Efficient and robust preparation of tyrosine phosphorylated intrinsically disordered proteins

Warning

This publication doesn't include Faculty of Medicine. It includes Central European Institute of Technology. Official publication website can be found on muni.cz.

Authors	BRÁZDA Pavel ŠEDO Ondrej KUBÍČEK Karel ŠTEFL Richard
Year of publication	2019
Type	Article in Periodical
Magazine / Source	BioTechniques
MU Faculty or unit	Central European Institute of Technology
Citation
Web	URL
Doi	http://dx.doi.org/10.2144/btn-2019-0033
Keywords	C-terminal domain; co-expression; CTD; IDP; intrinsically disordered proteins; phosphorylation; purification; RNA polymerase II; TRANSCRIPTION TERMINATION; LARGEST SUBUNIT; CELL-CYCLE; KINASE; STRATEGIES; SEMISYNTHESIS
Attached files	btn-2019-0033.pdf
Description	Intrinsically disordered proteins (IDPs) are subject to post-translational modifications. This allows the same polypeptide to undertake different interaction networks with different consequences, ranging from regulatory signalling networks to formation of membraneless organelles. We report a robust method for co-expression of modification enzyme and SUMO-tagged IDP with subsequent purification procedure allowing production of modified IDP. The robustness of our protocol is demonstrated on a challenging system, RNA polymerase II C-terminal domain (CM), that is a low-complexity repetitive region with multiple phosphorylation sites. In vitro phosphorylation approaches fail to yield multiple-site phosphorylated CTD, whereas our in vivo protocol allows to rapidly produce near homogeneous phosphorylated CTD at a low cost. These samples can be used in functional and structural studies.
Related projects:	Molekulární podstata pro specifické rozpoznávání histonu H3K4me2 pomocí Set3 PHD domény DECOR Czech Infrastructure for Integrative Structural Biology CEITEC 2020 Molecular architecture of ADAR - RNA complexes