Regional and fibre type glycogen utilization patterns in the hamster diaphragm following swimming.

The purpose of this study was to determine the regional and myofibrillar ATPase (M-ATPase) fibre type glycogen utilization patterns in response to increased ventilation induced by pre-exhaustive (Pre-Exh) and exhaustive (Exh) durations of swimming. Twenty-eight hamsters were studied: six controls (Con), 11 Pre-Exh (swam 82 min), 11 Exh (swam to exhaustion). We examined the optical density of PAS-stained fibres from the different regions of the diaphragm as a measure of glycogen remaining after the exercise or control period. The optical densities of PAS-stained fibres in most M-ATPase fibre types and diaphragmatic regions for the Pre-Exh and Exh groups was less than those in the Con hamsters except for the optical densities of all the M-ATPase fibre types in the sternal region. The optical densities of PAS-stained fibres in different regions and M-ATPase fibre types did not differ in the Exh and Pre-Exh groups. This data indicates that significant glycogen utilization occurred in all three M-ATPase fibre types in the costal, and both the thoracic and abdominal surface of the crural diaphragm in hamsters following pre-exhaustive and exhaustive durations of swimming. Glycogen utilization was greater in type 1 fibres of the thoracic surface of the crural region than in the type 1 fibres of the sternal region of the Pre-Exh group. Further, significant utilization of glycogen did not occur in any of the three M-ATPase fibre types of the sternal region of the diaphragm following prolonged durations of swimming. It would appear that glycogen is an important substrate in the hamster diaphragm during swimming.(ABSTRACT TRUNCATED AT 250 WORDS)

Circadian rhythm of glycogen in the hamster diaphragm.

The purpose of this study was to determine the diurnal fluctuation of glycogen stores for the whole hemidiaphragm and within a specific myofibrillar ATPase (M-ATPase) fibre type and diaphragmatic region. Fifty-six golden Syrian hamsters were randomly divided into six groups according to the time of sampling biopsies from the diaphragm: 03:00, 07:00, 11:00, 15:00, 19:00, and 23:00. The right hemidiaphragm was quick frozen and biochemically assayed for glycogen levels. Biopsies from the left hemidiaphragm of the same animal were cut from the anterior costal and crural regions, and stained with periodic acid--Schiff (PAS) and for M-ATPase. Optical density measures of PAS-stained fibres were determined to quantitate glycogen in different M-ATPase fibre types and diaphragmatic regions. Biochemical assay of the entire hemidiaphragm showed slightly greater glycogen content of biopsies taken at 11:00 and 15:00 than at 03:00, 19:00, and 23:00 (range of differences: 6.4-10.0%). However, glycogen levels within a specific M-ATPase fibre type and diaphragm region were not different in biopsies sampled at different times. Because the hamster has a small diurnal variation of glycogen in the diaphragm, which is similar to the small diurnal variation of glycogen in human skeletal muscle, this species may be a good animal model for metabolic studies of the diaphragm that could be affected by diurnal glycogen variability.