Literature DB >> 19056421

Intracellular delivery of proteins into mouse Müller glia cells in vitro and in vivo using Pep-1 transfection reagent.

Minhua H Wang1, Laura J Frishman, Deborah C Otteson.   

Abstract

Direct protein transfection is a potentially valuable tool for studying protein function in basic and clinical research. A major challenge is to enable a sufficiently large amount of protein to penetrate the plasma membrane of the transfected cells. Pep-1, a protein transfection reagent, was evaluated for its ability and efficiency in delivering proteins and antibodies into mouse Müller cells in vitro and in vivo. Pep-1 delivered active beta-galactosidase enzyme and antibodies (non-specific IgG and Cy3-conjugated anti-vimentin) into cultured Müller cells with high efficiency. Transfection efficiency increased with increasing concentration of the protein in the complex and with incubation time. Following intravitreal injection of Pep-1/IgG complexes in vivo, retinal histology was preserved and immunostaining showed that the antibodies were distributed widely across the retinal surface, with the most intense staining located near the retino-vitreal border. For complexes using non-specific IgG, double staining with anti-glutamine synthetase identified many IgG-positive cells as Müller glia. IgG immunoreactivity was also detected in the cytoplasm and occasionally in the nuclei of inner retinal neurons. Dark-adapted flash electroretinogram (ERG) recordings from injected eyes were nearly identical to ERG recordings from control eyes, suggesting that injection of Pep-1/IgG complex has minimal effects on retinal function. Therefore, Pep-1 is a useful tool for intracellular delivery of antibodies to study the role of proteins in living cells.

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Year:  2008        PMID: 19056421      PMCID: PMC2681185          DOI: 10.1016/j.jneumeth.2008.10.039

Source DB:  PubMed          Journal:  J Neurosci Methods        ISSN: 0165-0270            Impact factor:   2.390


  53 in total

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Authors:  J G Robson; H Maeda; S M Saszik; L J Frishman
Journal:  Vision Res       Date:  2004-12       Impact factor: 1.886

9.  Disruption of the vimentin intermediate filament system during adipose conversion of 3T3-L1 cells inhibits lipid droplet accumulation.

Authors:  J G Lieber; R M Evans
Journal:  J Cell Sci       Date:  1996-12       Impact factor: 5.285

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Authors:  V Prahlad; M Yoon; R D Moir; R D Vale; R D Goldman
Journal:  J Cell Biol       Date:  1998-10-05       Impact factor: 10.539

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  5 in total

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2.  A conditional immortalized mouse muller glial cell line expressing glial and retinal stem cell genes.

Authors:  Deborah C Otteson; M Joseph Phillips
Journal:  Invest Ophthalmol Vis Sci       Date:  2010-05-26       Impact factor: 4.799

3.  Inhibition of TXNIP expression in vivo blocks early pathologies of diabetic retinopathy.

Authors:  L Perrone; T S Devi; K-I Hosoya; T Terasaki; L P Singh
Journal:  Cell Death Dis       Date:  2010-08-19       Impact factor: 8.469

4.  Functional characterization of a competitive peptide antagonist of p65 in human macrophage-like cells suggests therapeutic potential for chronic inflammation.

Authors:  Mythily Srinivasan; Corinne Blackburn; Debomoy K Lahiri
Journal:  Drug Des Devel Ther       Date:  2014-12-03       Impact factor: 4.162

5.  Cell-Penetrating Peptides as a Tool for the Cellular Uptake of a Genetically Modified Nitroreductase for use in Directed Enzyme Prodrug Therapy.

Authors:  Simon D Anderson; Robert J Hobbs; Vanessa V Gwenin; Patrick Ball; Lindsey A Bennie; Jonathan A Coulter; Chris D Gwenin
Journal:  J Funct Biomater       Date:  2019-10-01
  5 in total

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