A high-throughput integrated microfluidics method enables tyrosine autophosphorylation discovery

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作者
Hadas Nevenzal
Meirav Noach-Hirsh
Or Skornik-Bustan
Lev Brio
Efrat Barbiro-Michaely
Yair Glick
Dorit Avrahami
Roxane Lahmi
Amit Tzur
Doron Gerber
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[1] Bar-Ilan University,The Mina and Everard Goodman Faculty of Life Sciences and the Institute of Nanotechnology and Advanced Materials
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Autophosphorylation of receptor and non-receptor tyrosine kinases is a common molecular switch with broad implications for pathogeneses and therapy of cancer and other human diseases. Technologies for large-scale discovery and analysis of autophosphorylation are limited by the inherent difficulty to distinguish between phosphorylation and autophosphorylation in vivo and by the complexity associated with functional assays of receptors kinases in vitro. Here, we report a method for the direct detection and analysis of tyrosine autophosphorylation using integrated microfluidics and freshly synthesized protein arrays. We demonstrate the efficacy of our platform in detecting autophosphorylation activity of soluble and transmembrane tyrosine kinases, and the dependency of in vitro autophosphorylation assays on membranes. Our method, Integrated Microfluidics for Autophosphorylation Discovery (IMAD), is high-throughput, requires low reaction volumes and can be applied in basic and translational research settings. To our knowledge, it is the first demonstration of posttranslational modification analysis of membrane protein arrays.
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