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	Structural basis of tethered agonism and G protein coupling of protease-activated receptors.
ジャーナル・号・ページ	Cell Res, Vol. 34, Issue 10, Page 725-734, Year 2024
掲載日	2024年7月12日
著者	Jia Guo / Yun-Li Zhou / Yixin Yang / Shimeng Guo / Erli You / Xin Xie / Yi Jiang / Chunyou Mao / H Eric Xu / Yan Zhang /
PubMed 要旨	Protease-activated receptors (PARs) are a unique group within the G protein-coupled receptor superfamily, orchestrating cellular responses to extracellular proteases via enzymatic cleavage, which ...Protease-activated receptors (PARs) are a unique group within the G protein-coupled receptor superfamily, orchestrating cellular responses to extracellular proteases via enzymatic cleavage, which triggers intracellular signaling pathways. Protease-activated receptor 1 (PAR1) is a key member of this family and is recognized as a critical pharmacological target for managing thrombotic disorders. In this study, we present cryo-electron microscopy structures of PAR1 in its activated state, induced by its natural tethered agonist (TA), in complex with two distinct downstream proteins, the G and G heterotrimers, respectively. The TA peptide is positioned within a surface pocket, prompting PAR1 activation through notable conformational shifts. Contrary to the typical receptor activation that involves the outward movement of transmembrane helix 6 (TM6), PAR1 activation is characterized by the simultaneous downward shift of TM6 and TM7, coupled with the rotation of a group of aromatic residues. This results in the displacement of an intracellular anion, creating space for downstream G protein binding. Our findings delineate the TA recognition pattern and highlight a distinct role of the second extracellular loop in forming β-sheets with TA within the PAR family, a feature not observed in other TA-activated receptors. Moreover, the nuanced differences in the interactions between intracellular loops 2/3 and the Gα subunit of different G proteins are crucial for determining the specificity of G protein coupling. These insights contribute to our understanding of the ligand binding and activation mechanisms of PARs, illuminating the basis for PAR1's versatility in G protein coupling.
リンク	Cell Res / PubMed:38997424 / PubMed Central
手法	EM (単粒子)
解像度	3.0 - 3.2 Å
構造データ	38538 8xor EMDB-38538, PDB-8xor: Cryo-EM structure of the tethered agonist-bound human PAR1-Gq complex 手法: EM (単粒子) / 解像度: 3.0 Å 38539 8xos EMDB-38539, PDB-8xos: Cryo-EM structure of the tethered agonist-bound human PAR1-Gi complex 手法: EM (単粒子) / 解像度: 3.2 Å
化合物	ChemComp-CLR: CHOLESTEROL / コレステロ-ル
由来	rattus (ネズミ) bos taurus (ウシ) homo sapiens (ヒト) mus musculus (ハツカネズミ)
キーワード	MEMBRANE PROTEIN / GPCR / protease-activated receptor