EMDB-40883: Raw consensus map of TRPM2 chanzyme in the presence of Magnesium,...

Basic information

Entry

Database: EMDB / ID: EMD-40883

• Title: Raw consensus map of TRPM2 chanzyme in the presence of Magnesium, Adenosine monophosphate, and Ribose-5-phosphate

Sample

• Complex: TRPM2 chanzyme incubated with Magnesium and ADP-ribose for 4min, ADP-ribose completely hydrolyzed to Adenosine monophosphate, and Ribose-5-phosphate
  • Protein or peptide: TRPM2 chanzyme

• Keywords: TRPM2 Chanzyme / Channel-enzyme / MEMBRANE PROTEIN
• Biological species: Salpingoeca rosetta (eukaryote)
• Method: single particle reconstruction / cryo EM / Resolution: 2.8 Å
• Authors: Huang Y / Kumar S / Lu W / Du J

Funding support

United States, 4 items

Organization	Grant number	Country
National Institutes of Health/National Heart, Lung, and Blood Institute (NIH/NHLBI)	HL153219	United States
National Institutes of Health/National Institute of Neurological Disorders and Stroke (NIH/NINDS)	NS112363	United States
National Institutes of Health/National Institute of Neurological Disorders and Stroke (NIH/NINDS)	NS111031	United States
National Institutes of Health/National Institute of General Medical Sciences (NIH/NIGMS)	GM129547	United States

• Citation: Journal: Nat Struct Mol Biol / Year: 2024; Title: Coupling enzymatic activity and gating in an ancient TRPM chanzyme and its molecular evolution.; Authors: Yihe Huang / Sushant Kumar / Junuk Lee / Wei Lü / Juan Du / ; Abstract: Channel enzymes represent a class of ion channels with enzymatic activity directly or indirectly linked to their channel function. We investigated a TRPM2 chanzyme from choanoflagellates that integrates two seemingly incompatible functions into a single peptide: a channel module activated by ADP-ribose with high open probability and an enzyme module (NUDT9-H domain) consuming ADP-ribose at a remarkably slow rate. Using time-resolved cryogenic-electron microscopy, we captured a complete series of structural snapshots of gating and catalytic cycles, revealing the coupling mechanism between channel gating and enzymatic activity. The slow kinetics of the NUDT9-H enzyme module confers a self-regulatory mechanism: ADPR binding triggers NUDT9-H tetramerization, promoting channel opening, while subsequent hydrolysis reduces local ADPR, inducing channel closure. We further demonstrated how the NUDT9-H domain has evolved from a structurally semi-independent ADP-ribose hydrolase module in early species to a fully integrated component of a gating ring essential for channel activation in advanced species.

History

Deposition	May 25, 2023	-
Header (metadata) release	May 29, 2024	-
Map release	May 29, 2024	-
Update	Oct 30, 2024	-
Current status	Oct 30, 2024	Processing site: RCSB / Status: Released

Map

• File: Download / File: emd_40883.map.gz / Format: CCP4 / Size: 325 MB / Type: IMAGE STORED AS FLOATING POINT NUMBER (4 BYTES)
• Voxel size: X=Y=Z: 0.826 Å

Density

Contour Level	By AUTHOR: 0.009
Minimum - Maximum	-0.003630515 - 0.022016462
Average (Standard dev.)	0.00014495054 (±0.00093115127)

• Symmetry: Space group: 1

Details

EMDB XML:

Map geometry	Axis order X Y Z Origin 0 0 0 Dimensions 440 440 440 Spacing 440 440 440
Cell	A=B=C: 363.44 Å α=β=γ: 90.0 °

Supplemental data

Additional map: #1

• File: emd_40883_additional_1.map

Half map: #1

• File: emd_40883_half_map_1.map

Half map: #2

• File: emd_40883_half_map_2.map

Sample components

Entire : TRPM2 chanzyme incubated with Magnesium and ADP-ribose for 4min, ...

• Entire: Name: TRPM2 chanzyme incubated with Magnesium and ADP-ribose for 4min, ADP-ribose completely hydrolyzed to Adenosine monophosphate, and Ribose-5-phosphate

Components

• Complex: TRPM2 chanzyme incubated with Magnesium and ADP-ribose for 4min, ADP-ribose completely hydrolyzed to Adenosine monophosphate, and Ribose-5-phosphate
  • Protein or peptide: TRPM2 chanzyme

Supramolecule #1: TRPM2 chanzyme incubated with Magnesium and ADP-ribose for 4min, ...

• Supramolecule: Name: TRPM2 chanzyme incubated with Magnesium and ADP-ribose for 4min, ADP-ribose completely hydrolyzed to Adenosine monophosphate, and Ribose-5-phosphate; type: complex / ID: 1 / Parent: 0 / Macromolecule list: all
• Source (natural): Organism: Salpingoeca rosetta (eukaryote)

Macromolecule #1: TRPM2 chanzyme

• Macromolecule: Name: TRPM2 chanzyme / type: protein_or_peptide / ID: 1 / Enantiomer: LEVO
• Source (natural): Organism: Salpingoeca rosetta (eukaryote)
• Recombinant expression: Organism: Homo sapiens (human)

Sequence

String:

MQRARPGELV EVIMFRPTGK ARVSNLDESM AMEFTDLRTR AMSSAAMIRQ SVAAKTLLIE NEDGKGSTRM EVQDFMKRFH MHASEDDKT GSPSTAWGTL RFPTKEATAP YLRLSVNDDP EDALLFVKAM LAQKYGETYD RPSLILSVTG GARNFTLPPR L ETAIAKGL RLAAQRTNAW VVTGGTNTGV MKLTGQIMEA LSKTQSHFIP PTIGIATYGV IIGGDDMTRG EPPKIGLEYE MH KKDPPKT TPLDDNHNLF LLVDDGSTNK FGKEIKFRAA FENAAGQAFA APVVTIVVQG GPGTLGTALQ AVRQGTPIVV VDG SGLAAD VLAYAYNFMH NPLTRFKSYT IDDLRQKVAQ TFNPKSSQQL TNLLDSALEC VQDPNLVVVY SLQESGIDEF DDCI LKAIF SSQGKLGNKL KQAMYFDQLD VAKRALSEAS KNGQHNEIAA CINDNLMAAM MHNKPHFVEL YLGFDAKIYE LKPSE EVAK TNITALDELP SFALAIEELY KREAKKPHSH VQRLVSLSNT DVLGRHYRVS TQRGDGTTRR IGRDLANTRA YNVLRM DQI FARLVSKDFS VNRDFTIYDS KYDKVPGIQF RRTAQASHML FLWAICLDRF RMARHFWLIG DQSIINALVA SRILERL ST HRALQGPHLA EERAKMQHNA KKFEELAVGV LGECHGSDSH MASEMLHSKN DMFNKKNAIN IAYDAKSLAF LSHPATQS V INADWYGHLK SVTSFWAVLF AFFFPFFVLP FINFSEDHAE QQVEAPRDFF TDAPRSSHSA NSTTSGAHRL RRKFAKFYS APYTRFISDL LSHFVLCVVT SYFVLDKLED TISAIEWILL VWFVALLLEE LRQMIFCDGI AEYISDTWNR LDLIMITLFF VGFFTHASD PSNQDSKVVS KGIHAFLVVV LWLRFMRYYA LSKNLGPKLI MMMEMMKDVS TFVFLLLIFL IGYGVAAQSL L SPDEDFSS RTFIGVLFRP YFQIYGELFL DDLNSEANCL GDTPFTECSR ETVRMVPFFL AVYILGSNVL LVNLLIAMFN DT YMKVQEA AEDLWRKQNY ELCAEYKDRP FLPAPFILLA HVHMLFMRLL RLCGVHTQEH EKIQDDETKR KITTFEELNT DKF LRRWER ERQEMLEARV KMTNDNVVQA MGMMDQLLEH MISFRFSLDQ QATKIKQEIR DDGLPSTEPT GLVSRTPSQP INRL NSAVA VHGHTAEAAE WYVPPEEYPK SGGVKRYLID ASMVPLSIMC PSYDPVEYTH PSVAAQPVWA DPADPRKIKF NVKDE VNGK VVDRTSCHPS GISIDSNTGR PINPWGRTGM TGRGLLGKWG VNQAADTVVT RWKRSPDGSI LERDGKKVLE FVAIQR QDN KMWAIPGGFV DNGEDVALTS GREFMEEALG MGTSADLMSA ESKDSLAALF SSGTIVARIY CEDPRNTDNA WVETTCV NF HDESGRHAAR LKLQGGDDAE HARWMMVHGG LNLFASHRTL LQHVTSALNA YF(RP5)(AMP)(MG)(MG)(MG)(MG) (CLR) (CLR)(CLR)

Experimental details

Structure determination

• Method: cryo EM
• Processing: single particle reconstruction
• Aggregation state: particle

Sample preparation

• Concentration: 8.5 mg/mL
• Buffer: pH: 8
• Vitrification: Cryogen name: ETHANE

Electron microscopy

• Microscope: FEI TITAN KRIOS
• Image recording: Film or detector model: GATAN K3 BIOQUANTUM (6k x 4k) / Average exposure time: 0.02 sec. / Average electron dose: 49.0 e/Ų
• Electron beam: Acceleration voltage: 300 kV / Electron source: FIELD EMISSION GUN
• Electron optics: Illumination mode: FLOOD BEAM / Imaging mode: BRIGHT FIELD / Nominal defocus max: 1.9000000000000001 µm / Nominal defocus min: 0.9 µm
• Experimental equipment: Model: Titan Krios / Image courtesy: FEI Company

Image processing

• Startup model: Type of model: NONE
• Final reconstruction: Resolution.type: BY AUTHOR / Resolution: 2.8 Å / Resolution method: FSC 0.143 CUT-OFF / Number images used: 634404
• Initial angle assignment: Type: RANDOM ASSIGNMENT
• Final angle assignment: Type: MAXIMUM LIKELIHOOD

Atomic model buiding 1

• Refinement: Space: REAL / Protocol: AB INITIO MODEL