Investigation of the relationship between phenylalanine in venous plasma and capillary blood using volumetric blood collection devices

Author:

Carling Rachel S.12ORCID,Barclay Zoe2,Cantley Nathan3,Emmett Erin C.2,Hogg Sarah L.4,Finezilber Yael5,Schulenburg‐Brand Danja6,Murphy Elaine5,Moat Stuart J.78

Affiliation:

1. GKT School Medical Education Kings College London London UK

2. Biochemical Sciences, Synnovis, Guys & St Thomas' NHSFT London UK

3. Department of Clinical Biochemistry, Severn Pathology Southmead Hospital, North Bristol NHS Trust Bristol UK

4. Biochemical Genetics Unit Cambridge University Hospitals Cambridge UK

5. Charles Dent Metabolic Unit National Hospital for Neurology and Neurosurgery, Queen Square London UK

6. Department of Haematology, Immunology and Metabolic Medicine University Hospital Wales Cardiff UK

7. Department of Medical Biochemistry, Immunology & Toxicology University Hospital Wales Cardiff UK

8. School of Medicine Cardiff University, University Hospital Wales Cardiff UK

Abstract

AbstractMeasurement of plasma and dried blood spot (DBS) phenylalanine (Phe) is key to monitoring patients with phenylketonuria (PKU). The relationship between plasma and capillary DBS Phe concentrations has been investigated previously, however, differences in methodology, calibration approach and assumptions about the volume of blood in a DBS sub‐punch has complicated this. Volumetric blood collection devices (VBCDs) provide an opportunity to re‐evaluate this relationship. Paired venous and capillary samples were collected from patients with PKU (n = 51). Capillary blood was collected onto both conventional newborn screening (NBS) cards and VBCDs. Specimens were analysed by liquid‐chromatography tandem mass‐spectrometry (LC–MS/MS) using a common calibrator. Use of VBCDs was evaluated qualitatively by patients. Mean bias between plasma and volumetrically collected capillary DBS Phe was −13%. Mean recovery (SD) of Phe from DBS was 89.4% (4.6). VBCDs confirmed that the volume of blood typically assumed to be present in a 3.2 mm sub‐punch is over‐estimated by 9.7%. Determination of the relationship between plasma and capillary DBS Phe, using a single analytical method, common calibration and VBCDs, demonstrated that once the under‐recovery of Phe from DBS has been taken into account, there is no significant difference in the concentration of Phe in plasma and capillary blood. Conversely, comparison of plasma Phe with capillary DBS Phe collected on a NBS card highlighted the limitations of this approach. Introducing VBCDs for the routine monitoring of patients with PKU would provide a simple, acceptable specimen collection technique that ensures consistent sample quality and produces accurate and precise blood Phe results which are interchangeable with plasma Phe.

Publisher

Wiley

Subject

Biochemistry, Genetics and Molecular Biology (miscellaneous),Endocrinology, Diabetes and Metabolism,Internal Medicine

Reference37 articles.

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