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LINK . SPRINGER . COM {}

  1. Analyzed Page
  2. Matching Content Categories
  3. CMS
  4. Monthly Traffic Estimate
  5. How Does Link.springer.com Make Money
  6. Keywords
  7. Topics
  8. Schema
  9. External Links
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We are analyzing https://link.springer.com/article/10.1186/s12951-015-0141-1.

Title:
Human mesenchymal stem cells labelled with dye-loaded amorphous silica nanoparticles: long-term biosafety, stemness preservation and traceability in the beating heart | Journal of Nanobiotechnology
Description:
Treatment of myocardial infarction with mesenchymal stem cells (MSCs) has proven beneficial effects in both animal and clinical studies. Engineered silica nanoparticles (SiO2-NPs) have been extensively used as contrast agents in regenerative medicine, due to their resistance to degradation and ease of functionalization. However, there are still controversies on their effective biosafety on cellular systems. In this perspective, the aims of the present study are: 1) to deeply investigate the impact of amorphous 50 nm SiO2-NPs on viability and function of human bone marrow-derived MSCs (hMSCs); 2) to optimize a protocol of harmless hMSCs labelling and test its feasibility in a beating heart model. Optimal cell labelling is obtained after 16 h exposure of hMSCs to fluorescent 50 nm SiO2-NPs (50 µg mL−1); interestingly, lysosomal activation consequent to NPs storage is not associated to oxidative stress. During prolonged culture hMSCs do not undergo cyto- or genotoxicity, preserve their proliferative potential and their stemness/differentiation properties. Finally, the bright fluorescence emitted by internalized SiO2-NPs allows both clear visualization of hMSCs in normal and infarcted rat hearts and ultrastructural analysis of cell engraftment inside myocardial tissue. Overall, 50 nm SiO2-NPs display elevated compatibility with hMSCs in terms of lack of cyto- and genotoxicity and maintenance of important features of these cells. The demonstrated biosafety, combined with proper cell labelling and visualization in histological sections, make these SiO2-NPs optimal candidates for the purpose of stem cell tracking inside heart tissue.
Website Age:
28 years and 1 months (reg. 1997-05-29).

Matching Content Categories {📚}

  • Science
  • Education
  • Telecommunications

Content Management System {📝}

What CMS is link.springer.com built with?

Custom-built

No common CMS systems were detected on Link.springer.com, and no known web development framework was identified.

Traffic Estimate {📈}

What is the average monthly size of link.springer.com audience?

🌠 Phenomenal Traffic: 5M - 10M visitors per month


Based on our best estimate, this website will receive around 8,123,328 visitors per month in the current month.

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How Does Link.springer.com Make Money? {💸}

We don’t know how the website earns money.

Many websites are intended to earn money, but some serve to share ideas or build connections. Websites exist for all kinds of purposes. This might be one of them. Link.springer.com could be getting rich in stealth mode, or the way it's monetizing isn't detectable.

Keywords {🔍}

hmscs, sionps, cells, article, cell, google, scholar, fig, stem, inside, cas, labelled, red, mesenchymal, analysis, hearts, min, pbs, heart, nanoparticles, time, treated, human, vitro, magnification, confocal, data, silica, fluorescent, tissue, additional, study, representative, file, internalized, cardiac, differentiation, medium, nuclei, nps, normal, distribution, scale, bar, cultured, experiments, γhax, stress, flow, number,

Topics {✒️}

dye-doped 50 nm sio2-nps hybrid cyanine—silica nanoparticles bone marrow-derived mscs 25 % trypsin-ethylenediamine-tetra acetate 50 nm sio2-nps 50 µg·ml−1 sarcomeric α-actinin allowed dna double-strand-breaks oxygenated krebs-henseleit buffer dna double-strand breaks sio2-nps-exposed hmscs labelled thioacetamide-induced liver injury ��1and insulin 10 µg·ml−1 sarcomeric α-actinin staining newly formed/daughter cells article download pdf amorphous 50 nm sio2-nps sio2-nps optimal candidates limit ros-dependent damage sio2-nps-dependent toxicity internalized fluorescent sio2-nps fluorescent 50 nm sio2-nps mesenchymal stem cells fluorescently labelled sio2-nps warm phosphate-buffered saline early-stage apoptotic cells sio2-nps-treated cells sio2-nps -treated cells internalized 50 nm sio2-nps sio2-nps-exposed cells sio2-nps internalization hmscs long-term cell monitoring sio2-nps-hmscs displayed p38 mapk-mediated alteration obtained sio2-nps exhibited privacy choices/manage cookies sio2-nps -labelled hmscs sio2-nps -treated hmscs sio2-nps-treated hmscs human endothelial cells optical inverted microscope sio2-nps-dependent cyto cell stem cell stem cell rev related subjects circulating stem cells stem cells dev contrast agents allowing bmc vet res adult murine heart powerful core shells

Schema {🗺️}

WebPage:
      mainEntity:
         headline:Human mesenchymal stem cells labelled with dye-loaded amorphous silica nanoparticles: long-term biosafety, stemness preservation and traceability in the beating heart
         description:Treatment of myocardial infarction with mesenchymal stem cells (MSCs) has proven beneficial effects in both animal and clinical studies. Engineered silica nanoparticles (SiO2-NPs) have been extensively used as contrast agents in regenerative medicine, due to their resistance to degradation and ease of functionalization. However, there are still controversies on their effective biosafety on cellular systems. In this perspective, the aims of the present study are: 1) to deeply investigate the impact of amorphous 50 nm SiO2-NPs on viability and function of human bone marrow-derived MSCs (hMSCs); 2) to optimize a protocol of harmless hMSCs labelling and test its feasibility in a beating heart model. Optimal cell labelling is obtained after 16 h exposure of hMSCs to fluorescent 50 nm SiO2-NPs (50 µg mL−1); interestingly, lysosomal activation consequent to NPs storage is not associated to oxidative stress. During prolonged culture hMSCs do not undergo cyto- or genotoxicity, preserve their proliferative potential and their stemness/differentiation properties. Finally, the bright fluorescence emitted by internalized SiO2-NPs allows both clear visualization of hMSCs in normal and infarcted rat hearts and ultrastructural analysis of cell engraftment inside myocardial tissue. Overall, 50 nm SiO2-NPs display elevated compatibility with hMSCs in terms of lack of cyto- and genotoxicity and maintenance of important features of these cells. The demonstrated biosafety, combined with proper cell labelling and visualization in histological sections, make these SiO2-NPs optimal candidates for the purpose of stem cell tracking inside heart tissue.
         datePublished:2015-10-29T00:00:00Z
         dateModified:2015-10-29T00:00:00Z
         pageStart:1
         pageEnd:14
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         keywords:
            Mesenchymal stem cells
            Silica nanoparticles
            Toxicity
            Stem cell tracking
            Heart
            Biotechnology
            Nanotechnology
            Molecular Medicine
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ScholarlyArticle:
      headline:Human mesenchymal stem cells labelled with dye-loaded amorphous silica nanoparticles: long-term biosafety, stemness preservation and traceability in the beating heart
      description:Treatment of myocardial infarction with mesenchymal stem cells (MSCs) has proven beneficial effects in both animal and clinical studies. Engineered silica nanoparticles (SiO2-NPs) have been extensively used as contrast agents in regenerative medicine, due to their resistance to degradation and ease of functionalization. However, there are still controversies on their effective biosafety on cellular systems. In this perspective, the aims of the present study are: 1) to deeply investigate the impact of amorphous 50 nm SiO2-NPs on viability and function of human bone marrow-derived MSCs (hMSCs); 2) to optimize a protocol of harmless hMSCs labelling and test its feasibility in a beating heart model. Optimal cell labelling is obtained after 16 h exposure of hMSCs to fluorescent 50 nm SiO2-NPs (50 µg mL−1); interestingly, lysosomal activation consequent to NPs storage is not associated to oxidative stress. During prolonged culture hMSCs do not undergo cyto- or genotoxicity, preserve their proliferative potential and their stemness/differentiation properties. Finally, the bright fluorescence emitted by internalized SiO2-NPs allows both clear visualization of hMSCs in normal and infarcted rat hearts and ultrastructural analysis of cell engraftment inside myocardial tissue. Overall, 50 nm SiO2-NPs display elevated compatibility with hMSCs in terms of lack of cyto- and genotoxicity and maintenance of important features of these cells. The demonstrated biosafety, combined with proper cell labelling and visualization in histological sections, make these SiO2-NPs optimal candidates for the purpose of stem cell tracking inside heart tissue.
      datePublished:2015-10-29T00:00:00Z
      dateModified:2015-10-29T00:00:00Z
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      pageEnd:14
      license:http://creativecommons.org/publicdomain/zero/1.0/
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      keywords:
         Mesenchymal stem cells
         Silica nanoparticles
         Toxicity
         Stem cell tracking
         Heart
         Biotechnology
         Nanotechnology
         Molecular Medicine
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      author:
            name:Clara Gallina
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                  address:
                     name:Department of Clinical and Biological Sciences, University of Turin, Orbassano, Italy
                     type:PostalAddress
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            type:Person
            name:Tânia Capelôa
            affiliation:
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                  address:
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            name:Silvia Saviozzi
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                  name:University of Turin
                  address:
                     name:Department of Clinical and Biological Sciences, University of Turin, Orbassano, Italy
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            name:Lisa Accomasso
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                  address:
                     name:Department of Clinical and Biological Sciences, University of Turin, Orbassano, Italy
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            name:Federico Catalano
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                  address:
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                  address:
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            name:Gianmario Martra
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            address:
               name:Department of Clinical and Biological Sciences, University of Turin, Orbassano, Italy
               type:PostalAddress
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      name:Federico Catalano
      affiliation:
            name:University of Turin
            address:
               name:Department of Clinical and Biological Sciences, University of Turin, Orbassano, Italy
               type:PostalAddress
            type:Organization
            name:University of Turin
            address:
               name:Department of Chemistry, Interdepartmental Centre “Nanostructured Interfaces and Surfaces”, University of Turin, Turin, Italy
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            type:Organization
      name:Francesca Tullio
      affiliation:
            name:University of Turin
            address:
               name:Department of Clinical and Biological Sciences, University of Turin, Orbassano, Italy
               type:PostalAddress
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      name:Gianmario Martra
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            name:University of Turin
            address:
               name:Department of Chemistry, Interdepartmental Centre “Nanostructured Interfaces and Surfaces”, University of Turin, Turin, Italy
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            type:Organization
      name:Claudia Penna
      affiliation:
            name:University of Turin
            address:
               name:Department of Clinical and Biological Sciences, University of Turin, Orbassano, Italy
               type:PostalAddress
            type:Organization
      name:Pasquale Pagliaro
      affiliation:
            name:University of Turin
            address:
               name:Department of Clinical and Biological Sciences, University of Turin, Orbassano, Italy
               type:PostalAddress
            type:Organization
      name:Valentina Turinetto
      affiliation:
            name:University of Turin
            address:
               name:Department of Clinical and Biological Sciences, University of Turin, Orbassano, Italy
               type:PostalAddress
            type:Organization
      name:Claudia Giachino
      affiliation:
            name:University of Turin
            address:
               name:Department of Clinical and Biological Sciences, University of Turin, Orbassano, Italy
               type:PostalAddress
            type:Organization
PostalAddress:
      name:Department of Clinical and Biological Sciences, University of Turin, Orbassano, Italy
      name:Department of Clinical and Biological Sciences, University of Turin, Orbassano, Italy
      name:Department of Clinical and Biological Sciences, University of Turin, Orbassano, Italy
      name:Department of Clinical and Biological Sciences, University of Turin, Orbassano, Italy
      name:Department of Clinical and Biological Sciences, University of Turin, Orbassano, Italy
      name:Department of Chemistry, Interdepartmental Centre “Nanostructured Interfaces and Surfaces”, University of Turin, Turin, Italy
      name:Department of Clinical and Biological Sciences, University of Turin, Orbassano, Italy
      name:Department of Chemistry, Interdepartmental Centre “Nanostructured Interfaces and Surfaces”, University of Turin, Turin, Italy
      name:Department of Clinical and Biological Sciences, University of Turin, Orbassano, Italy
      name:Department of Clinical and Biological Sciences, University of Turin, Orbassano, Italy
      name:Department of Clinical and Biological Sciences, University of Turin, Orbassano, Italy
      name:Department of Clinical and Biological Sciences, University of Turin, Orbassano, Italy

External Links {🔗}(138)

Analytics and Tracking {📊}

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