PDB-8t6q: Cryo-EM structure of dodecameric CaMKII beta holoenzyme T287A T30...

基本情報

• 登録情報: データベース: PDB / ID: 8t6q
• タイトル: Cryo-EM structure of dodecameric CaMKII beta holoenzyme T287A T306A T307A
• 要素: Venus-tagged CaMKII beta holoenzyme mutant
• キーワード: SIGNALING PROTEIN / High-order oligomer / Protein Kinase / Signaling / Memory

機能・相同性

分子機能:

regulation of synaptic transmission, cholinergic / activation of meiosis involved in egg activation / cell projection morphogenesis / HSF1-dependent transactivation / RAF activation / Ion transport by P-type ATPases / hippocampal neuron apoptotic process / calcium- and calmodulin-dependent protein kinase complex / cellular response to homocysteine / Interferon gamma signaling / positive regulation of synapse maturation / regulation of neuron migration / Ca2+/calmodulin-dependent protein kinase / structural constituent of postsynaptic actin cytoskeleton / regulation of synapse maturation / positive regulation of dendritic spine morphogenesis / calcium-dependent protein serine/threonine kinase activity / Trafficking of AMPA receptors / RAF/MAP kinase cascade / calcium/calmodulin-dependent protein kinase activity / response to psychosocial stress / Ion homeostasis / phospholipase binding / neuromuscular process controlling balance / Unblocking of NMDA receptors, glutamate binding and activation / regulation of protein localization to plasma membrane / spindle midzone / response to cadmium ion / sarcoplasmic reticulum membrane / bioluminescence / generation of precursor metabolites and energy / long-term synaptic potentiation / apoptotic signaling pathway / positive regulation of apoptotic signaling pathway / regulation of long-term neuronal synaptic plasticity / positive regulation of neuron projection development / G1/S transition of mitotic cell cycle / calcium ion transport / nervous system development / perikaryon / peptidyl-serine phosphorylation / protein autophosphorylation / postsynaptic density / cell differentiation / calmodulin binding / neuron projection / protein serine kinase activity / protein serine/threonine kinase activity / centrosome / glutamatergic synapse / dendrite / protein kinase binding / protein homodimerization activity / ATP binding / identical protein binding / cytoplasm / cytosol

ドメイン・相同性:

Calcium/calmodulin-dependent protein kinase II, association-domain / Calcium/calmodulin dependent protein kinase II association domain / NTF2-like domain superfamily / Green fluorescent protein, GFP / Green fluorescent protein-related / Green fluorescent protein / Green fluorescent protein / Serine/threonine-protein kinase, active site / Serine/Threonine protein kinases active-site signature. / Protein kinase domain / Serine/Threonine protein kinases, catalytic domain / Protein kinase, ATP binding site / Protein kinases ATP-binding region signature. / Protein kinase domain profile. / Protein kinase domain / Protein kinase-like domain superfamily

構成要素:

Calcium/calmodulin-dependent protein kinase type II subunit beta / Green fluorescent protein

• 生物種: Aequorea victoria (オワンクラゲ); Rattus norvegicus (ドブネズミ)
• 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: 3.5 Å
• データ登録者: Chien, C.-T. / Chiu, W. / Khan, S.

資金援助

米国, 1件

組織	認可番号	国
Other government	U24 GM129541	米国

• 引用: ジャーナル: Commun Biol / 年: 2024; タイトル: Hub stability in the calcium calmodulin-dependent protein kinase II.; 著者: Chih-Ta Chien / Henry Puhl / Steven S Vogel / Justin E Molloy / Wah Chiu / Shahid Khan / ; 要旨: The calcium calmodulin protein kinase II (CaMKII) is a multi-subunit ring assembly with a central hub formed by the association domains. There is evidence for hub polymorphism between and within CaMKII isoforms, but the link between polymorphism and subunit exchange has not been resolved. Here, we present near-atomic resolution cryogenic electron microscopy (cryo-EM) structures revealing that hubs from the α and β isoforms, either standalone or within an β holoenzyme, coexist as 12 and 14 subunit assemblies. Single-molecule fluorescence microscopy of Venus-tagged holoenzymes detects intermediate assemblies and progressive dimer loss due to intrinsic holoenzyme lability, and holoenzyme disassembly into dimers upon mutagenesis of a conserved inter-domain contact. Molecular dynamics (MD) simulations show the flexibility of 4-subunit precursors, extracted in-silico from the β hub polymorphs, encompassing the curvature of both polymorphs. The MD explains how an open hub structure also obtained from the β holoenzyme sample could be created by dimer loss and analysis of its cryo-EM dataset reveals how the gap could open further. An assembly model, considering dimer concentration dependence and strain differences between polymorphs, proposes a mechanism for intrinsic hub lability to fine-tune the stoichiometry of αβ heterooligomers for their dynamic localization within synapses in neurons.

履歴

登録	2023年6月16日	登録サイト: RCSB / 処理サイト: RCSB
改定 1.0	2024年6月19日	Provider: repository / タイプ: Initial release
改定 1.1	2024年7月10日	Group: Data collection / Database references / カテゴリ: citation / citation_author / em_admin Item: _citation.country / _citation.journal_abbrev / _citation.journal_id_CSD / _citation.journal_id_ISSN / _citation.journal_volume / _citation.page_first / _citation.page_last / _citation.pdbx_database_id_DOI / _citation.pdbx_database_id_PubMed / _citation.title / _citation.year / _citation_author.identifier_ORCID / _citation_author.name / _em_admin.last_update

集合体

登録構造単位

A: Venus-tagged CaMKII beta holoenzyme mutant

B: Venus-tagged CaMKII beta holoenzyme mutant

C: Venus-tagged CaMKII beta holoenzyme mutant

D: Venus-tagged CaMKII beta holoenzyme mutant

F: Venus-tagged CaMKII beta holoenzyme mutant

G: Venus-tagged CaMKII beta holoenzyme mutant

H: Venus-tagged CaMKII beta holoenzyme mutant

I: Venus-tagged CaMKII beta holoenzyme mutant

J: Venus-tagged CaMKII beta holoenzyme mutant

K: Venus-tagged CaMKII beta holoenzyme mutant

L: Venus-tagged CaMKII beta holoenzyme mutant

N: Venus-tagged CaMKII beta holoenzyme mutant

概要:

• 1.09 MDa, 12 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)	1,090,162	12
ポリマ－	1,090,162	12
非ポリマー	0	0
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: 電子顕微鏡法, not applicable

対称操作:

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

要素

#1: タンパク質

A B C D F G H I J K L N
Venus-tagged CaMKII beta holoenzyme mutant

詳細:

分子量: 90846.859 Da / 分子数: 12 / 変異: T287A,T306A,T307A / 由来タイプ: 組換発現
由来: (組換発現) Aequorea victoria (オワンクラゲ), (組換発現) Rattus norvegicus (ドブネズミ)
遺伝子: GFP, Camk2b / 発現宿主: Escherichia coli (大腸菌) / 参照: UniProt: P42212, UniProt: P08413

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: Venus-tagged CaMKII beta holoenzyme T287A T306A T307A; タイプ: COMPLEX / Entity ID: all / 由来: RECOMBINANT
• 分子量: 実験値: NO
• 由来(天然): 生物種: Rattus norvegicus (ドブネズミ)
• 由来(組換発現): 生物種: Escherichia coli (大腸菌)
• 緩衝液: pH: 7.5
• 試料: 濃度: 20 mg/ml / 包埋: NO / シャドウイング: NO / 染色: NO / 凍結: YES
• 急速凍結: 凍結剤: ETHANE / 湿度: 100 % / 凍結前の試料温度: 277 K

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 / 最大 デフォーカス（公称値）: 1500 nm / 最小 デフォーカス（公称値）: 600 nm
• 撮影: 電子線照射量: 60 e/Ų; フィルム・検出器のモデル: GATAN K3 BIOQUANTUM (6k x 4k)

解析

• CTF補正: タイプ: PHASE FLIPPING AND AMPLITUDE CORRECTION
• 3次元再構成: 解像度: 3.5 Å / 解像度の算出法: FSC 0.143 CUT-OFF / 粒子像の数: 332360 / 対称性のタイプ: POINT
• 精密化: 交差検証法: NONE; 立体化学のターゲット値: GeoStd + Monomer Library + CDL v1.2
• 原子変位パラメータ: B_iso mean: 88.4 Ų

拘束条件

Refine-ID	タイプ	Dev ideal	数
ELECTRON MICROSCOPY	f_bond_d	0.0031	13284
ELECTRON MICROSCOPY	f_angle_d	0.5402	18036
ELECTRON MICROSCOPY	f_chiral_restr	0.0419	1920
ELECTRON MICROSCOPY	f_plane_restr	0.0052	2400
ELECTRON MICROSCOPY	f_dihedral_angle_d	5.121	1752