1 Department of Evolutionary and Functional Biology, University of Parma, Viale delle Scienze 11/a, 43100 Parma, Italy
2 Division for Experimental Oncology 2, The National Cancer Institute, CRO-IRCCS, Via Pedemontana Occidentale 1, Aviano 33081, Italy
Author for correspondence (e-mail: paolo.malatesta{at}istge.it)
Accepted 25 May 2005
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Summary |
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Key words: Bone-marrow-derived stem cells, Neurogenesis, Transdifferentiation
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Introduction |
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Cells with neural characteristics appear to have been generated in vitro from adult stem cells of putative mesodermal origin and isolated from a variety of connective tissues, including bone marrow, umbilical cord blood, dermis and adipose tissue (Hermann et al., 2004; Jin et al., 2003
; Kang et al., 2004
; Padovan et al., 2003
; Sanchez-Ramos et al., 2000
; Sanchez-Ramos, 2002
; Wislet-Gendebien et al., 2005
; Wislet-Gendebien et al., 2003
). However, attempts to assert transdifferentiation of adult bone-marrow-derived cells into neural lineages in vivo have produced discordant results. Some authors have reported the integration and differentiation of such cells in the brain (Munoz-Elias et al., 2004
), whereas others have found that the few cells that were capable of engrafting into the nervous tissue fused with endogenous cells and thereby acquired the phenotype of the partner host cell (Alvarez-Dolado et al., 2003
; Weimann et al., 2003a
; Weimann et al., 2003b
). The beneficial effects observed following transplantation of bone marrow stromal cells into injured nervous tissue are now believed to occur independently of tissue integration and to be due to a potential local release of stimulating factors by the transplanted cells (Hofstetter et al., 2002
; Zhao et al., 2002
). Several recent reports propose that mesenchymal stem/progenitor cells may generate both endodermal derivatives, such as hepatocytes (Alison et al., 2000
; Krause et al., 2001
; Petersen et al., 1999
; Schwartz et al., 2002
; Wang et al., 2004
) and ectodermal ones, such as various types of neural cells (Deng et al., 2001
; Hung et al., 2002
; Jiang et al., 2003
; Jiang et al., 2002
; Kim et al., 2002
; Kohyama et al., 2001
; Levy et al., 2003
; Munoz-Elias et al., 2003
; Reyes et al., 2001
; Sanchez-Ramos et al., 2000
; Tzeng et al., 2004
).
Of these investigations, some have suggested that this capacity may be restricted to a rare subpopulation of bone-marrow-resident cells, termed multipotent adult progenitor cells (MAPCs), which can be selected on the basis of immunological criteria and expanded extensively in vitro (Jiang et al., 2003; Reyes et al., 2001
). Others have reported that neural differentiation can be observed in the predominant population of MSCs isolated according to standard procedures if these cells are sequentially exposed to a series of inducing factors (Deng et al., 2001
; Dezawa et al., 2004
; Levy et al., 2003
; Munoz-Elias et al., 2003
; Qian and Saltzman, 2004
; Rismanchi et al., 2003
; Sanchez-Ramos et al., 2000
; Suon et al., 2004
; Tzeng et al., 2004
; Wislet-Gendebien et al., 2005
; Wislet-Gendebien et al., 2003
; Woodbury et al., 2002
; Woodbury et al., 2000
). Significantly, some of these studies claim that neural cells may be obtained rapidly and with high yield from cultured human and rodent MSCs by applying simple chemical treatments (Munoz-Elias et al., 2003
; Woodbury et al., 2002
; Woodbury et al., 2000
). This latter observation would have a high conceptual relevance as it suggests that MSCs might be somehow precommitted toward a neural fate. However in such studies the accomplishment of in vitro neurogenic differentiation was concluded exclusively on the basis of changes of cell morphology and de novo expression of few markers, such as NSE, NeuN and Tau. In addition, some authors have raised doubts about the interpretation of these results, arguing about the authenticity of the observed neuron-like morphology and the reliability of the expression of the various markers (Lu et al., 2004
; Neuhuber et al., 2004
; Tondreau et al., 2004
).
This apparent controversy has not confirmed whether MSCs truly harbour the potential to be converted into neural cells with the proposed chemical methods and, hence, whether they are likely to be precommitted toward a neural phenotype. Using MSCs, we have therefore revisited the problem at the cellular and molecular level.
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Materials and Methods |
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Osteogenic and adipogenic differentiation
Osteogenic and adipogenic differentiation of hMSCs were induced according to a published protocol (Pittenger et al., 1999). To achieve osteogenic differentiation, cells were seeded at a density of 3x103 cells/cm2 and then cultured for 10 days in the presence of 100 nM dexamethasone, 50 µM ascorbic acid 2-phosphate and 10 mM ß-glycerophosphate. Osteoblast formation was assessed by alkaline phosphatase (AP) staining using Sigma Diagnostic Kit 85, according to the manufacturer's instructions. For adipogenic differentiation, cells were grown until they reached confluence and were then induced by three cycles of induction/maintenance with 1 µM dexamethasone, 0.2 mM indomethacin, 10 µg/ml insulin and 0.5 mM 3-isobutyl-l-methylxanthine. Adipogenesis was assayed by staining of intracellular lipid droplets with Oil Red O (Sigma) as previously described (Sottile et al., 2002
).
Neural induction and drug treatments
The protocol for neural induction of hMSCs (DMSO/BHA neural induction) was as reported (Woodbury et al., 2002; Woodbury et al., 2000
). Briefly, cells at passage 4-7 were cultured in standard conditions on plastic or glass coverslips until they became subconfluent and then incubated for 24 hours in pre-induction medium consisting of DMEM supplemented with 20% FBS and 10 ng/ml FGF-2 (Calbiochem). Thereafter, the medium was replaced with an equal volume of the induction medium composed of DMEM supplemented with 2% DMSO, 100 µM butylated hydroxyanisole (BHA), 10 µM forskolin, 2 mM valproic acid, 10 mM KCl, 5 nM K252a (Sigma) and N2 supplement (Invitrogen). The cells were treated for 6 hours, 48 hours or 6 days before fixation or harvesting. In some cases, hMSCs at a similar density were incubated for 1 hour in serum-free DMEM with 10 µM cytochalasin D (Sigma) or 4 mM EDTA. Dose-dependent tests determined these concentrations were suitable to cause contraction and substrate-detachment of the cells.
The effects of DMSO/BHA neural induction protocol on cell morphology were evaluated in hMSCs derived from three different donors. For each donor, two independent experiments were performed in duplicate by treating cells for 6 and 48 hours (24 cultures in total). Two additional cultures for each donor were maintained in the induction medium for 6 days. In each culture the percentage of affected or unaffected cells was evaluated by scoring more than 500 cells from five randomly selected fields. Results are reported as the mean percentage±s.e.m. calculated across all the cultures for any given treatment period.
Immunocytochemistry
Immunocytochemical staining was performed in cells grown on glass coverslips and fixed with 4% paraformaldehyde as previously described (Malatesta et al., 2003; Malatesta et al., 2000
). The following antibodies were used: mouse monoclonal antibodies against CD31, CD44, CD73, CD105, CD117 and CD147 (1:100, BD Biosciences),
SMA (1:400, Sigma), calponin (1:500, Sigma), caldesmon (1:100, Sigma), fibronectin (1:50, Sigma), the myofibroblastic antigen 1B10 (1:500, Sigma), nestin (1:4, Dev. Hybridoma Bank), NeuN (1:50, Chemicon), 200 kDa neurofilament isoform (NF-200; 1:200, Sigma), synaptophysin (1:100, Sigma), Tau protein (1:100, Sigma), ßIII-tubulin (1:100, Sigma), GFAP (1:200, Sigma), S100 (1:500, Sigma), CNPase (1:500, Sigma), O4 (1:40, Chemicon) and ß-galactosidase (1:500, Promega); rabbit polyclonal antibodies against MyoD (1:100, Santa Cruz), parvalbumin (1:500, Swant), NSE (1:2, Sigma) and GFP (1:500, RDI).
Binding of primary antibodies was revealed with specific secondary antisera, conjugated with FITC, TRITC (Immucor) or biotin (Dako), and subsequently developed with the ABC kit from Vector laboratories, according to the procedure provided by the suppliers. Primary antibodies against CD34, CD45, CD10, CD38, CD90 and CD133 directly conjugated with phycoerythrin or FITC (BD Biosciences) were also used at 1:100 dilution.
Western blotting
For western blot analysis, confluent cultures of either untreated hMSCs or hMSCs treated with the DMSO/BHA neural induction medium were lysed with RIPA buffer (Sigma) supplemented with 2 mM EDTA and `Complete Mini' protease inhibitor kit (Roche) at the concentration recommended by the supplier. Total protein content of the lysates was quantified using Bradford reagent (Sigma). Approximately 30 µg of each cell lysate were diluted in sample buffer (50 mM Tris-HCl pH 6.8, 7% glycerol, 0.5% SDS, 25 mM DTT, 0.005% Bromophenol Blue) and separated on 8% SDS-polyacrylamide gels. After electrophoresis, the proteins were blotted onto a nitrocellulose membrane to perform the antibody detection. The primary antibodies were used at the following concentrations: anti-ßIII-tubulin (1:1000), anti-NF-200 (1:800), anti-NeuN (1:500), anti-NSE (1:200), anti-SMA (1:3000) and anti-fibronectin (1:200). Rabbit polyclonal anti-ß-actin (1:3000, Abcam) was used for normalization. Primary antibodies were detected with specific antisera conjugated with HRP (Sigma) and developed with the ECL Plus chemiluminescent detection system (Amersham Biosciences). Quantification of protein expression was performed on digitized images using ImageJ (Wayne Rasband, NIH, USA). The intensity of ß-actin bands was used to normalize the densitometric measurements of each band analysed for different samples.
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DNA microarray analysis
Total RNA from hMSC cultures was extracted with the RNeasy Mini kit (Qiagen) and total RNA of human foetal brain and adult liver were purchased from Chemicon. Representative amplification of mRNA and fluorescent labelling were carried out using an Amino Allyl MessageAmp aRNA kit (Ambion) and NHS ester fluorescent dyes (Amersham Bioscience) following the protocol suggested by the supplier. Hybridization was performed on a human Operon oligo V2.0 microarray platform printed by MicroCRIBI service at CRIBI facility (University of Padua, Italy) containing 21,329 human gene probes (GEO Platform accession number GPL 2136). The arrays were previously blocked in hybridization buffer [5x SSC, 0.1% SDS, 0.2 mg/ml Torula Yeast RNA (Sigma), 5x Denhardt's solution, 25% formamide] for 2 hours. 120 pmol of each dye-labelled aRNA sample, diluted in 100 µl hybridization buffer, were denatured for 5 minutes at 65C and were then applied to the glass slide. A 60-mm glass coverslip was used to uniformly spread the sample solution. Incubation was carried out for 24 hours at 48°C in a humid chamber and was followed by six washing steps with decreasing concentrations of SSC and SDS. Array-scanning was performed by using a ScanArray Lite (PerkinElmer Life Sciences). Background subtraction, normalization and statistical analysis were performed using the TIGR TM4 suite (Saeed et al., 2003
) and SAM (Tusher et al., 2001
). The non-linear LOWESS-based lockfit algorithm was used for normalization. Principal component analysis (PCA) was performed using SPSS13.
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Results |
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It was also confirmed that hMSCs maintained their ability to undergo osteogenic and adipogenic differentiation with increasing number of passages. Following osteogenic induction with the appropriate medium, hMSCs changed their morphology, expressed alkaline phosphatase within 7-10 days (Fig. 1D) and deposited a mineralized matrix (data not shown). Following the adipogenic induction, cells showed a reduced proliferation rate and within 10 days accumulated lipid vacuoles in their cytoplasm that were evidenced by Oil Red O staining (Fig. 1F). Taken together these results indicate that the population of hMSCs under examination was comparable to that described by other authors (Colter et al., 2001; Conget and Minguell, 1999
; Deans and Moseley, 2000
; Pittenger et al., 1999
; Vogel et al., 2003
; Woodbury et al., 2002
).
`Neural induction'
When hMSCs were exposed to the DMSO/BHA neural induction medium, they rapidly underwent dramatic morphological changes. Within a few hours, the majority of the cells rounded up and showed thin radial processes vaguely reminiscent of neurites (Fig. 2B). Some of the cells partially lost contact with the substratum and others completely detached, whereas a limited fraction of hMSCs appeared to be unaffected by the treatment (15±5%, mean±s.e.m.) (Fig. 2B). These morphological changes were transitory and reverted spontaneously even if the cells were maintained in the same medium. After 48 hours only 20±5% (mean±s.e.m.) of cells still displayed a pseudo-neural appearance (Fig. 2C) and after 6 days of continuous treatment cultures were almost indistinguishable from untreated ones (data not shown).
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Rather than being representative of a differentiation event, the morphological alterations exhibited by hMSCs following incubation with the DMSO/BHA neural induction medium seemed to be a consequence of cytoskeletal collapse and/or disruption of focal contacts. We therefore assayed by video time-lapse whether drug-induced interference of cell-substratum contacts or cytoskeletal rearrangement evoked similar effects. Treatment of hMSCs with both EDTA, causing loss of cell-substratum anchorage, and cytochalasin D, known to disrupt the cytoskeletal architecture, resulted in shape changes virtually indistinguishable from those caused by treatment with DMSO/BHA (Fig. 2E-F).
There remained the possibility that the morphological changes observed in hMSCs following the putative neural induction could still reflect a specific trait of pluripotent cells and were, in fact, a display of an incipient in vitro neurogenesis process. We therefore incubated normal human prostate fibroblasts in the same neural induction medium and, in parallel, challenged them with the osteogenic induction protocol to verify that they diverged from hMSCs in their multipotency. These fibroblastic cells failed to differentiate into osteoblasts (Fig. 3D), but, under DMSO/BHA treatment, showed an analogous retraction of the cell margins and rapidly assumed a similar stellate pseudo-neural morphology (Fig. 3B), as displayed by hMSCs.
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We then suspected that the apparent increase in immunoreactivity could simply be an artefact deriving from immunolabelling of shrunken cells having potentially altered membrane properties. To test this hypothesis, we immunolabelled hMSCs that had been partly detached from their substrate by treatment with EDTA, or in which their focal adhesions had been disrupted through treatment with cytochalasin D (Fig. 4H-K), but which had not been exposed to the DMSO/BHA neural induction medium. These cells too exhibited enhanced staining for the neural markers. In further support of the idea of a possible pitfall and misinterpretation of the previously reported immunocytochemical patterns was the aberrant localization of the neural markers NeuN and Tau. The former should have shown a preferentially nuclear distribution and the second a microtubule-associated localization along the pseudo-neurites. Both in our immunostaining experiments and in those reported by other investigators adopting DMSO/BHA neural induction protocol (Munoz-Elias et al., 2003; Woodbury et al., 2002
; Woodbury et al., 2000
), immunoreactivity for these two antigens was evenly distributed in the cytoplasm of the treated hMSCs indicating that the staining patterns did not reflect proper immunolocalization of these markers.
Western blot analysis of cell lineage markers
Biochemical techniques based on protein extracts are not influenced by cell morphology and we therefore examined the relative levels of marker expression in treated and untreated hMSCs by western blotting using human brain as a positive control and a human kidney cell line HEK293 as a negative control. Neither NeuN nor NF-200 was detectable in hMSCs before the treatment or after 6 and 48 hours of neural induction (Fig. 5A). Analogously, the levels of markers that are constitutively expressed in untreated cells, such as NSE (Fig. 5A) and Tau (data not shown), were not significantly increased following treatment with the neural induction medium (Fig. 5A). A slight upregulation after DMSO/BHA treatment was seen for ßIII-tubulin. However, this could hardly be considered as an indication of a neural differentiation programme as the expression of this tubulin isoform is not strictly neurospecific in humans (Pontius et al., 2003; Tondreau et al., 2004
). A modulation of the expression of fibronectin and the smooth muscle marker
SMA was also observed (Fig. 5B). Rather than being a trait in favour of a differentiation process, the down-regulation of
SMA was probably due to collapse of the actin microfilaments.
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Microarray gene profiling
The most severe limitation of previous studies is that very few markers were examined in the induced MSCs. In order to overcome these limitations, we performed a DNA microarray-based global expression profiling of treated and untreated hMSCs using a 21,329 oligonucleotide platform. RNA extracted from untreated hMSCs from different donors and RNA isolated from hMSCs treated for 6 or 48 hours with DMSO/BHA neural induction medium were used as reference and test samples, respectively. Control experiments were performed with RNA derived from human foetal brain, in order to provide information on the set of genes that would be differentially expressed in human neural tissue compared to untreated hMSCs. Data obtained from microarray experiments are expressed as the logarithm (base 2) of the ratio between the expression level in the probe compared to that of the reference sample (fold change). Eight independent experiments (GEO accession number: GSE2776), each one with an internal replicate, were used to derive 16 datasets that were first evaluated for their consistency by a Principal Component Analysis (PCA) statistical approach. The contribution of each dataset to the two principal components was determined (Fig. 6A). The datasets are tightly clustered into three groups, corresponding to the three different probes that were used. The cluster containing the datasets relative to the comparison between foetal brain and untreated hMSCs is well separated from the others and contributes almost entirely to the first principal component. Such data sets, therefore, constitute a coherent group that is the main source of variance between all the data sets. As expected, the other two clusters are more similar to each other, contributing only to the second principal component. These results show that the set of genes modulated by the DMSO/BHA neural induction treatment is different from the set of genes differentially expressed between untreated hMSCs and neural tissue. Moreover, the number of genes that show a significant modulation after the 6 or 48 hours treatment is extremely small compared to the number of genes differentially expressed between untreated hMSCs and neural tissue (Fig. 6B). In particular, the numbers of genes that showed a fold change in absolute value equal or greater to 1.5 were 55 after the 6-hour treatment and 104 after the 48-hour treatment. In comparison, 854 genes showed a significant differential expression between untreated hMSCs and neural tissue. These results show that the change in the transcriptome of hMSCs due to the DMSO/BHA neural induction treatment is dramatically different to the change that would be expected in the case of conversion between hMSCs and neural tissue.
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The absolute number of genes differentially expressed after the treatment, however, may also depend on the number of cells that are influenced by the treatment. In order to rule out the possibility that the DMSO/BHA neural induction medium was actually promoting the differentiation of a small subpopulation in the culture, we examined whether at least the set of genes that were most significantly modulated by the treatment matched the set of genes most differentially expressed between hMSCs and neural tissue. The sets containing the 100 genes that were most significantly modulated by the 6- and 48-hour treatments had extremely small intersections (respectively three and four genes) with the set of the 100 most significant genes differentially expressed between hMSCs and neural tissue (Fig. 6C). Noticeably, similar intersections could be found when comparing the set of genes modulated by the treatments and the set of genes differentially expressed between non-induced hMSCs and adult liver (three and five genes respectively) (Fig. 6D). Moreover, the genes belonging to the intersections (Table 2) do not show any obvious relation to neural differentiation pathways. Taken together, these data highlight that the modest changes in gene expression levels promoted by the treatment of hMSCs with the DMSO/BHA medium do not resemble at any level a differentiation cascade conducive to neurogenesis.
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Discussion |
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Our time-lapse recordings of the behaviour of hMSCs following treatment with the DMSO/BHA neural induction medium, are in agreement with recent data obtained on murine MSCs (Neuhuber et al., 2004) and show that the morphological changes are due to cell shrinkage rather than to a process of neurite extension typical of neuronal differentiation. These observations, therefore, suggest that the change in cell morphology could be an artefact rather than a differentiation trait. However, some doubts still remain as chemical treatment appears able to induce the expression of genes that are commonly considered as markers of neuronal differentiation. The most critical point in these studies is the reliability of these markers and in particular their capability to give information about the differentiation fate of cells found in a heterodox context. In most cases, cell type-specific markers have been deemed to be reliable in the identification of particular cell types in a given context, but they can be misleading in other contexts. For instance, in the CNS, the calcium binding protein calbindin is used as marker for the horizontal cells, a population of interneurons in the retina (Matsuda and Cepko, 2004
), but it is also the standard marker for Purkinje projection neurons in the cerebellum (McAlhany et al., 1997
). A cell expressing calbindin cannot be classified as a Purkinje cell (or horizontal cell) if its origin is not known or, worse, if it is different from both retina and cerebellum. In addition, some markers have a different specificity in different species. The well-established neuronal marker ßIII-tubulin is extremely useful for identification of neurons in murine nervous system cultures, whereas in humans its expression is less restricted and can be found in different tissues including lung, pancreas and bone marrow (Pontius et al., 2003
). Therefore, an increase of ßIII-tubulin immunoreactivity, or expression levels, in a population of bone-marrow-derived cells hardly supports the notion of their transdifferentiation.
Moreover, many of the immunostaining patterns presented by other investigators do not show the expected localization of the corresponding antigens. For instance, NeuN immunoreactivity appears to be spread outside the perinuclear region, being present also in cell processes (Levy et al., 2003; Sanchez-Ramos et al., 2000
; Sanchez-Ramos, 2002
). Conversely, Tau, a typical axonal marker, appears to be more widely expressed in the cytoplasm of the cells and is not distinctly associated with cell protrusions (Munoz-Elias et al., 2003
; Woodbury et al., 2002
). Taken together with our observations highlighting that immunoreactivity for all tested antigens apparently increased in both the pseudo-neurally shaped cells and in the cells partially detached from the substratum by EDTA or cytochalasin D treatment, these considerations undermine the evidence in favour of a neural transdifferentiation event.
As, in the absence of functional data, the analysis of a few markers is not sufficient to allocate a cell, taken out of its normal physiological context, to a particular lineage, a more appropriate approach is to compare its entire transcriptome to that of cells belonging to the lineage of interest. We therefore compared the changes in gene expression profile of hMSCs treated with the protocol proposed by Woodbury and colleagues with the set of genes that are differentially expressed between hMSCs and brain tissue. This comparison showed that although the set of genes differentially expressed between hMSCs and brain was rather large, the set of genes modulated by the chemical treatment was about tenfold smaller and the two sets did not show significant correlation. Moreover, we found that the few genes in common among these sets were not overtly referable to a neural differentiation pathway. Strikingly, we found an even higher number of common elements in the set of genes modulated by the DMSO/BHA treatment and in the set of genes differentially expressed between untreated hMSCs and adult liver cells (Fig. 6D); in other words, the adopted neural induction protocol was not driving the cells toward the neural lineage more than toward the hepatic one.
The presence of common elements between the set of genes modulated by the induction and the genes differentially expressed between non-induced hMSCs and foetal brain (or adult liver) is probably due to the peculiar level of expression of such genes in the reference sample, i.e. untreated hMSCs. This may for example be the case for the caldesmon 1 gene CALD1, which encodes a calmodulin and actin binding protein, that appears to be expressed at high levels by bone marrow (Pontius et al., 2003) and untreated hMSCs, but is expressed at lower levels by both the nervous system and liver. The expression of the caldesmon 1 gene is probably reduced by the treatment with DMSO/BHA as a consequence of cytoskeleton collapse. These data provide a stronger basis for rejecting the idea that the adopted chemical treatment is able to induce a transdifferentiation process of hMSCs in vitro. We found that hMSCs undergo shape changes, assuming a pseudo-neural morphology when they are exposed to different kinds of chemical stresses that induce their detachment from the substratum and/or cause the collapse of the actin cytoskeleton. Taken together with the observation that a high percentage of apoptotic cells are present in the cultures exposed to the DMSO/BHA neural induction protocol (Rismanchi et al., 2003
), our results support the notion that the morphological changes observed in hMSCs are caused by a cytotoxic effect of BHA and/or DMSO. Although this study cannot rule out the possibility that specific culture conditions, i.e. co-culturing with neural primary cells, as described recently (Wislet-Gendebien et al., 2005
), may induce hMSCs to form neuronal elements in vitro, it unequivocally shows that the treatment with DMSO/BHA does not. Moreover, it raises doubts on other claims about transdifferentiation of hMSCs toward a neural fate based exclusively upon cell shape changes and analyses of a few precocious lineage markers.
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Acknowledgments |
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Footnotes |
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* Present address: National Institute for Cancer Research (IST), 16132 Genoa, Italy
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References |
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