Sarcopenia Clinical Trial
— PA-AGEOfficial title:
Determining the Muscle Anabolic Properties of Phosphatidic Acid in Ageing.
| Verified date | February 2018 |
| Source | University of Birmingham |
| Contact | n/a |
| Is FDA regulated | No |
| Health authority | |
| Study type | Interventional |
Ageing is characterized by a loss of muscle mass that is detrimental for physical function
and metabolic health and increases the risk of mortality. The loss of muscle protein mass
with ageing is characterized by a blunted muscle anabolic response to nutrition and exercise.
Thus, interventions to counteract muscle anabolic blunting in old age might assist in the
long-term maintenance of muscle mass.
Phosphatidic acid (hereafter defined as 'PA') is a novel nutrient compound that has been
suggested to play an important role in muscle growth. Oral consumption of PA may amplify the
signalling response to nutrition and exercise and restore muscle anabolic sensitivity in
older adults. In order for PA to be 'clinically' applied as a means to mitigate muscle loss
in aged populations, we must first understand the efficacy and mechanisms underlying the
anabolic properties of this compound, which have yet to be defined in man. The proposed pilot
study is needed to investigate the acute muscle metabolic properties of oral PA
supplementation in older individuals.
Sixteen healthy (non-obese, non-diabetic, non-smokers) older males aged 65-75 yrs will
initially complete a lower-limb strength assessment and undergo a body composition scan.
Between 4-14 days after these initial assessments, participants will be assigned to co-ingest
1.5g of either phosphatidic acid (N= 8; PA) or a non-caloric placebo (N=8; PL) after
following a bout of moderate intensity, single leg resistance exercise. A stable isotope
infusion will be combined with serial muscle biopsies from the thigh of each leg to determine
the measure rates of muscle protein synthesis in the fasted state and in the 'early' and
'late' phase of feeding-only and exercise-plus-feeding.
| Status | Completed |
| Enrollment | 16 |
| Est. completion date | September 2017 |
| Est. primary completion date | March 2017 |
| Accepts healthy volunteers | Accepts Healthy Volunteers |
| Gender | Male |
| Age group | 65 Years to 80 Years |
| Eligibility |
Inclusion Criteria: - Be a non-smoking male between 65 and 80 years. - Have a BMI between 18 and 25 kg/m2. - Be in good general health: no cardiovascular or metabolic diseases. Exclusion Criteria: - Health problems such as: heart disease, rheumatoid arthritis, uncontrolled hypertension, poor lung function, or any health condition that might put you at risk when participating in this study. - Generalised neuromuscular disease (such as Parkinson's disease or motorneurone disease). - Failure to obtain clearance for exercise participation from your GP or negative advice given by your GP concerning exercise participation. - Involvement in regular structured resistance exercise training at the time of the study. - Consumption of any analgesic drugs, anti-inflammatory drugs, or medication that is known to affect protein metabolism (beta-blockers, corticosteroids, NSAIDs). - Participants who have undergone muscle biopsy testing or isotope infusion procedures within the last 5 years. |
| Country | Name | City | State |
|---|---|---|---|
| United Kingdom | University of Birmingham, School of Sport, Exercise and Rehabilitation Sciences | Edgbaston | West Midlands |
| Lead Sponsor | Collaborator |
|---|---|
| University of Birmingham | University of Nottingham |
United Kingdom,
| Type | Measure | Description | Time frame | Safety issue |
|---|---|---|---|---|
| Primary | Myofibrillar protein synthesis in response to oral phosphatidic acid or placebo ingestion alone or in combination with resistance exercise | Myofibrillar protein synthesis will be determined via mass spectrometry to assess stable isotope enrichment of 13C6 phenylalanine isotope in the myofibrillar protein fraction of biopsy tissue. The standard precursor-product calculations will be applied, using plasma isotope enrichment as the precursor. | The change in myofibrillar protein synthesis after treatment ingestion will be determined over 0-to-2.5 hours and 2.5-to-5 hours post-ingestion in rested and exercised legs | |
| Secondary | Anabolic and proteolytic signalling phosphorylation | Phosphorylation of key anabolic and proteolytic signalling intermediates that modulate myofibrillar protein synthesis will be determined via western blot technique | The change in signaling protein phosphorylation from rest will be measured at 2.5 and 5 h after treatment ingestion in rested and exercised legs |
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