Generation and Characterization of Virus-Enhancing Peptide Nanofibrils Functionalized with Fluorescent Labels | Zendy

Sascha Rode | Zendy; Manuel Hayn | Zendy; Annika Röcker | Zendy; Stefanie Sieste | Zendy; Markus Lamla | Zendy; Daniel Markx | Zendy; Christoph A. Meier | Zendy; Frank Kirchhoff | Zendy; Paul Walther | Zendy; Marcus Fändrich | Zendy; Tanja Weil | Zendy; Jan Münch | Zendy

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Generation and Characterization of Virus-Enhancing Peptide Nanofibrils Functionalized with Fluorescent Labels

Author(s) -

Sascha Rode,

Manuel Hayn,

Annika Röcker,

Stefanie Sieste,

Markus Lamla,

Daniel Markx,

Christoph A. Meier,

Frank Kirchhoff,

Paul Walther,

Marcus Fändrich,

Tanja Weil,

Jan Münch

Publication year - 2017

Publication title -

bioconjugate chemistry

Language(s) - English

Resource type - Journals

SCImago Journal Rank - 1.279

H-Index - 172

eISSN - 1520-4812

pISSN - 1043-1802

DOI - 10.1021/acs.bioconjchem.7b00079

Subject(s) - transduction (biophysics) , chemistry , peptide , fluorescence , biophysics , fluorescence microscope , covalent bond , green fluorescent protein , flow cytometry , förster resonance energy transfer , membrane , signal transduction , confocal microscopy , biochemistry , amyloid (mycology) , gene , microbiology and biotechnology , biology , physics , organic chemistry , quantum mechanics , inorganic chemistry

Retroviral gene transfer is the method of choice for the stable introduction of genetic material into the cellular genome. However, efficient gene transfer is often limited by low transduction rates of the viral vectors. We have recently described a 12-mer peptide, termed EF-C, that forms amyloid-like peptide nanofibrils (PNF), strongly increasing viral transduction efficiencies. These nanofibrils are polycationic and bind negatively charged membranes of virions and cells, thereby overcoming charge repulsions and resulting in increased rates of virion attachment and gene transfer. EF-C PNF enhance vector transduction more efficiently than other soluble additives and offer prospects for clinical applications. However, while the transduction-enhancing activity of PNF has been well-characterized, the exact mechanism and the kinetics underlying infection enhancement as well as the cellular fate of the fibrils are hardly explored. This is partially due to the fact that current labeling techniques for PNF rely on amyloid probes that cause high background staining or lose signal intensities after cellular uptake. Here, we sought to generate EF-C PNF covalently coupled with fluorescent labels. To achieve such covalent bioconjugates, the free amino groups of the EF-C peptide were coupled to the ATTO 495 or 647N NHS ester dyes. When small amounts of the labeled peptides were mixed with a 100- to 10 000-fold excess of the native peptide, PNF formed that were morphologically indistinguishable from those derived from the unlabeled peptide. The fluorescence of the fibrils could be readily detected using fluorescence spectroscopy, microscopy, and flow cytometry. In addition, labeled and nonlabeled fibrils captured viral particles and increased retroviral transduction with similar efficacy. These covalently fluorescence-labeled PNF are valuable tools with which to elucidate the mechanism(s) underlying transduction attachment and the fate of the fibrils in cells, tissues, and animal models.

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