EMDB/PDB/SASBDBから引用されている文献のデータベース

キーワード
構造解析手法	All X線回折 NMR 電子顕微鏡小角散乱中性子線回折線維回折粉末回折赤外分光 EPR FRET 理論モデルハイブリッド
著者・登録者
ジャーナル
IF	>30 >20 >10 >5 all

タイトル	Nucleoside diphosphate kinase A (NME1) catalyses its own oligophosphorylation.
ジャーナル・号・ページ	Nat Chem, Vol. 17, Issue 11, Page 1757-1767, Year 2025
掲載日	2025年8月20日
著者	Arif Celik / Felix Schöpf / Christian E Stieger / Sarah Lampe / Björn Hanf / Jeremy A M Morgan / Max Ruwolt / Fan Liu / Christian P R Hackenberger / Daniel Roderer / Dorothea Fiedler /
PubMed 要旨	Protein phosphorylation is a central signalling mechanism in eukaryotic cells. The scope of this post-translational modification includes protein pyro- and polyphosphorylation. Here we report the ...Protein phosphorylation is a central signalling mechanism in eukaryotic cells. The scope of this post-translational modification includes protein pyro- and polyphosphorylation. Here we report the discovery of another mode of phosphorylation: protein oligophosphorylation. Using site-specifically phosphorylated and pyrophosphorylated nucleoside diphosphate kinase A (NME1), the effects of these modifications on enzyme activity were investigated. Phosphorylation, and more so pyrophosphorylation, on Thr94 reduced the nucleoside diphosphate kinase activity. Nevertheless, both phosphoprotein and pyrophosphoprotein catalysed their own oligophosphorylation-up to the formation of a hexaphosphate chain-using ATP as a cofactor. Oligophosphorylation was critically dependent on the catalytic histidine residue His118, and cryogenic electron microscopy analysis of the modified proteins suggests an intramolecular phosphoryl transfer mechanism. Oligophosphorylation of NME1 in biochemical samples, and in cell lysates, was further confirmed using mass spectrometry, and was found to promote a new set of protein interactions. Our results highlight the complex nature of phosphoregulation, and the methods described here provide the opportunity to investigate the impact of this unusual modification in the future.
リンク	Nat Chem / PubMed:40835738 / PubMed Central
手法	EM (単粒子)
解像度	2.8 - 3.8 Å
構造データ	51248 9gd6 EMDB-51248, PDB-9gd6: NME1 94-Phosphoserine 手法: EM (単粒子) / 解像度: 2.8 Å 51250 9gd8 EMDB-51250, PDB-9gd8: NME1 94-Diphosphoserine 手法: EM (単粒子) / 解像度: 3.3 Å 51251 9gd9 EMDB-51251, PDB-9gd9: NME1 94-Oligophosphoserine 手法: EM (単粒子) / 解像度: 3.8 Å
由来	homo sapiens (ヒト)
キーワード	TRANSFERASE / nucleotide kinase / post-translational modification / phosphorylation