Gene Expression Profile during Chondrogenesis in Human Bone Marrow derived Mesenchymal Stem Cells using a cDNA Microarray

Yoo, Hyun Jung; Yoon, Sung Soo; Park, Seon Yang; Lee, Eun Young; Lee, Eun Bong; Kim, Ju Han

doi:10.3346/jkms.2011.26.7.851

Cited by 18 publications

(11 citation statements)

References 29 publications

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“…Transcriptome studies of hMSCs have focused on differential expression patterns among cells obtained from different sources 19 – 26 , different stages of the differentiation process 27 – 30 , and different cultivation times 31 – 35 . Differentially expressed genes have already been identified in bone marrow stem cells (hBMSC) at the 20 th passage compared to the 1st passage, adipose tissue stem cells (ASCs) at the 30th passage compared to the 1st passage 31 , hBM-MSC at the 15th passage compared to the 7th passage 32 , umbilical cord mesenchymal stem cells (UC-MSC) at the 15th passage compared to the 3rd passage 33 , hBMSCs at 33 population doubling levels (PDL) compared to 3 PDL 34 , and in BMSC at the 15th passage compared to 10th passage 35 .…”

Section: Introductionmentioning

confidence: 99%

Identification of new genes associated to senescent and tumorigenic phenotypes in mesenchymal stem cells

Marques

Cornélio

Silbiger

et al. 2017

Sci Rep

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Although human mesenchymal stem cells (hMSCs) are a powerful tool for cell therapy, prolonged culture times result in replicative senescence or acquisition of tumorigenic features. To identify a molecular signature for senescence, we compared the transcriptome of senescent and young hMSCs with normal karyotype (hMSCs/n) and with a constitutional inversion of chromosome 3 (hMSC/inv). Senescent and young cells from both lineages showed differentially expressed genes (DEGs), with higher levels in senescent hMSCs/inv. Among the 30 DEGs in senescent hMSC/inv, 11 are new candidates for biomarkers of cellular senescence. The functional categories most represented in senescent hMSCs were related to cellular development, cell growth/proliferation, cell death, cell signaling/interaction, and cell movement. Mapping of DEGs onto biological networks revealed matrix metalloproteinase-1, thrombospondin 1, and epidermal growth factor acting as topological bottlenecks. In the comparison between senescent hMSCs/n and senescent hMSCs/inv, other functional annotations such as segregation of chromosomes, mitotic spindle formation, and mitosis and proliferation of tumor lines were most represented. We found that many genes categorized into functional annotations related to tumors in both comparisons, with relation to tumors being highest in senescent hMSCs/inv. The data presented here improves our understanding of the molecular mechanisms underlying the onset of cellular senescence as well as tumorigenesis.

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Section: Introductionmentioning

confidence: 99%

Identification of new genes associated to senescent and tumorigenic phenotypes in mesenchymal stem cells

Marques

Cornélio

Silbiger

et al. 2017

Sci Rep

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“…Current methods for human cells reported in the literature employ various passage conditions and culture media formulae to support growth of chondrocytes (e.g. (Adesida et al , ; Alves da Silva et al , ; Bian et al , ; de Mara et al , ; Ghone and Grayson, ; Handorf and Li, ; Matsumoto et al , ; Mendelson et al , ; Park et al , ; Perrier et al , ; Wu et al , ; Yin et al , ; Yoo et al , )).…”

Section: Introductionmentioning

confidence: 99%

Human chondrocyte migration behaviour to guide the development of engineered cartilage

O’Connell

Tan

Cui

et al. 2015

J Tissue Eng Regen Med

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Tissue-engineering techniques have been successful in developing cartilage-like tissues in vitro using cells from animal sources. The successful translation of these strategies to the clinic will likely require cell expansion to achieve sufficient cell numbers. Using a two-dimensional (2D) cell migration assay to first identify the passage at which chondrocytes exhibited their greatest chondrogenic potential, the objective of this study was to determine a more optimal culture medium for developing three-dimensional (3D) cartilage-like tissues using human cells. We evaluated combinations of commonly used growth factors that have been shown to promote chondrogenic growth and development. Human articular chondrocytes (AC) from osteoarthritic (OA) joints were cultured in 3D environments, either in pellets or encapsulated in agarose. The effect of growth factor supplementation was dependent on the environment, such that matrix deposition differed between the two culture systems. ACs in pellet culture were more responsive to bone morphogenetic protein (BMP2) alone or combinations containing BMP2 (i.e. BMP2 with PDGF or FGF). However, engineered cartilage development within agarose was better for constructs cultured with TGFβ3. These results with agarose and pellet culture studies set the stage for the development of conditions appropriate for culturing 3D functional engineered cartilage for eventual use in human therapies.

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“…In addition, in a reanalysis of the data which included 5HTTLPR polymorphism genotyping, an interaction between 5HTTLPR polymorphisms and SSRI treatment was found for the total lumbar BMD z-score [24]. Effects of SSRIs on chondrocytes and cartilaginous tissue growth have not been studied, but serotonin receptors have been identified in embryonic and adult cartilaginous tissue [55, 56]. …”

Section: Discussionmentioning

confidence: 99%

Bone growth in juvenile rhesus monkeys is influenced by 5HTTLPR polymorphisms and interactions between 5HTTLPR polymorphisms and fluoxetine

Golub

Bulleri

Hogrefe

et al. 2015

Bone

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Male rhesus monkeys received a therapeutic oral dose of the selective serotonin reuptake inhibitor (SSRI) fluoxetine daily from 1 to 3 years of age. Puberty is typically initiated between 2 and 3 years of age in male rhesus and reproductive maturity is reached at 4 years. The study group was genotyped for polymorphisms in the monoamine oxidase A (MAOA) and serotonin transporter (SERT) genes that affect serotonin neurotransmission. Growth was assessed with morphometrics at 4 month intervals and radiographs of long bones were taken at 12 month intervals to evaluate skeletal growth and maturation. No effects of fluoxetine, or MAOA or SERT genotype were found for growth during the first year of the study. Linear growth began to slow during the second year of the study and serotonin reuptake transporter (SERT) long polymorphic region (5HTTLPR) polymorphism effects with drug interactions emerged. Monkeys with two SERT 5HTTLPR L alleles (LL, putative greater transcription) had 25–39% less long bone growth, depending on the bone, than monkeys with one S and one L allele (SL). More advanced skeletal maturity was also seen in the LL group, suggesting earlier onset of puberty. An interaction between 5HTTLPR polymorphisms and fluoxetine was identified for femur and tibia growth; the 5HTTLPR effect was seen in controls (40% less growth for LL) but not in the fluoxetine treated group (10% less growth for LL). A role for serotonin in peripubertal skeletal growth and maturation has not previously been investigated but may be relevant to treatment of children with SSRIs.

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Gene Expression Profile during Chondrogenesis in Human Bone Marrow derived Mesenchymal Stem Cells using a cDNA Microarray

Cited by 18 publications

References 29 publications

Identification of new genes associated to senescent and tumorigenic phenotypes in mesenchymal stem cells

Identification of new genes associated to senescent and tumorigenic phenotypes in mesenchymal stem cells

Human chondrocyte migration behaviour to guide the development of engineered cartilage

Bone growth in juvenile rhesus monkeys is influenced by 5HTTLPR polymorphisms and interactions between 5HTTLPR polymorphisms and fluoxetine

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