The crystal structure of
            <i>apo</i>
            -FtsH reveals domain movements necessary for substrate unfolding and translocation

Bieniossek, Christoph; Niederhauser, Barbara; Baumann, Ulrich

doi:10.1073/pnas.0910708106

Cited by 84 publications

(93 citation statements)

References 46 publications

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“…The resolution of the structure, determined at 12 Å, was sufficient to confirm the presence of six FtsH protomers within each complex, obtained by fitting the atomic structures of cytosolic fragments of FtsH into the cryo-EM model (Bieniossek et al, 2006(Bieniossek et al, , 2009, but was insufficient to determine the structural organization of the two types of subunit within the ring.…”

Section: Introductionmentioning

confidence: 99%

“…To aid interpretation of the three-dimensional reconstruction, the crystallographically derived hexameric structure of a soluble fragment of FtsH, containing residues 146 to 603 of the 610-amino acid sequence of Thermotoga maritima FtsH (Bieniossek et al, 2009), encompassing the conserved AAA domain and PD, was modeled by visual inspection into the molecular envelope, contoured at a threshold of 2.5 s ( Figure 7A). The crystal structure fitted remarkably well into the central core, providing clear evidence to support the presence of six FtsH subunits in the GST-tagged FtsH complex.…”

Section: Electron Microscopy and Single-particle Analysis Of The Ftshmentioning

confidence: 99%

“…Coordinate data sets were obtained from the Research Collaboratory Structural Bioinformatics Data Bank (www.rcsb.org) for 3KDS.pdb (structure of the cytosolic region of the Thermotoga maritima FtsH protease at 2.60 Å; Bieniossek et al, 2009) and 1GTA.pdb (structure of GST at 2.4 Å; McTigue et al, 1995). Structures were modeled into the final calculated three-dimensional map using PyMol (DeLano, 2008).…”

Section: Single-particle Analysismentioning

confidence: 99%

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Subunit Organization of a Synechocystis Hetero-Oligomeric Thylakoid FtsH Complex Involved in Photosystem II Repair

Boehm

Krynická

et al. 2012

The Plant Cell

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FtsH metalloproteases are key components of the photosystem II (PSII) repair cycle, which operates to maintain photosynthetic activity in the light. Despite their physiological importance, the structure and subunit composition of thylakoid FtsH complexes remain uncertain. Mutagenesis has previously revealed that the four FtsH homologs encoded by the cyanobacterium Synechocystis sp PCC 6803 are functionally different: FtsH1 and FtsH3 are required for cell viability, whereas FtsH2 and FtsH4 are dispensable. To gain insights into FtsH2, which is involved in selective D1 protein degradation during PSII repair, we used a strain of Synechocystis 6803 expressing a glutathione S-transferase (GST)-tagged derivative (FtsH2-GST) to isolate FtsH2-containing complexes. Biochemical analysis revealed that FtsH2-GST forms a hetero-oligomeric complex with FtsH3. FtsH2 also interacts with FtsH3 in the wild-type strain, and a mutant depleted in FtsH3, like ftsH2 2 mutants, displays impaired D1 degradation. FtsH3 also forms a separate heterocomplex with FtsH1, thus explaining why FtsH3 is more important than FtsH2 for cell viability. We investigated the structure of the isolated FtsH2-GST/FtsH3 complex using transmission electron microscopy and single-particle analysis. The three-dimensional structural model obtained at a resolution of 26 Å revealed that the complex is hexameric and consists of alternating FtsH2/FtsH3 subunits.

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Section: Introductionmentioning

confidence: 99%

Section: Electron Microscopy and Single-particle Analysis Of The Ftshmentioning

confidence: 99%

Section: Single-particle Analysismentioning

confidence: 99%

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Subunit Organization of a Synechocystis Hetero-Oligomeric Thylakoid FtsH Complex Involved in Photosystem II Repair

Boehm

Krynická

et al. 2012

The Plant Cell

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“…Next, to improve the envelope fit, we replaced the AAA domain of apo-FtsH Cyt (7) with that of the nucleotide-bound structure (6) by superimposing the small helical domain from each structure. Because the pore loop-2 (residues 393-404 in Yta10 and 453-463 in Yta12) is disordered in the T. maritima FtsH Cyt crystal structure, the loop was modeled according to the conformation seen in the x-ray structure of Thermus thermophilus FtsH Cyt (PDB code 2DHR (5)), followed by manually adjusting the position of the AAA domains.…”

Section: ϫHis6mentioning

confidence: 99%

“…X-ray crystal structures of the soluble cytosolic domains of the bacterial AAA protease FtsH (FtsH Cyt ) bound to ADP and in the absence of nucleotide (apo) have been reported (5)(6)(7). Although the AAA ring of the apo-FtsH Cyt hexamer was 6-fold symmetric (7), the ADP-bound structures revealed a 2-(6) and 3-fold symmetrical hexamer (5).…”

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confidence: 99%

Electron Cryomicroscopy Structure of a Membrane-anchored Mitochondrial AAA Protease

Lee

Augustin

Tatsuta

et al. 2011

Journal of Biological Chemistry

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FtsH-related AAA proteases are conserved membrane-anchored, ATP-dependent molecular machines, which mediate the processing and turnover of soluble and membrane-embedded proteins in eubacteria, mitochondria, and chloroplasts. Homo-and hetero-oligomeric proteolytic complexes exist, which are composed of homologous subunits harboring an ATPase domain of the AAA family and an H41 metallopeptidase domain. Mutations in subunits of mitochondrial m-AAA proteases have been associated with different neurodegenerative disorders in human, raising questions on the functional differences between homo-and hetero-oligomeric AAA proteases. Here, we have analyzed the hetero-oligomeric yeast m-AAA protease composed of homologous Yta10 and Yta12 subunits. We combined genetic and structural approaches to define the molecular determinants for oligomer assembly and to assess functional similarities between Yta10 and Yta12. We demonstrate that replacement of only two amino acid residues within the metallopeptidase domain of Yta12 allows its assembly into homo-oligomeric complexes. To provide a molecular explanation, we determined the 12 Å resolution structure of the intact yeast m-AAA protease with its transmembrane domains by electron cryomicroscopy (cryo-EM) and atomic structure fitting. The full-length m-AAA protease has a bipartite structure and is a hexamer in solution. We found that residues in Yta12, which facilitate homo-oligomerization when mutated, are located at the interface between neighboring protomers in the hexamer ring. Notably, the transmembrane and intermembrane space domains are separated from the main body, creating a passage on the matrix side, which is wide enough to accommodate unfolded but not folded polypeptides.These results suggest a mechanism regarding how proteins are recognized and degraded by m-AAA proteases.Energy-dependent proteases form oligomeric ring complexes and harbor conserved ATPase domains of the AAA ϩ family (1). It is widely accepted that AAA ϩ machines utilize the energy derived from ATP hydrolysis to thread substrate proteins through a central pore resulting in substrate unfolding. FtsH-related AAA proteases form a distinct membraneassociated group of AAA ϩ machines, present in eubacteria and in mitochondria and chloroplasts of eukaryotic cells (2, 3). Members of this group feature an N-terminal membrane targeting signal, followed by one or two transmembrane helices, and a canonical AAA domain that is covalently linked to the metallopeptidase domain (3, 4).X-ray crystal structures of the soluble cytosolic domains of the bacterial AAA protease FtsH (FtsH Cyt ) bound to ADP and in the absence of nucleotide (apo) have been reported (5-7). Although the AAA ring of the apo-FtsH Cyt hexamer was 6-fold symmetric (7), the ADP-bound structures revealed a 2-(6) and 3-fold symmetrical hexamer (5). However, the protease ring was 6-fold symmetric in all three structures. Therefore, it remained unclear what symmetry the full-length protease adopts and which of the stereo-specific interactions between ne...

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Self‐Assembly of a Supramolecular, Three‐Dimensional, Spoked, Bicycle‐like Wheel

Cao

et al. 2013

Angewandte Chemie

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The function and properties of materials and biological organisms are not only related to the chemical structure and connectivity, but also through higher-order domain structure, such as in the magnetic domain of magnetic materials [1] as well as the secondary and tertiary structures of proteins and DNA. [2] Weak interactions such as hydrogen bonding and coordination exist widely in biological systems and are vital for biological metabolism and many other essential functions. [3] These supramolecular interactions [4] have attracted attention both in biology [5] as well as in numerous other fields, [6] such as supramolecular catalysis, chemical sensing, and molecular electronics. [7] 2,2':6',2''-Terpyridine (tpy) has been a widely used ligand for the creation of such motifs, partly because of its ability to coordinate diverse metals. There are numerous examples of tpy-based supramolecular systems, from 2D-based macrocycles and grids [8] to 3D arrangements, such as cages and prisms. [9] A two-dimensional, tpy-based supramolecular spoked wheel was previously reported. [10] In this three-component ensemble, two different terpyridine ligands and one type of metal were self-assembled. This 2D wheel structure is more rigid than macrocyclic hexagons because of its fixed spacefilling centerpiece, which also serves as a template for the outer ligands. Notably, very few supramolecular spokedwheel systems have been reported, [10,11] since the self-assembly of multiple components can be a synthetic challenge that requires more precise control over the geometry and connectivity. [12] To further functionalize the well-established tpy-based spoked-wheel assembly, the backbone and connectivity components of its original structure were redesigned. The framework, in this case, includes two parts: the spokes (S3) and rims (R3; core and outer ligands, respectively; numbers equate to the available tpy units). The core that originally consisted of the single, hexakis(terpyridine) S6 was replaced by two aromatic cores functionalized with three terpyridine ligands at 1208 that adopt a staggered conformation (Scheme 1). Thus, the new construct involves the two tris(terpyridine)s S3, six rim units R3 in which the three tris(terpyridine)s are separated by angles of 608, and twelve metals in a precise 2:6:12 ratio, respectively. The two central tris-tpy ligands are stacked with a common perpendicular axis to impart the 3D bicycle-wheel motif. b-Glucose moieties were attached to the tris-tpy rim component R3 to increase the solubility of the desired complex.The synthesis of rim ligand R3 (Scheme 2) started with bromination of 2,6-dimethoxyphenol to afford 1, followed by etherification with benzyl bromide to give 2. Next, 3 was prepared (67 %) through a Suzuki cross-coupling reaction between 2 and 4'-boronatophenyl-2,2':6',2''-terpyridine [13] by utilizing [PdCl 2 (PPh 3 ) 2 ] as a catalyst. The benzyl group in 3 was removed with ammonium formate in the presence of a Pd/C catalyst to afford 4, which underwent alkylation with N-(6-bromohe...

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The crystal structure of apo -FtsH reveals domain movements necessary for substrate unfolding and translocation

Cited by 84 publications

References 46 publications

Subunit Organization of a Synechocystis Hetero-Oligomeric Thylakoid FtsH Complex Involved in Photosystem II Repair

Subunit Organization of a Synechocystis Hetero-Oligomeric Thylakoid FtsH Complex Involved in Photosystem II Repair

Electron Cryomicroscopy Structure of a Membrane-anchored Mitochondrial AAA Protease

Self‐Assembly of a Supramolecular, Three‐Dimensional, Spoked, Bicycle‐like Wheel

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