PDB-7mdm: Structure of human p97 ATPase L464P mutant

基本情報

• 登録情報: データベース: PDB / ID: 7mdm
• タイトル: Structure of human p97 ATPase L464P mutant
• 要素: Transitional endoplasmic reticulum ATPase
• キーワード: MOTOR PROTEIN

機能・相同性

分子機能:

positive regulation of Lys63-specific deubiquitinase activity / flavin adenine dinucleotide catabolic process / positive regulation of oxidative phosphorylation / VCP-NSFL1C complex / cytoplasm protein quality control / endosome to lysosome transport via multivesicular body sorting pathway / endoplasmic reticulum stress-induced pre-emptive quality control / cellular response to arsenite ion / Derlin-1 retrotranslocation complex / BAT3 complex binding / protein-DNA covalent cross-linking repair / positive regulation of protein K63-linked deubiquitination / deubiquitinase activator activity / ubiquitin-modified protein reader activity / regulation of protein localization to chromatin / aggresome assembly / NADH metabolic process / mitotic spindle disassembly / VCP-NPL4-UFD1 AAA ATPase complex / vesicle-fusing ATPase / cellular response to misfolded protein / stress granule disassembly / negative regulation of protein localization to chromatin / positive regulation of mitochondrial membrane potential / retrograde protein transport, ER to cytosol / K48-linked polyubiquitin modification-dependent protein binding / regulation of aerobic respiration / regulation of synapse organization / positive regulation of ATP biosynthetic process / ATPase complex / ubiquitin-specific protease binding / MHC class I protein binding / ubiquitin-like protein ligase binding / RHOH GTPase cycle / polyubiquitin modification-dependent protein binding / autophagosome maturation / HSF1 activation / negative regulation of hippo signaling / endoplasmic reticulum to Golgi vesicle-mediated transport / translesion synthesis / proteasomal protein catabolic process / Protein methylation / interstrand cross-link repair / ATP metabolic process / negative regulation of smoothened signaling pathway / endoplasmic reticulum unfolded protein response / ERAD pathway / Attachment and Entry / proteasome complex / viral genome replication / lipid droplet / Josephin domain DUBs / N-glycan trimming in the ER and Calnexin/Calreticulin cycle / Hh mutants are degraded by ERAD / macroautophagy / Hedgehog ligand biogenesis / Defective CFTR causes cystic fibrosis / positive regulation of protein-containing complex assembly / ADP binding / Translesion Synthesis by POLH / establishment of protein localization / ABC-family proteins mediated transport / : / autophagy / Aggrephagy / cytoplasmic stress granule / positive regulation of non-canonical NF-kappaB signal transduction / positive regulation of protein catabolic process / azurophil granule lumen / KEAP1-NFE2L2 pathway / positive regulation of canonical Wnt signaling pathway / Ovarian tumor domain proteases / double-strand break repair / positive regulation of proteasomal ubiquitin-dependent protein catabolic process / E3 ubiquitin ligases ubiquitinate target proteins / site of double-strand break / Neddylation / cellular response to heat / ubiquitin-dependent protein catabolic process / protein phosphatase binding / secretory granule lumen / regulation of apoptotic process / proteasome-mediated ubiquitin-dependent protein catabolic process / ficolin-1-rich granule lumen / Attachment and Entry / protein ubiquitination / protein domain specific binding / intracellular membrane-bounded organelle / DNA repair / lipid binding / DNA damage response / glutamatergic synapse / ubiquitin protein ligase binding / Neutrophil degranulation / endoplasmic reticulum membrane / perinuclear region of cytoplasm / endoplasmic reticulum / ATP hydrolysis activity / protein-containing complex / RNA binding

ドメイン・相同性:

AAA ATPase, CDC48 family / Cell division protein 48 (CDC48), N-terminal domain / CDC48, N-terminal subdomain / Cell division protein 48 (CDC48) N-terminal domain / CDC48, domain 2 / Cell division protein 48 (CDC48), domain 2 / Cell division protein 48 (CDC48) domain 2 / CDC48 domain 2-like superfamily / : / Aspartate decarboxylase-like domain superfamily / AAA ATPase, AAA+ lid domain / AAA+ lid domain / ATPase, AAA-type, conserved site / AAA-protein family signature. / ATPase family associated with various cellular activities (AAA) / ATPase, AAA-type, core / ATPases associated with a variety of cellular activities / AAA+ ATPase domain / P-loop containing nucleoside triphosphate hydrolase

構成要素:

ADENOSINE-5'-DIPHOSPHATE / Transitional endoplasmic reticulum ATPase

• 生物種: Homo sapiens (ヒト)
• 手法: 電子顕微鏡法 / 単粒子再構成法 / クライオ電子顕微鏡法 / 解像度: 4.86 Å
• データ登録者: Zhang, X. / Gui, L. / Li, S. / Nandi, P. / Columbres, R.C. / Wong, D.E. / Moen, D.R. / Lin, H.J. / Chiu, P.-L. / Chou, T.-F.

資金援助

米国, 2件

組織	認可番号	国
National Institutes of Health/National Institute of Neurological Disorders and Stroke (NIH/NINDS)	R01NS100815	米国
National Institutes of Health/National Institute of Neurological Disorders and Stroke (NIH/NINDS)	R01NS102279	米国

• 引用: ジャーナル: Biochem J / 年: 2021; タイトル: Conserved L464 in p97 D1-D2 linker is critical for p97 cofactor regulated ATPase activity.; 著者: Xiaoyi Zhang / Lin Gui / Shan Li / Purbasha Nandi / Rod Carlo Columbres / Daniel E Wong / Derek R Moen / Henry J Lin / Po-Lin Chiu / Tsui-Fen Chou / ; 要旨: p97 protein is a highly conserved, abundant, functionally diverse, structurally dynamic homohexameric AAA enzyme-containing N, D1, and D2 domains. A truncated p97 protein containing the N and D1 domains and the D1-D2 linker (ND1L) exhibits 79% of wild-type (WT) ATPase activity whereas the ND1 domain alone without the linker only has 2% of WT activity. To investigate the relationship between the D1-D2 linker and the D1 domain, we produced p97 ND1L mutants and demonstrated that this 22-residue linker region is essential for D1 ATPase activity. The conserved amino acid leucine 464 (L464) is critical for regulating D1 and D2 ATPase activity by p97 cofactors p37, p47, and Npl4-Ufd1 (NU). Changing leucine to alanine, proline, or glutamate increased the maximum rate of ATP turnover (kcat) of p47-regulated ATPase activities for these mutants, but not for WT. p37 and p47 increased the kcat of the proline substituted linker, suggesting that they induced linker conformations facilitating ATP hydrolysis. NU inhibited D1 ATPase activities of WT and mutant ND1L proteins, but activated D2 ATPase activity of full-length p97. To further understand the mutant mechanism, we used single-particle cryo-EM to visualize the full-length p97L464P and revealed the conformational change of the D1-D2 linker, resulting in a movement of the helix-turn-helix motif (543-569). Taken together with the biochemical and structural results we conclude that the linker helps maintain D1 in a competent conformation and relays the communication to/from the N-domain to the D1 and D2 ATPase domains, which are ∼50 Å away.

履歴

登録	2021年4月5日	登録サイト: RCSB / 処理サイト: RCSB
改定 1.0	2021年8月25日	Provider: repository / タイプ: Initial release
改定 1.1	2021年9月1日	Group: Database references / カテゴリ: citation / Item: _citation.pdbx_database_id_PubMed / _citation.title
改定 1.2	2021年9月22日	Group: Database references / カテゴリ: citation Item: _citation.journal_volume / _citation.page_first / _citation.page_last
改定 1.3	2024年5月29日	Group: Data collection / Refinement description カテゴリ: chem_comp_atom / chem_comp_bond / em_3d_fitting_list / pdbx_initial_refinement_model Item: _em_3d_fitting_list.accession_code / _em_3d_fitting_list.initial_refinement_model_id / _em_3d_fitting_list.source_name / _em_3d_fitting_list.type

集合体

登録構造単位

B: Transitional endoplasmic reticulum ATPase

C: Transitional endoplasmic reticulum ATPase

D: Transitional endoplasmic reticulum ATPase

E: Transitional endoplasmic reticulum ATPase

A: Transitional endoplasmic reticulum ATPase

F: Transitional endoplasmic reticulum ATPase

ヘテロ分子

概要:

• 539 kDa, 6 ポリマー

構成要素の詳細:

	分子量 (理論値)	分子数
合計 (水以外)	539,088	12
ポリマ－	536,525	6
非ポリマー	2,563	6
水	0	0

1

概要:

• 登録構造と同一
• 登録者が定義した集合体
• 根拠: gel filtration

対称操作:

タイプ	名称	対称操作	数
identity operation	1_555		1

計算値:

Buried area	42480 Å2
ΔGint	-237 kcal/mol
Surface area	170970 Å2

要素

#1: タンパク質

B C D E A F
Transitional endoplasmic reticulum ATPase / TER ATPase / 15S Mg(2+)-ATPase p97 subunit / Valosin-containing protein / VCP

詳細:

分子量: 89420.773 Da / 分子数: 6 / 由来タイプ: 組換発現 / 由来: (組換発現) Homo sapiens (ヒト) / 遺伝子: VCP / 発現宿主: Escherichia coli (大腸菌) / 参照: UniProt: P55072, vesicle-fusing ATPase

#2: 化合物

B-901 C-901 D-901 E-901 A-901 F-901
ChemComp-ADP / ADENOSINE-5'-DIPHOSPHATE / ADP

詳細:

分子量: 427.201 Da / 分子数: 6 / 由来タイプ: 合成 / 式: C₁₀H₁₅N₅O₁₀P₂ / コメント: ADP, エネルギー貯蔵分子*YM

• 研究の焦点であるリガンドがあるか: N

実験情報

実験

• 実験: 手法: 電子顕微鏡法
• EM実験: 試料の集合状態: PARTICLE / ３次元再構成法: 単粒子再構成法

試料調製

• 構成要素: 名称: Human p97 L464P mutant / タイプ: COMPLEX / Entity ID: #1 / 由来: RECOMBINANT
• 分子量: 値: 0.536 MDa / 実験値: NO
• 由来(天然): 生物種: Homo sapiens (ヒト)
• 由来(組換発現): 生物種: Escherichia coli (大腸菌)
• 緩衝液: pH: 7.4
• 試料: 包埋: NO / シャドウイング: NO / 染色: NO / 凍結: YES
• 試料支持: グリッドのタイプ: C-flat-2/1
• 急速凍結: 凍結剤: ETHANE

電子顕微鏡撮影

• 実験機器: モデル: Titan Krios / 画像提供: FEI Company
• 顕微鏡: モデル: FEI TITAN KRIOS
• 電子銃: 電子線源: FIELD EMISSION GUN / 加速電圧: 300 kV / 照射モード: FLOOD BEAM
• 電子レンズ: モード: BRIGHT FIELD / Cs: 2.7 mm / C2レンズ絞り径: 70 µm
• 試料ホルダ: 凍結剤: NITROGEN; 試料ホルダーモデル: FEI TITAN KRIOS AUTOGRID HOLDER
• 撮影: 電子線照射量: 64.8 e/Ų / 検出モード: COUNTING; フィルム・検出器のモデル: GATAN K2 SUMMIT (4k x 4k)

解析

• ソフトウェア: 名称: PHENIX / バージョン: 1.18.2_3874: / 分類: 精密化

EMソフトウェア

ID	名称	バージョン	カテゴリ
1	Topaz	0.2.3	粒子像選択
2	SerialEM	3.9	画像取得
4	cryoSPARC	3.1	CTF補正
10	cryoSPARC	3.1	初期オイラー角割当
11	cryoSPARC	3.1	最終オイラー角割当
13	cryoSPARC	3.1	３次元再構成

• CTF補正: タイプ: PHASE FLIPPING AND AMPLITUDE CORRECTION
• 3次元再構成: 解像度: 4.86 Å / 解像度の算出法: FSC 0.143 CUT-OFF / 粒子像の数: 81865 / アルゴリズム: BACK PROJECTION / 対称性のタイプ: POINT
• 原子モデル構築: プロトコル: RIGID BODY FIT

原子モデル構築

PDB-ID: 5FTK

5ftk

Accession code: 5FTK / Source name: PDB / タイプ: experimental model

拘束条件

Refine-ID	タイプ	Dev ideal	数
ELECTRON MICROSCOPY	f_bond_d	0.005	32516
ELECTRON MICROSCOPY	f_angle_d	1.169	43942
ELECTRON MICROSCOPY	f_dihedral_angle_d	11.118	4446
ELECTRON MICROSCOPY	f_chiral_restr	0.07	4978
ELECTRON MICROSCOPY	f_plane_restr	0.008	5767