Distinct microRNA and protein profiles of extracellular vesicles secreted from myotubes from morbidly obese donors with type 2 diabetes in response to electrical pulse stimulation

Vigdis Aas; Reidun Øvstebø; Berit Sletbakk Brusletto; Trude Aspelin; Anne-Marie Siebke Trøseid; Saba Qureshi; Desima Shitandi Otundo Eid; Ole Kristoffer Olstad; Tuula A Nyman; Kari Bente Foss Haug

doi:10.3389/fphys.2023.1143966

Distinct microRNA and protein profiles of extracellular vesicles secreted from myotubes from morbidly obese donors with type 2 diabetes in response to electrical pulse stimulation

Front Physiol. 2023 Mar 30:14:1143966. doi: 10.3389/fphys.2023.1143966. eCollection 2023.

Affiliations

¹ Department of Life Sciences and Health, Oslo Metropolitan University (OsloMet), Oslo, Norway.
² Department of Medical Biochemistry, Oslo University Hospital, Ullevål, Oslo, Norway.
³ Department of Immunology, University of Oslo, and Oslo University Hospital, Rikshospitalet, Oslo, Norway.

Abstract

Lifestyle disorders like obesity, type 2 diabetes (T2D), and cardiovascular diseases can be prevented and treated by regular physical activity. During exercise, skeletal muscles release signaling factors that communicate with other organs and mediate beneficial effects of exercise. These factors include myokines, metabolites, and extracellular vesicles (EVs). In the present study, we have examined how electrical pulse stimulation (EPS) of myotubes, a model of exercise, affects the cargo of released EVs. Chronic low frequency EPS was applied for 24 h to human myotubes isolated and differentiated from biopsy samples from six morbidly obese females with T2D, and EVs, both exosomes and microvesicles (MV), were isolated from cell media 24 h thereafter. Size and concentration of EV subtypes were characterized by nanoparticle tracking analysis, surface markers were examined by flow cytometry and Western blotting, and morphology was confirmed by transmission electron microscopy. Protein content was assessed by high-resolution proteomic analysis (LC-MS/MS), non-coding RNA was quantified by Affymetrix microarray, and selected microRNAs (miRs) validated by real time RT-qPCR. The size and concentration of exosomes and MV were unaffected by EPS. Of the 400 miRs identified in the EVs, EPS significantly changed the level of 15 exosome miRs, of which miR-1233-5p showed the highest fold change. The miR pattern of MV was unaffected by EPS. Totally, about 1000 proteins were identified in exosomes and 2000 in MV. EPS changed the content of 73 proteins in exosomes, 97 in MVs, and of these four were changed in both exosomes and MV (GANAB, HSPA9, CNDP2, and ATP5B). By matching the EPS-changed miRs and proteins in exosomes, 31 targets were identified, and among these several promising signaling factors. Of particular interest were CNDP2, an enzyme that generates the appetite regulatory metabolite Lac-Phe, and miR-4433b-3p, which targets CNDP2. Several of the regulated miRs, such as miR-92b-5p, miR-320b, and miR-1233-5p might also mediate interesting signaling functions. In conclusion, we have used a combined transcriptome-proteome approach to describe how EPS affected the cargo of EVs derived from myotubes from morbidly obese patients with T2D, and revealed several new factors, both miRs and proteins, that might act as exercise factors.

Keywords: electrical pulse stimulation (EPS); extracellular vescicles; human myotubes; microRNA; morbid obesity; proteomic; transcriptomic; type 2 diabetes (T2D).

Grants and funding

The study was funded by the Norwegian Diabetes Association, The Blood Cell Research Group, Department of Medical Biochemistry, Oslo University Hospital and OsloMet.