Literature DB >> 18397318

Study of uptake of cell penetrating peptides and their cargoes in permeabilized wheat immature embryos.

Archana Chugh1, François Eudes.   

Abstract

The uptake of five fluorescein labeled cell-penetrating peptides (Tat, Tat(2), mutated-Tat, peptide vascular endothelial-cadherin and transportan) was studied in wheat immature embryos. Interestingly, permeabilization treatment of the embryos with toluene/ethanol (1 : 20, v/v with permeabilization buffer) resulted in a remarkably higher uptake of cell-penetrating peptides, whereas nonpermeabilized embryos failed to show significant cell-penetrating peptide uptake, as observed under fluorescence microscope and by fluorimetric analysis. Among the cell-penetrating peptides investigated, Tat monomer (Tat) showed highest fluorescence uptake (4.2-fold greater) in permeabilized embryos than the nonpermeabilized embryos. On the other hand, mutated-Tat serving as negative control did not show comparable fluorescence levels even in permeabilized embryos. A glucuronidase histochemical assay revealed that Tat peptides can efficiently deliver functionally active beta-glucuronidase (GUS) enzyme in permeabilized immature embryos. Tat(2)-mediated GUS enzyme delivery showed the highest number of embryos with GUS uptake (92.2%) upon permeabilization treatment with toluene/ethanol (1 : 40, v/v with permeabilization buffer) whereas only 51.8% of nonpermeabilized embryos showed Tat(2)-mediated GUS uptake. Low temperature, endocytosis and macropinocytosis inhibitors reduced delivery of the Tat(2)-GUS enzyme cargo complex. The results suggest that more than one mechanism of cell entry is involved simultaneously in cell-penetrating peptide-cargo uptake in wheat immature embryos. We also studied Tat(2)-plasmid DNA (carrying Act-1GUS) complex formation by gel retardation assay, DNaseI protection assay and confocal laser microscopy. Permeabilized embryos transfected with Tat(2)-plasmid DNA complex showed 3.3-fold higher transient GUS gene expression than the nonpermeabilized embryos. Furthermore, addition of cationic transfecting agent Lipofectamine 2000 to the Tat(2)-plasmid DNA complex resulted in 1.5-fold higher transient GUS gene expression in the embryos. This is the first report demonstrating translocation of various cell-penetrating peptides and their potential to deliver macromolecules in wheat immature embryos in the presence of a cell membrane permeabilizing agent.

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Year:  2008        PMID: 18397318     DOI: 10.1111/j.1742-4658.2008.06384.x

Source DB:  PubMed          Journal:  FEBS J        ISSN: 1742-464X            Impact factor:   5.542


  12 in total

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3.  A novel method of transgene delivery into triticale plants using the Agrobacterium transferred DNA-derived nano-complex.

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Review 4.  Applications of CPPs in Genome Editing of Plants.

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5.  Gene Delivery to Tobacco Root Cells with Single-Walled Carbon Nanotubes and Cell-Penetrating Fusogenic Peptides.

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6.  Cell-penetrating peptide-driven Cre recombination in porcine primary cells and generation of marker-free pigs.

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Journal:  PLoS One       Date:  2018-01-09       Impact factor: 3.240

7.  A mitochondria-targeted coenzyme Q peptoid induces superoxide dismutase and alleviates salinity stress in plant cells.

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8.  A Peptoid Delivers CoQ-derivative to Plant Mitochondria via Endocytosis.

Authors:  Kinfemichael Geressu Asfaw; Qiong Liu; Jan Maisch; Stephan W Münch; Ilona Wehl; Stefan Bräse; Ivan Bogeski; Ute Schepers; Peter Nick
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9.  Tetrabutylphosphonium Bromide Reduces Size and Polydispersity Index of Tat2:siRNA Nano-Complexes for Triticale RNAi.

Authors:  Jordan T Pepper; Priti Maheshwari; Alicja Ziemienowicz; Paul Hazendonk; Igor Kovalchuk; François Eudes
Journal:  Front Mol Biosci       Date:  2017-05-16

10.  Library screening of cell-penetrating peptide for BY-2 cells, leaves of Arabidopsis, tobacco, tomato, poplar, and rice callus.

Authors:  Keiji Numata; Yoko Horii; Kazusato Oikawa; Yu Miyagi; Taku Demura; Misato Ohtani
Journal:  Sci Rep       Date:  2018-07-20       Impact factor: 4.379

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