Applicability of the Dyes CFSE, CM-DiI and PKH26 for Tracking of Human Preadipocytes to Evaluate Adipose Tissue Engineering

Hemmrich, Karsten; Meersch, Melanie; Heimburg, Dennis von; Pallua, Norbert

doi:10.1159/000099618

Cited by 41 publications

(48 citation statements)

References 62 publications

(43 reference statements)

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“…Recently, it has been reported by Banas et al [2007] that TTR is expressed in ADSC CD105+ differentiated into hepatic lineage. In our previous study [Raposio et al, 2008], we verified that MTT test, DNA assay and CFSE staining were suitable analyses to evaluate cell proliferation in undifferentiated ADSC, in accordance with other data in the literature [Hemmrich et al, 2006;Liu et al, 2008;Zaminv et al, 2008]. So, we apply the above analyses to evaluate the proliferation rate of HA and HB cells.…”

Section: Discussionsupporting

confidence: 82%

A Comparative Study of Proliferation and Hepatic Differentiation of Human Adipose-Derived Stem Cells

Coradeghini

Guida

Scanarotti

et al. 2009

Cells Tissues Organs

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Human adipose-derived stem cells possess a lot of stem cell characteristics, so they may be considered a source of stem cell population. On the basis of that, we have investigated the hepatic potential of adipose-derived stem cells, obtained from liposuction, following two differentiation protocols. In the first procedure, medium was supplemented with epidermal growth factor (EGF), basic fibroblast growth factor, hepatocyte growth factor (HGF) and nicotinamide; the second involved the addition of factors such as dexametasone, EGF, insulin-transferrin-sodium selenite, HGF, dimethyl sulfoxide and oncostatin. In parallel, we carried out our study in the Hep G2 cell line, as human hepatic differentiated in vitro model. Immunocytochemical analysis and RT-PCR were performed using hepatic markers to evaluate cell differentiation. DNA content, MTT test and carboxyl fluorescein succinimidyl ester staining were carried out to evaluate cell proliferation. We reported the evidence of basal hepatic marker in undifferentiated adipose-derived stem cells, which confirmed their multipotency. A strong expression of albumin and α-fetoprotein was observed in hepatic-induced adipose-derived stem cells following both differentiation procedures. Morphological aspects of the two types of hepatic adipose-derived stem cells were alike. Proliferation index suggested that the first differentiation procedure promoted better growth than the second. These preliminary findings suggest adipose-derived stem cells may be induced into hepatic lineage, and the most significant difference between the two standard differentiation procedures concerns proliferation rate. This aspect is to be considered when adipose-derived stem cells are employed in research and clinical studies.

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Section: Discussionsupporting

confidence: 82%

A Comparative Study of Proliferation and Hepatic Differentiation of Human Adipose-Derived Stem Cells

Coradeghini

Guida

Scanarotti

et al. 2009

Cells Tissues Organs

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“…Multipotent NSCs are found in the developing and adult mammalian CNS, including that of humans. 15,27,28 The human NSC line F3 carries the normal human karyotype (46XX) and has the ability to selfrenew, differentiate into cells of neuronal or glial lineage, and integrate into the damaged CNS on transplantation in animal locally converts 5-fluorocytosine into 5-fluorouracil, which interferes with DNA synthesis and results in the death of dividing cells. 27,30,31 Similarly, the TK gene converts the nontoxic drug ganciclovir into a phosphorylated metabolite that acts as a potent killer of dividing cancer cells.…”

Section: Figure 3 Coronal Section 10 Days After F3 Cell Neural Stem mentioning

confidence: 99%

Stereological Analysis on Migration of Human Neural Stem Cells in the Brain of Rats Bearing Glioma

Kim

Lee

Kim³

et al. 2010

Neurosurgery

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“…These include luciferase transfection [Bereziat et al, 2005;Wolbank et al, 2007;Bai et al, 2011], green fluorescent protein [Bereziat et al, 2005;Lin et al, 2006;Yan et al, 2007;Wolbank et al, 2007;Bai et al, 2011], fluorescence in situ hybridization [Li et al, 2008], various fluorochromes [Rieck and Schlaak, 2003;Hemmrich et al, 2006;Yan et al, 2007;Li et al, 2008;Li et al, 2009;Lequeux et al, 2011], iron oxide labeling for MRI [Heymer et al, 2008;Kraitchman and Bulte, 2008;Yan et al, 2007] as well as radionuclide labeling strategies [Hofmann et al, 2005;Yan et al, 2007].…”

Section: Introductionmentioning

confidence: 99%

“…Fluorochromes such as PKH26, a fluorescent surface marker [Rieck and Schlaak, 2003;Hemmrich et al, 2006], BrdU (5-bromo-2-deoxyuridine) which replaces thymidine and incorporates into DNA strands during cell proliferation [Lequeux et al, 2011] and CSFE (Vybrant ® CFDA-SE cell tracer kit) which diffuses passively into the cells [Hemmrich et al, 2006] were analyzed for their applicability to ASCs. In addition, gene transfection procedures resulting in the expression of green fluorescence protein or luciferase were also used to label ASCs [Béréziat et al, 2005;Wolbank et al, 2007].…”

Section: Introductionmentioning

confidence: 99%

DiI Labeling of Human Adipose-Derived Stem Cells: Evaluation of DNA Damage, Toxicity and Functional Impairment

Froelich¹,

Steussloff²,

Schmidt

et al. 2013

Cells Tissues Organs

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Introduction: Adipose tissue-derived stem cells (ASCs) have become the primary focus of tissue engineering research. To understand their functions and behavior in in vitro and in vivo models, it is mandatory to track the implanted cells and distinguish them from the resident or host cells. A common labeling method is the use of fluorescent dyes, e.g. the lipophilic carbocyanine dye, DiI. This study aimed to analyze potential DNA damage, toxicity and impairment of the functional properties of human ASCs after labeling with DiI. Methods: Cytotoxicity was measured using the MTT assay and DNA damage was determined by means of the comet assay. Potential apoptotic effects were determined using the annexin V-propidium iodide test. Differentiation potential was evaluated by trilineage differentiation procedures in labeled and unlabeled ASCs. Proliferation as well as migration capability was analyzed, and the duration and stability of DiI labeling in ASCs during in vitro expansion was observed over a period of 35 days. Results: DiI labeling did not cause genotoxic effects 15, or 30 min or 24 h after the labeling procedure, and there were no cytotoxic effects until 72 h afterwards. No impairment of proliferation or migration capability or differentiation potential could be determined. However, after 35 days, only 37% of labeled cells could be detected using the fluorescence microscope, which indicates a decrease in staining stability during in vitro expansion. Conclusion: DiI is a convenient method for ASCs labeling which causes no toxic effects and does not impair the proliferation, migration or differentiation potential of ASCs after the labeling procedure.

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Applicability of the Dyes CFSE, CM-DiI and PKH26 for Tracking of Human Preadipocytes to Evaluate Adipose Tissue Engineering

Cited by 41 publications

References 62 publications

A Comparative Study of Proliferation and Hepatic Differentiation of Human Adipose-Derived Stem Cells

A Comparative Study of Proliferation and Hepatic Differentiation of Human Adipose-Derived Stem Cells

Stereological Analysis on Migration of Human Neural Stem Cells in the Brain of Rats Bearing Glioma

DiI Labeling of Human Adipose-Derived Stem Cells: Evaluation of DNA Damage, Toxicity and Functional Impairment

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