Dried blood spot proteomics as a diagnostic framework for citrin deficiency

  1. Eriko Totsune
  2. Daisuke Nakajima
  3. Ryo Konno
  4. Yasuko Mikami-Saito
  5. Natsuko Arai-Ichinoi
  6. Hikaru Nishida
  7. Hiroko Yagi
  8. Takashi Ishige
  9. Hoshiro Suzuki
  10. Matsuyuki Shirota
  11. Jun Takayama
  12. Chika Takano-Asai
  13. Masaru Shimura
  14. Hideo Sasai
  15. Tomoko Lee
  16. Jun Kido
  17. Yoko Nakajima
  18. Hironori Kobayashi
  19. Atsuo Kikuchi
  20. Chikahiko Numakura
  21. Takashi Hamazaki
  22. Kimihiko Oishi
  23. Kimitoshi Nakamura
  24. Yusuke Kawashima
  25. Osamu Ohara
  26. Yoichi Wada
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Abstract

Background

Citrin deficiency, caused by biallelic pathogenic variants in SLC25A13 , must be identified early to prevent serious complications such as hyperammonemia and liver failure. However, clinical diagnosis is often delayed due to its nonspecific presentation and limited sensitivity of amino acid–based newborn screening methods. Although genome-based evaluations are being investigated to address these issues, concerns about their cost, turnaround time, variant interpretation ability, and data handling highlight the need for a more practical yet reliable alternative. We investigated the feasibility of applying proteomic approach on dried blood spots (DBS), which are routinely used in newborn screening.

Methods

We performed untargeted liquid chromatography-tandem mass spectrometry to analyze the proteome of DBS using a previously developed “non-targeted analysis of non-specifically DBS-absorbed proteins” (NANDA) workflow. SLC25A13 protein abundance was quantified in individuals with biallelic loss-of-function mutations, compound loss-of-function/missense mutations, and heterozygous carriers; this was also evaluated in healthy and diseased controls representing relevant differential diagnoses. To leverage proteomic information, we derived a multivariate proteomic signature using feature selection and evaluated its performance with leave-one-out cross-validation. Biological relevance was assessed by enrichment analysis, and complementary transcriptomics was performed using RNA sequencing.

Results

A total of 7,474 proteins, including SLC25A13, were consistently detected in DBS. SLC25A13 was undetectable in individuals with biallelic loss-of-function mutations. However, individuals with compound loss-of-function/missense genotypes showed reduced but measurable SLC25A13 levels, comparable to those observed in heterozygous carriers. In contrast, a compact 15-protein signature accurately identified individuals with compound loss-of-function/missense genotypes (AUC, 0.99; sensitivity, 1.00; specificity, 0.95). The signature was enriched for Ca 2+ -response, and transcriptomics showed downregulation of genes related to multimodal ion channels in affected individuals compared to controls.

Conclusions

DBS-based proteomic profiling may assist in the diagnosis of citrin deficiency through SLC25A13-quantification and a biologically plausible multivariate signature. More broadly, this strategy offers a promising new diagnostic layer for protein disorders, providing a proteomic readout in a clinically practical DBS format with potential utility for future diagnostic and screening applications.

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  1. Version published to 10.64898/2026.05.26.26354012 on medRxiv