Highlights d A deep learning model is trained to predict antibiotics based on structure d Halicin is predicted as an antibacterial molecule from the Drug Repurposing Hub d Halicin shows broad-spectrum antibiotic activities in mice d More antibiotics with distinct structures are predicted from the ZINC15 database
SummaryPlasmodium gene functions in mosquito and liver stages remain poorly characterized due to limitations in the throughput of phenotyping at these stages. To fill this gap, we followed more than 1,300 barcoded P. berghei mutants through the life cycle. We discover 461 genes required for efficient parasite transmission to mosquitoes through the liver stage and back into the bloodstream of mice. We analyze the screen in the context of genomic, transcriptomic, and metabolomic data by building a thermodynamic model of P. berghei liver-stage metabolism, which shows a major reprogramming of parasite metabolism to achieve rapid growth in the liver. We identify seven metabolic subsystems that become essential at the liver stages compared with asexual blood stages: type II fatty acid synthesis and elongation (FAE), tricarboxylic acid, amino sugar, heme, lipoate, and shikimate metabolism. Selected predictions from the model are individually validated in single mutants to provide future targets for drug development.
Highlights d We present a metabolic model for T. gondii harmonized with experimental fitness scores d T. gondii can tolerate the loss of fatty acid biosynthesis with FA supplementation d Biosynthesis of Vitamin B6 is essential in vivo and is a potential drug target d Heme biosynthesis is essential for parasite survival
Novel antimalarial therapies are urgently needed for the fight against drug-resistant parasites. The metabolism of malaria parasites in infected cells is an attractive source of drug targets but is rather complex. Computational methods can handle this complexity and allow integrative analyses of cell metabolism. In this study, we present a genome-scale metabolic model (iPfa) of the deadliest malaria parasite, Plasmodium falciparum, and its thermodynamics-based flux analysis (TFA). Using previous absolute concentration data of the intraerythrocytic parasite, we applied TFA to iPfa and predicted up to 63 essential genes and 26 essential pairs of genes. Of the 63 genes, 35 have been experimentally validated and reported in the literature, and 28 have not been experimentally tested and include previously hypothesized or novel predictions of essential metabolic capabilities. Without metabolomics data, four of the genes would have been incorrectly predicted to be non-essential. TFA also indicated that substrate channeling should exist in two metabolic pathways to ensure the thermodynamic feasibility of the flux. Finally, analysis of the metabolic capabilities of P. falciparum led to the identification of both the minimal nutritional requirements and the genes that can become indispensable upon substrate inaccessibility. This model provides novel insight into the metabolic needs and capabilities of the malaria parasite and highlights metabolites and pathways that should be measured and characterized to identify potential thermodynamic bottlenecks and substrate channeling. The hypotheses presented seek to guide experimental studies to facilitate a better understanding of the parasite metabolism and the identification of targets for more efficient intervention.
Understanding the adaptive responses of individual bacterial strains is crucial for microbiome engineering approaches that introduce new functionalities into complex microbiomes, such as xenobiotic compound metabolism for soil bioremediation. Adaptation requires metabolic reprogramming of the cell, which can be captured by multi-omics, but this data remains formidably challenging to interpret and predict. Here we present a new approach that combines genome-scale metabolic modeling with transcriptomics and exometabolomics, both of which are common tools for studying dynamic population behavior. As a realistic demonstration, we developed a genome-scale model of Pseudomonas veronii 1YdBTEX2, a candidate bioaugmentation agent for accelerated metabolism of mono-aromatic compounds in soil microbiomes, while simultaneously collecting experimental data of P. veronii metabolism during growth phase transitions. Predictions of the P. veronii growth rates and specific metabolic processes from the integrated model closely matched experimental observations. We conclude that integrative and network-based analysis can help build predictive models that accurately capture bacterial adaptation responses. Further development and testing of such models may considerably improve the successful establishment of bacterial inoculants in more complex systems.npj Systems Biology and Applications (2020) 6:1 ; https://doi.
A large number of genome-scale models of cellular metabolism are available for various organisms. These models include all known metabolic reactions based on the genome annotation. However, the reactions that are active are dependent on the cellular metabolic function or environmental condition. Constraint-based methods that integrate condition-specific transcriptomics data into models have been used extensively to investigate condition-specific metabolism. Here, we present a method (TEX-FBA) for modeling condition-specific metabolism that combines transcriptomics and reaction thermodynamics data to generate a thermodynamically-feasible condition-specific metabolic model. TEX-FBA is an extension of thermodynamic-based flux balance analysis (TFA), which allows the simultaneous integration of different stages of experimental data (e.g., absolute gene expression, metabolite concentrations, thermodynamic data, and fluxomics) and the identification of alternative metabolic states that maximize consistency between gene expression levels and condition-specific reaction fluxes. We applied TEX-FBA to a genome-scale metabolic model of Escherichia coli by integrating available condition-specific experimental data and found a marked reduction in the flux solution space. Our analysis revealed a marked correlation between actual gene expression profile and experimental flux measurements compared to the one obtained from a randomly generated gene expression profile. We identified additional essential reactions from the membrane lipid and folate metabolism when we integrated transcriptomics data of the given condition on the top of metabolomics and thermodynamics data. These results show TEX-FBA is a promising new approach to study condition-specific metabolism when different types of experimental data are available.Author summaryCells utilize nutrients via biochemical reactions that are controlled by enzymes and synthesize required compounds for their survival and growth. Genome-scale models of metabolism representing these complex reaction networks have been reconstructed for a wide variety of organisms ranging from bacteria to human cells. These models comprise all possible biochemical reactions in a cell, but cells choose only a subset of reactions for their immediate needs and functions. Usually, these models allow for a large flux solution space and one can integrate experimental data in order to reduce it and potentially predict the physiology for a specific condition. We developed a method for integrating different types of omics data, such as fluxomics, transcriptomics, metabolomics into genome-scale metabolic models that reduces the flux solution space. Using gene expression data, the algorithm maximizes the consistency between the predicted and experimental flux for the reactions and predicts biologically relevant flux ranges for the remaining reactions in the network. This method is useful for determining fluxes of metabolic reactions with reduced uncertainty and suitable for performing context- and condition-specific analysis in metabolic models using different types of experimental data.
Advances in medicine and biotechnology rely on a deep understanding of biological processes. Despite the increasingly available types and amounts of omics data, significant knowledge gaps remain, with current approaches to identify and curate missing annotations being limited to a set of already known reactions. Here, we introduce N etwork I ntegrated C omputational E xplorer for G ap A nnotation of Me tabolism (NICEgame), a workflow to identify and curate nonannotated metabolic functions in genomes using the ATLAS of Biochemistry and genome-scale metabolic models (GEMs). To resolve gaps in GEMs, NICEgame provides alternative sets of known and hypothetical reactions, assesses their thermodynamic feasibility, and suggests candidate genes to catalyze these reactions. We identified metabolic gaps and applied NICEgame in the latest GEM of Escherichia coli , iML1515, and enhanced the E. coli genome annotation by resolving 47% of these gaps. NICEgame, applicable to any GEM and functioning from open-source software, should thus enhance all GEM-based predictions and subsequent biotechnological and biomedical applications.
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