto de Bioquímica y Microbiología, Facultad de Ciencias, Universidad Austral de Chile
Pablo Caviedes: Programa de Farmacología Molecular y Clínica, ICBM, Facultad de Medicina, Universidad de Chile

DOI: https://doi.org/10.1186/s13098-020-00573-9
Journal volume & issue: Vol. 12, no. 1
pp. 1 – 11

Abstract

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Abstract Background In type I diabetes mellitus (T1DM) pancreatic β cells are destroyed. Treatment entails exogenous insulin administration and strict diet control, yet optimal glycemic control is hardly attainable. Islet transplant could be an alternative in patients with poor glycemic control, but inefficient islet purification and autoimmune response of patients is still a challenge. For these reasons, it is necessary to explore new cellular sources and immunological isolation methods oriented to develop T1DM cell-based therapies. Aims We postulate human adipose-derived stem cell (hASC) as an adequate source to generate pancreatic islet cells in vitro, and to produce islet-like structures. Furthermore, we propose microencapsulation of these aggregates as an immunological isolation strategy. Methods hASC obtained from lipoaspirated fat tissue from human donors were differentiated in vitro to insulin (Ins) and glucagon (Gcg) producing cells. Then, insulin producing cells (IPC) and glucagon producing cells (GPC) were cocultured in low adhesion conditions to form cellular aggregates, and later encapsulated in a sodium alginate polymer. Expression of pancreatic lineage markers and secretion of insulin or glucagon in vitro were analyzed. Results The results show that multipotent hASC efficiently differentiate to IPC and GPC, and express pancreatic markers, including insulin or glucagon hormones which they secrete upon stimulation (fivefold for insulin in IPC, and fourfold for glucagon, compared to undifferentiated cells). In turn, calculation of the Feret diameter and area of cellular aggregates revealed mean diameters of ~ 80 µm, and 65% of the aggregates reached 4000 µm2 at 72 h of formation. IPC/GPC aggregates were then microencapsulated in sodium-alginate polymer microgels, which were found to be more stable when stabilized with Ba2+, yielding average diameters of ~ 300 µm. Interestingly, Ba2+-microencapsulated aggregates respond to high external glucose with insulin secretion. Conclusions The IPC/GPC differentiation process from hASC, followed by the generation of cellular aggregates that are later microencapsulated, could represent a possible treatment for T1DM.

Published in Diabetology & Metabolic Syndrome

ISSN: 1758-5996 (Online)
Publisher: BMC
Country of publisher: United Kingdom
LCC subjects: Medicine: Internal medicine: Specialties of internal medicine: Nutritional diseases. Deficiency diseases
Website: https://dmsjournal.biomedcentral.com

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