Increased detection of primary carnitine deficiency through second-tier newborn genetic screening

Yiming Lin; Weifeng Zhang; Chenggang Huang; Chunmei Lin; Weihua Lin; Weilin Peng; Qingliu Fu; Dongmei Chen

doi:10.1186/s13023-021-01785-6

Orphanet Journal of Rare Diseases (Mar 2021)

Increased detection of primary carnitine deficiency through second-tier newborn genetic screening

Yiming Lin,
Weifeng Zhang,
Chenggang Huang,
Chunmei Lin,
Weihua Lin,
Weilin Peng,
Qingliu Fu,
Dongmei Chen

Affiliations

Yiming Lin: Neonatal Disease Screening Center, Quanzhou Maternity and Children’s Hospital
Weifeng Zhang: Department of Neonatal Intensive Care Unit, Quanzhou Maternity and Children’s Hospital
Chenggang Huang: Zhejiang Biosan Biochemical Technologies Co., Ltd
Chunmei Lin: Neonatal Disease Screening Center, Quanzhou Maternity and Children’s Hospital
Weihua Lin: Neonatal Disease Screening Center, Quanzhou Maternity and Children’s Hospital
Weilin Peng: Neonatal Disease Screening Center, Quanzhou Maternity and Children’s Hospital
Qingliu Fu: Neonatal Disease Screening Center, Quanzhou Maternity and Children’s Hospital
Dongmei Chen: Department of Neonatal Intensive Care Unit, Quanzhou Maternity and Children’s Hospital

DOI: https://doi.org/10.1186/s13023-021-01785-6
Journal volume & issue: Vol. 16, no. 1
pp. 1 – 7

Abstract

Read online

Abstract Background Newborn screening for primary carnitine deficiency (NBS) is commonly implemented worldwide; however, it has poor sensitivity. This study aimed to evaluate the feasibility of improving screening by including a second-tier genetic assay. Results An Agena iPLEX assay was developed to identify 17 common SLC22A5 mutations in Chinese populations and was applied in NBS as a second-tier screening. From January 2017 to December 2018, 204,777 newborns were screened for PCD using tandem mass spectrometry. A total of 316 (0.15%) residual NBS-positive specimens with low free carnitine (C0) levels were subjected to this second-tier screening. The screening identified 20 screen-positive newborns who harboured biallelic mutations in theSLC22A5 gene, 99 carriers with one mutation, and 197 screen-negative newborns with no mutations. Among the 99 carriers, four newborns were found to have a second disease-causing SLC22A5mutation by further genetic analysis. Among the 197 screen-negatives were four newborns with persistently low C0 levels, and further genetic analysis revealed that one newborn had two novel SLC22A5 pathogenic variants. In total, 25 newborns were diagnosed with PCD, for a positive predictive value of 7.91% (25/316). Based on these data, we estimate the incidence of PCD in Quanzhou is estimated to be 1:8191.Thirteen distinct SLC22A5 variants were identified, and the most common was c.760C > T, with an allelic frequency of 32% (16/50), followed by c.1400C > G (7/50, 14%), and c.51C > G (7/50, 14%). Conclusion Data from this study revealed that 24% (6/25) of PCD cases would have been missed by conventional NBS. This high-throughput iPLEX assay is a powerful tool for PCD genotyping. The addition of this second-tier genetic screening to the current NBS program could identify missed PCD cases, thereby increasing PCD detection. However, further studies are needed to optimise the workflow of the new screening algorithm and to evaluate the cost-effectiveness of this screening approach.

Published in Orphanet Journal of Rare Diseases

ISSN: 1750-1172 (Online)
Publisher: BMC
Country of publisher: United Kingdom
LCC subjects: Medicine
Website: https://ojrd.biomedcentral.com

About the journal

Abstract

Keywords