Akt deficiency attenuates muscle size and function but not the response to ActRIIB inhibition

MD Goncalves, EE Pistilli, A Balduzzi, MJ Birnbaum… - PloS one, 2010 - journals.plos.org
PloS one, 2010journals.plos.org
Background Akt is a critical mediator of developmental skeletal muscle growth. Treatment
with a soluble ActRIIB fusion protein (ActRIIB-mFc) increases skeletal muscle mass and
strength by inhibiting myostatin and related peptides. Recent in vitro studies have suggested
that Akt signaling is necessary for the ability of ActRIIB inhibition to induce muscle
hypertrophy. Thus, we hypothesized that mice deficient in either Akt1 or Akt2 would not
respond to in vivo inhibition of ActRIIB with ActRIIB-mFc treatment. Methodology and …
Background
Akt is a critical mediator of developmental skeletal muscle growth. Treatment with a soluble ActRIIB fusion protein (ActRIIB-mFc) increases skeletal muscle mass and strength by inhibiting myostatin and related peptides. Recent in vitro studies have suggested that Akt signaling is necessary for the ability of ActRIIB inhibition to induce muscle hypertrophy. Thus, we hypothesized that mice deficient in either Akt1 or Akt2 would not respond to in vivo inhibition of ActRIIB with ActRIIB-mFc treatment.
Methodology and Principal Findings
We analyzed body composition and muscle parameters in wild-type C57BL/6J and Akt1 and Akt2 knockout mice, and compared the responses to blockade of ActRIIB signaling via ActRIIB-mFc treatment. Mice lacking Akt1 or Akt2 had reduced muscle mass, grip strength and contractile force. However, deficiency of Akt1 or Akt2 did not prevent the ability of ActRIIB-mFc treatment to induce muscle hypertrophy, or increase grip strength and contractile force. Akt1 and Akt2 deficient mice responded similarly as wild type mice to ActRIIB-mFc treatment by increasing fiber size.
Conclusions and Significance
Akt1 and Akt2 are important for the regulation of skeletal muscle mass and function. However, these Akt isoforms are not essential for the ability of ActRIIB inhibition to regulate muscle size, fiber type, strength or contractile force.
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