Characterization of the Optimal Culture Conditions for Clinical Scale Production of Human Mesenchymal Stem Cells

Sotiropoulou, Panagiota A.; Perez, Sonia A.; Salagianni, Maria; Baxevanis, Constantin N.; Papamichail, Michael

doi:10.1634/stemcells.2004-0331

Cited by 558 publications

(464 citation statements)

References 52 publications

Supporting

Mentioning

416

Contrasting

Unclassified

Order By: Relevance

“…11 In our study, an aberrant HLA-DR expression on BM-derived MSCs was documented in some LPD, thus suggesting unreported possible interactions between BM stromal cells and early lymphoid progenitor cells. Furthermore, because cytokines treatment (IL-1b, INF-y and TGF-b) was reported to modulate the expression of antigenpresenting molecules on cultured human fibroblasts and epithelial cells, 12 in this study, we gave evidence that HLA-DR expression on MSCs was also found to be related to different culture conditions, 13 as it was more expressed under angiogenic conditions. As MSCs heterogeneity could suggest specialization of function, the occurrence of immunophenotypic changes of ex vivo expanded MSCs could be relevant for MSCs properties; based on these considerations, we speculated that the BM microenvironmental conditions play a pivotal role in controlling MSCs function.…”

mentioning

confidence: 55%

Aberrant expression of HLA-DR antigen by bone marrow-derived mesenchymal stromal cells from patients affected by acute lymphoproliferative disorders

et al. 2006

View full text Add to dashboard Cite

tic stem cells. 3 As a single activating mutation in Janus kinase (JAK-2) is considered a very good new marker of clonality in chronic myeloproliferative syndromes (cMPDs), 4 we determined whether the marrow microenvironment is an abnormal stromal compartment carrying the JAK-2 mutation. After obtaining informed consent, we generated bone marrow mesenchymal cells 5 from 20 patients (10 with polycythemia vera, five with essential thrombocythemia and five with idiopathic myelofibrosis) carrying the V617F mutation (Table 1). After a median of 2 months, nHSC were detached and analysed with direct fluorescence for expression of CD45-FITC, CD90-FITC, CD105-FITC (Beckman-Coulter Corporation, Hialeah, FL, USA) and STRO1-PE (Caltag Laboratories, Burlingame, CA, USA) by Epics XL cytometer (Coulter). Polymerase chain reaction (PCR) analysis determined CD45 mRNA expression. 3 Cells were analysed for the Jak-2 mutation by allele-specific PCR 4 and by microelectronic DNA chip that allows automated calculation of the allelic ratio (mutated V617F vs wild type). 6 No differences emerged in the generation of the stromal layer from the different cMPDs. Furthermore, the cases with allelic ratios 450% V617F did not show any disadvantages in the stromal generation. In 15/ 20 cases, flow cytometry analysis revealed that nHSC were negative for CD45 and positive for CD90, CD105 and STRO-1. The other five cases still had residual haematopoietic cells as shown by 1-2% positivity for CD45 at immunophenotyping and strong PCR positivity for CD45 mRNA expression. Five other cases had faint positivity at PCR and 10 were negative. The distribution of CD45 PCR-positive/negative cases was not disease specific. V617F Jak-2 mutation analysis demonstrated that the mutation was not present in the 10 cases that were CD45 negative at immunophenotyping and PCR. A faint positivity emerged in cases with only mRNA positivity at CD45 PCR. The mutation was strongly present in the five cases that were CD45 positive by cytofluorimetry analysis and/or PCR. All JAK-2-positive cases were treated with leucyl-leucine methyl ester, the antilysosomal compound 5 that induces selective depletion of monocyte-macrophages. After treatment, all cases were JAK-2 negative. Macrophages persisting long term in cultures may account for the false positive results reported by Singer et al. 2 These data strongly suggest nHSC do not form part of the malignant clone in cMPDs and support the finding that haematopoietic and stromal cells are not derived from a common stem-cell precursor.

show abstract

mentioning

confidence: 55%

Aberrant expression of HLA-DR antigen by bone marrow-derived mesenchymal stromal cells from patients affected by acute lymphoproliferative disorders

et al. 2006

View full text Add to dashboard Cite

show abstract

“…The DJ9 corresponding antigen, HLA-DR is normally expressed in antigen presenting cells, and not MSCs . However, expression of HLA-DR in cultured MSCs has been described previously as a result of induction by interferon-γ (Chan et al, 2008) or basic fibroblast growth factor (Sotiropoulou et al, 2006) present in the culture medium. Thus, the expression of HLA-DR in telemorase immortalized MSCs, but not primary derived MSCs, may reflect the long term in vitro culture of these cells.…”

Section: Discussionmentioning

confidence: 94%

Development of Novel Monoclonal Antibodies that Define Differentiation Stages of Human Stromal (Mesenchymal) Stem Cells

Andersen

Kortesidis

Zannettino

et al. 2011

Molecules and Cells

View full text Add to dashboard Cite

Human mesenchymal stem cells (hMSC) are currently being introduced for cell therapy, yet, antibodies specific for native and differentiated MSCs are required for their identification prior to clinical use. Herein, high quality antibodies against MSC surface proteins were developed by immunizing mice with hMSC, and by using a panel of subsequent screening methods. Flow cytometry analysis revealed that 83.5, 1.1, and 8.5% of primary cultures of hMSC were double positive for STRO-1 and either of DJ 3, 9, and 18, respectively. However, none of the three DJ antibodies allowed enrichment of clonogenic hMSC from BMMNCs as single reagents. Using mass-spectrometric analysis, we identified the antigen recognised by DJ3 as CD44, whereas DJ9 and DJ18 recognized HLA-DRB1 and Collagen VI, respectively. The identified proteins were highly expressed throughout in vitro osteogenic-and adipogenic differentiation. Interestingly, undifferentiated cells revealed a sole cytoplasmic distribution pattern of Collagen VI, which however changed to an extracellular matrix appearance upon osteogenic-and adipogenic differentiation. In relation to this, we found that STRO-1 +/-/Collagen VI -sorted hMSC contained fewer differentiated alkaline phosphatase + cells compared to STRO-1 +/-/Collagen VI + hMSC, suggesting that Collagen VI on the cell membrane exclusively defines differentiated MSCs. In conclusion, we have generated a panel of high quality antibodies to be used for characterization of MSCs, and in addition our results may suggest that the DJ18 generated antibody against Collagen VI can be used for negative selection of cultured undifferentiated MSCs.

show abstract

“…Refl ecting the complexity of the stromal system in bone marrow, MSC populations expanded from marrow aspirates are heterogeneous in nature with the exact composition depending on the donor (Rickard et al, 1996;Majors et al, 1997;Muschler et al, 2001), the individual aspirate (Lazarus et al, 1997;Muschler et al, 1997;Phinney et al, 1999;Muschler et al, 2001;Hernigou et al, 2006), applied isolation methods and expansion conditions, the latter of which differ largely among investigators (Phinney, 2002;Shahdadfar et al, 2005;Sotiropoulou et al, 2006;Mannello and Tonti, 2007;Wagner and Ho, 2007). Cloned populations of MSC demonstrate that only part of the cells is multipotent while the remaining population shows varied phenotypes (Russell et al, 2010).…”

Section: Introductionmentioning

confidence: 99%

Prediction of in vivo bone forming potency of bone marrow-derived human mesenchymal stem cells

Janicki

Boeuf²,

Steck³

et al. 2011

eCM

View full text Add to dashboard Cite

Characterization of the Optimal Culture Conditions for Clinical Scale Production of Human Mesenchymal Stem Cells

Cited by 558 publications

References 52 publications

Aberrant expression of HLA-DR antigen by bone marrow-derived mesenchymal stromal cells from patients affected by acute lymphoproliferative disorders

Aberrant expression of HLA-DR antigen by bone marrow-derived mesenchymal stromal cells from patients affected by acute lymphoproliferative disorders

Development of Novel Monoclonal Antibodies that Define Differentiation Stages of Human Stromal (Mesenchymal) Stem Cells

Prediction of in vivo bone forming potency of bone marrow-derived human mesenchymal stem cells

Contact Info

Product

Resources

About