4.8 Article

Nerve growth factor expression by PLG-mediated lipofection

Journal

BIOMATERIALS
Volume 27, Issue 11, Pages 2477-2486

Publisher

ELSEVIER SCI LTD
DOI: 10.1016/j.biomaterials.2005.11.016

Keywords

gene transfer; PLG; nerve growth factor; nerve regeneration; nerve guide

Funding

  1. NIBIB NIH HHS [R01 EB003806, R01 EB003806-01] Funding Source: Medline
  2. NINDS NIH HHS [F31 NS042364, F31 NS042364-01] Funding Source: Medline

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Biomaterials capable of efficient gene delivery provide a fundamental tool for basic and applied research models, such as promoting neural regeneration. We developed a system for the encapsulation and sustained release of plasmid DNA complexed with a cationic lipid and investigated their efficacy using in vitro models of neurite outgrowth. Sustained lipoplex release was obtained for up to 50 days, with rates controlled by the fabrication conditions. Released lipoplexes retained their activity, transfecting 48.2 +/- 8.3% of NIH3T3 cells with luciferase activity of 3.97 x 10(7) RLU/nig. Expression of nerve growth factor (NGF) was employed in two models of neurite outgrowth: PC12 and primary dorsal root ganglia (DRG) co-culture. Polymer-mediated lipofection of PC12 produced. bioactive NGF, eliciting robust neurite outgrowth. An EGFP/NGF dual-expression vector identified transfected cells (GFP-positive) while neurite outgrowth verified NGF secretion. A co-culture model examined the ability of NGF secretion by an accessory cell population to stimulate DRG neurite outgrowth. Polymer-mediated transfection of HEK293T with an NGF-encoding plasmid induced outgrowth by DRG neurons. This system could be fabricated as implants or nerve guidance conduits to support cellular and tissue regeneration. Combining this physical support with the ability to locally express neurotrophic factors will potentiate regeneration in nerve injury and disease models. (c) 2005 Elsevier Ltd. All rights reserved.

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