The Journal of General and Applied Microbiology

Decolorization and degradation of azo dyes by the thermal and heavy metal tolerant bacterial consortium BPA-1

An efficient bacterial consortium (designated BPA-1), comprising Bacillus subtilis SX-6, Pseudomonas sp. SX-10, and Georgenia sp. SY-1, was successfully constructed for the decolorization of the azo dye Congo Red (CR). BPA-1 exhibited significant thermotolerance and heavy metal resistance, achieving over 90% CR decolorization within 60 h at 47°C under co-stress conditions with Zn²⁺, Mn²⁺, and Pb²⁺ (50 mg/L each). The consortium demonstrated broad substrate specificity, effectively decolorizing 12 structurally diverse azo dyes. Enzymatic assays revealed the involvement of laccase, manganese peroxidase, lignin peroxidase, and azoreductase in CR biodegradation. Metabolic pathway analysis indicated a three-stage degradation mechanism: (1) Asymmetric cleavage of azo bonds (-N=N-) generated 4,4'-diazaldenylbiphenyl and 4-amino-1-naphthalenesulfonic acid (Intermediate II); (2) Deamination converted Intermediate II to 3,4-dihydroxy-1-naphthalenesulfonic acid, followed by desulfurization to form naphthalene-1,2,3,4-tetraol; (3) Complete mineralization of intermediates occurred through subsequent oxidative steps. Notably, 4,4'-diazaldenylbiphenyl was further transformed into 4,4'-diaminobiphenyl, confirming the consortium’s capacity for multi-step detoxification.

Characterization of rice rhizospheric Bacillus thuringiensis as biocide against leaf folder (Cnaphalocrocis medinalis), stripe stem borer (Chilo suppresalis), plant pathogens, and plant growth promotion traits

Bacillus thuringiensis (Bt) has broad spectrum multipotent functionalities for pest and disease suppression, and growth promotion (PGP) of plants. Therefore, potency of 27 rice rhizospheric and 2 commercial Bt isolates was assessed for biocidal and PGP traits. Functionally rhizospheric Bts were broadly superior than commercial Bts. Virulence of the Bts varied against rice leaf folder (LF, Cnaphalocrocis medinalis) and stripe stem borer (SSB, Chilo suppresalis) larvae in laboratory, net house and field tests. Drosophila diet (DD) incorporation, cut leaf and field assays proved virulence of 5-9 Bt isolates against LF larvae with LC₅₀s 1.99 - 6.31 x 10⁸, 2.18 x 10⁶ - 2.25 x 10⁹ and 3.16 x 10⁶ – 1.25 x 10⁹ bacteria-spore-crystal (BSC)/ml, respectively, and TB261 was most (LC₅₀s 2.18 x 10⁶ – 3.98 x 10⁸ BSC/ml) infective. DD and cut stem assays for SSB proved virulence of 5 and 6 Bts with LC₅₀s 9.20 x 10⁶ - 3.62 x 10⁸ and 9.21 x 10⁶- 3.24 x 10⁸ BSC/ml, respectively, and maximum (LC₅₀s 9.20 – 9.21 x 10⁸ BSC/ml) infectivity of TB263. Eight Bts inhibited 1-4 out of 7 rice pathogens and 16 Bts antagonized 1-4 out of 9 entomopathogenic fungi. Biocidal principles of the Bts were cell wall/membrane hydrolyzing exoenzymes, toxin/inhibitors and crystal toxins. Furthermore, the Bts were also inhibited by 3 insecticides and 2 fungicides. The Bts possessed 1-4 PGP and phytostimulation traits also. The potent rhizospheric Bt can be prospected for overall improvement/sustenance of rice.

Functional diversification of five superoxide dismutase genes in Aspergillus nidulans against oxidative stress: distinct cellular roles of SodA and SodB

Superoxide dismutases (SODs) play crucial roles in protecting cells against oxidative stress by catalyzing the dismutation of superoxide radicals. In Aspergillus nidulans, five putative SOD genes have been predicted in the genome; however, their comparative expression profiles and physiological functions remain largely uncharacterized. In this study, we analyzed the expression levels of all five SOD genes at different growth stages and examined the oxidative stress sensitivity of corresponding gene-disrupted strains. We found that sodA exhibited high and constitutive expression across all growth stages, while sodB was predominantly expressed in conidia (asexual spores). Disruption mutants of sodA and sodB showed increased sensitivity to oxidative agents, confirming their functional importance. Subcellular fractionation and SOD activity assays revealed that SodA was localized in the cytoplasm, whereas SodB was primarily localized in mitochondria. These results highlight the growth stage-specific expression and distinct cellular roles of SodA and SodB in A. nidulans, providing novel insights into the oxidative stress defense system in filamentous fungi.

Superoxide dismutase SodB is essential for growth on non-fermentable carbon sources and conidiation under mitochondrial stress in Aspergillus nidulans

Superoxide dismutases (SODs) play crucial roles in cellular oxidative stress defense. In Aspergillus nidulans, SodB is a mitochondria-localized SOD whose physiological function remains poorly understood. Here, we show that a ΔsodB mutant displays impaired growth on non-fermentable carbon sources including acetate, ethanol, threonine, and Tween 20/80, suggesting compromised mitochondrial function. Oxygen consumption assays using an extracellular oxygen consumption reagent revealed a ~50% reduction in respiratory activity in the ΔsodB strain compared to the wild type. When mitochondrial respiration was inhibited by Antimycin A or salicylhydroxamic acid, giant colony growth was equally suppressed across wild-type, ΔsodA, ΔsodB, and complemented strains. However, conidial production was significantly reduced in ΔsodB under Antimycin treatment, and morphological abnormalities in conidiophore heads were observed under this condition. These results indicate that SodB is not only involved in mitochondrial respiration but also required for maintaining normal sporulation under mitochondrial stress conditions. This study provides new insights into the role of mitochondrial ROS defense systems in filamentous fungal development.

Characterization of bacterial bioluminescence using a large liquid culture of Photobacterium kishitanii KH-2005

At the 2025 Osaka/Kansai Expo, a bacterial-bioluminescence-based lighting system, called BIOLIGHT, was exhibited. It consists of 80 liters of liquid culture medium and produces enough brightness to illuminate a room. In this study, to make clear the relationship between the liquid culture thickness and the brightness using BIOLIGHT, the world's largest liquid culture aquarium of bioluminescent bacteria, we investigated the brightness of the bacterial liquid culture in relation to optical density (OD). The theoretical brightness of BIOLIGHT was calculated using the transmittance of the liquid culture at 475 nm (the peak luminescence wavelength) derived from the measured OD and was then compared with the brightness actually measured. The calculated (theoretical) brightness was lower than the measured one, suggesting that the light output of BIOLIGHT is influenced not only by cell-induced light shielding but also by another factor, presumably forward scattering. Additionally, depth-dependent brightness measurements showed that brightness became saturated at a liquid culture thickness greater than 7 cm. These findings will contribute to the design of future lighting solutions using bacterial bioluminescence.

Anti-Cancer Activity of Methionine gamma-lyase Isolated from Mucor irregularis PQ344458 Against Cervical Adenocarcinoma HeLa Cells and Pleural Lymphoma U937 Cells

Methionine gamma-lyase enzyme was isolated and purified from Mucor irregularis PQ344458 fungal isolates, that obtained from plant root, the isolates were identified through observation of their colony morphological features, implementation of PCR and DNA sequencing via sanger-chain termination approach, then data of DNA sequence alignment, phylogenetic tree, percent identity was generated. Through implementation of several stages that involved using of ion-exchange chromatography, gel-filtration chromatography, ammonium sulphate, enzyme isolation and purification stages were accomplished. The enzyme extract then, was analyzed for its protein content, specific activity and Impact of pH, temperature, inhibitors and activators on its kinetics. Additionally, MTT and DPPH radical scavenging assays were carried-out to reveal information about anti-cancer and anti-oxidant activities of methionine gamma-lyase enzyme. MTT assay results of %viable cells were 15% for HeLa cells and 6.6% for U937 cells at maximum concentration of the enzyme extract. Moreover, DPPH scavenging activity results were 82% at maximum concentration.

Effects of cloned murE gene for peptidoglycan synthesis on morphology and amino acid composition of peptidoglycan of Escherichia coli

In the biosynthesis of peptidoglycan (PG), murE protein (MurE) adds a diamino acid at position 3 of the peptide chain of peptidoglycan. The diamino acid that is added by MurE and makes cross-linkage with adjacent peptide chain differs depending on the bacterial species: Gram-negative bacteria add meso-diaminopimelic acid (DAP), while most Gram-positive bacteria add L-lysine (Lys). In this study, the murE gene of Levilactobacillus brevis that transfers Lys in PG synthesis was cloned into Escherichia coli that has DAP-type PG. The transformant cells harboring L. brevis murE showed reduction of colony forming units during cultivation, and were elongated or burst when murE was expressed. Amino acid analysis of solubilized PG revealed that the Lys/DAP ratio increased in the PG of the transformants. Interestingly, aspartic acid that is responsible for the formation of cross-linkages between Lys and other peptide chain in the PG of L. brevis also increased, suggesting that Lys-type PG with Asp cross-linkage was partially formed by the cloning of murE gene.

Mechanosensitive channels are versatile exporters in microbial cell factories

The extracellular export of target chemicals is essential for achieving the target productivity of microbial cell factories (MCFs). We demonstrated that MscCG, a mechanosensitive channel responsible for glutamate export in glutamate-producing MCF of Corynebaterium glutamicum, can export various intracellular low-molecular-weight chemicals outside the cell. The mechanosensitive channels exporter improved L-Lys productivity and conferred substantial 5′-IMP fermentative production ability to the Escherichia coli MCF, which lacks inherent 5′-IMP exporters, indicating that mechanosensitive channels, which are low selective, functioned effectively as MCF exporters. We also demonstrated the effectiveness of a gain-of-function (GOF) mutation of mechanosensitive channels as MCF exporters; however, the essential mechanism underlying this GOF mutation remains unknown. Therefore, we performed molecular dynamics simulations to identify this mechanism at the atomic level. Consequently, we partially elucidated the underlying mechanism of G46D-induced GOF in MscL, which was effective as a 5′-IMP exporter. Specifically, the kink at A38 in the inner transmembrane helix of MscL forming its pore can affect GOF behavior. Based on these results, we conclude that mechanosensitive channels have potential as innovative and versatile exporters of MCFs, capable of enhancing the production efficiency of target chemicals and enabling their production in the absence of natural exporters.

Characterization of the acylglycerolphosphate acyltransferase in Actinoplanes missouriensis

Actinoplanes missouriensis grows by forming branched substrate mycelia and produces terminal sporangia. Each sporangium contains a few hundred spores, which swim as zoospores after being released from sporangia. Previously, we disrupted 22 putative acyltransferase genes and examined their involvement in morphological differentiation. Here, we described the characterization of one of them, a putative 1-acyl-2-hydroxy-sn-glycerol-3-phosphate acyltransferase (AGPAT) encoded by plsC (AMIS_11360). The plsC null (∆plsC) mutant exhibited a conditional growth defect in a nutrient-poor medium. No differences were observed between the wild-type and ∆plsC strains in sporangium formation, spore release, or zoospore motility. We confirmed the AGPAT activity of PlsC; the recombinant polyhistidine-tagged PlsC protein transferred the acyl group from palmitoyl-coenzyme A to 1-palmitoyl-2-hydroxy-sn-glycero-3-phosphate, resulting in the production of 1,2-dipalmitoyl-sn-glycero-3-phosphate.

Diverse fungal communities in commercial karebushi produced with or without a starter culture

We investigated the effect of a starter culture on the fungal communities of commercial karebushi. Aspergillus pseudoglaucus was initially identified as the starter fungus. In karebushi samples from two manufacturers relying on naturally occurring molds, Aspergillus chevalieri was the dominant species, accompanied by Aspergillus montevidensis and Aspergillus sydowii, while A. pseudoglaucus was not detected. Among samples from six manufacturers that used the starter culture, A. pseudoglaucus was dominant in only three; in the remaining three, A. chevalieri predominated despite the starter being used. These results suggest that indigenous fungi, particularly A. chevalieri, present in the processing environment can outcompete the starter culture, influence the fungal community, and potentially contribute to the qualitative diversity of karebushi.