Your search keyword '"Flaibani, Marina"' showing total 3 results

1. A combining method to enhance the in vitro differentiation of hepatic precursor cells.

Author

Carraro A, Flaibani M, Cillo U, Michelotto L, Magrofuoco E, Buggio M, Abatangelo G, Cortivo R, Herrera MB, Tetta C, Elvassore N, and Zavan B

Subjects

Adult, Cell Culture Techniques methods, Cell Proliferation, Cell Survival, Cells, Cultured, Coculture Techniques methods, Hepatocytes cytology, Humans, Liver cytology, Models, Biological, Models, Theoretical, Adult Stem Cells cytology, Adult Stem Cells physiology, Cell Differentiation physiology, Hepatocytes physiology, Tissue Engineering methods

Abstract

The ideal bioartificial liver should be designed to reproduce as nearly as possible in vitro the habitat that hepatic cells find in vivo. In the present work, we investigated the in vitro perfusion condition with a view to improving the hepatic differentiation of pluripotent human liver stem cells (HLSCs) from adult liver. Tissue engineering strategies based on the cocultivation of HLSCs with hepatic stellate cells (ITO) and with several combinations of medium were applied to improve viability and differentiation. A mathematical model estimated the best flow rate for perfused cultures lasting up to 7 days. Morphological and functional assays were performed. Morphological analyses confirmed that a flow of perfusion medium (assured by the bioreactor system) enabled the in vitro organization of the cells into liver clusters even in the deeper levels of the sponge. Our results showed that, when cocultured with ITO using stem cell medium, HLSCs synthesized a large amount of albumin and the MTT test confirmed an improvement in cell proliferation. In conclusion, this study shows that our in vitro cell conditions promote the formation of clusters of HLSCs and enhance the functional differentiation into a mature hepatic population.

Published

2010

2. Muscle differentiation and myotubes alignment is influenced by micropatterned surfaces and exogenous electrical stimulation.

Author

Flaibani M, Boldrin L, Cimetta E, Piccoli M, De Coppi P, and Elvassore N

Subjects

Animals, Cell Separation, Cells, Cultured, Desmin genetics, Desmin metabolism, Electric Stimulation, Gene Expression Regulation drug effects, Lactic Acid pharmacology, Membranes, Artificial, Muscle Fibers, Skeletal drug effects, Muscle Fibers, Skeletal metabolism, Myoblasts drug effects, Myoblasts metabolism, Myogenin genetics, Myogenin metabolism, Nitrogen Dioxide metabolism, Polyesters, Polymers pharmacology, Rats, Rats, Wistar, Reproducibility of Results, Reverse Transcriptase Polymerase Chain Reaction, Surface Properties drug effects, Troponin I metabolism, Cell Differentiation drug effects, Muscle Fibers, Skeletal cytology, Myoblasts cytology, Tissue Engineering methods

Abstract

An in vitro muscle-like structure with parallel-oriented contractile myotubes is needed as a model of muscle tissue regeneration. For this purpose, it is necessary to reproduce a controllable microscale environment mimicking the in vivo cues. In this work we focused on the application of topological and electrical stimuli on muscle precursor cell (MPC) culture to influence MPC orientation and induce myotube alignment. The two stimulations were tested both independently and together. A structural and topological template was achieved using micropatterned poly-(L-lactic acid) membranes. Electrical stimulation, consisting of square pulses of 70 mV/cm amplitude each 30 s, was applied to the MPC culture. The effect of different pulse durations on cultures was evaluated by galvanotaxis analysis. The highest cell displacement rate toward the cathode was observed for 3 ms pulse stimulation, which was then applied in combination with topological stimuli. Topological and electrical stimuli had an additive effect in enhancing differentiation of cultured MPC, shown by high Troponin I protein production and, in parallel, Myogenin and Desmin genes, down- and upregulation respectively.

Published

2009

3. Ultrastructure of Glioblastoma cells in baseline conditions and following mTOR inhibtion

Author

Ryskalin, Larisa, Lenzi, Paola, Falleni, Alessandra, Guagnozzi, Mariangela, Paparelli, Silvio, Bartalucci, Alessia, Flaibani, Marina, and Fornai, Francesco

Subjects

Rapamycin, autophagy, electron microscopy, cell differentiation, autophagy vacuoles

Abstract

Glioblastoma Multiforme (GBM), a WHO grade IV malignant glioma, is the most common, aggressive and lethal primary brain tumor [1]. GBM poses a unique challenge due to its propensity for proliferation and tissue invasion. Multiple experimental and pathological findings suggest that, at molecular level, the up-regulation of the molecular complex mTOR plays a pivotal role in determining cell growth, stem cell proliferation, infiltration, relapse and resistance to standard treatments [2]. When activated, mTOR controls and modulates, directly or indirectly, several cellular events and biochemical pathways [3,4]; in particular, mTOR acts as a negative modulator of autophagy, resulting in a defective autophagy in GBM. In the present study we analyzed the ultrastructural correlates of autophagy inhibition in GBM cells and we reverted various alterations by administering the mTOR inhibitor rapamycin. Rapamycin effects were both dose- and time-dependent and consisted in reducing cell proliferation and inducing cell differentiation. In particular, rapamycin was able to restore autophagy vacuoles and it increased specific markers of neuronal differentiation while it inhibited stem cell-like phenotype. The present data lend substance to mTOR and autophagy as critical determinant in astrocytomas and provide the first ultrastructural evidence of autophagy modulation in these brain tumors., Italian Journal of Anatomy and Embryology, Vol 119, No 1 (Supplement) 2014

Published

2015