Duchenne Muscular Dystrophy Clinical Trial
Official title:
Restoring Dystrophin Expression in Duchenne Muscular Dystrophy: A Phase I/II Clinical Trial Using AVI-4658
Duchenne muscular dystrophy (DMD), a fatal muscle degenerative disorder, arises from
mutations in the dystrophin gene. Antisense therapy with the use of antisense
oligonucleotides (AON) has the potential to restore effectively the production of dystrophin,
the defective protein, in >70% of DMD. This could result in increased life expectancy through
improved muscle survival and function. Recent scientific research has demonstrated the
potential of this technique to skip mutated dystrophin exons, restore the reading frame and
generate functional dystrophin protein. Having demonstrated proof-of-principle in human cell
culture and animal model studies, we now intend to determine efficacy and safety of this
approach to induce dystrophin exon skipping in children with DMD.
The specific aim of this phase I/II study is to assess efficacy (dystrophin production) and
safety of intramuscular administered morpholino oligomer directed against exon 51 (AVI-4658
PMO). We are performing parallel preclinical studies to develop methods of systemic delivery
that will be necessary for future phase II/III clinical studies.
Duchenne Muscular Dystrophy (DMD) is the most common form of muscular dystrophy affecting 1
in every 3500 live male births. The disease is characterised by severe muscle wasting and
weakness, which becomes clinically evident between the ages of 3 to 5 years. Affected
individuals stop walking by 12 years of age and usually do not survive beyond the age of 20
unless ventilated. In general DMD is caused by mutations that disrupt the reading frame thus
leading to a failure to express dystrophin.
Recent scientific research has led to the belief that DMD may be treated by correcting the
genetic error in the dystrophin gene which causes DMD. Most children with DMD have a
deletion, i.e., a mutation which removes part of the dystrophin gene. A novel technique using
antisense technology to skip a specific exon and bypass faulty genetic material, thus
allowing production of functional dystrophin to be produced, has been developed.These
antisense oligonucleotides (AON) target and bypass faulty genetic material and allow
production of functional protein.This has been successfully demonstrated in cultured human
DMD cells and in mouse and canine DMD models.The restored production of dystrophin is
predicted to reduce muscle pathology significantly.
In the early part of the study we compared different antisense oligomers chemical
modification and concluded that the morpholino backbone is significantly superior when
administered to skeletal muscle compared to a number of other types of antisense.
The aim of this phase I/II clinical study is to assess efficacy and safety of AVI-4658, a
morpholino antisense directed against exon 51, in DMD individuals with deletions which would
benefit from skipping exon 51.
The proposed work is presented in 4 sections detailing the main approaches.
Study design
This dose escalation IM trial will involve of up to 9 subjects, subdivided in three groups,
of three subjects each. Patients in group 1 will be recruited sequentially whilst patients in
groups 2 and 3 will be recruited serially.
- Group 1 (3 patients) will receive intramuscular administration of a low concentration of
study drug (extensor digitorum brevis muscle, EDB) and will undergo a muscle biopsy
between days 14 and 28 after intramuscular (IM) administration of the AVI-4658.
- Group 2 (3 patients) will undergo an identical procedure but receiving an intermediate
dose of the AVI-4658.
- Group 3 (3 patients) will be recruited to receive the highest dose of the AVI-4658 but
only if the results in the first 2 cohort of patients show a lack of efficacy of the
lower doses. Up to an additional 3 subjects may be enrolled in cohorts 1 or 2, should
cohort 3 not be enrolled.
Screening
- A physical examination, including body weight, height, arm span, neuromuscular
examination and vital signs (blood pressure, pulse, respiration, and temperature).
- Neuropsychiatric assessment of both subject and the family.
- Molecular genetic on blood sample and dystrophin analysis of original muscle biopsy
obtained at diagnosis.
- Muscle MRI scans of lower limbs to assess the preservation of the muscle to be targeted
with the injection of AON.
- Biochemical (blood) and urine investigation to include standard biochemistry and
haematology (full blood count; coagulation screen; liver function test; serum Ig;
protein electrophoresis; inflammatory markers; creatinine kinase; gamma glutamyl
transferase; urine biochemistry).
- Cardiovascular assessments: ECG and heart echocardiogram.
- Pulmonary assessments: Forced vital capacity, overnight oxygen saturation monitoring.
- Skin biopsy for MyoD-transfection.
Procedure
- The muscle to be used is the extensor digitorum brevis, a foot muscle with very little
function in children with mobility difficulties.
- Local injection will be performed directly through the skin using a combined
EMG-delivery needle. While the procedure could be performed under local anaesthetic;
where possible, it will be performed under general anaesthetic in order to reduce
distress to the subject. A skin tattoo featuring a 1 cm x 1 cm grid with 2 lines in
between to divide it in 9 smaller squares will be used to mark the site of the injection
precisely and for a subsequent muscle biopsy.
- The total volume of each injection will be 100 μL containing the AVI-4658. Nine
injections will be performed at 3 mm intervals inside the 1 cm2 grid tattoo. The depth
of the injection will be carefully recorded.
Observation
- Patients will be closely monitored within the clinical research facility by designated
nursing staff educated in the trial protocol and with experience in similar Phase I/II
studies.
- The clinical research facility has close access to intensive care unit facilities in the
event of an unforeseen adverse reaction.
Follow-up Day 2 - Patients will be discharged. Prior to discharge, a brief physical
examination and systems review will be performed.
Day 3 - A further brief physical examination and systems review including examination of the
injection sites and reporting of any reactions. This examination can be performed at the
local surgery or at the hospital of the referring clinician.
Days 5, 7 - Contact with the subject and inquire as to current status.
Day 14 to 28 - The subject is admitted to hospital. Perform systems assessment (physical
examination), body weight and vital signs. Blood and urine biochemistry will be repeated then
as well as open biopsies of both injected muscles will be performed under general or local
anaesthetic.
Day 30 - Contact with the subject and inquiry as to current status.
Day 60 - Contact the subject and inquiry as to current status.
Day 120 - (Final Visit at the hospital where the study drug was administered). A brief
physical examination and systems review will be performed.
MDEX Consortium.
The PRECLINICAL studies were performed by the following groups, who are all members of the
MDEX consortium:
1. Prof Francesco Muntoni, Dr. Jennifer Morgan. Dubowitz Neuromuscular Centre, Department
of Paediatrics, Imperial College Hammersmith Hospital Campus, Du Cane Road London W12
ONN
2. Prof Dominic Wells; Dr Kim Wells. Gene Targeting Group, Department of Cellular and
Molecular Neuroscience Division of Neuroscience and Mental Health, Imperial College,
Charing Cross Campus, St. Dunstan's Road, London W6 8RP
3. Prof George Dickson; Dr Ian Graham. Gene Therapy Laboratory, Centre for Biomedical
Sciences, Royal Holloway - University of London, Egham
4. Dr Matthew Wood. Department of Physiology, Anatomy and Genetics, South Parks Road,Oxford
OX1 3QX, United Kingdom (UK).
5. Professor Steve Wilton. Experimental Molecular Medicine Group, Centre for Neuromuscular
and Neurological Disorders, University of Western Australia
Additional CLINICAL SUPPORT other than the Study officials will be provided by:
Dubowitz Neuromuscular Centre, Department of Paediatrics, Hammersmith Hospital Campus, Du
Cane Road, W12ONN: Prof Caroline Sewry; Dr. Maria Kinali; Dr Virginia Arechavala; Dr Lucy
Feng
Department of Surgery, St Mary's Hospital Trust, Imperial College Praed Street, London, W2
1NY: Mr David Hunt
DNA Laboratory, Genetics Centre, 5th Floor Guy's Tower, Guy's Hospital London SE1 9RT: Dr
Steve Abbs
Academic Unit of Child and Adolescent Psychiatry, Division of Neuroscience and Mental Health,
Imperial College, St Mary's Campus, Norfolk Place, Paddington,London, W2 1PG: Professor Elena
Garralda
MDEX Study coordinator:
Dr K Ganeshaguru, Dubowitz Neuromuscular Centre, Department of Paediatrics, Hammersmith
Hospital Campus, Imperial College London, Du Cane Road, W12ONN, k.ganeshaguru@imperial.ac.uk
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