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	N-terminal Transmembrane-Helix Epitope Tag for X-ray Crystallography and Electron Microscopy of Small Membrane Proteins.
ジャーナル・号・ページ	J Mol Biol, Vol. 433, Issue 16, Page 166909, Year 2021
掲載日	2021年8月6日
著者	Benjamin C McIlwain / Amanda L Erwin / Alexander R Davis / B Ben Koff / Louise Chang / Tatsiana Bylund / Gwo-Yu Chuang / Peter D Kwong / Melanie D Ohi / Yen-Ting Lai / Randy B Stockbridge /
PubMed 要旨	Structural studies of membrane proteins, especially small membrane proteins, are associated with well-known experimental challenges. Complexation with monoclonal antibody fragments is a common ...Structural studies of membrane proteins, especially small membrane proteins, are associated with well-known experimental challenges. Complexation with monoclonal antibody fragments is a common strategy to augment such proteins; however, generating antibody fragments that specifically bind a target protein is not trivial. Here we identify a helical epitope, from the membrane-proximal external region (MPER) of the gp41-transmembrane subunit of the HIV envelope protein, that is recognized by several well-characterized antibodies and that can be fused as a contiguous extension of the N-terminal transmembrane helix of a broad range of membrane proteins. To analyze whether this MPER-epitope tag might aid structural studies of small membrane proteins, we determined an X-ray crystal structure of a membrane protein target that does not crystallize without the aid of crystallization chaperones, the Fluc fluoride channel, fused to the MPER epitope and in complex with antibody. We also demonstrate the utility of this approach for single particle electron microscopy with Fluc and two additional small membrane proteins that represent different membrane protein folds, AdiC and GlpF. These studies show that the MPER epitope provides a structurally defined, rigid docking site for antibody fragments that is transferable among diverse membrane proteins and can be engineered without prior structural information. Antibodies that bind to the MPER epitope serve as effective crystallization chaperones and electron microscopy fiducial markers, enabling structural studies of challenging small membrane proteins.
リンク	J Mol Biol / PubMed:33676924 / PubMed Central
手法	EM (単粒子) / X線回折
解像度	3.26 - 16.0 Å
構造データ	EMDB-23247: MPER Fluc Bpe in complex with VRC42 手法: EM (単粒子) / 解像度: 16.0 Å PDB-6x58: MPER-Fluc-Ec2 bound to 10E8v4 antibody 手法: X-RAY DIFFRACTION / 解像度: 3.26 Å
由来	Bordetella pertussis (百日咳菌) homo sapiens (ヒト) human immunodeficiency virus (ヒト免疫不全ウイルス) escherichia coli (大腸菌)
キーワード	MEMBRANE PROTEIN (膜タンパク質) / antibody (抗体) / chaperone (シャペロン) / MEMBRANE PROTEIN-IMMUNE SYSTEM complex (生体膜)