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The influence of xeno-free culture conditions on the angiogenic and adipogenic differentiation properties of adipose tissue-derived stem cells
Umeå universitet, Medicinska fakulteten, Institutionen för medicinsk och translationell biologi. Umeå universitet, Medicinska fakulteten, Institutionen för diagnostik och intervention.
Umeå universitet, Medicinska fakulteten, Institutionen för medicinsk och translationell biologi.
Umeå universitet, Medicinska fakulteten, Institutionen för medicinsk och translationell biologi. Umeå universitet, Medicinska fakulteten, Institutionen för diagnostik och intervention.ORCID-id: 0000-0002-2777-8184
Umeå universitet, Medicinska fakulteten, Institutionen för diagnostik och intervention. Umeå universitet, Medicinska fakulteten, Institutionen för medicinsk och translationell biologi.
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2024 (Engelska)Ingår i: Regenerative Therapy, ISSN 2352-3204, Vol. 26, s. 901-910Artikel i tidskrift (Refereegranskat) Published
Abstract [en]

Introduction: Before performing cell therapy clinical trials, it is important to understand how cells are influenced by different growth conditions and to find optimal xeno-free medium formulations. In this study we have investigated the properties of adipose tissue-derived stem cells (ASCs) cultured under xeno-free conditions.

Methods: Human lipoaspirate samples were digested to yield the stromal vascular fraction cells which were then seeded in i) Minimum Essential Medium-α (MEM-α) supplemented with 10 % (v/v) fetal bovine serum (FBS), ii) MEM-α supplemented with 2 % (v/v) human platelet lysate (PLT) or iii) PRIME-XV MSC expansion XSFM xeno-free, serum free medium (XV). Flow cytometry for ASCs markers CD73, CD90 and CD105 together with the putative pericyte marker CD146 was performed. Growth rates were monitored over multiple passages and adipogenic differentiation performed at early and expanded passage culture. Growth factor gene expression was analyzed and an in vitro angiogenesis assay performed.

Results: Cells in FBS and PLT grew at similar rates whereas the cells cultured in XV medium proliferated significantly faster up to 60 days in culture. All cultures were >98 % positive for CD73, CD90 and CD105, whereas CD146 expression was significantly higher in XV cells. Adipogenic differentiation was most pronounced in cells which had been cultured in XV medium whilst cells grown in PLT were inferior compared with cells from the FBS cultures. IGF1 gene expression was highest in cells cultured in PLT whilst cells grown in XV medium showed 10-fold lower expression compared with FBS cells. In contrast, HGF gene expression was 90-fold greater in cells cultured in XV medium compared with those cultured in FBS. Conditioned medium from XV cultured cells showed the most angiogenic activity, inducing the greatest endothelial cell network formation and maturation.

Conclusion: Culture under different conditions alters the ASCs characteristics. Since cells cultured in XV medium showed the best adipogenic and angiogenic profile this might be a preferred medium formulation for preparing cells required for reconstructive surgical applications such as cell-assisted fat grafting.
Ort, förlag, år, upplaga, sidor
Elsevier, 2024. Vol. 26, s. 901-910
Nyckelord [en]
Cell-assisted lipotransfer, Mesenchymal stem cells, Regenerative medicine, Stem cell therapy, Xeno-free
Nationell ämneskategori
Medicinsk bioteknologi
Identifikatorer
URN: urn:nbn:se:umu:diva-230771DOI: 10.1016/j.reth.2024.09.013ISI: 001338899200001Scopus ID: 2-s2.0-85205929562OAI: oai:DiVA.org:umu-230771DiVA, id: diva2:1904769
Forskningsfinansiär
Vinnova, 2017-02130Umeå universitetRegion VästerbottenTillgänglig från: 2024-10-10 Skapad: 2024-10-10 Senast uppdaterad: 2025-04-24Bibliografiskt granskad

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Lauvrud, Anne ThereseGiraudo, Maria VittoriaWiberg, RebeccaWiberg, MikaelKingham, Paul J.Brohlin, Maria

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Lauvrud, Anne ThereseGiraudo, Maria VittoriaWiberg, RebeccaWiberg, MikaelKingham, Paul J.Brohlin, Maria
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Institutionen för medicinsk och translationell biologiInstitutionen för diagnostik och interventionInstitutionen för klinisk mikrobiologi
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