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1. Mössbauer studies of the redox state of the ferric uptake regulator [2Fe–2S]2+ cluster in Escherichia coli

   https://doi.org/10.1016/j.jinorgbio.2025.112928  

   Fontenot, Chelsey R; Hoepner, Thomas; Xiong, Jin; Ding, Huangen; Popescu, Codrina V (September 2025, Journal of Inorganic Biochemistry)

   Ciurli, S (Ed.)

   The Ferric uptake regulator (Fur) proteins from Haemophilus influenzae and Escherichia coli overexpressed in E. coli cells (MC4100) grown in M9 medium supplemented with 57Fe were studied with Mössbauer spectroscopy. Previous studies have shown that Fur proteins from H. influenzae and E. coli bind a [2Fe-2S]2+ cluster in response to elevation of intracellular free iron content. Here we find that when the [2Fe-2S] 2+ clusters in purified Fur proteins are reduced with dithionite, the reduced clusters are quickly decomposed, forming compounds with two distinct spectral signatures of high spin Fe(II) in tetrahedral and octahedral coordination, respectively. The instability of the reduced [2Fe-2S]1+ cluster in Fur is unique, as the [2Fe-2S]2+ clusters in many other proteins can reversibly undergo one-electron reduction-oxidation. The Mössbauer spectra of whole E. coli cells overexpressing Fur proteins show a quadrupole doublet with the isomer shift of δ1 = 0.28 mm/s and ΔEQ1 = 0.52 mm/s, typical for oxidized [2Fe-2S]2+ clusters and identical with that in the purified Fur protein. The corresponding spectra in large applied magnetic fields show the diamagnetic pattern that unambiguously reveals an exchange-coupled system with a diamagnetic electronic ground state, which confirms its assignment to the oxidized [2Fe-2S]2+ cluster clusters from Fur. No reduced [2Fe-2S]1+ clusters of Fur are observed in the whole-cell E. coli spectra. The Mössbauer spectra of the whole-cell E. coli without the Fur expression do not contain the components associated with the [2Fe-2S]2+ cluster of Fur. 

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2. Production and secretion of recombinant spider silk in Bacillus megaterium

   https://doi.org/10.1186/s12934-024-02304-5  

   Connor, Alexander; Zha, R. Helen; Koffas, Mattheos (January 2024, Microbial Cell Factories)

   Abstract BackgroundSilk proteins have emerged as versatile biomaterials with unique chemical and physical properties, making them appealing for various applications. Among them, spider silk, known for its exceptional mechanical strength, has attracted considerable attention. Recombinant production of spider silk represents the most promising route towards its scaled production; however, challenges persist within the upstream optimization of host organisms, including toxicity and low yields. The high cost of downstream cell lysis and protein purification is an additional barrier preventing the widespread production and use of spider silk proteins. Gram-positive bacteria represent an attractive, but underexplored, microbial chassis that may enable a reduction in the cost and difficulty of recombinant silk production through attributes that include, superior secretory capabilities, frequent GRAS status, and previously established use in industry. ResultsIn this study, we explore the potential of gram-positive hosts by engineering the first production and secretion of recombinant spider silk in theBacillusgenus. Using an industrially relevantB. megateriumhost, it was found that the Sec secretion pathway enables secretory production of silk, however, the choice of signal sequence plays a vital role in successful secretion. Attempts at increasing secreted titers revealed that multiple translation initiation sites in tandem do not significantly impact silk production levels, contrary to previous findings for other gram-positive hosts and recombinant proteins. Notwithstanding, targeted amino acid supplementation in minimal media was found to increase production by 135% relative to both rich media and unaltered minimal media, yielding secretory titers of approximately 100 mg/L in flask cultures. ConclusionIt is hypothesized that the supplementation strategy addressed metabolic bottlenecks, specifically depletion of ATP and NADPH within the central metabolism, that were previously observed for anE. colihost producing the same recombinant silk construct. Furthermore, this study supports the hypothesis that secretion mitigates the toxicity of the produced silk protein on the host organism and enhances host performance in glucose-based minimal media. While promising, future research is warranted to understand metabolic changes more precisely in theBacillushost system in response to silk production, optimize signal sequences and promoter strengths, investigate the mechanisms behind the effect of tandem translation initiation sites, and evaluate the performance of this system within a bioreactor. 

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3. Metabolic engineering of Escherichia coli for optimized biosynthesis of nicotinamide mononucleotide, a noncanonical redox cofactor

   https://doi.org/10.1186/s12934-020-01415-z  

   Black, William B.; Aspacio, Derek; Bever, Danielle; King, Edward; Zhang, Linyue; Li, Han (December 2020, Microbial Cell Factories)

   null (Ed.)

   Abstract Background Noncanonical redox cofactors are emerging as important tools in cell-free biosynthesis to increase the economic viability, to enable exquisite control, and to expand the range of chemistries accessible. However, these noncanonical redox cofactors need to be biologically synthesized to achieve full integration with renewable biomanufacturing processes. Results In this work, we engineered Escherichia coli cells to biosynthesize the noncanonical cofactor nicotinamide mononucleotide (NMN + ), which has been efficiently used in cell-free biosynthesis. First, we developed a growth-based screening platform to identify effective NMN + biosynthetic pathways in E. coli . Second, we explored various pathway combinations and host gene disruption to achieve an intracellular level of ~ 1.5 mM NMN + , a 130-fold increase over the cell’s basal level, in the best strain, which features a previously uncharacterized nicotinamide phosphoribosyltransferase (NadV) from Ralstonia solanacearum. Last, we revealed mechanisms through which NMN + accumulation impacts E. coli cell fitness, which sheds light on future work aiming to improve the production of this noncanonical redox cofactor. Conclusion These results further the understanding of effective production and integration of NMN + into E. coli . This may enable the implementation of NMN + -directed biocatalysis without the need for exogenous cofactor supply. 

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4. Tetrazine Amino Acid Encoding for Rapid and Complete Protein Bioconjugation

   https://doi.org/10.21769/BioProtoc.5048  

   Eddins, Alex; Pung, Abigail; Cooley, Richard; Mehl, Ryan (January 2024, BIO-PROTOCOL)

   Generating protein conjugates using the bioorthogonal ligation between tetrazines and trans-cyclooctene groups avoids the need to manipulate cysteine amino acids, and the ligation is rapid, site-specific, stoichiometric and allows for labeling of proteins in complex biological environments. Here, we provide a protocol for the expression of conjugation-ready proteins at high yields in Escherichia coli with greater than 95% encoding and labeling fidelity. This protocol focuses on installing the “Tet2” tetrazine amino acid using an optimized genetic code expansion (GCE) machinery system, Tet2 “pAJE-E7”, to direct Tet2 encoding at TAG stop codons in BL21 E. coli strains, enabling reproducible expression of Tet2-proteins that quantitatively react with trans-cyclooctene (TCO) groups within 5 minutes at room temperature and physiological pH. Use of the BL21 derivative B95(DE3) minimizes premature truncation byproducts caused by incomplete suppression of TAG stop codons and this makes it possible to use more diverse protein construct designs. Here, using a superfolder green fluorescent protein construct as an example protein, we describe in detail a four-day process for encoding Tet2 with yields of ~200 mg per liter culture. Additionally, a simple and fast diagnostic gel electrophoretic mobility shift assay to confirm Tet2-Et encoding, and reactivity is described. Finally, strategies to adapt the protocol to alternative proteins of interest and optimize expression yields and reactivity for that protein are discussed. 

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5. Global protein turnover quantification in Escherichia coli reveals cytoplasmic recycling under nitrogen limitation

   https://doi.org/10.1038/s41467-024-49920-8  

   Gupta, Meera; Johnson, Alex_N_T; Cruz, Edward_R; Costa, Eli_J; Guest, Randi_L; Li, Sophia_Hsin-Jung; Hart, Elizabeth_M; Nguyen, Thao; Stadlmeier, Michael; Bratton, Benjamin_P; et al (July 2024, Nature Communications)

   Abstract Protein turnover is critical for proteostasis, but turnover quantification is challenging, and even in well-studiedE. coli, proteome-wide measurements remain scarce. Here, we quantify the turnover rates of ~3200E. coliproteins under 13 conditions by combining heavy isotope labeling with complement reporter ion quantification and find that cytoplasmic proteins are recycled when nitrogen is limited. We use knockout experiments to assign substrates to the known cytoplasmic ATP-dependent proteases. Surprisingly, none of these proteases are responsible for the observed cytoplasmic protein degradation in nitrogen limitation, suggesting that a major proteolysis pathway inE. coliremains to be discovered. Lastly, we show that protein degradation rates are generally independent of cell division rates. Thus, we present broadly applicable technology for protein turnover measurements and provide a rich resource for protein half-lives and protease substrates inE. coli, complementary to genomics data, that will allow researchers to study the control of proteostasis. 

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