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Journal of Receptors and Signal Transduction Volume 36, 2016 - Issue 1
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Research Article

Botulinum neurotoxin A and an engineered derivate targeted secretion inhibitor (TSI) A enter cells via different vesicular compartments

Elena FonfriaSyntaxin Ltd an Ipsen Company, Abingdon, UKCorrespondence[email protected]
,
Sarah DonaldSyntaxin Ltd an Ipsen Company, Abingdon, UK
&
Verity A. CaddSyntaxin Ltd an Ipsen Company, Abingdon, UK
Pages 79-88 | Received 13 Jan 2015, Accepted 04 May 2015, Published online: 31 Aug 2015
 
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Abstract

Botulinum neurotoxins (BoNTs) are highly potent multi-domain proteins, responsible for botulism in animals and humans. The modular structural organization of BoNTs has led to the development of novel engineered bio-therapeutic proteins called targeted secretion inhibitors (TSIs). We report here that botulinum neurotoxin A (BoNT/A) and a TSI/A in which the neuronal binding domain of BoNT/A has been substituted by an epidermal growth factor (EGF) ligand, named EGFR-targeted TSI/A, exploit different routes to gain entry in the same in vitro neuroblastoma cell system, SiMa cells. We found that the EGF ligand conferred the affinity to the EGFR-targeted TSI/A at the EGF receptor when compared to an untargeted TSI/A and also the ability to internalize into the cells and cleave its cytosolic target protein SNAP-25. Using high content analysis we found that both BoNT/A and the EGFR-targeted TSI/A enter the cell in a concentration-dependent manner and in compartments which are able to translocate the proteins into the cytosol within 4 h. The EGFR-targeted TSI/A internalized into a compartment which gave a punctate staining pattern by immunofluorescence and partially overlapped with structures positive for the early endosomal marker EAA1; whereas BoNT/A did not internalize into a punctate compartment but did so in an acidifying compartment consistent with local synaptic vesicle recycling. These findings show that the BoNT/A translocation domain, common to both BoNT/A and the EGFR-targeted TSI/A, is a versatile tool for cytosolic delivery from distinct intracellular vesicular compartments.

Acknowledgements

We thank Dr. K. A. Foster and Dr. J. A. Chaddock for their contributions to the TSI field. We also thank Dr. J. K. Krupp, Dr. M. Beard and Dr. M. S. J. Elliott for their comments on the manuscript.

Declaration of interest

This study was funded by Syntaxin Ltd, an Ipsen Company. All authors are employees of Syntaxin Ltd., an Ipsen Company.

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