Mitochondrial-bacterial hybrids of BamA/Tob55 suggest variable requirements for the membrane integration of β-barrel proteins

Pfitzner, Anna-Katharina; Steblau, Nadja; Ulrich, Thomas A.; Oberhettinger, Philipp; Autenrieth, Ingo B.; Schütz, Monika; Rapaport, Doron

doi:10.1038/srep39053

Cited by 8 publications

(14 citation statements)

References 50 publications

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“…This is consistent with recent kinetic simulations showing that when Skp foldase rates are set to be equivalent to those mediated by SurA, the experimentally observed severity of the ∆ surA phenotype is not reproduced [20] . Interestingly, a recent study in yeast demonstrated that expression of E. coli Skp in the mitochondrial intermembrane space assists the assembly of some E. coli OMPs (OmpX, PhoE) into the mitochondrial OM, but not others (OmpA) [54] , consistent with the view that chaperones and BAM components perform different roles in OMP assembly, depending on substrate [55] .…”

Section: Discussionsupporting

confidence: 55%

Effects of Periplasmic Chaperones and Membrane Thickness on BamA-Catalyzed Outer-Membrane Protein Folding

Schiffrin

Calabrese

Higgins

et al. 2017

Journal of Molecular Biology

100

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The biogenesis of outer-membrane proteins (OMPs) in gram-negative bacteria involves delivery by periplasmic chaperones to the β-barrel assembly machinery (BAM), which catalyzes OMP insertion into the outer membrane. Here, we examine the effects of membrane thickness, the Escherichia coli periplasmic chaperones Skp and SurA, and BamA, the central subunit of the BAM complex, on the folding kinetics of a model OMP (tOmpA) using fluorescence spectroscopy, native mass spectrometry, and molecular dynamics simulations. We show that prefolded BamA promotes the release of tOmpA from Skp despite the nM affinity of the Skp:tOmpA complex. This activity is located in the BamA β-barrel domain, but is greater when full-length BamA is present, indicating that both the β-barrel and polypeptide transport-associated (POTRA) domains are required for maximal activity. By contrast, SurA is unable to release tOmpA from Skp, providing direct evidence against a sequential chaperone model. By varying lipid acyl chain length in synthetic liposomes we show that BamA has a greater catalytic effect on tOmpA folding in thicker bilayers, suggesting that BAM catalysis involves lowering of the kinetic barrier imposed by the hydrophobic thickness of the membrane. Consistent with this, molecular dynamics simulations reveal that increases in membrane thinning/disorder by the transmembrane domain of BamA is greatest in thicker bilayers. Finally, we demonstrate that cross-linking of the BamA barrel does not affect tOmpA folding kinetics in 1,2-dimyristoyl-sn-glycero-3-phosphocholine (DMPC) liposomes, suggesting that lateral gating of the BamA barrel and/or hybrid barrel formation is not required, at least for the assembly of a small 8-stranded OMP in vitro.

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Section: Discussionsupporting

confidence: 55%

Effects of Periplasmic Chaperones and Membrane Thickness on BamA-Catalyzed Outer-Membrane Protein Folding

Schiffrin

Calabrese

Higgins

et al. 2017

Journal of Molecular Biology

100

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“…The large diversity of bacterial β-barrel proteins and the involvement of multiple POTRA domains and accessory Bam proteins (5, 15, 51, 60) raise the possibility that additional precursor-specific folding pathways may complement the central mechanism of β-signal exchange and sorting via the lateral gate elucidated here. For example assembly of oligomeric β-barrels in bacteria might be stalled at the BAM complex until all subunits are assembled (65), similar to the arrest of shortened precursor constructs of monomeric β-barrels (Fig.…”

Section: Discussionmentioning

confidence: 92%

“…The hidden-Markov model based homology search identified templates in the PDB with good p- and E-values. This included structures from FhaC [PDB code: 4QL0 (51)] and TamA [PDB code: 4C00 (18)] as well as several structures from BamA [PDB codes: 4K3B and 4K3C (16); 4C4V (21); 4N75 (22) and 5EKQ (23)], which exhibit considerable variations in the interaction between the β1 and β16-strands. A Sam50 model was calculated from each template using Modeller (72).…”

Section: Methodsmentioning

confidence: 99%

“…In addition to the β-barrel channel, Sam50 possesses two major characteristic elements, an N-terminal polypeptide transport associated (POTRA) domain exposed to the intermembrane space and a highly conserved loop 6 that extends from the cytosolic side of the β-barrel. (i) Whereas bacterial BamA proteins contain several POTRA domains that interact with β-barrel precursors and are crucial for precursor transfer from the periplasm into the outer membrane (17, 46–49), Sam50 contains a single POTRA domain that is not essential for cell viability (13, 50, 51). Disulfide formation between the Por1 precursor and Sam50 β-strands 1 and 16 was not blocked in mitochondria lacking the entire POTRA domain (fig.…”

Section: Sam50 Loop 6 Is Required For β-Signal Bindingmentioning

confidence: 99%

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Membrane protein insertion through a mitochondrial β-barrel gate

Höhr

Lindau

Wirth

et al. 2018

Science

125

139

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The biogenesis of mitochondria, chloroplasts, and Gram-negative bacteria requires the insertion of β-barrel proteins into the outer membranes. Homologous Omp85 proteins are essential for membrane insertion of β-barrel precursors. It is unknown if precursors are threaded through the Omp85-channel interior and exit laterally or if they are translocated into the membrane at the Omp85-lipid interface. We have mapped the interaction of a precursor in transit with the mitochondrial Omp85-channel Sam50 in the native membrane environment. The precursor is translocated into the channel interior, interacts with an internal loop, and inserts into the lateral gate by β-signal exchange. Transport through the Omp85-channel interior followed by release through the lateral gate into the lipid phase may represent a basic mechanism for membrane insertion of β-barrel proteins.

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“…TOM40 and SAM50 together have representatives in 97.93 % of the studied proteomes (1042 out of 1064 proteomes) and this reflects their crucial biological role in the translocation of OMPs into the MOM in all eukaryotes. This process begins with the translation of mitochondrial OMPs in cytosolic ribosomes and then follows their import into the target organelles 61,62,97 . Mitochondrial proteins reach the mitochondrial surface and then are translocated into the intermembrane space across the outer membrane via the translocase of the MOM (TOM) complex 45,98 .…”

mentioning

confidence: 99%

Landscape of Eukaryotic Transmembrane Beta Barrel Proteins

et al. 2020

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Even though in the last few years several families of eukaryotic β-barrel outer membrane proteins (OMPs) have been discovered, their computational characterization and their annotation in public databases is far from complete. The PFAM database includes only very few characteristic profiles for these families and, in most cases, the profile Hidden Markov Models (pHMMs) have been trained using prokaryotic and eukaryotic proteins together. Here, we present for the first time a comprehensive computational analysis of eukaryotic transmembrane β-barrels. 12 characteristic pHMMs were built, based on an extensive literature search, that can discriminate eukaryotic β-barrels from other classes of proteins (globular and bacterial β-barrel ones), as well as between mitochondrial and chloroplastic ones. We built eight novel profiles for the chloroplastic β-barrel families that are not present in the PFAM database and, also, updated the profile for the MDM10 family 2 (PF12519) in PFAM and split the porin family (PF01459) into two separate families, namely VDAC and TOM40.

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Mitochondrial-bacterial hybrids of BamA/Tob55 suggest variable requirements for the membrane integration of β-barrel proteins

Cited by 8 publications

References 50 publications

Effects of Periplasmic Chaperones and Membrane Thickness on BamA-Catalyzed Outer-Membrane Protein Folding

Effects of Periplasmic Chaperones and Membrane Thickness on BamA-Catalyzed Outer-Membrane Protein Folding

Membrane protein insertion through a mitochondrial β-barrel gate

Landscape of Eukaryotic Transmembrane Beta Barrel Proteins

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