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1. Atomic Force Microscopy Reveals Complexity Underlying General Secretory System Activity

   https://doi.org/10.3390/ijms24010055  

   Weaver, Dylan R.; King, Gavin M. (January 2023, International Journal of Molecular Sciences)

   The translocation of specific polypeptide chains across membranes is an essential activity for all life forms. The main components of the general secretory (Sec) system of E. coli include integral membrane translocon SecYEG, peripheral ATPase SecA, and SecDF, an ancillary complex that enhances polypeptide secretion by coupling translocation to proton motive force. Atomic force microscopy (AFM), a single-molecule imaging technique, is well suited to unmask complex, asynchronous molecular activities of membrane-associated proteins including those comprising the Sec apparatus. Using AFM, the dynamic structure of membrane-external protein topography of Sec system components can be directly visualized with high spatial-temporal precision. This mini-review is focused on AFM imaging of the Sec system in near-native fluid conditions where activity can be maintained and biochemically verified. Angstrom-scale conformational changes of SecYEG are reported on 100 ms timescales in fluid lipid bilayers. The association of SecA with SecYEG, forming membrane-bound SecYEG/SecA translocases, is directly visualized. Recent work showing topographical aspects of the translocation process that vary with precursor species is also discussed. The data suggests that the Sec system does not employ a single translocation mechanism. We posit that differences in the spatial frequency distribution of hydrophobic content within precursor sequences may be a determining factor in mechanism selection. Precise AFM investigations of active translocases are poised to advance our currently vague understanding of the complicated macromolecular movements underlying protein export across membranes. 

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2. Automated Registration and Clustering for Enhanced Localization Atomic Force Microscopy of Flexible Membrane Proteins

   https://doi.org/10.1101/2025.06.30.662259  

   Lisowski, Creighton M; King, Gavin M; Kosztin, Ioan (July 2025, bioRxiv)

   Atomic Force Microscopy (AFM) can create images of biomolecules under near-native conditions but suffers from limited lateral resolution due to the finite AFM tip size and recording frequency. The recently developed Localization Atomic Force Microscopy or LAFM (Heath et al., Nature 594, 385 (2021)) enhances lateral resolution by reconstructing peak positions in AFM image stacks, but it is less effective for flexible proteins with multiple conformations. Here we introduce an unsupervised deep learning algorithm that simultaneously registers and clusters images by protein conformation, thus making LAFM applicable to more flexible proteins. Using simulated AFM images from molecular dynamics simulations of the SecYEG translocon as a model membrane protein system, we demonstrate improved resolution for individual protein conformations. This work represents a step towards a more general LAFM algorithm that can handle biological macromolecules with multiple distinct conformational states such as SecYEG. Author summaryAtomic Force Microscopy (AFM) enables high-resolution imaging of biomolecules under near-native conditions but faces lateral resolution limits due to the finite AFM tip size and recording frequency. The recently developed Localization Atomic Force Microscopy (LAFM) method addresses this by reconstructing peak positions from AFM image stacks, achieving almost atomic resolution for rigid proteins like bacteriorhodopsin (Heath et al., Nature 594, 385 (2021)). However, flexible membrane proteins with dynamic conformations, such as the SecYEG translocon, which exhibits large and highly mobile cytoplasmic loops, lead to non-physical smearing in standard LAFM reconstructions. Here, we present a computational framework combining unsupervised deep clustering and LAFM to enhance the lateral resolution of AFM images of flexible membrane proteins. Our neural network algorithm (i) groups AFM images into conformationally homogeneous clusters and (ii) registers images within each cluster. Applying LAFM separately to these clusters minimizes smearing artifacts, yielding high-resolution reconstructions for distinct conformations. We validate this approach using synthetic AFM images generated from all-atom molecular dynamics simulations of SecYEG in a solvated POPE lipid bilayer. This advancement extends LAFM’s utility to encompass conformationally diverse membrane proteins. 

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3. An investigation of the YidC-mediated membrane insertion of Pf3 coat protein using molecular dynamics simulations

   https://doi.org/10.3389/fmolb.2022.954262  

   Polasa, Adithya; Hettige, Jeevapani; Immadisetty, Kalyan; Moradi, Mahmoud (August 2022, Frontiers in Molecular Biosciences)

   YidC is a membrane protein that facilitates the insertion of newly synthesized proteins into lipid membranes. Through YidC, proteins are inserted into the lipid bilayer via the SecYEG-dependent complex. Additionally, YidC functions as a chaperone in protein folding processes. Several studies have provided evidence of its independent insertion mechanism. However, the mechanistic details of the YidC SecY-independent protein insertion mechanism remain elusive at the molecular level. This study elucidates the insertion mechanism of YidC at an atomic level through a combination of equilibrium and non-equilibrium molecular dynamics (MD) simulations. Different docking models of YidC-Pf3 in the lipid bilayer were built in this study to better understand the insertion mechanism. To conduct a complete investigation of the conformational difference between the two docking models developed, we used classical molecular dynamics simulations supplemented with a non-equilibrium technique. Our findings indicate that the YidC transmembrane (TM) groove is essential for this high-affinity interaction and that the hydrophilic nature of the YidC groove plays an important role in protein transport across the cytoplasmic membrane bilayer to the periplasmic side. At different stages of the insertion process, conformational changes in YidC’s TM domain and membrane core have a mechanistic effect on the Pf3 coat protein. Furthermore, during the insertion phase, the hydration and dehydration of the YidC’s hydrophilic groove are critical. These results demonstrate that Pf3 coat protein interactions with the membrane and YidC vary in different conformational states during the insertion process. Finally, this extensive study directly confirms that YidC functions as an independent insertase. 

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4. Conserved lipid-facing basic residues promote the insertion of the porin OmpC into the E. coli outer membrane

   https://doi.org/10.1128/mbio.03319-24  

   Peterson, Janine H; Yang, Lixinhao; Gumbart, James C; Bernstein, Harris D (March 2025, mBio)

   Trent, M Stephen; Konovalova, Anna (Ed.)

   ABSTRACT Almost all integral membrane proteins that reside in the outer membrane (OM) of gram-negative bacteria contain a closed amphipathic β sheet (“β barrel”) that serves as a membrane anchor. The membrane integration of β barrel structures is catalyzed by a highly conserved heterooligomer called thebarrelassemblymachine (BAM). Although charged residues that are exposed to the lipid bilayer are infrequently found in outer membrane protein β barrels, the β barrels of OmpC/OmpF-type trimeric porins produced by Enterobacterales contain multiple conserved lipid-facing basic residues located near the extracellular side of the OM. Here, we show that these residues are required for the efficient insertion of theEscherichia coliOmpC protein into the OMin vivo. We found that the mutation of multiple basic residues to glutamine or alanine slowed insertion and reduced insertion efficiency. Furthermore, molecular dynamics simulations provided evidence that the basic residues promote the formation of hydrogen bonds and salt bridges with lipopolysaccharide, a unique glycolipid located exclusively in the outer leaflet of the OM. Taken together, our results support a model in which hydrophilic interactions between OmpC and LPS help to anchor the protein in the OM when the local environment is perturbed by BAM during membrane insertion and suggest a surprising role for membrane lipids in the insertion reaction.IMPORTANCEThe assembly (folding and membrane insertion) of bacterial outer membrane proteins (OMPs) is an essential cellular process that is a potential target for novel antibiotics. A heterooligomer called thebarrelassemblymachine (BAM) plays a major role in catalyzing OMP assembly. Here, we show that a group of highly conserved lipid-facing basic residues inEscherichia coliOmpC, a member of a major family of abundant OMPs known as trimeric porins, is required for the efficient integration of the protein into the outer membrane (OM). Based on our work and previous studies, we propose that the basic residues form interactions with a unique OM lipid (lipopolysaccharide) that promotes the insertion reaction. Our results provide strong evidence that interactions between specific membrane lipids and at least a subset of OMPs are required to supplement the activity of BAM and facilitate the integration of the proteins into the membrane. 

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5. Recurrent co-domestication of PIF/Harbinger transposable element proteins in insects

   https://doi.org/10.1186/s13100-022-00282-2  

   Markova, Dragomira N.; Ruma, Fatema B.; Casola, Claudio; Mirsalehi, Ayda; Betrán, Esther (December 2022, Mobile DNA)

   Abstract Background Transposable elements (TEs) are selfish DNA sequences capable of moving and amplifying at the expense of host cells. Despite this, an increasing number of studies have revealed that TE proteins are important contributors to the emergence of novel host proteins through molecular domestication. We previously described seven transposase-derived domesticated genes from the PIF/Harbinger DNA family of TEs in Drosophila and a co-domestication. All PIF TEs known in plants and animals distinguish themselves from other DNA transposons by the presence of two genes. We hypothesize that there should often be co-domestications of the two genes from the same TE because the transposase (gene 1) has been described to be translocated to the nucleus by the MADF protein (gene 2). To provide support for this model of new gene origination, we investigated available insect species genomes for additional evidence of PIF TE domestication events and explored the co-domestication of the MADF protein from the same TE insertion. Results After the extensive insect species genomes exploration of hits to PIF transposases and analyses of their context and evolution, we present evidence of at least six independent PIF transposable elements proteins domestication events in insects: two co-domestications of both transposase and MADF proteins in Anopheles (Diptera), one transposase-only domestication event and one co-domestication in butterflies and moths (Lepidoptera), and two transposases-only domestication events in cockroaches (Blattodea). The predicted nuclear localization signals for many of those proteins and dicistronic transcription in some instances support the functional associations of co-domesticated transposase and MADF proteins. Conclusions Our results add to a co-domestication that we previously described in fruit fly genomes and support that new gene origination through domestication of a PIF transposase is frequently accompanied by the co-domestication of a cognate MADF protein in insects, potentially for regulatory functions. We propose a detailed model that predicts that PIF TE protein co-domestication should often occur from the same PIF TE insertion. 

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