Accessing isotopically labeled proteins containing genetically encoded phosphoserine for NMR with optimized expression conditions

Cat Hoang Vesely; Patrick N Reardon; Zhen Yu; Elisar Barbar; Ryan A Mehl; Richard B Cooley

doi:10.1016/j.jbc.2022.102613

Accessing isotopically labeled proteins containing genetically encoded phosphoserine for NMR with optimized expression conditions

J Biol Chem. 2022 Dec;298(12):102613. doi: 10.1016/j.jbc.2022.102613. Epub 2022 Oct 17.

Authors

Cat Hoang Vesely¹, Patrick N Reardon², Zhen Yu³, Elisar Barbar³, Ryan A Mehl¹, Richard B Cooley⁴

Affiliations

¹ GCE4All Research Center, Oregon State University, Corvallis, Oregon, USA; Department of Biochemistry and Biophysics, Oregon State University, Corvallis, Oregon, USA.
² Oregon State University NMR Facility, Oregon State University, Corvallis, Oregon, USA.
³ Department of Biochemistry and Biophysics, Oregon State University, Corvallis, Oregon, USA.
⁴ GCE4All Research Center, Oregon State University, Corvallis, Oregon, USA; Department of Biochemistry and Biophysics, Oregon State University, Corvallis, Oregon, USA. Electronic address: rick.cooley@oregonstate.edu.

Abstract

Phosphoserine (pSer) sites are primarily located within disordered protein regions, making it difficult to experimentally ascertain their effects on protein structure and function. Therefore, the production of ¹⁵N- (and ¹³C)-labeled proteins with site-specifically encoded pSer for NMR studies is essential to uncover molecular mechanisms of protein regulation by phosphorylation. While genetic code expansion technologies for the translational installation of pSer in Escherichia coli are well established and offer a powerful strategy to produce site-specifically phosphorylated proteins, methodologies to adapt them to minimal or isotope-enriched media have not been described. This shortcoming exists because pSer genetic code expansion expression hosts require the genomic ΔserB mutation, which increases pSer bioavailability but also imposes serine auxotrophy, preventing growth in minimal media used for isotopic labeling of recombinant proteins. Here, by testing different media supplements, we restored normal BL21(DE3) ΔserB growth in labeling media but subsequently observed an increase of phosphatase activity and mis-incorporation not typically seen in standard rich media. After rounds of optimization and adaption of a high-density culture protocol, we were able to obtain ≥10 mg/L homogenously labeled, phosphorylated superfolder GFP. To demonstrate the utility of this method, we also produced the intrinsically disordered serine/arginine-rich region of the SARS-CoV-2 Nucleocapsid protein labeled with ¹⁵N and pSer at the key site S188 and observed the resulting peak shift due to phosphorylation by 2D and 3D heteronuclear single quantum correlation analyses. We propose this cost-effective methodology will pave the way for more routine access to pSer-enriched proteins for 2D and 3D NMR analyses.

Keywords: genetic code expansion; nuclear magnetic resonance; phosphoserine; post-translation modification; protein expression; protein phosphorylation; protein synthesis.

Publication types

Research Support, N.I.H., Extramural
Research Support, Non-U.S. Gov't
Research Support, U.S. Gov't, Non-P.H.S.

MeSH terms

COVID-19*
Escherichia coli / genetics
Escherichia coli / metabolism
Humans
Magnetic Resonance Spectroscopy
Phosphoserine / metabolism
Recombinant Proteins / chemistry
SARS-CoV-2 / metabolism
Serine / genetics
Serine / metabolism

Substances

Phosphoserine
Recombinant Proteins
Serine

Grants and funding

RM1 GM144227/GM/NIGMS NIH HHS/United States