Stem Cell Research & Therapy (Jun 2023)

Significant improvement of bone marrow-derived MSC expansion from MDS patients by defined xeno-free medium

  • Eva Altrock,
  • Carla Sens-Albert,
  • Franziska Hofmann,
  • Vladimir Riabov,
  • Nanni Schmitt,
  • Qingyu Xu,
  • Johann-Christoph Jann,
  • Felicitas Rapp,
  • Laurenz Steiner,
  • Alexander Streuer,
  • Verena Nowak,
  • Julia Obländer,
  • Nadine Weimer,
  • Iris Palme,
  • Melda Göl,
  • Ali Darwich,
  • Patrick Wuchter,
  • Georgia Metzgeroth,
  • Mohamad Jawhar,
  • Wolf-Karsten Hofmann,
  • Daniel Nowak

DOI
https://doi.org/10.1186/s13287-023-03386-5
Journal volume & issue
Vol. 14, no. 1
pp. 1 – 13

Abstract

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Abstract Background Robust and reliable in vitro and in vivo models of primary cells are necessary to study the pathomechanisms of Myelodysplastic Neoplasms (MDS) and identify novel therapeutic strategies. MDS-derived hematopoietic stem and progenitor cells (HSPCs) are reliant on the support of bone marrow (BM) derived mesenchymal stroma cells (MSCs). Therefore, isolation and expansion of MCSs are essential for successfully modeling this disease. For the clinical use of healthy MSCs isolated from human BM, umbilical cord blood or adipose tissue, several studies showed that xeno-free (XF) culture conditions resulted in superior growth kinetics compared to MSCs cultured in the presence of fetal bovine serum (FBS). In this present study, we investigate, whether the replacement of a commercially available MSC expansion medium containing FBS with a XF medium is beneficial for the expansion of MSCs derived from BM of MDS patients which are often difficult to cultivate. Methods MSCs isolated from BM of MDS patients were cultured and expanded in MSC expansion medium with FBS or XF supplement. Subsequently, the impact of culture media on growth kinetics, morphology, immunophenotype, clonogenic potential, differentiation capacity, gene expression profiles and ability to engraft in immunodeficient mouse models was evaluated. Results Significant higher cell numbers with an increase in clonogenic potential were observed during culture of MDS MSCs with XF medium compared to medium containing FBS. Differential gene expression showed an increase in transcripts associated with MSC stemness after expansion with XF. Furthermore, immunophenotypes of the MSCs and their ability to differentiate into osteoblasts, adipocytes or chondroblasts remained stable. MSCs expanded with XF media were similarly supportive for creating MDS xenografts in vivo as MSCs expanded with FBS. Conclusion Our data indicate that with XF media, higher cell numbers of MDS MSCs can be obtained with overall improved characteristics in in vitro and in vivo experimental models.

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