Development of a sandwich ELISA to detect circulating, soluble IRAP as a potential disease biomarker

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作者
Anika Vear
Claudia Thalmann
Kristina Youngs
Natalie Hannan
Tracey Gaspari
Siew Yeen Chai
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[1] Monash University,Department of Physiology, Biomedicine Discovery Institute
[2] University of Melbourne,Department of Obstetrics and Gynaecology
[3] Mercy Perinatal,Department of Pharmacology, Biomedicine Discovery Institute
[4] Mercy Hospital for Women,undefined
[5] Monash University,undefined
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There is growing interest in the use of the enzyme, insulin regulated aminopeptidase (IRAP), as a biomarker for conditions such as cardio-metabolic diseases and ischemic stroke, with upregulation in its tissue expression in these conditions. However, quantification of circulating IRAP has been hampered by difficulties in detecting release of the truncated, soluble form of this enzyme into the blood stream. The current study aimed to develop a sandwich ELISA using novel antibodies directed towards the soluble portion of IRAP (sIRAP), to improve accuracy in detection and quantification of low levels of sIRAP in plasma. A series of novel anti-IRAP antibodies were developed and found to be highly specific for sIRAP in Western blots. A sandwich ELISA was then optimised using two distinct antibody combinations to detect sIRAP in the low nanogram range (16–500 ng/ml) with a sensitivity of 9 ng/ml and intra-assay variability < 10%. Importantly, the clinical validity of the ELISA was verified by the detection of significant increases in the levels of sIRAP throughout gestation in plasma samples from pregnant women. The specific and sensitive sandwich ELISA described in this study has the potential to advance the development of IRAP as a biomarker for certain diseases.
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