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1. Sensing devices fabricated with Escherichia coli expressing genetically tunable nanowires incorporated into a water-stable polymer

   https://doi.org/0.1016/j.bios.2025.117378  

   Sonawane, Jayesh M; Chia, Eric; Ueki, Toshiyuki; Woodard, Trevor; Greener, Jesse; Nonnenmann, Stephen S; Yao, Jun; Lovley, Derek R (March 2025, Biosensors and Bioelectronics)

   Electrically conductive, genetically tunable, pilin-based protein nanowires (ePNs) expressed in Escherichia coli grown on the biodiesel byproduct glycerol are a sustainable electronic material. They were previously shown to effectively function as sensing components for volatile analytes when deployed as thin films in electronic devices. However, thin-film devices are not suitable for analyzing components dissolved in water. To evaluate the possibility of fabricating a water-stable ePN matrix, ePNs purified from cells were mixed with polyvinyl butyral (PVB) to produce a transparent, electrically conductive, water-stable composite. ePN/PVB composite conductivity was tuned by changing the concentration of ePNs in the composite or genetically tailoring ePNs for different conductivities. Devices with an ePN/PVB sensing component rapidly responded in a linear fashion to changes in concentrations of dissolved ammonia or acetate. Genetically modifying nanowires to display an analyte-binding peptide on the ePN outer surface that was specific for ammonia or acetate increased sensing sensitivity and specificity. Composites comprised of whole cells of E. coli expressing ePNs and PVB were also electrically conductive. They functioned as sensing components whose sensitivity could also be tuned with the expression of ePNs displaying specific analyte-binding peptides. This approach avoids the laborious and time-consuming purification of protein nanowires from cells. The simplicity of sustainably fabricating an electronic sensing component with ePN-expressing E. coli mixed with a polymer, coupled with the potential of exquisitely tuning sensing specificity with facile ‘plug and play’ nanowire design, demonstrates the possibility of simply and inexpensively producing sensing devices for detecting a broad range of analytes. 

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2. Microbial nanowires with genetically modified peptide ligands to sustainably fabricate electronic sensing devices

   https://doi.org/10.1016/j.bios.2023.115147  

   Lekbach, Yassir; Ueki, Toshiyuki; Liu, Xiaomeng; Woodard, Trevor; Yao, Jun; Lovley, Derek R. (April 2023, Biosensors and Bioelectronics)

   Nanowires have substantial potential as the sensor component in electronic sensing devices. However, surface functionalization of traditional nanowire and nanotube materials with short peptides that increase sensor selectivity and sensitivity requires complex chemistries with toxic reagents. In contrast, microorganisms can assemble pilin monomers into protein nanowires with intrinsic conductivity from renewable feedstocks, yielding an electronic material that is robust and stable in applications, but also biodegradable. Here we report that the sensitivity and selectivity of protein nanowire-based sensors can be modified with a simple plug and play genetic approach in which a short peptide sequence, designed to bind the analyte of interest, is incorporated into the pilin protein that is microbially assembled into nanowires. We employed a scalable Escherichia coli chassis to fabricate protein nanowires that displayed either a peptide previously demonstrated to effectively bind ammonia, or a peptide known to bind acetic acid. Sensors comprised of thin films of the nanowires amended with the ammonia-specific peptide had a ca. 100-fold greater response to ammonia than sensors made with unmodified protein nanowires. Protein nanowires with the peptide that binds acetic acid yielded a 4-fold higher response than nanowires without the peptide. The protein nanowire-based sensors had greater responses than previously reported sensors fabricated with other nanomaterials. The results demonstrate that protein nanowires with enhanced sensor response for analytes of interest can be fabricated with a flexible genetic strategy that sustainably eliminates the energy, environmental, and health concerns associated with other common nanomaterials. 

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3. Structure and dynamics determine G protein coupling specificity at a class A GPCR

   https://doi.org/10.1101/2024.03.28.587240  

   Casiraghi, Marina; Wang, Haoqing; Brennan, Patrick; Habrian, Chris; Hubner, Harald; Schmidt, Maximilian F; Maul, Luis; Pani, Biswaranjan; Bahriz, Sherif MFM; Xu, Bing; et al (March 2024, bioRxiv)

   G protein coupled receptors (GPCRs) exhibit varying degrees of selectivity for different G protein isoforms. Despite the abundant structures of GPCR-G protein complexes, little is known about the mechanism of G protein coupling specificity. The β2-adrenergic receptor is an example of GPCR with high selectivity for Gαs, the stimulatory G protein for adenylyl cyclase, and much weaker for the Gαi family of G proteins inhibiting adenylyl cyclase. By developing a new Gαi-biased agonist (LM189), we provide structural and biophysical evidence supporting that distinct conformations at ICL2 and TM6 are required for coupling of the different G protein subtypes Gαs and Gαi. These results deepen our understanding of G protein specificity and bias and can accelerate the design of ligands that select for preferred signaling pathways. 

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4. Lipid-Mediated Modulation of mGluR2 Embedded in Micelle and Bilayer Environments: Insights from Molecular Dynamics

   https://doi.org/10.1101/2025.04.06.647485  

   Khodadadi, Ehsaneh; badiee, Shadi A; Khodadadi, Ehsan; Moradi, Mahmoud (April 2025, bioRxiv)

   Abstract Metabotropic glutamate receptor 2 (mGluR2), a subclass C member of the G protein-coupled receptor (GPCR) superfamily, is essential for regulating neurotransmitter signaling and facilitating synaptic adaptability in the central nervous system. This receptor, like other GPCRs, is highly sensitive to its surrounding lipid environment, where specific lipid compositions can influence its stability, conformational dynamics, and function. In particular, cholesteryl hemisuccinate (CHS) plays a critical role in stabilizing mGluR2 and modulating its structural states within cellular membranes and micellar environments. However, the molecular basis for this lipid-mediated modulation remains largely unexplored. To investigate the effects of CHS and lipid composition on mGluR2, we employed all-atom molecular dynamics simulations of mGluR2 embedded in both detergent micelles (BLMNG and CHS) and a POPC lipid bilayer containing 0%, 10%, and 25% CHS. These simulations were conducted for both active and inactive states of the receptor. Our findings reveal that CHS concentration modulates mGluR2’s structural stability and conformational behavior, with a marked impact observed within transmembrane helices TM1, TM2, and TM3, which constitute the core of the receptor’s transmembrane domain. In micelle environments, mGluR2 displayed unique conformational dynamics influenced by CHS, underscoring the receptor’s sensitivity to its lipid surroundings. Notably, a CHS concentration of 10% elicited more pronounced conformational changes than either cholesterol-depleted (0%) or cholesterol-enriched (25%) systems, indicating an optimal CHS range for maintaining structural stability. Our study provides atomistic insights into how lipid composition and CHS concentration impact mGluR2’s conformational landscape in distinct micelle and bilayer environments. These findings advance our understanding of lipid-mediated modulation in GPCR function, highlighting potential avenues for receptor-targeted drug design, particularly in cases where lipid interactions play a significant role in therapeutic efficacy. 

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5. Layer-Dependent Gas Sensing Mechanism of 2D Titanium Carbide (Ti3C2Tx) MXene

   https://doi.org/10.1021/acsnano.4c08225  

   Loes, Michael J; Bagheri, Saman; Sinitskii, Alexander (September 2024, ACS Nano)

   Monolayers of Ti3C2Tx MXene and bilayer structures formed by partially overlapping monolayer flakes exhibit opposite sensing responses to a large scope of molecular analytes. When exposed to reducing analytes, monolayer MXene flakes show increased electrical conductivity, i.e., an n-type behavior, while bilayer structures become less conductive, exhibiting a p-type behavior. On the contrary, both monolayers and bilayers show unidirectional sensing responses with increased resistivity when exposed to oxidizing analytes. The sensing responses of Ti3C2Tx monolayers and bilayers are dominated by entirely different mechanisms. The sensing behavior of MXene monolayers is dictated by the charge transfer from adsorbed molecules and the response direction is consistent with the donor/acceptor properties of the analyte and the intrinsic n-type character of Ti3C2Tx. In contrast, the bilayer MXene structures always show the same response regardless of the donor/acceptor character of the analyte, and the resistivity always increases because of the intercalation of molecules between the Ti3C2Tx layers. This study explains the sensing behavior of bulk MXene sensors based on multiflake assemblies, in which this intercalation mechanism results in universal increase in resistance that for many analytes is seemingly inconsistent with the n-type character of the material. By scaling MXene sensors down from multiflake to single-flake level, we disentangled the charge transfer and intercalation effects and unraveled their contributions. In particular, we show that the charge transfer has a much faster kinetics than the intercalation process. Finally, we demonstrate that the layer-dependent gas sensing properties of MXenes can be employed for the design of sensor devices with enhanced molecular recognition. 

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