Lactate oxidation for the detection of mitochondrial dysfunction in human skin fibroblasts.

[neonatal adrenoleukodystrophy]

To screen fibroblasts for defects in lactate /pyruvate oxidation , cells were grown to confluence in 25 -cm 2 flasks , rinsed , and incubated in glucose-free media containing 25 microM L-lactate and 0 .1 microCi [D ,L-1 -14 C ]lactate . Lactate oxidation was measured as the amount of lactate oxidized in nmol of 14 CO 2 generated /mg protein /min . Fibroblasts from patients with mitochondrial or peroxisomal disorders had decreased lactate oxidation compared to the control (CON ): CON , 1 .9 +/- 0 .13 nmol /mg /min ; neonatal adrenoleukodystrophy (NALD ), 0 .45 +/- 0 .01 (P < 0 .001 ); rhizomelic chondrodysplasia punctata (RCDP ), 0 .13 +/- 0 .002 (P < 0 .001 ); mitochondrial defect of unknown etiology (MIT ), 0 .77 +/- 0 .003 (P < 0 .001 ); pyruvate dehydrogenase (PDH ) deficiency , 0 .98 +/- 0 .02 (P < 0 .001 ). This method is useful for screening fibroblasts for defects in lactate oxidation in patients with mitochondrial or peroxisomal disorders . Confirmation of the site of the defect may then be investigated with specific assays , e .g ., PDH , in cellular homogenates : CON , 0 .93 +/- 0 .02 nmol /mg /min ; NALD , 0 .55 +/- 0 .02 ; RCDP , 0 .44 +/- 0 .02 ; MIT , 0 .53 +/- 0 .03 ; PDH deficiency , 0 .19 +/- 0 .02 .