Your search keyword '"Receptor-Like Protein Tyrosine Phosphatases, Class 8 metabolism"' showing total 2 results

1. Azide and Tween-20 reduce binding to autoantibody epitopes of islet antigen-2; implications for assay performance and reproducibility.

Author

Williams AJ, Somerville M, Rokni S, Bonifacio E, Yu L, Eisenbarth G, Akolkar B, Steffes M, and Bingley PJ

Subjects

Autoantibodies blood, Azides, Diabetes Mellitus, Type 1 blood, Diabetes Mellitus, Type 1 immunology, Epitopes immunology, Humans, Polysorbates, Protein Binding, Reproducibility of Results, Diabetes Mellitus, Type 1 diagnosis, Epitopes metabolism, Radioligand Assay, Receptor-Like Protein Tyrosine Phosphatases, Class 8 immunology, Receptor-Like Protein Tyrosine Phosphatases, Class 8 metabolism

Abstract

Autoantibodies to islet antigen 2 (IA-2A) are important markers for predicting diabetes in children and young adults. Harmonization of IA-2A assay measurement is essential if results from different laboratories are to be compared. We investigated whether sodium azide, a bacteriostatic agent added to some assays, could affect IA-2A binding and thereby contribute to differences in IA-2A measurement between laboratories. Addition of 0.1% azide to assay buffer was found to reduce median IA-2A binding of 18 selected sera from IA-2A positive patients with type 1 diabetes and their relatives by 41% (range, 78 to -33%, p<0.001). The effect on binding was epitope specific; median IA-2A binding by 14 sera with antibodies to the protein tyrosine phosphatase region of IA-2 was reduced by 48% (range, 11 to 78%, p<0.001), while binding by 4 sera with antibodies specific to only the juxtamembrane region of IA-2 showed no change (median increase 16% (range 6 to 33%, p=0.125). When the Tween-20 concentration was reduced from 1% to 0.15% the median reduction in IA-2A binding with azide by the 18 sera was only 10% (range, -12 to 41%, p<0.001). Tween-20 also exerted an independent effect, since median IA-2A binding increased by 23% (range 3% to 86%, p<0.001) when Tween-20 concentration was reduced from 1% to 0.15% in the absence of azide. We conclude that common assay reagents such as azide and Tween-20 can strongly influence IA-2A binding in an epitope-related manner, and their use may explain some of the differences between laboratories in IA-2A measurement.

Published

2009

2. Radiobinding assay for detecting autoantibodies to single epitopes.

Author

Lampasona V, Belloni C, Piquer S, Bonicchio S, Furlan R, and Bonifacio E

Subjects

Adolescent, Adult, Animals, Autoantibodies immunology, Child, Child, Preschool, Diabetes Mellitus, Type 1 diagnosis, Diabetes Mellitus, Type 1 immunology, Encephalomyelitis, Autoimmune, Experimental immunology, Enzyme-Linked Immunosorbent Assay, Epitope Mapping, Epitopes metabolism, Female, Humans, Infant, Male, Mice, Peptides metabolism, Receptor-Like Protein Tyrosine Phosphatases, Class 8 metabolism, Recombinant Fusion Proteins immunology, Recombinant Fusion Proteins metabolism, Sensitivity and Specificity, Thioredoxins immunology, Thioredoxins metabolism, Autoantibodies blood, Epitopes immunology, Peptides immunology, Radioligand Assay methods, Receptor-Like Protein Tyrosine Phosphatases, Class 8 immunology

Abstract

Autoantibodies, a hallmark of autoimmune disease, are directed against diverse antigens and epitopes. This diversity aids in characterising disease progression and identifying disease-associated autoantibodies. Here we aimed to develop a sensitive assay to detect and quantify epitope-specific autoantibodies. We generated constructs to integrate known peptide epitopes into the TrxA protein, and used these to in vitro synthesize radio-labelled proteins for a radiobinding assay (RBA). This assay was first validated with an animal model using mice immunized with the MOG(40-55) peptide. Using type 1 diabetes-associated protein tyrosine phosphatase-like autoantigen IA-2 as a human model, we expressed IA-2(609-621), IA-2(619-631), or IA-2(609-631) peptide in the TrxA construct and used the RBA to test sera from 113 patients with type 1 diabetes and 87 controls. Antibodies were detected to the IA-2(609-631) epitope in 37 of 113 patient sera and one control; 17 sera were reactive to the IA-2(609-621) (JM1) epitope, and 16 to the IA-2(619-631) (JM2) epitope. Interestingly, a novel third epitope (JM3) was identified in 7 sera that reacted to IA-2(609-631) but not the JM1 and JM2 sub-specificities. An ELISA using IA-2(609-631) was less sensitive than the RBA, as it detected only some of the JM1 and JM3 antibody positive sera and none of the JM2. Mutagenesis of single IA-2(609-631) amino acids in combination with the RBA showed that antibodies to JM2 and JM3 were highly diverse in their specific residue requirements. Our strategy using in vitro synthesized antigens and the RBA was thus a highly sensitive and versatile method to identify epitopes and quantify epitope-specific antibodies.

Published

2008