Direct optogenetic activation of upper airway muscles in an acute model of upper airway hypotonia mimicking sleep onset

Author:

Knapman Fiona L12ORCID,Cohen E Myfanwy1,Kulaga Tom2,Lovell Nigel2ORCID,Lisowski Leszek34,McMullan Simon5ORCID,Burke Peter G R125,Bilston Lynne E12ORCID

Affiliation:

1. Neuroscience Research Australia , Sydney, NSW , Australia

2. School of Clinical Medicine, University of New South Wales , Sydney, NSW , Australia

3. Translational Vectorology Research Unit, Children’s Medical Research Institute , Sydney, NSW , Australia

4. Laboratory of Molecular Oncology and Innovative Therapies, Military Institute of Medicine , Warsaw , Poland

5. Macquarie Medical School, Macquarie University , Sydney, NSW , Australia

Abstract

Abstract Study Objectives Obstructive sleep apnea (OSA), where the upper airway collapses repeatedly during sleep due to inadequate dilator muscle tone, is challenging to treat as current therapies are poorly tolerated or have variable and unpredictable efficacy. We propose a novel, optogenetics-based therapy, that stimulates upper airway dilator muscle contractions in response to light. To determine the feasibility of a novel optogenetics-based OSA therapy, we developed a rodent model of human sleep-related upper airway muscle atonia. Using this model, we evaluated intralingual delivery of candidate optogenetic constructs, notably a muscle-targeted approach that will likely have a favorable safety profile. Methods rAAV serotype 9 viral vectors expressing a channelrhodopsin-2 variant, driven by a muscle-specific or nonspecific promoter were injected into rat tongues to compare strength and specificity of opsin expression. Light-evoked electromyographic responses were recorded in an acute, rodent model of OSA. Airway dilation was captured with ultrasound. Results The muscle-specific promoter produced sufficient opsin expression for light stimulation to restore and/or enhance electromyographic signals (linear mixed model, F = 140.0, p < 0.001) and induce visible tongue contraction and airway dilation. The muscle-specific promoter induced stronger (RM-ANOVA, F(1,8) = 10.0, p = 0.013) and more specific opsin expression than the nonspecific promoter in an otherwise equivalent construct. Viral DNA and RNA were robust in the tongue, but low or absent in all other tissues. Conclusions Significant functional responses to direct optogenetic muscle activation were achieved following muscle-specific promoter-driven rAAV-mediated transduction, providing proof-of-concept for an optogenetic therapy for patients with inadequate dilator muscle activity during sleep.

Funder

Biomedical Engineering seed

National Health and Medical Research Council

Publisher

Oxford University Press (OUP)

Subject

Physiology (medical),Neurology (clinical)

Reference65 articles.

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