Structure-based peptide ligand design for improved epidermal growth factor receptor targeted gene delivery

[Display omitted] The epidermal growth factor receptor EGFR allows targeted delivery of macromolecular drugs to tumors. Its ligand, epidermal growth factor, binds EGFR with high affinity but acts mitogenic. Non-mitogenic peptides are utilized as targeting ligands, like the dodecapeptide GE11, althou...

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Published inEuropean journal of pharmaceutics and biopharmaceutics Vol. 176; pp. 211 - 221
Main Authors Decker, Simon, Taschauer, Alexander, Geppl, Emanuela, Pirhofer, Viktoria, Schauer, Michael, Pöschl, Stephan, Kopp, Florian, Richter, Lars, Ecker, Gerhard F., Sami, Haider, Ogris, Manfred
Format Journal Article
LanguageEnglish
Published Netherlands Elsevier B.V 01.07.2022
Subjects
EGFR
GE11
Polyplex
Targeted gene delivery
Transfection
Polyplex
RU
EDC
Gln
NaOH
LPEI
HBG
EGFR
TFA
hEGFR
HRMS
GLuc
Transfection
SPR
NHS
ESI
Fmoc
RLU
GE11
CID
BCA
SDS
OPSS
AF
EGF
Targeted gene delivery
RP-HPLC
PEG
pDNA
HEPES
ζ
FCS
S-NHS
ITC
DPBS
targeted gene delivery
transfection
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Summary:[Display omitted] The epidermal growth factor receptor EGFR allows targeted delivery of macromolecular drugs to tumors. Its ligand, epidermal growth factor, binds EGFR with high affinity but acts mitogenic. Non-mitogenic peptides are utilized as targeting ligands, like the dodecapeptide GE11, although its low binding affinity warrants improvement. We applied a two-step computational approach with database search and molecular docking to design GE11 variants with improved binding. Synthesized peptides underwent binding studies on immobilized EGFR using surface plasmon resonance. Conjugates of peptides coupled via heterobifunctional PEG linker to linear polyethylenimine (LPEI) were used for transfection studies on EGFR-overexpressing cells using reporter gene encoding plasmid DNA. Docking studies unraveled similarities between GE11 and the EGFR dimerization arm. By skipping non-overlapping amino acids, a less hydrophobic segment (YTPQNVI) was identified to be directly involved in EGFR binding. By replacing valine by tyrosine, a full-length version with proposed enhanced binding (GE11m3) was developed. While hydrophobic or hydrophilic segments and variations thereof exhibited low binding, GE11m3 exhibited 3-fold increase in binding compared to GE11, validating in silico predictions. In transfection studies, polyplexes with GE11m3 induced a significantly higher reporter gene expression when compared to GE11 polyplexes both on murine and human cancer cells overexpressing EGFR.
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ISSN:0939-6411
1873-3441
DOI:10.1016/j.ejpb.2022.05.004