Commercial insulin immunoassays fail to detect commonly prescribed insulin analogues

Blood insulin and C-peptide are key investigations in the differential diagnosis of hypoglycaemia. Analogues of insulin have modified primary-sequences compared to native human insulin, as such may not cross react with insulin assays. This has important implications in detecting surreptitious or mal...

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Published inClinical biochemistry Vol. 48; no. 18; pp. 1354 - 1357
Main Authors Parfitt, C., Church, D., Armston, A., Couchman, L., Evans, C., Wark, G., McDonald, T.J.
Format Journal Article
LanguageEnglish
Published United States Elsevier Inc 01.12.2015
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Abstract Blood insulin and C-peptide are key investigations in the differential diagnosis of hypoglycaemia. Analogues of insulin have modified primary-sequences compared to native human insulin, as such may not cross react with insulin assays. This has important implications in detecting surreptitious or malicious insulin administration. The aim of this study is to assess the cross-reactivity of all insulins currently listed in the British National Formulary (BNF65, 2013) in clinical insulin assays currently used in UK clinical laboratories. Sample sets were prepared for all 15 exogenous insulin classes listed in the BNF, at concentrations of 1000pmol/L and 300pmol/L, using pooled human serum. Samples were sent blinded to 5 participating analytical laboratories to cover analysis on the 10 major clinical insulin assays used in the UK. The ability of insulin assays to detect exogenous insulin preparations was highly variable and ranged from 0% to >140% for a single exogenous insulin. Four assays were highly specific for the human insulin sequence and had no cross-reactivity with any synthetic analogue insulin. Two detected all insulin types (human sequence, animal and synthetic analogue), with the remaining having variable cross-reactivity. The cross-reactivity of the 15 exogenous insulin preparations is highly variable in the assays used in clinical laboratories around the UK. It is important that laboratories and clinicians are aware of the limitations of their local assays to avoid missing the important diagnosis of hypoglycaemia secondary to excessive exogenous insulin. Where necessary, samples should be referred to specialist centres for insulin analysis and ideally by a validated and fully-quantitative mass spectrometry-based method. •We assess the cross reactivity of 15 exogenous insulins in 10 clinical insulin assays.•Detection of insulin analogues was highly variable and ranged from 0% to >140%.•Most assays failed to detect insulins with more than 1 amino acid difference.•Physicians need to be aware of the limitation of laboratory methods to detect exogenous insulin.
AbstractList Blood insulin and C-peptide are key investigations in the differential diagnosis of hypoglycaemia. Analogues of insulin have modified primary-sequences compared to native human insulin, as such may not cross react with insulin assays. This has important implications in detecting surreptitious or malicious insulin administration. The aim of this study is to assess the cross-reactivity of all insulins currently listed in the British National Formulary (BNF65, 2013) in clinical insulin assays currently used in UK clinical laboratories. Sample sets were prepared for all 15 exogenous insulin classes listed in the BNF, at concentrations of 1000 pmol/L and 300 pmol/L, using pooled human serum. Samples were sent blinded to 5 participating analytical laboratories to cover analysis on the 10 major clinical insulin assays used in the UK. The ability of insulin assays to detect exogenous insulin preparations was highly variable and ranged from 0% to >140% for a single exogenous insulin. Four assays were highly specific for the human insulin sequence and had no cross-reactivity with any synthetic analogue insulin. Two detected all insulin types (human sequence, animal and synthetic analogue), with the remaining having variable cross-reactivity. The cross-reactivity of the 15 exogenous insulin preparations is highly variable in the assays used in clinical laboratories around the UK. It is important that laboratories and clinicians are aware of the limitations of their local assays to avoid missing the important diagnosis of hypoglycaemia secondary to excessive exogenous insulin. Where necessary, samples should be referred to specialist centres for insulin analysis and ideally by a validated and fully-quantitative mass spectrometry-based method.
Blood insulin and C-peptide are key investigations in the differential diagnosis of hypoglycaemia. Analogues of insulin have modified primary-sequences compared to native human insulin, as such may not cross react with insulin assays. This has important implications in detecting surreptitious or malicious insulin administration. The aim of this study is to assess the cross-reactivity of all insulins currently listed in the British National Formulary (BNF65, 2013) in clinical insulin assays currently used in UK clinical laboratories. Sample sets were prepared for all 15 exogenous insulin classes listed in the BNF, at concentrations of 1000pmol/L and 300pmol/L, using pooled human serum. Samples were sent blinded to 5 participating analytical laboratories to cover analysis on the 10 major clinical insulin assays used in the UK. The ability of insulin assays to detect exogenous insulin preparations was highly variable and ranged from 0% to >140% for a single exogenous insulin. Four assays were highly specific for the human insulin sequence and had no cross-reactivity with any synthetic analogue insulin. Two detected all insulin types (human sequence, animal and synthetic analogue), with the remaining having variable cross-reactivity. The cross-reactivity of the 15 exogenous insulin preparations is highly variable in the assays used in clinical laboratories around the UK. It is important that laboratories and clinicians are aware of the limitations of their local assays to avoid missing the important diagnosis of hypoglycaemia secondary to excessive exogenous insulin. Where necessary, samples should be referred to specialist centres for insulin analysis and ideally by a validated and fully-quantitative mass spectrometry-based method. •We assess the cross reactivity of 15 exogenous insulins in 10 clinical insulin assays.•Detection of insulin analogues was highly variable and ranged from 0% to >140%.•Most assays failed to detect insulins with more than 1 amino acid difference.•Physicians need to be aware of the limitation of laboratory methods to detect exogenous insulin.
Author Armston, A.
Evans, C.
Church, D.
Parfitt, C.
McDonald, T.J.
Couchman, L.
Wark, G.
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Issue 18
Keywords Immunoassay
Analogues
Hypoglycaemia
Insulin
Cross-reactivity
Language English
License Copyright © 2015 The Canadian Society of Clinical Chemists. Published by Elsevier Inc. All rights reserved.
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Snippet Blood insulin and C-peptide are key investigations in the differential diagnosis of hypoglycaemia. Analogues of insulin have modified primary-sequences...
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pubmed
elsevier
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StartPage 1354
SubjectTerms Analogues
Antibodies, Monoclonal - chemistry
Biomarkers - blood
C-Peptide - blood
Cross Reactions
Cross-reactivity
Humans
Hypoglycaemia
Hypoglycemia - blood
Hypoglycemia - chemically induced
Hypoglycemia - diagnosis
Immunoassay
Immunoassay - standards
Insulin
Insulin - adverse effects
Insulin - analogs & derivatives
Insulin - blood
Prescription Drugs - administration & dosage
Prescription Drugs - metabolism
Sensitivity and Specificity
Title Commercial insulin immunoassays fail to detect commonly prescribed insulin analogues
URI https://dx.doi.org/10.1016/j.clinbiochem.2015.07.017
https://www.ncbi.nlm.nih.gov/pubmed/26171976
Volume 48
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