Chemical proteomic analysis of 6-benzylaminopurine molecular partners in wheat grains

Radim Simerský; Ivo Chamrád; Jindřich Kania; Miroslav Strnad; Marek Šebela; René Lenobel

doi:10.1007/s00299-017-2174-4

Chemical proteomic analysis of 6-benzylaminopurine molecular partners in wheat grains

Plant Cell Rep. 2017 Oct;36(10):1561-1570. doi: 10.1007/s00299-017-2174-4. Epub 2017 Jul 7.

Authors

Radim Simerský¹, Ivo Chamrád², Jindřich Kania^{3

4}, Miroslav Strnad³, Marek Šebela¹, René Lenobel¹

Affiliations

¹ Department of Protein Biochemistry and Proteomics, Centre of the Region Haná for Biotechnological and Agricultural Research, Palacký University, Šlechtitelů 241/27, 783 71, Olomouc, Czech Republic.
² Department of Protein Biochemistry and Proteomics, Centre of the Region Haná for Biotechnological and Agricultural Research, Palacký University, Šlechtitelů 241/27, 783 71, Olomouc, Czech Republic. ivo.chamrad@upol.cz.
³ Laboratory of Growth Regulators, Centre of the Region Haná for Biotechnological and Agricultural Research, Palacký University, Šlechtitelů 241/27, 783 71, Olomouc, Czech Republic.
⁴ R&D, Production, Polypure AS, Oslo Research Park, Gaustadallen 21, 0349, Oslo, Norway.

PMID: 28688084
DOI: 10.1007/s00299-017-2174-4

Abstract

An affinity-based chemical proteomic technique enabled direct identification of BAP-interacting proteins in wheat, including the well-known cytokinin-binder, cytokinin-binding protein 1. In this work, we show the development of a chemical proteomic technique for the identification of proteins binding to natural aromatic cytokinins (CKs). 6-benzylaminopurine (BAP) and documented CK-binder, wheat germ-allocated cytokinin-binding protein 1 (CBP-1), were suggested as an ideal proof-of concept affinity pair. Therefore, wheat grains were chosen as a model plant material. The BAP affinity beads were prepared by the immobilization of synthesized BAP-derived ligand to a commercial, pre-activated resin and used to isolate target proteins. The proteomic analysis of complex plant extracts is often complicated by the presence of highly abundant background proteins; in this case, the omnipresent alpha-amylase inhibitors (AAIs). To cope with this problem, we included SDS-PAGE, in-gel trypsin digestion and fraction pooling prior to shotgun analysis, which brought about an obvious drop in the signals belonging to the obstructing proteins. This was accompanied by a sharp increase in the number of identified BAP targets in comparison to a conventional in-solution digestion approach. To distinguish specific CK-binding proteins from those having a general affinity for nucleotide-like compounds, competitive pull-downs with natural nucleotides and free BAP were included in every affinity experiment. By this approach, we were able to identify a group of BAP-interacting proteins, which were subsequently found to be related to biological processes affected by CKs. Moreover, the selected affinity enrichment strategy was verified by the detection of the aforementioned CK-interacting protein, CBP-1. We propose that the developed method represents a promising tool for appealing research of as yet unknown CK molecular partners in plants.

Keywords: Affinity purification; Chemical proteomics; Cytokinin; Molecular target identification; Plant proteomics; Wheat.

MeSH terms

Benzyl Compounds / metabolism*
Chromatography, Liquid
Cytokinins / metabolism
Edible Grain / metabolism*
Electrophoresis, Polyacrylamide Gel
Plant Proteins / metabolism*
Protein Binding
Proteome / metabolism
Proteomics / methods*
Purines / metabolism*
Tandem Mass Spectrometry
Triticum / metabolism*

Substances

Benzyl Compounds
Cytokinins
Plant Proteins
Proteome
Purines
benzylaminopurine

Grants and funding

LO1204/Ministry of Education, Youth and Sports, Czech Republic