PDB-5m5m: Pseudo-atomic model of microtubule-bound S.pombe kinesin-5 motor ...

Basic information

• Entry: Database: PDB / ID: 5m5m
• Title: Pseudo-atomic model of microtubule-bound S.pombe kinesin-5 motor domain in the AMPPNP state (based on cryo-electron microscopy experiment): the N-terminus adopts multiple conformations.

Components

• Kinesin-like protein cut7
• Tubulin alpha-1D chain
• Tubulin beta-2B chain

• Keywords: MOTOR PROTEIN / microtubule-bound S.pombe kinesin-5 / motor domain / AMPPNP bound state / MODELLER 9.10 2013-08 complex

Function / homology

Function:

mitotic spindle formation (spindle phase one) / mitotic spindle elongation (spindle phase three) / Kinesins / initial mitotic spindle pole body separation / microtubule plus-end directed mitotic chromosome migration / meiotic spindle assembly / meiotic spindle pole / mitotic spindle midzone assembly / mitotic spindle midzone / mitotic spindle pole body / spindle elongation / polar microtubule / minus-end-directed microtubule motor activity / plus-end-directed microtubule motor activity / meiotic spindle / positive regulation of axon guidance / microtubule associated complex / microtubule motor activity / microtubule-based process / mitotic spindle assembly / spindle microtubule / structural constituent of cytoskeleton / mitotic spindle / kinetochore / microtubule cytoskeleton organization / microtubule cytoskeleton / mitotic cell cycle / nervous system development / microtubule binding / Hydrolases; Acting on acid anhydrides; Acting on GTP to facilitate cellular and subcellular movement / microtubule / hydrolase activity / protein heterodimerization activity / cell division / GTPase activity / GTP binding / ATP hydrolysis activity / ATP binding / nucleus / metal ion binding / cytoplasm

Domain/homology:

: / : / Kinesin motor domain signature. / Kinesin motor domain, conserved site / Kinesin motor domain profile. / Kinesin motor, catalytic domain. ATPase. / Kinesin motor domain / Kinesin motor domain / Kinesin motor domain superfamily / Alpha tubulin / Tubulin-beta mRNA autoregulation signal. / Beta tubulin, autoregulation binding site / Beta tubulin / Tubulin / Tubulin, C-terminal / Tubulin C-terminal domain / Tubulin, conserved site / Tubulin subunits alpha, beta, and gamma signature. / Tubulin/FtsZ family, C-terminal domain / Tubulin/FtsZ-like, C-terminal domain / Tubulin/FtsZ, C-terminal / Tubulin/FtsZ, 2-layer sandwich domain / Tubulin/FtsZ family, GTPase domain / Tubulin/FtsZ family, GTPase domain / Tubulin/FtsZ, GTPase domain / Tubulin/FtsZ, GTPase domain superfamily / P-loop containing nucleoside triphosphate hydrolase

Component:

PHOSPHOAMINOPHOSPHONIC ACID-ADENYLATE ESTER / GUANOSINE-5'-DIPHOSPHATE / GUANOSINE-5'-TRIPHOSPHATE / TAXOL / Kinesin-like protein cut7 / Tubulin alpha-1D chain / Tubulin beta-2B chain

• Biological species: Schizosaccharomyces pombe (fission yeast); Bos taurus (cattle)
• Method: ELECTRON MICROSCOPY / single particle reconstruction / cryo EM / Resolution: 9.3 Å
• Authors: Goulet, A. / Moores, C.A. / Cross, R.A.
• Citation: Journal: Proc Natl Acad Sci U S A / Year: 2016; Title: Schizosaccharomyces pombe kinesin-5 switches direction using a steric blocking mechanism.; Authors: Mishan Britto / Adeline Goulet / Syeda Rizvi / Ottilie von Loeffelholz / Carolyn A Moores / Robert A Cross / ; Abstract: Cut7, the sole kinesin-5 in Schizosaccharomyces pombe, is essential for mitosis. Like other yeast kinesin-5 motors, Cut7 can reverse its stepping direction, by mechanisms that are currently unclear. Here we show that for full-length Cut7, the key determinant of stepping direction is the degree of motor crowding on the microtubule lattice, with greater crowding converting the motor from minus end-directed to plus end-directed stepping. To explain how high Cut7 occupancy causes this reversal, we postulate a simple proximity sensing mechanism that operates via steric blocking. We propose that the minus end-directed stepping action of Cut7 is selectively inhibited by collisions with neighbors under crowded conditions, whereas its plus end-directed action, being less space-hungry, is not. In support of this idea, we show that the direction of Cut7-driven microtubule sliding can be reversed by crowding it with non-Cut7 proteins. Thus, crowding by either dynein microtubule binding domain or Klp2, a kinesin-14, converts Cut7 from net minus end-directed to net plus end-directed stepping. Biochemical assays confirm that the Cut7 N terminus increases Cut7 occupancy by binding directly to microtubules. Direct observation by cryoEM reveals that this occupancy-enhancing N-terminal domain is partially ordered. Overall, our data point to a steric blocking mechanism for directional reversal through which collisions of Cut7 motor domains with their neighbors inhibit their minus end-directed stepping action, but not their plus end-directed stepping action. Our model can potentially reconcile a number of previous, apparently conflicting, observations and proposals for the reversal mechanism of yeast kinesins-5.

History

Deposition	Oct 21, 2016	Deposition site: PDBE / Processing site: PDBE
Revision 1.0	Nov 30, 2016	Provider: repository / Type: Initial release
Revision 1.1	Dec 14, 2016	Group: Database references
Revision 1.2	Aug 2, 2017	Group: Data collection / Derived calculations / Experimental preparation / Refinement description Category: em_3d_fitting / em_image_scans / em_sample_support / em_software / pdbx_struct_conn_angle Item: _em_3d_fitting.target_criteria / _em_sample_support.grid_type / _em_software.name / _em_software.version
Revision 1.3	May 8, 2024	Group: Data collection / Database references / Category: chem_comp_atom / chem_comp_bond / database_2 Item: _database_2.pdbx_DOI / _database_2.pdbx_database_accession

Assembly

Deposited unit

A: Tubulin alpha-1D chain

B: Tubulin beta-2B chain

C: Kinesin-like protein cut7

hetero molecules

Summary:

• 143 kDa, 3 polymers
• Cα atoms only: ABC

Component details:

	Theoretical mass	Number of molelcules
Total (without water)	143,257	9
Polymers	140,882	3
Non-polymers	2,375	6
Water	0	0

1

Summary:

• Idetical with deposited unit
• defined by author

Symmetry operations:

Type	Name	Symmetry operation	Number
identity operation	1_555		1

Components

Protein , 3 types, 3 molecules A B C

#1: Protein

A Tubulin alpha-1D chain / Coordinate model: Cα atoms only

Details:

Mass: 50236.352 Da / Num. of mol.: 1 / Source method: isolated from a natural source / Source: (natural) Bos taurus (cattle) / References: UniProt: Q2HJ86

#2: Protein

B Tubulin beta-2B chain / Coordinate model: Cα atoms only

Details:

Mass: 49907.770 Da / Num. of mol.: 1 / Source method: isolated from a natural source / Source: (natural) Bos taurus (cattle) / References: UniProt: Q6B856

#3: Protein

C Kinesin-like protein cut7 / Cell untimely torn protein 7 / Coordinate model: Cα atoms only

Details:

Mass: 40737.527 Da / Num. of mol.: 1
Source method: isolated from a genetically manipulated source
Source: (gene. exp.) Schizosaccharomyces pombe (strain 972 / ATCC 24843) (yeast)
Gene: cut7, SPAC25G10.07c / Production host: Escherichia coli BL21(DE3) (bacteria) / References: UniProt: P24339

Non-polymers , 5 types, 6 molecules

#4: Chemical

A-501 C-501 ChemComp-MG / MAGNESIUM ION

Details:

Mass: 24.305 Da / Num. of mol.: 2 / Source method: obtained synthetically / Formula: Mg

#5: Chemical

A-502 ChemComp-GTP / GUANOSINE-5'-TRIPHOSPHATE

Details:

Mass: 523.180 Da / Num. of mol.: 1 / Source method: obtained synthetically / Formula: C₁₀H₁₆N₅O₁₄P₃ / Comment: GTP, energy-carrying molecule*YM

#6: Chemical

B-501 ChemComp-GDP / GUANOSINE-5'-DIPHOSPHATE

Details:

Type: RNA linking / Mass: 443.201 Da / Num. of mol.: 1 / Source method: obtained synthetically / Formula: C₁₀H₁₅N₅O₁₁P₂ / Comment: GDP, energy-carrying molecule*YM

#7: Chemical

B-502 ChemComp-TA1 / TAXOL

Details:

Mass: 853.906 Da / Num. of mol.: 1 / Source method: obtained synthetically / Formula: C₄₇H₅₁NO₁₄ / Comment: medication, chemotherapy*YM

#8: Chemical

C-502 ChemComp-ANP / PHOSPHOAMINOPHOSPHONIC ACID-ADENYLATE ESTER

Details:

Mass: 506.196 Da / Num. of mol.: 1 / Source method: obtained synthetically / Formula: C₁₀H₁₇N₆O₁₂P₃ / Comment: AMP-PNP, energy-carrying molecule analogue*YM

Experimental details

Experiment

• Experiment: Method: ELECTRON MICROSCOPY
• EM experiment: Aggregation state: HELICAL ARRAY / 3D reconstruction method: single particle reconstruction

Sample preparation

• Component: Name: microtubule-bound S. pombe kinesin-5 motor domain in the AMPPNP state; Type: COMPLEX / Entity ID: #1-#3 / Source: MULTIPLE SOURCES
• Molecular weight: Experimental value: NO
• Buffer solution: pH: 6.8

Buffer component

ID	Conc.	Formula	Buffer-ID
1	25 mM	PIPES	1
2	30 mM	NaCl	1
3	7 mM	MgCl2	1
4	1 mM	EGTA	1
5	5 mM	AMPPNP	1

• Specimen: Embedding applied: NO / Shadowing applied: NO / Staining applied: NO / Vitrification applied: YES
• Specimen support: Grid material: COPPER / Grid mesh size: 400 divisions/in. / Grid type: C-flat-2/2
• Vitrification: Instrument: FEI VITROBOT MARK I / Cryogen name: ETHANE / Humidity: 100 % / Chamber temperature: 294 K

Electron microscopy imaging

• Experimental equipment: Model: Tecnai F20 / Image courtesy: FEI Company
• Microscopy: Model: FEI TECNAI F20
• Electron gun: Electron source: FIELD EMISSION GUN / Accelerating voltage: 200 kV / Illumination mode: FLOOD BEAM
• Electron lens: Mode: BRIGHT FIELD / Calibrated magnification: 68000 X / Nominal defocus min: 700 nm
• Specimen holder: Cryogen: NITROGEN; Specimen holder model: GATAN CT3500 SINGLE TILT LIQUID NITROGEN CRYO TRANSFER HOLDER
• Image recording: Electron dose: 20 e/Ų / Film or detector model: GATAN ULTRASCAN 4000 (4k x 4k)

Processing

EM software

ID	Name	Version	Category
1	EMAN		particle selection
4	CTFFIND	3	CTF correction
5	FREALIGN		CTF correction
8	UCSF Chimera		model fitting
9	Flex-EM		model fitting
11	SPIDER		initial Euler assignment
12	FREALIGN		final Euler assignment
14	FREALIGN		3D reconstruction
15	Flex-EM		model refinement
16	MODELLER		model refinement

• CTF correction: Type: PHASE FLIPPING AND AMPLITUDE CORRECTION
• 3D reconstruction: Resolution: 9.3 Å / Resolution method: FSC 0.5 CUT-OFF / Num. of particles: 144300 / Symmetry type: POINT
• Atomic model building: Protocol: FLEXIBLE FIT / Space: REAL / Target criteria: Cross-correlation coefficient; Details: An initial homology model of S. pombe cut7 kinesin-5 motor domain based on human kinesin-5 structure (PDB 3HQD) was prepared using Modeller. The coordinates of motor bound to an alpha-beta tubulin dimer (PDB 1JFF) were rigidly fitted into the cryo-EM map using Chimera and refined by flexible fitting using Flex-EM. Structural models of loop5 and loop10 were generated using Modeller. The conformation of the neck-linker and the N-terminus were calculated using a conjugate-gradient energy minimization approach.