Multicenter evaluation of use of dried blood spot compared to conventional plasma in measurements of globotriaosylsphingosine (LysoGb3) concentration in 104 Fabry patients

Author:

Malvagia Sabrina1,Ferri Lorenzo2,Della Bona Maria1,Borsini Walter3,Cirami Calogero Lino4,Dervishi Egrina4,Feriozzi Sandro5,Gasperini Serena6,Motta Serena6,Mignani Renzo7,Trezzi Barbara8,Pieruzzi Federico9,Morrone Amelia210,Daniotti Marta11,Donati Maria Alice11,la Marca Giancarlo112ORCID

Affiliation:

1. Newborn Screening, Clinical Chemistry and Pharmacology Lab , Meyer Children’s University Hospital , Florence , Italy

2. Molecular and Cell Biology Laboratory of Neurometabolic Diseases, Neuroscience Department , Meyer Children’s Hospital , Florence , Italy

3. Casa di Cura Villa Ulivella e Glicini , Florence , Italy

4. Nephrology Dialysis Transplant Unit , Careggi Hospital , Florence , Italy

5. Nephrology and Dialysis Unit , Belcolle Hospital , Viterbo , Italy

6. Pediatric Rare Diseases Unit, Department of Pediatrics , MBBM Foundation, San Gerardo Hospital , Monza , Italy

7. Department of Nephrology , Infermi Hospital , Rimini , Italy

8. Clinical Nephrology, School of Medicine and Surgery , University of Milano , Milan , Italy

9. Clinical Nephrology, School of Medicine and Surgery , University of Milano-Bicocca and Nephrology and Dialysis Unit, ASST-Monza San Gerardo Hospital , Monza , Italy

10. Department of Neurofarba , University of Florence , Florence , Italy

11. Metabolic Disease Unit , Meyer Children’s University Hospital , Florence , Italy

12. Department of Experimental and Clinical Biomedical Sciences , University of Florence , Florence , Italy

Abstract

Abstract Objectives Fabry disease (FD) is an X-linked lysosomal storage disorder, resulting from a deficiency of the enzyme α-galactosidase A, responsible for breaking down glycolipids such as globotriaosylceramide and its deacylated derivative, globotriaosylsphingosine (LysoGb3). Here, we compare the levels of LysoGb3 in dried blood spots (DBS) and plasma in patients with classic and late-onset phenotypes. Methods LysoGb3 measurements were performed in 104 FD patients, 39 males and 65 females. Venous blood was collected. A portion was spotted onto filter paper and another portion separated to obtain plasma. The LysoGb3 concentrations in DBS and plasma were determined by highly sensitive electrospray ionization liquid chromatography tandem mass spectrometry. Agreement between different matrices was assessed using linear regression and Bland Altman analysis. Results The method on DBS was validated by evaluating its precision, accuracy, matrix effect, recovery, and stability. The analytical performances were verified by comparison of a total of 104 paired DBS and plasma samples from as many FD patients (representing 46 GLA variants). There was a strong correlation between plasma and the corresponding DBS LysoGb3 concentrations, with few exceptions. Discrepancies were observed in anemic patients with typically low hematocrit levels compared to the normal range. Conclusions The method proved to be efficient for the rapid analysis of LysoGb3. DBS provides a convenient, sensitive, and reproducible method for measuring LysoGb3 levels for diagnosis, initial phenotypic assignment, and therapeutic monitoring in patients with FD.

Publisher

Walter de Gruyter GmbH

Subject

Biochemistry (medical),Clinical Biochemistry,General Medicine

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