Improved analysis of C26:0-lysophosphatidylcholine in dried-blood spots via negative ion mode HPLC-ESI-MS/MS for X-linked adrenoleukodystrophy newborn screening.

[x-linked adrenoleukodystrophy]

X-linked adrenoleukodystrophy (X-ALD ) is the most common human peroxisomal disorder , and is caused by mutations in the peroxisomal transmembrane ALD protein (ALDP , ABCD 1 ). The biochemical defect associated with X-ALD is an accumulation of very long -chain fatty acids (VLCFA , e .g . C 2 4 :0 and C 2 6 :0 ), which has been shown to result in the accumulation of C 2 6 :0 -lysophosphatidylcholine (C 2 6 :0 -LPC ).We describe the analysis of C 2 6 :0 -LPC in dried-blood spots (DBS ) using a rapid (30 min ) and simple extraction procedure , isocratic HPLC resolution of LPC , and structure-specific analysis via negative ion mode tandem mass spectrometry .In putative normal DBS specimens from newborns (N =223 ) C 2 6 :0 -LPC was 0 .09 ±0 .03 μmol /l whole blood , while in peroxisomal biogenesis disorder (including X-ALD ) patients (N =28 ) C 2 6 :0 -LPC was 1 .13 ±0 .67 μmol /l whole blood . Both multiple reaction monitoring and a neutral loss scan (225 .1 Da ) analysis of DBS were used to analyze LPC .Compared to a previous report of C 2 6 :0 -LPC analysis in DBS , the method described here is simpler , faster , and more structure-specific for LPC with C 2 6 :0 acyl chains .