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Dive into the research topics where Francesca Pagliari is active.

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Featured researches published by Francesca Pagliari.


Nano-micro Letters | 2017

Fabrication and Applications of Micro/Nanostructured Devices for Tissue Engineering

Tania Limongi; Luca Tirinato; Francesca Pagliari; Andrea Giugni; Marco Allione; Gerardo Perozziello; Patrizio Candeloro; Enzo Di Fabrizio

Nanotechnology allows the realization of new materials and devices with basic structural unit in the range of 1–100xa0nm and characterized by gaining control at the atomic, molecular, and supramolecular level. Reducing the dimensions of a material into the nanoscale range usually results in the change of its physiochemical properties such as reactivity, crystallinity, and solubility. This review treats the convergence of last research news at the interface of nanostructured biomaterials and tissue engineering for emerging biomedical technologies such as scaffolding and tissue regeneration. The present review is organized into three main sections. The introduction concerns an overview of the increasing utility of nanostructured materials in the field of tissue engineering. It elucidates how nanotechnology, by working in the submicron length scale, assures the realization of a biocompatible interface that is able to reproduce the physiological cell–matrix interaction. The second, more technical section, concerns the design and fabrication of biocompatible surface characterized by micro- and submicroscale features, using microfabrication, nanolithography, and miscellaneous nanolithographic techniques. In the last part, we review the ongoing tissue engineering application of nanostructured materials and scaffolds in different fields such as neurology, cardiology, orthopedics, and skin tissue regeneration.


BioMed Research International | 2009

Interfacing Sca-1pos Mesenchymal Stem Cells with Biocompatible Scaffolds with Different Chemical Composition and Geometry

Giancarlo Forte; Ornella Franzese; Stefania Pagliari; Francesca Pagliari; A. M. Di Francesco; Paolo Cossa; A. Laudisi; Roberta Fiaccavento; Marilena Minieri; E. Bonmassar; P. Di Nardo

An immortalized murine mesenchymal stem cell line (mTERT-MSC) enriched for Linneg/Sca-1pos fraction has been obtained through the transfection of MSC with murine TERT and single-cell isolation. Such cell line maintained the typical MSC self-renewal capacity and continuously expressed MSC phenotype. Moreover, mTERT-MSC retained the functional features of freshly isolated MSC in culture without evidence of senescence or spontaneous differentiation events. Thus, mTERT-MSC have been cultured onto PLA films, 30 and 100 μm PLA microbeads, and onto unpressed and pressed HYAFF-11 scaffolds. While the cells adhered preserving their morphology on PLA films, clusters of mTERT-MSC were detected on PLA beads and unpressed fibrous scaffolds. Finally, mTERT-MSC were not able to colonize the inner layers of pressed HYAFF-11. Nevertheless, such cell line displayed the ability to preserve Sca-1 expression and to retain multilineage potential when appropriately stimulated on all the scaffolds tested.


Stem Cells International | 2017

An Overview of Lipid Droplets in Cancer and Cancer Stem Cells

Luca Tirinato; Francesca Pagliari; Tania Limongi; Monica Marini; Andrea Falqui; J. Seco; P. Candeloro; Carlo Liberale; E. Di Fabrizio

For decades, lipid droplets have been considered as the main cellular organelles involved in the fat storage, because of their lipid composition. However, in recent years, some new and totally unexpected roles have been discovered for them: (i) they are active sites for synthesis and storage of inflammatory mediators, and (ii) they are key players in cancer cells and tissues, especially in cancer stem cells. In this review, we summarize the main concepts related to the lipid droplet structure and function and their involvement in inflammatory and cancer processes.


Archive | 2017

Cardiac Progenitor Cell Extraction from Human Auricles

Paolo Di Nardo; Francesca Pagliari

For many years, myocardial tissue has been considered terminally differentiated and, thus, incapable of regenerating. Recent studies have shown, instead, that cardiomyocytes, at least in part, are slowly substituted by new cells originating by precursor cells mostly embedded into the heart apex and in the atria. We have shown that an elective region of progenitor cell embedding is represented by the auricles, non-contractile atria appendages that can be easily sampled without harming the patient. The protocol here reported describes how from auricles a population of multipotent, cardiogenic cells can be isolated, cultured, and differentiated. Further studies are needed to fully exploit this cell population, but, sampling auricles, it could be possible to treat cardiac patients using their own cells circumventing rejection or organ shortage limitations.


Archive | 2016

The New Youth of the In Situ Transmission Electron Microscopy

Alberto Casu; Elisa Sogne; Alessandro Genovese; Cristiano DiBenedetto; Sergio Lentijo Mozo; Efisio Zuddas; Francesca Pagliari; Andrea Falqui

The idea of in situ transmission electron microscopy (TEM) and its possible ramifica‐ tions were proposed at the very dawn of electron microscopy, but the translation from theory to practice encountered many technological setbacks, which hindered the feasibility of the most elaborated approaches until recent times. However, the several technological improvements achieved in the last 10–15 years filled this gap, allowing the direct observation of the dynamic response of materials to external stimuli under a vast range of conditions going from vacuum to gaseous or liquid environment. This resulted in a blossoming of the in situ TEM and scanning TEM (STEM) techniques to a new youth for a vast, growing range of applications, which cannot be rightfully detailed in a short span; therefore, this chapter should be intended as a guide highlighting a selection of the most inspiring, recently achieved results.


TERMIS World Congress | 2012

Human cardiac progenitor cell sheets as a source of autologous contractile and vascular cells for cardiac repair

Giancarlo Forte; Stefano Pietronave; Giorgia Nardone; Andrea Zamperone; Stefania Pagliari; Francesca Pagliari; Teruo Okano; Marilena Minieri; Maria Prat; P Di Nardo

Adequate cellular in-growth into biomaterials is one of the fundamental requirements in regenerative medicine. Type-I-collagen is the most commonly used material for soft tissue engineering, because it is nonimmunogenic and a highly porous network for cellular support. However, adequate cell in-growth and cell seeding has been suboptimal. Different densities of collagen scaffolds (0.3% to 0.8% (w/v)) with/without polymer knitting (poly-caprolactone (PCL)) were prepared. The structure of collagen scaffolds was characterized using scanning electronic microscopy (SEM) and HE staining. The mechanical strength of hybrid scaffolds was determined using tensile strength analysis. Cellular penetration and interconnectivity were evaluated using fluorescent bead distribution and human bladder smooth muscle cells and urothelium seeding. SEM and HE analysis showed the honeycomb structure and the hybrid scaffolds were adequately connected. The hybrid scaffolds were much stronger than collagen alone. The distribution of the beads and cells were highly dependent on the collagen density: at lower densities the beads and cells were more evenly distributed and penetrated deeper into the scaffold. The lower density collagen scaffolds showed remarkably deeper cellular penetration and by combining it with PCL knitting the tensile strength was enhanced. This study indicated that a 0.4% hybrid scaffold strengthened with knitting achieved the best cellular distribution.Human adult heart harbors a population of resident progenitor cells nthat can be isolated by Sca-1 antibody and expanded in culture. These ncells can differentiate into cardiomyocytes and vascular cells in vitro nand contribute to cardiac regeneration in vivo. However, when directly ninjected as single cell suspension, the survival rate and retention is nreally poor, less than 1% of injected cells being detectable in the hosttissue within few weeks. The present study aimed at investigating the npossibility to produce scaffoldless, thick cardiac progenitor cell-derived ncardiac patches by thermo-responsive technology. Human cardiac progenitors nobtained from the auricles of patients were cultured as scaffoldless nengineered tissues fabricated using temperature-responsive nsurfaces obtained by poly-N-isopropylacrylamide (PNIPAAm) surface nimmobilization. In the engineered tissue, progenitor cells established nproper three-dimensional intercellular relationships and produced nabundant extracellular matrix, while preserving their phenotype and nplasticity. Cell phenotype and viability within the 3D construct were followed nfor 1 week, showing that no significant differentiation or apoptotic nevents occurred within the construct. After engineered tissues nwere leant on visceral pericardium, a number of cells migrated into the nmyocardium and in the vascular walls, where they integrated in the nrespective textures. The study demonstrates the suitability of such napproach to deliver stem cells.Spinal cord injury and repair is one of the important focus areas in tissue regeneration. Mechanical trauma caused due to factors such as contusion, compression or involuntary stretching induce post-traumatic secondary tissue damage in many Spinal Cord Injury (SCI) patients. Therefore, there is a need for scaffolds that provide a conducive threedimensionsal (3D) environment for injured cells to attach and grow. In this study we propose to synthesize 3D polymeric scaffolds in order to study the mechanical and adhesive properties & the nature of the interactions between hyaluronan-based (HY) biomaterials and cells and tissues both in vitroandin vivo. Here we have synthesized 3D HY-based hydrogels with robust mechanical and adhesive properties and demonstrate the use of this material for neuronal-related applications such as the treatment of SCI. Cell culture and survivability studies were done with NSC-34 cells. Live/Dead assay performed on the cells revealed significant differences in the staining of live cells and showed increased viability and proliferation. The number of live cells in the HY-based hydrogels with 0.1% collagen showed higher cell numbers compared with the other hydrogels. In this study we show that Injectable HYbased hydrogels with high elasticity, comparable to the mechanical properties of nervous tissue have been used in this study to study their biocompatibility and neuroprotective properties and they show better affinity for neuronal cells.Calcium phosphates (CaP) obtained by biomineralisation in Simulated Boby Fluid have been used for decades to assess the mineralisation capability of biomaterials. Recently, they have been envisioned as potential agents to promote bone formation. In this study, we have fabricated and coated with calcium phosphate melt electrospun scaffolds whereby macropores permit adequate cell migration and nutrient transfer. We have systematically investigated the effect of coating and osteoinduction onto the response of ovine osteoblasts and we observed that the coating up-regulated alkaline phosphatase activity regardless of the in vitro culture conditions. Micro Computed Tomography revealed that only scaffolds cultured in an osteoinductive cocktail were capable of depositing mineralised matrix, and that CaP coated scaffolds were more efficient at promoting mineralisation. Theses scaffolds were subcutaneously implanted in athymic rats and this demonstrated that the osteoinduction was a pre-requisite for bone formation in this ectopic model. It showed that although the bone formation was not significantly different after 8 weeks, the CaP coated scaffolds were superior at inducing bone formation as evidenced by higher levels of mineralisation at earlier time points. This work demonstrated that CaP coating is not sufficient to induce bone formation; however the combination of osteoinduction and CaP coating resulted in earlier bone formation in an ectopic model.Introduction: Bladder regeneration using minced bladder mucosa is an alternative to costly and time-consuming conventional in vitro culturing of urothelial cells. In this method, the uroepithelium ...


Microelectronic Engineering | 2017

Laboratory injection molder for the fabrication of polymeric porous poly-epsilon-caprolactone scaffolds for preliminary mesenchymal stem cells tissue engineering applications

Tania Limongi; Lucia Lizzul; Andrea Giugni; Luca Tirinato; Francesca Pagliari; Hua Tan; Gobind Das; Manola Moretti; Monica Marini; Giovanna Brusatin; Andrea Falqui; Bruno Torre; Cristiano Di Benedetto; Enzo Di Fabrizio


Journal of Molecular and Cellular Cardiology | 2008

Stem cell-derived cardiac patches: A tissue engineering approach to cardiac healing

Giancarlo Forte; Felicia Carotenuto; Francesca Pagliari; Stefania Pagliari; Paolo Cossa; Roberta Fiaccavento; Arti Ahluwalia; Giovanni Vozzi; B. Vinci; Annalucia Serafino; Marilena Minieri; P. Di Nardo


Bio-Optics: Design and Application | 2017

Quantum cascade laser infrared spectroscopy of single cancer cells

Imran I. Patel; Vijayakumar P. Rajamanickam; Andrea Bertoncini; Francesca Pagliari; Luca Tirinato; Sergey Laptenok; Carlo Liberale


Disputationes - Adult Progenitor Cell Standardization | 2010

Developing an Organotypic in vitro 3D Toxicological Test by a Continuous, Stable, non-Tumourogeic Mesenchymal Progenitors Cell Line Derived from the Rat Dental Pulp

Gn Berta; Francesca Pagliari; F Di Scipio; Stefania Pagliari; Andrea Elio Sprio; P Salamone; Eugenio Magnani; Giorgia Nardone; Giancarlo Forte; P Di Nardo

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Giancarlo Forte

University of Rome Tor Vergata

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Stefania Pagliari

University of Rome Tor Vergata

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Marilena Minieri

University of Rome Tor Vergata

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Luca Tirinato

King Abdullah University of Science and Technology

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Paolo Cossa

University of Rome Tor Vergata

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Roberta Fiaccavento

University of Rome Tor Vergata

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Andrea Falqui

King Abdullah University of Science and Technology

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Tania Limongi

King Abdullah University of Science and Technology

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Carlo Liberale

Istituto Italiano di Tecnologia

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