Quantitative analysis of 1H NMR detected proteins in the rat cerebral cortex in vivo and in vitro

Abstract

Spectral editing experiments were used to quantify CH₃ groups from macromolecular species in the chemical shift region from 1.2 to 1.4 ppm of rat cerebrum in vivo. Two peaks centred at 1.22 and 1.40 ppm were revealed when irradiation was positioned at 4.35 or 4.30 ppm. These peaks had lower saturation factors (1 vs. 1.72±0.10) than N‐acetyl aspartate (NAA) and shorter T₂ [60±5.8 (1.22 ppm) and 51±2.2 (1.40 ppm) vs. 123±12 (NAA) ms]. The concentrations of the peaks at 1.22 and 1.40 ppm were calculated to be 0.65±0.09 and 1.37±0.18 mmol of CH₃, equivalents/kg brain. Acid extract from cerebral corticies contained macromolecular peaks at the same chemical shifts with approximately the same area ratios to NAA as in vivo. These data show that the macromolecular peaks in the brain at TE>100 ms arise predominantly from proteins which are acid soluble. The assignment of macromolecular signals in the cerebral spectrum to a given polypeptide (thymosin β4 and histone H1) is discussed in the light of protein analyses of brain acid extracts.