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Application of ADA1 as a new marker enzyme in sandwich ELISA to study the effect of adenosine on activated monocytes

Chengqian Liu; Maksym Skaldin; Yuanan Lu; Andrey V. Zavialov; Chengxiang Wu

Application of ADA1 as a new marker enzyme in sandwich ELISA to study the effect of adenosine on activated monocytes

Chengqian Liu
Maksym Skaldin
Yuanan Lu
Andrey V. Zavialov
Chengxiang Wu
Katso/Avaa
Publisher's version (1.196Mb)
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NATURE PUBLISHING GROUP
doi:10.1038/srep31370
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Julkaisun pysyvä osoite on:
https://urn.fi/URN:NBN:fi-fe2021042715518
Tiivistelmä

Enzyme-linked immunosorbent assay (ELISA) is a valuable technique to detect antigens in biological fluids. Horse radish peroxidase (HRP) is one of the most common enzymes used for signal amplification in ELISA. Despite new advances in technology, such as a large-scale production of recombinant enzymes and availability of new detection systems, limited research is devoted to finding alternative enzymes and their substrates to amplify the ELISA signals. Here, HRP-avidin was substituted with the human adenosine deaminase (hADA1)-streptavidin complex and adenosine as a detection system in commercial ELISA kits. The hADA1 ELISA was successfully used to demonstrate that adenosine, bound to A1 and A3 adenosine receptors, increases cytokine secretion by LPS activated monocytes. We show that hADA1-based ELISA has the same sensitivity, and also provides identical results, as HRP ELISA. In addition, the sensitivity of hADA1-based ELISA could be easily adjusted by changing the adenosine concentration and the incubation time. Therefore, hADA1 could be used as a detection enzyme with any commercial ELISA kit with a wide range of concentration of antigens.

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