Structural basis of trehalose recycling by the ABC transporter LpqY-SugABC

In bacteria, adenosine 5′-triphosphate (ATP)–binding cassette (ABC) importers are essential for the uptake of nutrients including the nonreducing disaccharide trehalose, a metabolite that is crucial for the survival and virulence of several human pathogens including Mycobacterium tuberculosis. SugABC is an ABC transporter that translocates trehalose from the periplasmic lipoprotein LpqY into the cytoplasm of mycobacteria. Here, we report four high-resolution cryo–electron microscopy structures of the mycobacterial LpqY-SugABC complex to reveal how it binds and passes trehalose through the membrane to the cytoplasm. A unique feature observed in this system is the initial mode of capture of the trehalose at the LpqY interface. Uptake is achieved by a pivotal rotation of LpqY relative to SugABC, moving from an open and accessible conformation to a clamped conformation upon trehalose binding. These findings enrich our understanding as to how ABC transporters facilitate substrate transport across the membrane in Gram-positive bacteria.

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Cryo-EM structure and polymorphism of Aβ amyloid fibrils purified from Alzheimer’s brain tissue

Nature Communications ◽

10.1038/s41467-019-12683-8 ◽

2019 ◽

Vol 10 (1) ◽

Cited By ~ 85

Author(s):

Marius Kollmer ◽

William Close ◽

Leonie Funk ◽

Jay Rasmussen ◽

Aref Bsoul ◽

...

Keyword(s):

Electron Microscopy ◽

Brain Tissue ◽

Amyloid Fibrils ◽

Structural Basis ◽

Amyloid Angiopathy ◽

Cryo Electron Microscopy ◽

Aβ Amyloid ◽

Cerebral Amyloid ◽

Aβ Fibrils

Abstract The formation of Aβ amyloid fibrils is a neuropathological hallmark of Alzheimer’s disease and cerebral amyloid angiopathy. However, the structure of Aβ amyloid fibrils from brain tissue is poorly understood. Here we report the purification of Aβ amyloid fibrils from meningeal Alzheimer’s brain tissue and their structural analysis with cryo-electron microscopy. We show that these fibrils are polymorphic but consist of similarly structured protofilaments. Brain derived Aβ amyloid fibrils are right-hand twisted and their peptide fold differs sharply from previously analyzed Aβ fibrils that were formed in vitro. These data underscore the importance to use patient-derived amyloid fibrils when investigating the structural basis of the disease.

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Cryo-electron Microscopy Structure and Transport Mechanism of a Wall Teichoic Acid ABC Transporter

mBio ◽

10.1128/mbio.02749-19 ◽

2020 ◽

Vol 11 (2) ◽

Cited By ~ 8

Author(s):

Li Chen ◽

Wen-Tao Hou ◽

Tao Fan ◽

Banghui Liu ◽

Ting Pan ◽

...

Keyword(s):

Abc Transporter ◽

Conformational Changes ◽

Abc Transporters ◽

Rational Design ◽

Teichoic Acid ◽

Inhibitory Mechanism ◽

Wall Teichoic Acid ◽

Content Type ◽

Design And Optimization ◽

Cryo Electron Microscopy

ABSTRACT The wall teichoic acid (WTA) is a major cell wall component of Gram-positive bacteria, such as methicillin-resistant Staphylococcus aureus (MRSA), a common cause of fatal clinical infections in humans. Thus, the indispensable ABC transporter TarGH, which flips WTA from cytoplasm to extracellular space, becomes a promising target of anti-MRSA drugs. Here, we report the 3.9-Å cryo-electron microscopy (cryo-EM) structure of a 50% sequence-identical homolog of TarGH from Alicyclobacillus herbarius at an ATP-free and inward-facing conformation. Structural analysis combined with activity assays enables us to clearly decode the binding site and inhibitory mechanism of the anti-MRSA inhibitor Targocil, which targets TarGH. Moreover, we propose a “crankshaft conrod” mechanism utilized by TarGH, which can be applied to similar ABC transporters that translocate a rather big substrate through relatively subtle conformational changes. These findings provide a structural basis for the rational design and optimization of antibiotics against MRSA. IMPORTANCE The wall teichoic acid (WTA) is a major component of cell wall and a pathogenic factor in methicillin-resistant Staphylococcus aureus (MRSA). The ABC transporter TarGH is indispensable for flipping WTA precursor from cytoplasm to the extracellular space, thus making it a promising drug target for anti-MRSA agents. The 3.9-Å cryo-EM structure of a TarGH homolog helps us to decode the binding site and inhibitory mechanism of a recently reported inhibitor, Targocil, and provides a structural platform for rational design and optimization of potential antibiotics. Moreover, we propose a “crankshaft conrod” mechanism to explain how a big substrate is translocated through subtle conformational changes of type II exporters. These findings advance our understanding of anti-MRSA drug design and ABC transporters.

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How Good Can Single-Particle Cryo-EM Become? What Remains Before It Approaches Its Physical Limits?

Annual Review of Biophysics ◽

10.1146/annurev-biophys-070317-032828 ◽

2019 ◽

Vol 48 (1) ◽

pp. 45-61 ◽

Cited By ~ 26

Author(s):

Robert M. Glaeser

Keyword(s):

Electron Microscopy ◽

High Resolution ◽

Single Particle ◽

Energy Use ◽

Optimal Choice ◽

Structural Basis ◽

Detective Quantum Efficiency ◽

Quantum Metrology ◽

Cryo Electron Microscopy ◽

Induced Motion

Impressive though the achievements of single-particle cryo–electron microscopy are today, a substantial gap still remains between what is currently accomplished and what is theoretically possible. As is reviewed here, twofold or more improvements are possible as regards ( a) the detective quantum efficiency of cameras at high resolution, ( b) converting phase modulations to intensity modulations in the image, and ( c) recovering the full amount of high-resolution signal in the presence of beam-induced motion of the specimen. In addition, potential for improvement is reviewed for other topics such as optimal choice of electron energy, use of aberration correctors, and quantum metrology. With the help of such improvements, it does not seem to be too much to imagine that determining the structural basis for every aspect of catalytic control, signaling, and regulation, in any type of cell of interest, could easily be accelerated fivefold or more.

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Granular Layer in the Periplasmic Space of Gram-Positive Bacteria and Fine Structures of Enterococcus gallinarum and Streptococcus gordonii Septa Revealed by Cryo-Electron Microscopy of Vitreous Sections

Journal of Bacteriology ◽

10.1128/jb.00391-06 ◽

2006 ◽

Vol 188 (18) ◽

pp. 6652-6660 ◽

Cited By ~ 63

Author(s):

Benoît Zuber ◽

Marisa Haenni ◽

Tânia Ribeiro ◽

Kathrin Minnig ◽

Fátima Lopes ◽

...

Keyword(s):

Electron Microscopy ◽

Plasma Membrane ◽

Granular Layer ◽

Streptococcus Gordonii ◽

Periplasmic Space ◽

Gram Positive ◽

Gram Positive Bacteria ◽

Cryo Electron Microscopy ◽

Enterococcus Gallinarum ◽

Peptidoglycan Layer

ABSTRACT High-resolution structural information on optimally preserved bacterial cells can be obtained with cryo-electron microscopy of vitreous sections. With the help of this technique, the existence of a periplasmic space between the plasma membrane and the thick peptidoglycan layer of the gram-positive bacteria Bacillus subtilis and Staphylococcus aureus was recently shown. This raises questions about the mode of polymerization of peptidoglycan. In the present study, we report the structure of the cell envelope of three gram-positive bacteria (B. subtilis, Streptococcus gordonii, and Enterococcus gallinarum). In the three cases, a previously undescribed granular layer adjacent to the plasma membrane is found in the periplasmic space. In order to better understand how nascent peptidoglycan is incorporated into the mature peptidoglycan, we investigated cellular regions known to represent the sites of cell wall production. Each of these sites possesses a specific structure. We propose a hypothetic model of peptidoglycan polymerization that accommodates these differences: peptidoglycan precursors could be exported from the cytoplasm to the periplasmic space, where they could diffuse until they would interact with the interface between the granular layer and the thick peptidoglycan layer. They could then polymerize with mature peptidoglycan. We report cytoplasmic structures at the E. gallinarum septum that could be interpreted as cytoskeletal elements driving cell division (FtsZ ring). Although immunoelectron microscopy and fluorescence microscopy studies have demonstrated the septal and cytoplasmic localization of FtsZ, direct visualization of in situ FtsZ filaments has not been obtained in any electron microscopy study of fixed and dehydrated bacteria.

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Structural basis for the mechanism of ABC transporters

Biochemical Society Transactions ◽

10.1042/bst20150047 ◽

2015 ◽

Vol 43 (5) ◽

pp. 889-893 ◽

Cited By ~ 69

Author(s):

Konstantinos Beis

Keyword(s):

Drug Resistance ◽

Binding Site ◽

Abc Transporter ◽

Abc Transporters ◽

Eukaryotic Cells ◽

Structural Basis ◽

Multi Drug Resistance ◽

Hydrolysis Of ◽

Transport Molecules ◽

Alternating Access

The ATP-binding cassette (ABC) transporters are primary transporters that couple the energy stored in adenosine triphosphate (ATP) to the movement of molecules across the membrane. ABC transporters can be divided into exporters and importers; importers mediate the uptake of essential nutrients into cells and are found predominantly in prokaryotes whereas exporters transport molecules out of cells or into organelles and are found in all organisms. ABC exporters have been linked with multi-drug resistance in both bacterial and eukaryotic cells. ABC transporters are powered by the hydrolysis of ATP and transport their substrate via the alternating access mechanism, whereby the protein alternates between a conformation in which the substrate-binding site is accessible from the outside of the membrane, outward-facing and one in which it is inward-facing. In this mini-review, the structures of different ABC transporter types in different conformations are presented within the context of the alternating access mechanism and how they have shaped our current understanding of the mechanism of ABC transporters.

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Structural basis of actin filament capping at the barbed-end: a cryo-electron microscopy study

The EMBO Journal ◽

10.1038/sj.emboj.7601395 ◽

2006 ◽

Vol 25 (23) ◽

pp. 5626-5633 ◽

Cited By ~ 71

Author(s):

Akihiro Narita ◽

Shuichi Takeda ◽

Atsuko Yamashita ◽

Yuichiro Maéda

Keyword(s):

Electron Microscopy ◽

Actin Filament ◽

Microscopy Study ◽

Electron Microscopy Study ◽

Structural Basis ◽

Cryo Electron Microscopy

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Elucidation of AMPA receptor–stargazin complexes by cryo–electron microscopy

Science ◽

10.1126/science.aaf8411 ◽

2016 ◽

Vol 353 (6294) ◽

pp. 83-86 ◽

Cited By ~ 76

Author(s):

Edward C. Twomey ◽

Maria V. Yelshanskaya ◽

Robert A. Grassucci ◽

Joachim Frank ◽

Alexander I. Sobolevsky

Keyword(s):

Electron Microscopy ◽

Cognitive Processes ◽

Electrostatic Interactions ◽

Structural Basis ◽

Cryo Electron Microscopy ◽

Activated State ◽

Ampar Trafficking ◽

Excitatory Neurotransmission ◽

Binding Interfaces ◽

The Brain

AMPA-subtype ionotropic glutamate receptors (AMPARs) mediate fast excitatory neurotransmission and contribute to high cognitive processes such as learning and memory. In the brain, AMPAR trafficking, gating, and pharmacology is tightly controlled by transmembrane AMPAR regulatory proteins (TARPs). Here, we used cryo–electron microscopy to elucidate the structural basis of AMPAR regulation by one of these auxiliary proteins, TARP γ2, or stargazin (STZ). Our structures illuminate the variable interaction stoichiometry of the AMPAR-TARP complex, with one or two TARP molecules binding one tetrameric AMPAR. Analysis of the AMPAR-STZ binding interfaces suggests that electrostatic interactions between the extracellular domains of AMPAR and STZ play an important role in modulating AMPAR function through contact surfaces that are conserved across AMPARs and TARPs. We propose a model explaining how TARPs stabilize the activated state of AMPARs and how the interactions between AMPARs and their auxiliary proteins control fast excitatory synaptic transmission.

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Cryo-EM Reveals the Structural Basis of Microtubule Depolymerization by Kinesin-13s

10.1101/206268 ◽

2017 ◽

Author(s):

Matthieu P. M. H. Benoit ◽

Ana B. Asenjo ◽

Hernando Sosa

Keyword(s):

Electron Microscopy ◽

Conformational Changes ◽

Distinct Group ◽

Atomic Resolution ◽

Structural Basis ◽

Structural Elements ◽

Microtubule Depolymerization ◽

Cryo Electron Microscopy ◽

Kinesin Superfamily ◽

Motile Activity

SummaryKinesin-13s constitute a distinct group within the kinesin superfamily of motor proteins that promotes microtubule depolymerization and lacks motile activity. The molecular mechanism by which the kinesins depolymerize microtubules and are adapted to perform a seemingly very different activity from other kinesins is still unclear. To address this issue we obtained near atomic resolution cryo-electron microscopy (cryo-EM) structures of Drosophila melanogaster kinesin-13 KLP10A constructs bound to curved or straight tubulin in different nucleotide states. The structures show how nucleotide induced conformational changes near the catalytic site are coupled with kinesin-13-specific structural elements to induce tubulin curvature leading to microtubule depolymerization. The data highlight a modular structure that allows similar kinesin core motor-domains to be used for different functions, such as motility or microtubule depolymerization.

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Molecular basis for the ATPase-powered substrate translocation by the Lon AAA+ protease

10.1101/2020.04.29.068361 ◽

2020 ◽

Cited By ~ 1

Author(s):

Kaiming Zhang ◽

Shanshan Li ◽

Kan-Yen Hsieh ◽

Shih-Chieh Su ◽

Grigore D. Pintilie ◽

...

Keyword(s):

Electron Microscopy ◽

Conformational Changes ◽

Molecular Basis ◽

Structural Basis ◽

Cryo Electron Microscopy ◽

Adenosine Triphosphatases ◽

Translocation Mechanism ◽

Atp Binding And Hydrolysis ◽

Proteolytic Chamber ◽

Specific Nucleotide

AbstractThe Lon AAA+ (adenosine triphosphatases associated with diverse cellular activities) protease (LonA) converts ATP-fuelled conformational changes into sufficient mechanical force to drive translocation of the substrate into a hexameric proteolytic chamber. To understand the structural basis for the substrate translocation process, we have determined the cryo-electron microscopy (cryo-EM) structure of Meiothermus taiwanensis LonA (MtaLonA) at 3.6 Å resolution in a substrate-engaged state. Substrate interactions are mediated by the dual pore-loops of the ATPase domains, organized in spiral staircase arrangement from four consecutive protomers in different ATP-binding and hydrolysis states; a closed AAA+ ring is nevertheless maintained by two disengaged ADP-bound protomers transiting between the lowest and highest position. The structure reveals a processive rotary translocation mechanism mediated by LonA-specific nucleotide-dependent allosteric coordination among the ATPase domains, which is induced by substrate binding.

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Structural basis of ER-associated protein degradation mediated by the Hrd1 ubiquitin ligase complex

Science ◽

10.1126/science.aaz2449 ◽

2020 ◽

Vol 368 (6489) ◽

pp. eaaz2449 ◽

Cited By ~ 7

Author(s):

Xudong Wu ◽

Marc Siggel ◽

Sergey Ovchinnikov ◽

Wei Mi ◽

Vladimir Svetlov ◽

...

Keyword(s):

Electron Microscopy ◽

Ubiquitin Ligase ◽

Dynamics Simulation ◽

Structural Basis ◽

Cryo Electron Microscopy ◽

Ubiquitin Ligase Complex ◽

Electron Microscopy Analysis ◽

Microscopy Analysis ◽

Simulation Results ◽

Membrane Region

Misfolded luminal endoplasmic reticulum (ER) proteins undergo ER-associated degradation (ERAD-L): They are retrotranslocated into the cytosol, polyubiquitinated, and degraded by the proteasome. ERAD-L is mediated by the Hrd1 complex (composed of Hrd1, Hrd3, Der1, Usa1, and Yos9), but the mechanism of retrotranslocation remains mysterious. Here, we report a structure of the active Hrd1 complex, as determined by cryo–electron microscopy analysis of two subcomplexes. Hrd3 and Yos9 jointly create a luminal binding site that recognizes glycosylated substrates. Hrd1 and the rhomboid-like Der1 protein form two “half-channels” with cytosolic and luminal cavities, respectively, and lateral gates facing one another in a thinned membrane region. These structures, along with crosslinking and molecular dynamics simulation results, suggest how a polypeptide loop of an ERAD-L substrate moves through the ER membrane.

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