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Absolute quantification of phosphorus metabolite concentrations in human muscle in vivo by 31 P MRS: a quantitative review
Author(s) -
Kemp Graham J.,
Meyerspeer Martin,
Moser Ewald
Publication year - 2007
Publication title -
nmr in biomedicine
Language(s) - English
Resource type - Journals
SCImago Journal Rank - 1.278
H-Index - 114
eISSN - 1099-1492
pISSN - 0952-3480
DOI - 10.1002/nbm.1192
Subject(s) - phosphocreatine , creatine , creatine kinase , pi , metabolite , in vivo , chemistry , oxidative phosphorylation , biology , biochemistry , endocrinology , energy metabolism , microbiology and biotechnology
31 P MRS offers a unique view of muscle metabolism in vivo , but correct quantification is important. Inter‐study correlation of estimates of [Pi] and [phosphocreatine (PCr)] in a number of published studies suggest that the main technical problem in calibrated 31 P MRS studies is the measurement of PCr and Pi signal intensities, rather than absolute quantification of [ATP]. For comparison, we discuss the few published biopsy studies of calf muscle and a selection of the many studies of quadriceps muscle. The ATP concentration is close to the value that we obtained in calf muscle in our own study, presented here, on four healthy subjects, by localised 31 P MRS using a surface coil incorporating an internal reference and calibrated using an external phantom. However, the freeze‐clamp biopsy PCr concentration is ∼20% lower than the value obtained by 31 P MRS, consistent with PCr breakdown by creatine kinase during freezing. Finally, we illustrate some consequences of uncertainty in resting [PCr] for analysis of mitochondrial function from PCr kinetics using a published 31 P MRS study of exercise and recovery: the lower the assumed resting [PCr], the lower the absolute rate of oxidative ATP synthesis estimated from the PCr resynthesis rate; in addition, the lower the assumed resting [PCr], or the higher the assumed [total creatine], the higher the apparent resting [ADP], and therefore the more sigmoid the relationship between the rate of oxidative ATP synthesis and [ADP]. Correct quantification of resting metabolite concentrations is crucially important for this sort of analysis. Our own results ([PCr] = 33 ± 2 mM, [Pi] = 4.5 ± 0.2 mM, and [ATP] = 8.2 ± 0.4 mM; mean ± SEM) are close to the overall mean values of the 10 published studies on calf muscle by ‘calibrated’ 31 P MRS (as in the present work), and of [PCr] and [Pi] in a representative selection of ‘uncalibrated’ 31 P MRS studies (i.e. from measured PCr/ATP and Pi/ATP ratios, assuming a literature value for [ATP]). Copyright © 2007 John Wiley & Sons, Ltd.