Cavitation‐Mediated Transcutaneous Delivery of Protein and Nucleotide‐based Antigen for Rapid High‐level Immune Responses

Author:

Hettinga Johanna K1,Lyons Brian1,Balkaran Joel1,Rijal Pramila2,Dunn‐Lawless Darcy1,Caproni Lisa3,Gray Michael1,Suslick Kenneth S.4,Coussios Constantin C1,Carlisle Robert C1ORCID

Affiliation:

1. BUBBL group Institute of Biomedical Engineering Department of Engineering Science University of Oxford Oxford OX3 7LD UK

2. Centre for Translational Immunology Chinese Academy of Medical Sciences Oxford Institute University of Oxford Oxford OX3 7BN UK

3. Touchlight Ltd Morelands & Riverdale Buildings Lower Sunbury Road Hampton TW12 2ER UK

4. Department of Chemistry University of Illinois Urbana IL 61801 USA

Abstract

AbstractAlternatives are needed to remove the pain, injury, cross‐infection, and hazardous waste associated with needle and syringe (N+S)‐based vaccination. Reported here is the use of novel ultrasound‐responsive protein cavitation nuclei (pCaN), formed using the model antigen bovine serum albumin (BSA), to achieve effective transcutaneous delivery. Upon exposure to ultrasound (US), these pCaN instigate cavitation events which propel themselves and co‐located DNA vectors into the skin. US parameters as well as pCaN and DNA concentration are refined to achieve optimal expression of encoded luciferase transgene. Twenty‐four hours post‐treatment, luciferase expression in the skin, by IVIS imaging,  was 1.67 × 106 ±941943, photons per sec for N+S intradermal injection and 1.49 × 106 ±261832 for cavitation‐mediated delivery (p>0.05). Hence, there is no significant difference in luciferase level achieved, but improved homogeneity and reproducibility of expression are evident in mice treated using US‐mediated cavitation. Despite this equivalence in luciferase levels, a >5× higher level (p<0.02) of anti‐luciferase antibodies is achieved when cavitation is used versus N+S injection. Antibody levels against BSA, resulting from the use of BSA pCaN, are equivalent for the two groups. PCaN can be formed from a range of antigenic proteins and DNA can encode a range of antigenic proteins, so this approach has wide‐ranging implications for needle‐free vaccination.

Funder

Engineering and Physical Sciences Research Council

Publisher

Wiley

Subject

Pharmacology (medical),Biochemistry (medical),Genetics (clinical),Pharmaceutical Science,Pharmacology,Medicine (miscellaneous)

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