Accuracy of 1H and 31P MRS analyses of lactate in skeletal muscle

## Abstract We have made __in vivo__ ^1^H NMR measurements of the time course of pH and lactate in human skeletal muscle after exercise. Spectra were obtained in a 4.7‐T 30 cm bore Bruker Biospec spectrometer with a 2.5‐cm diameter single surface coil. pH was determined from the shift of the endoge

## Abstract The aim of this study was to determine if muscle energy metabolism, as measured by ^31^P‐magnetic resonance spectroscopy (MRS), is a metabolic marker for the efficacy of treatment of Machado‐Joseph disease (MJD). We obtained ^31^P‐MRS in the calf muscle of 8 male patients with MJD and 1

## Abstract Traditional setups for in situ MR investigation of skeletal muscle function in animals use invasive systems for muscle stimulation and force measurement. These systems require surgical preparation and therefore exclude repetitive investigations on the same animal. This article describes

## Abstract Non‐invasive determination of mitochondrial content is an important objective in clinical and sports medicine. ^31^P MRS approaches to obtain information on this parameter at low field strength typically require in‐magnet exercise. Direct observation of the intra‐mitochondrial inorganic

Double quantum (DQ), J-resolved (1)H NMR spectra from rat and bovine skeletal muscle showed a splitting frequency ( approximately 24 Hz) for the lactate methyl protons that varied with the orientation of the muscle fibers relative to the magnetic field. In contrast, spectra of lactate in solution co

## Abstract Skeletal muscle contraction and glycogenolysis are closely coupled. The standard explanation for this coupling, as taught in modern biochemistry textbooks, is that the metabolic products of contraction (ADP, AMP, P~i~) feed back to activate glycogenolytic enzymes, thus providing for res