Increased C-Peptide Immunoreactivity in Insulin Autoimmune Syndrome (Hirata Disease) Due to High Molecular Weight Proinsulin

Author:

Kay Richard G1,Barker Peter2,Burling Keith2,Cohen Mark3,Halsall David4,Reimann Frank15,Gribble Fiona M15,Semple Robert K6,Church David4

Affiliation:

1. University of Cambridge Metabolic Research Laboratories, Wellcome Trust–MRC Institute of Metabolic Science, Cambridge, UK

2. Core Biochemical Assay Laboratory, Cambridge University Hospitals NHS Foundation Trust, Cambridge, UK

3. Department of Diabetes & Endocrinology, Royal Free London NHS Foundation Trust, London, UK

4. Department of Clinical Biochemistry and Immunology, Cambridge University Hospitals NHS Foundation Trust, Cambridge, UK

5. National Institute for Health Research Cambridge Biomedical Research Centre, Cambridge, UK

6. University of Edinburgh Centre for Cardiovascular Science, Queen’s Medical Research Institute, Edinburgh, UK

Abstract

Abstract Background Determination of C-peptide is important in the investigation of unexplained hyperinsulinemic hypoglycemia because a high C-peptide concentration usually indicates endogenous insulin hypersecretion. Insulin autoimmune syndrome (IAS) denotes hyperinsulinemic hypoglycemia due to insulin-binding antibodies that prolong insulin half-life. C-peptide clearance is considered to be unaffected, and although a marked C-peptide immunoreactivity in hypoglycemic samples has been reported, it has been suspected to be artifactual. High-resolution mass spectrometry enables examination of the basis of C-peptide-immunoreactivity in IAS. Methods Precipitation of plasma with polyethylene glycol was followed by C-peptide immunoassay. Plasma peptides extracted by solvent precipitation were characterized by nano-LC–MS/MS and analyzed using an untargeted data-dependent method. Peptides related to proinsulin, in amino acid sequence, were identified using proprietary bioinformatics software and confirmed by repeat LC–MS/MS analysis. Gel filtration chromatography coupled to LC–MS/MS was used to identify proinsulin-related peptides present in IAS immunocomplexes. Results were compared with those from C-peptide immunoassay. Results Polyethylene glycol precipitation of IAS plasma, but not control plasma, depleted C-peptide immunoreactivity consistent with immunoglobulin-bound C-peptide immunoreactivity. LC–MS/MS detected proinsulin and des 31,32 proinsulin at higher abundance in IAS plasma compared with control plasma. Analysis by gel filtration chromatography coupled to LC–MS/MS demonstrated proinsulin and des 31,32 proinsulin, but no C-peptide, in plasma immunocomplexes. Conclusions Antibody binding can enrich proinsulin and des 31,32 proinsulin in IAS immunocomplexes. Proinsulin cross-reactivity in some C-peptide immunoassays can lead to artifactually increased C-peptide results.

Funder

Diabetes Research & Wellness Foundation

Sutherland–Earl Clinical Fellowship

Wellcome Trust

MRC Metabolic Diseases Unit

MRC

NIHR Cambridge Biomedical Research Centre

Medical Research Council

Enhancing UK Clinical Research

Publisher

Oxford University Press (OUP)

Subject

Biochemistry, medical,Clinical Biochemistry

Reference42 articles.

1. Insulin autoimmune syndrome is the third leading cause of spontaneous hypoglycemic attacks in Japan;Takayama-Hasumi;Diabetes Res Clin Pract,1990

2. Insulin autoimmune syndrome (Hirata disease): clinical features and epidemiology in Japan;Uchigata;Diabetes Res Clin Pract,1994

3. Insulin antibodies prevent insulin-receptor interactions;de Pirro;Diabetologia,1980

4. Imaging of the buffering effect of insulin antibodies in the autoimmune hypoglycemic syndrome;Dozio;J Clin Endocrinol Metab,1998

5. Diagnosis of insulin autoimmune syndrome using polyethylene glycol precipitation and gel filtration chromatography with ex vivo insulin exchange;Church;Clin Endocrinol (Oxf),2017

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