Your search keyword '"Operon"' showing total 250 results

1. Comprehensive Characterization of fucAO Operon Activation in Escherichia coli

Author

Zhang, Zhongge, Zhang, Zhongge, Huo, Jialu, Velo, Juan, Zhou, Harry, Flaherty, Alex, Saier, Milton H, Zhang, Zhongge, Zhang, Zhongge, Huo, Jialu, Velo, Juan, Zhou, Harry, Flaherty, Alex, and Saier, Milton H

Abstract

Wildtype Escherichia coli cells cannot grow on L-1,2-propanediol, as the fucAO operon within the fucose (fuc) regulon is thought to be silent in the absence of L-fucose. Little information is available concerning the transcriptional regulation of this operon. Here, we first confirm that fucAO operon expression is highly inducible by fucose and is primarily attributable to the upstream operon promoter, while the fucO promoter within the 3'-end of fucA is weak and uninducible. Using 5'RACE, we identify the actual transcriptional start site (TSS) of the main fucAO operon promoter, refuting the originally proposed TSS. Several lines of evidence are provided showing that the fucAO locus is within a transcriptionally repressed region on the chromosome. Operon activation is dependent on FucR and Crp but not SrsR. Two Crp-cAMP binding sites previously found in the regulatory region are validated, where the upstream site plays a more critical role than the downstream site in operon activation. Furthermore, two FucR binding sites are identified, where the downstream site near the first Crp site is more important than the upstream site. Operon transcription relies on Crp-cAMP to a greater degree than on FucR. Our data strongly suggest that FucR mainly functions to facilitate the binding of Crp to its upstream site, which in turn activates the fucAO promoter by efficiently recruiting RNA polymerase.

Published

2024

2. SatR Is a Repressor of Fluoroquinolone Efflux Pump SatAB

Author

San Millán, Álvaro, Gutierrez, Belén, Martínez Ovejero, Cristina, Carrilero, Laura, Escudero García-Calderón, José Antonio, Montero Serra, Natalia, González Zorn, Bruno, San Millán, Álvaro, Gutierrez, Belén, Martínez Ovejero, Cristina, Carrilero, Laura, Escudero García-Calderón, José Antonio, Montero Serra, Natalia, and González Zorn, Bruno

Abstract

Streptococcus suis is an emerging zoonotic agent responsible for high-mortality outbreaks among the human population in China. In this species, the ABC transporter SatAB mediates fluoroquinolone resistance when overexpressed. Here, we describe and characterize satR, an open reading frame (ORF) encoding a MarR superfamily regulator that acts as a repressor of satAB. satR is cotranscribed with satAB, and its interruption entails the overexpression of the pump, leading to a clinically relevant in- crease in resistance to fluoroquinolones., Universidad Complutense de Madrid, Ministerio de Ciencia e Innovación, Comunidad de Madrid, Depto. de Sanidad Animal, Fac. de Veterinaria, TRUE, pub

Published

2024

3. A systems approach discovers the role and characteristics of seven LysR type transcription factors in Escherichia coli.

Author

Rodionova, Irina A, Rodionova, Irina A, Gao, Ye, Monk, Jonathan, Hefner, Ying, Wong, Nicholas, Szubin, Richard, Lim, Hyun Gyu, Rodionov, Dmitry A, Zhang, Zhongge, Saier, Milton H, Palsson, Bernhard O, Rodionova, Irina A, Rodionova, Irina A, Gao, Ye, Monk, Jonathan, Hefner, Ying, Wong, Nicholas, Szubin, Richard, Lim, Hyun Gyu, Rodionov, Dmitry A, Zhang, Zhongge, Saier, Milton H, and Palsson, Bernhard O

Abstract

Although Escherichia coli K-12 strains represent perhaps the best known model bacteria, we do not know the identity or functions of all of their transcription factors (TFs). It is now possible to systematically discover the physiological function of TFs in E. coli BW25113 using a set of synergistic methods; including ChIP-exo, growth phenotyping, conserved gene clustering, and transcriptome analysis. Among 47 LysR-type TFs (LTFs) found on the E. coli K-12 genome, many regulate nitrogen source utilization or amino acid metabolism. However, 19 LTFs remain unknown. In this study, we elucidated the regulation of seven of these 19 LTFs: YbdO, YbeF, YcaN, YbhD, YgfI, YiaU, YneJ. We show that: (1) YbdO (tentatively re-named CitR) regulation has an effect on bacterial growth at low pH with citrate supplementation. CitR is a repressor of the ybdNM operon and is implicated in the regulation of citrate lyase genes (citCDEFG); (2) YgfI (tentatively re-named DhfA) activates the dhaKLM operon that encodes the phosphotransferase system, DhfA is involved in formate, glycerol and dihydroxyacetone utilization; (3) YiaU (tentatively re-named LpsR) regulates the yiaT gene encoding an outer membrane protein, and waaPSBOJYZU operon is also important in determining cell density at the stationary phase and resistance to oxacillin microaerobically; (4) YneJ, re-named here as PtrR, directly regulates the expression of the succinate-semialdehyde dehydrogenase, Sad (also known as YneI), and is a predicted regulator of fnrS (a small RNA molecule). PtrR is important for bacterial growth in the presence of L-glutamate and putrescine as nitrogen/energy sources; and (5) YbhD and YcaN regulate adjacent y-genes on the genome. We have thus established the functions for four LTFs and identified the target genes for three LTFs.

Published

2022

4. Identifying candidate structured RNAs in CRISPR operons.

Author

Fremin, Brayon J, Fremin, Brayon J, Kyrpides, Nikos C, Fremin, Brayon J, Fremin, Brayon J, and Kyrpides, Nikos C

Abstract

Noncoding RNAs with secondary structures play important roles in CRISPR-Cas systems. Many of these structures likely remain undiscovered. We used a large-scale comparative genomics approach to predict 156 novel candidate structured RNAs from 36,111 CRISPR-Cas systems. A number of these were found to overlap with coding genes, including palindromic candidates that overlapped with a variety of Cas genes in type I and III systems. Among these 156 candidates, we identified 46 new models of CRISPR direct repeats and 1 tracrRNA. This tracrRNA model occasionally overlapped with predicted cas9 coding regions, emphasizing the importance of expanding our search windows for novel structure RNAs in coding regions. We also demonstrated that the antirepeat sequence in this tracrRNA model can be used to accurately assign thousands of predicted CRISPR arrays to type II-C systems. This study highlights the importance of unbiased identification of candidate structured RNAs across CRISPR-Cas systems.

Published

2022

5. Understanding the Formation and Mechanism of Anticipatory Responses in Escherichia coli.

Author

Rai, Navneet, Rai, Navneet, Kim, Minseung, Tagkopoulos, Ilias, Rai, Navneet, Rai, Navneet, Kim, Minseung, and Tagkopoulos, Ilias

Abstract

Microorganisms often live in complex habitats, where changes in the environment are predictable, providing an opportunity for microorganisms to learn, anticipate the upcoming environmental changes and prepare in advance for better survival and growth. One such environment is the mammalian intestine, where the abundance of different carbon sources is spatially distributed. In this study, we identified seven spatially distributed carbon sources in the mammalian intestine and tested whether Escherichia coli exhibits phenotypes that are consistent with an anticipatory response given their spatial order and abundance within the mammalian intestine. Through RNA-Seq and RT-PCR validation measurements, we found that there was a 67% match in the expression patterns between the measured phenotypes and what would otherwise be expected in the case of anticipatory behavior, while 83% and 0% were in agreement with the homeostatic and random response, respectively. To understand the genetic and phenotypic basis of the discrepancies between the expected and measured anticipatory responses, we thoroughly investigated the discrepancy in D-galactose treatment and the expression of maltose operon in E. coli. Here, the expected anticipatory response, based on the spatial distribution of D-galactose and D-maltose, was that D-galactose should upregulate the maltose operon, but it was the opposite in experimental validation. We performed whole genome random mutagenesis and screening and identified E. coli strains with positive expression of maltose operon in D-galactose. Targeted Sanger sequencing and mutation repair identified that the mutations in the promoter region of malT and in the coding region of the crp gene were the factors responsible for the reversion in the association. Further, to identify why positive association in the D-galactose treatment and the expression of the maltose operon did not evolve naturally, fitness measurements were performed. Fitness experiments demonstrate

Published

2022

6. A systems approach discovers the role and characteristics of seven LysR type transcription factors in Escherichia coli.

Author

Rodionova, Irina A, Rodionova, Irina A, Gao, Ye, Monk, Jonathan, Hefner, Ying, Wong, Nicholas, Szubin, Richard, Lim, Hyun Gyu, Rodionov, Dmitry A, Zhang, Zhongge, Saier, Milton H, Palsson, Bernhard O, Rodionova, Irina A, Rodionova, Irina A, Gao, Ye, Monk, Jonathan, Hefner, Ying, Wong, Nicholas, Szubin, Richard, Lim, Hyun Gyu, Rodionov, Dmitry A, Zhang, Zhongge, Saier, Milton H, and Palsson, Bernhard O

Abstract

Although Escherichia coli K-12 strains represent perhaps the best known model bacteria, we do not know the identity or functions of all of their transcription factors (TFs). It is now possible to systematically discover the physiological function of TFs in E. coli BW25113 using a set of synergistic methods; including ChIP-exo, growth phenotyping, conserved gene clustering, and transcriptome analysis. Among 47 LysR-type TFs (LTFs) found on the E. coli K-12 genome, many regulate nitrogen source utilization or amino acid metabolism. However, 19 LTFs remain unknown. In this study, we elucidated the regulation of seven of these 19 LTFs: YbdO, YbeF, YcaN, YbhD, YgfI, YiaU, YneJ. We show that: (1) YbdO (tentatively re-named CitR) regulation has an effect on bacterial growth at low pH with citrate supplementation. CitR is a repressor of the ybdNM operon and is implicated in the regulation of citrate lyase genes (citCDEFG); (2) YgfI (tentatively re-named DhfA) activates the dhaKLM operon that encodes the phosphotransferase system, DhfA is involved in formate, glycerol and dihydroxyacetone utilization; (3) YiaU (tentatively re-named LpsR) regulates the yiaT gene encoding an outer membrane protein, and waaPSBOJYZU operon is also important in determining cell density at the stationary phase and resistance to oxacillin microaerobically; (4) YneJ, re-named here as PtrR, directly regulates the expression of the succinate-semialdehyde dehydrogenase, Sad (also known as YneI), and is a predicted regulator of fnrS (a small RNA molecule). PtrR is important for bacterial growth in the presence of L-glutamate and putrescine as nitrogen/energy sources; and (5) YbhD and YcaN regulate adjacent y-genes on the genome. We have thus established the functions for four LTFs and identified the target genes for three LTFs.

Published

2022

7. Understanding the Formation and Mechanism of Anticipatory Responses in Escherichia coli.

Author

Rai, Navneet, Rai, Navneet, Kim, Minseung, Tagkopoulos, Ilias, Rai, Navneet, Rai, Navneet, Kim, Minseung, and Tagkopoulos, Ilias

Abstract

Microorganisms often live in complex habitats, where changes in the environment are predictable, providing an opportunity for microorganisms to learn, anticipate the upcoming environmental changes and prepare in advance for better survival and growth. One such environment is the mammalian intestine, where the abundance of different carbon sources is spatially distributed. In this study, we identified seven spatially distributed carbon sources in the mammalian intestine and tested whether Escherichia coli exhibits phenotypes that are consistent with an anticipatory response given their spatial order and abundance within the mammalian intestine. Through RNA-Seq and RT-PCR validation measurements, we found that there was a 67% match in the expression patterns between the measured phenotypes and what would otherwise be expected in the case of anticipatory behavior, while 83% and 0% were in agreement with the homeostatic and random response, respectively. To understand the genetic and phenotypic basis of the discrepancies between the expected and measured anticipatory responses, we thoroughly investigated the discrepancy in D-galactose treatment and the expression of maltose operon in E. coli. Here, the expected anticipatory response, based on the spatial distribution of D-galactose and D-maltose, was that D-galactose should upregulate the maltose operon, but it was the opposite in experimental validation. We performed whole genome random mutagenesis and screening and identified E. coli strains with positive expression of maltose operon in D-galactose. Targeted Sanger sequencing and mutation repair identified that the mutations in the promoter region of malT and in the coding region of the crp gene were the factors responsible for the reversion in the association. Further, to identify why positive association in the D-galactose treatment and the expression of the maltose operon did not evolve naturally, fitness measurements were performed. Fitness experiments demonstrate

Published

2022

8. Identifying candidate structured RNAs in CRISPR operons.

Author

Fremin, Brayon J, Fremin, Brayon J, Kyrpides, Nikos C, Fremin, Brayon J, Fremin, Brayon J, and Kyrpides, Nikos C

Abstract

Noncoding RNAs with secondary structures play important roles in CRISPR-Cas systems. Many of these structures likely remain undiscovered. We used a large-scale comparative genomics approach to predict 156 novel candidate structured RNAs from 36,111 CRISPR-Cas systems. A number of these were found to overlap with coding genes, including palindromic candidates that overlapped with a variety of Cas genes in type I and III systems. Among these 156 candidates, we identified 46 new models of CRISPR direct repeats and 1 tracrRNA. This tracrRNA model occasionally overlapped with predicted cas9 coding regions, emphasizing the importance of expanding our search windows for novel structure RNAs in coding regions. We also demonstrated that the antirepeat sequence in this tracrRNA model can be used to accurately assign thousands of predicted CRISPR arrays to type II-C systems. This study highlights the importance of unbiased identification of candidate structured RNAs across CRISPR-Cas systems.

Published

2022

9. Short- and long-read metabarcoding of the eukaryotic rRNA operon : Evaluation of primers and comparison to shotgun metagenomics sequencing

Author

Latz, Meike, Grujcic, Vesna, Brugel, S., Lycken, J., John, U., Karlson, B., Andersson, A., Andersson, Anders F., Latz, Meike, Grujcic, Vesna, Brugel, S., Lycken, J., John, U., Karlson, B., Andersson, A., and Andersson, Anders F.

Abstract

High-throughput sequencing-based analysis of microbial diversity has evolved vastly over the last decade. Currently, the go-to method for studying microbial eukaryotes is short-read metabarcoding of variable regions of the 18S rRNA gene with <500 bp amplicons. However, there is a growing interest in applying long-read sequencing of amplicons covering the rRNA operon for improving taxonomic resolution. For both methods, the choice of primers is crucial. It determines if community members are covered, if they can be identified at a satisfactory taxonomic level, and if the obtained community profile is representative. Here, we designed new primers targeting 18S and 28S rRNA based on 177,934 and 21,072 database sequences, respectively. The primers were evaluated in silico along with published primers on reference sequence databases and marine metagenomics data sets. We further evaluated a subset of the primers for short- and long-read sequencing on environmental samples in vitro and compared the obtained community profile with primer-unbiased metagenomic sequencing. Of the short-read pairs, a new V6-V8 pair and the V4_Balzano pair used with a simplified PCR protocol provided good results in silico and in vitro. Fewer differences were observed between the long-read primer pairs. The long-read amplicons and ITS1 alone provided higher taxonomic resolution than V4. Together, our results represent a reference and guide for selection of robust primers for research on and environmental monitoring of microbial eukaryotes., QC 20230206

Published

2022

10. A phage satellite tunes inducing phage gene expression using a domesticated endonuclease to balance inhibition and virion hijacking.

Author

Netter, Zoe, Netter, Zoe, Boyd, Caroline M, Silvas, Tania V, Seed, Kimberley D, Netter, Zoe, Netter, Zoe, Boyd, Caroline M, Silvas, Tania V, and Seed, Kimberley D

Abstract

Bacteria persist under constant threat of predation by bacterial viruses (phages). Bacteria-phage conflicts result in evolutionary arms races often driven by mobile genetic elements (MGEs). One such MGE, a phage satellite in Vibrio cholerae called PLE, provides specific and robust defense against a pervasive lytic phage, ICP1. The interplay between PLE and ICP1 has revealed strategies for molecular parasitism allowing PLE to hijack ICP1 processes in order to mobilize. Here, we describe the mechanism of PLE-mediated transcriptional manipulation of ICP1 structural gene transcription. PLE encodes a novel DNA binding protein, CapR, that represses ICP1's capsid morphogenesis operon. Although CapR is sufficient for the degree of capsid repression achieved by PLE, its activity does not hinder the ICP1 lifecycle. We explore the consequences of repression of this operon, demonstrating that more stringent repression achieved through CRISPRi restricts both ICP1 and PLE. We also discover that PLE transduces in modified ICP1-like particles. Examination of CapR homologs led to the identification of a suite of ICP1-encoded homing endonucleases, providing a putative origin for the satellite-encoded repressor. This work unveils a facet of the delicate balance of satellite-mediated inhibition aimed at blocking phage production while successfully mobilizing in a phage-derived particle.

Published

2021

11. A phage satellite tunes inducing phage gene expression using a domesticated endonuclease to balance inhibition and virion hijacking.

Author

Netter, Zoe, Netter, Zoe, Boyd, Caroline M, Silvas, Tania V, Seed, Kimberley D, Netter, Zoe, Netter, Zoe, Boyd, Caroline M, Silvas, Tania V, and Seed, Kimberley D

Abstract

Bacteria persist under constant threat of predation by bacterial viruses (phages). Bacteria-phage conflicts result in evolutionary arms races often driven by mobile genetic elements (MGEs). One such MGE, a phage satellite in Vibrio cholerae called PLE, provides specific and robust defense against a pervasive lytic phage, ICP1. The interplay between PLE and ICP1 has revealed strategies for molecular parasitism allowing PLE to hijack ICP1 processes in order to mobilize. Here, we describe the mechanism of PLE-mediated transcriptional manipulation of ICP1 structural gene transcription. PLE encodes a novel DNA binding protein, CapR, that represses ICP1's capsid morphogenesis operon. Although CapR is sufficient for the degree of capsid repression achieved by PLE, its activity does not hinder the ICP1 lifecycle. We explore the consequences of repression of this operon, demonstrating that more stringent repression achieved through CRISPRi restricts both ICP1 and PLE. We also discover that PLE transduces in modified ICP1-like particles. Examination of CapR homologs led to the identification of a suite of ICP1-encoded homing endonucleases, providing a putative origin for the satellite-encoded repressor. This work unveils a facet of the delicate balance of satellite-mediated inhibition aimed at blocking phage production while successfully mobilizing in a phage-derived particle.

Published

2021

12. Asymmetric localization of the cell division machinery during Bacillus subtilis sporulation.

Author

Khanna, Kanika, Khanna, Kanika, Lopez-Garrido, Javier, Sugie, Joseph, Pogliano, Kit, Villa, Elizabeth, Khanna, Kanika, Khanna, Kanika, Lopez-Garrido, Javier, Sugie, Joseph, Pogliano, Kit, and Villa, Elizabeth

Abstract

The Gram-positive bacterium Bacillus subtilis can divide via two modes. During vegetative growth, the division septum is formed at the midcell to produce two equal daughter cells. However, during sporulation, the division septum is formed closer to one pole to yield a smaller forespore and a larger mother cell. Using cryo-electron tomography, genetics and fluorescence microscopy, we found that the organization of the division machinery is different in the two septa. While FtsAZ filaments, the major orchestrators of bacterial cell division, are present uniformly around the leading edge of the invaginating vegetative septa, they are only present on the mother cell side of the invaginating sporulation septa. We provide evidence suggesting that the different distribution and number of FtsAZ filaments impact septal thickness, causing vegetative septa to be thicker than sporulation septa already during constriction. Finally, we show that a sporulation-specific protein, SpoIIE, regulates asymmetric divisome localization and septal thickness during sporulation.

Published

2021

13. A phage satellite tunes inducing phage gene expression using a domesticated endonuclease to balance inhibition and virion hijacking.

Author

Netter, Zoe, Netter, Zoe, Boyd, Caroline M, Silvas, Tania V, Seed, Kimberley D, Netter, Zoe, Netter, Zoe, Boyd, Caroline M, Silvas, Tania V, and Seed, Kimberley D

Abstract

Bacteria persist under constant threat of predation by bacterial viruses (phages). Bacteria-phage conflicts result in evolutionary arms races often driven by mobile genetic elements (MGEs). One such MGE, a phage satellite in Vibrio cholerae called PLE, provides specific and robust defense against a pervasive lytic phage, ICP1. The interplay between PLE and ICP1 has revealed strategies for molecular parasitism allowing PLE to hijack ICP1 processes in order to mobilize. Here, we describe the mechanism of PLE-mediated transcriptional manipulation of ICP1 structural gene transcription. PLE encodes a novel DNA binding protein, CapR, that represses ICP1's capsid morphogenesis operon. Although CapR is sufficient for the degree of capsid repression achieved by PLE, its activity does not hinder the ICP1 lifecycle. We explore the consequences of repression of this operon, demonstrating that more stringent repression achieved through CRISPRi restricts both ICP1 and PLE. We also discover that PLE transduces in modified ICP1-like particles. Examination of CapR homologs led to the identification of a suite of ICP1-encoded homing endonucleases, providing a putative origin for the satellite-encoded repressor. This work unveils a facet of the delicate balance of satellite-mediated inhibition aimed at blocking phage production while successfully mobilizing in a phage-derived particle.

Published

2021

14. A method for achieving complete microbial genomes and improving bins from metagenomics data.

Author

Lui, Lauren M, Langille, Morgan1, Lui, Lauren M, Nielsen, Torben N, Arkin, Adam P, Lui, Lauren M, Langille, Morgan1, Lui, Lauren M, Nielsen, Torben N, and Arkin, Adam P

Abstract

Metagenomics facilitates the study of the genetic information from uncultured microbes and complex microbial communities. Assembling complete genomes from metagenomics data is difficult because most samples have high organismal complexity and strain diversity. Some studies have attempted to extract complete bacterial, archaeal, and viral genomes and often focus on species with circular genomes so they can help confirm completeness with circularity. However, less than 100 circularized bacterial and archaeal genomes have been assembled and published from metagenomics data despite the thousands of datasets that are available. Circularized genomes are important for (1) building a reference collection as scaffolds for future assemblies, (2) providing complete gene content of a genome, (3) confirming little or no contamination of a genome, (4) studying the genomic context and synteny of genes, and (5) linking protein coding genes to ribosomal RNA genes to aid metabolic inference in 16S rRNA gene sequencing studies. We developed a semi-automated method called Jorg to help circularize small bacterial, archaeal, and viral genomes using iterative assembly, binning, and read mapping. In addition, this method exposes potential misassemblies from k-mer based assemblies. We chose species of the Candidate Phyla Radiation (CPR) to focus our initial efforts because they have small genomes and are only known to have one ribosomal RNA operon. In addition to 34 circular CPR genomes, we present one circular Margulisbacteria genome, one circular Chloroflexi genome, and two circular megaphage genomes from 19 public and published datasets. We demonstrate findings that would likely be difficult without circularizing genomes, including that ribosomal genes are likely not operonic in the majority of CPR, and that some CPR harbor diverged forms of RNase P RNA. Code and a tutorial for this method is available at https://github.com/lmlui/Jorg and is available on the DOE Systems Biology Knowledge

Published

2021

15. Asymmetric localization of the cell division machinery during Bacillus subtilis sporulation.

Author

Khanna, Kanika, Khanna, Kanika, Lopez-Garrido, Javier, Sugie, Joseph, Pogliano, Kit, Villa, Elizabeth, Khanna, Kanika, Khanna, Kanika, Lopez-Garrido, Javier, Sugie, Joseph, Pogliano, Kit, and Villa, Elizabeth

Abstract

The Gram-positive bacterium Bacillus subtilis can divide via two modes. During vegetative growth, the division septum is formed at the midcell to produce two equal daughter cells. However, during sporulation, the division septum is formed closer to one pole to yield a smaller forespore and a larger mother cell. Using cryo-electron tomography, genetics and fluorescence microscopy, we found that the organization of the division machinery is different in the two septa. While FtsAZ filaments, the major orchestrators of bacterial cell division, are present uniformly around the leading edge of the invaginating vegetative septa, they are only present on the mother cell side of the invaginating sporulation septa. We provide evidence suggesting that the different distribution and number of FtsAZ filaments impact septal thickness, causing vegetative septa to be thicker than sporulation septa already during constriction. Finally, we show that a sporulation-specific protein, SpoIIE, regulates asymmetric divisome localization and septal thickness during sporulation.

Published

2021

16. Exploration of Bacterial Bottlenecks and Streptococcus pneumoniae Pathogenesis by CRISPRi-Seq.

Author

Liu, Xue, Liu, Xue, Kimmey, Jacqueline M, Matarazzo, Laura, de Bakker, Vincent, Van Maele, Laurye, Sirard, Jean-Claude, Nizet, Victor, Veening, Jan-Willem, Liu, Xue, Liu, Xue, Kimmey, Jacqueline M, Matarazzo, Laura, de Bakker, Vincent, Van Maele, Laurye, Sirard, Jean-Claude, Nizet, Victor, and Veening, Jan-Willem

Abstract

Streptococcus pneumoniae is an opportunistic human pathogen that causes invasive diseases, including pneumonia, with greater health risks upon influenza A virus (IAV) co-infection. To facilitate pathogenesis studies in vivo, we developed an inducible CRISPR interference system that enables genome-wide fitness testing in one sequencing step (CRISPRi-seq). We applied CRISPRi-seq to assess bottlenecks and identify pneumococcal genes important in a murine pneumonia model. A critical bottleneck occurs at 48 h with few bacteria causing systemic infection. This bottleneck is not present during IAV superinfection, facilitating identification of pneumococcal pathogenesis-related genes. Top in vivo essential genes included purA, encoding adenylsuccinate synthetase, and the cps operon required for capsule production. Surprisingly, CRISPRi-seq indicated no fitness-related role for pneumolysin during superinfection. Interestingly, although metK (encoding S-adenosylmethionine synthetase) was essential in vitro, it was dispensable in vivo. This highlights advantages of CRISPRi-seq over transposon-based genetic screens, as all genes, including essential genes, can be tested for pathogenesis potential.

Published

2021

17. Spatial control of gene expression in flies using bacterially derived binary transactivation systems.

Author

Gamez, S, Gamez, S, Vesga, LC, Mendez-Sanchez, SC, Akbari, OS, Gamez, S, Gamez, S, Vesga, LC, Mendez-Sanchez, SC, and Akbari, OS

Abstract

Controlling gene expression is an instrumental tool for biotechnology, as it enables the dissection of gene function, affording precise spatial-temporal resolution. To generate this control, binary transactivational systems have been used employing a modular activator consisting of a DNA binding domain(s) fused to activation domain(s). For fly genetics, many binary transactivational systems have been exploited in vivo; however, as the study of complex problems often requires multiple systems that can be used in parallel, there is a need to identify additional bipartite genetic systems. To expand this molecular genetic toolbox, we tested multiple bacterially derived binary transactivational systems in Drosophila melanogaster including the p-CymR operon from Pseudomonas putida, PipR operon from Streptomyces coelicolor, TtgR operon from Pseudomonas putida and the VanR operon from Caulobacter crescentus. Our work provides the first characterization of these systems in an animal model in vivo. For each system, we demonstrate robust tissue-specific spatial transactivation of reporter gene expression, enabling future studies to exploit these transactivational systems for molecular genetic studies.

Published

2021

18. Systematic reconstruction of an effector-gene network reveals determinants of Salmonella cellular and tissue tropism.

Author

Chen, Didi, Chen, Didi, Burford, Wesley B, Pham, Giang, Zhang, Lishu, Alto, Laura T, Ertelt, James M, Winter, Maria G, Winter, Sebastian E, Way, Sing Sing, Alto, Neal M, Chen, Didi, Chen, Didi, Burford, Wesley B, Pham, Giang, Zhang, Lishu, Alto, Laura T, Ertelt, James M, Winter, Maria G, Winter, Sebastian E, Way, Sing Sing, and Alto, Neal M

Abstract

The minimal genetic requirements for microbes to survive within multiorganism communities, including host-pathogen interactions, remain poorly understood. Here, we combined targeted gene mutagenesis with phenotype-guided genetic reassembly to identify a cooperative network of SPI-2 T3SS effector genes that are sufficient for Salmonella Typhimurium (STm) to cause disease in a natural host organism. Five SPI-2 effector genes support pathogen survival within the host cell cytoplasm by coordinating bacterial replication with Salmonella-containing vacuole (SCV) division. Unexpectedly, this minimal genetic repertoire does not support STm systemic infection of mice. In vivo screening revealed a second effector-gene network, encoded by the spv operon, that expands the life cycle of STm from growth in cells to deep-tissue colonization in a murine model of typhoid fever. Comparison between Salmonella infection models suggests how cooperation between effector genes drives tissue tropism in a pathogen group.

Published

2021

19. Adaptations of Escherichia coli strains to oxidative stress are reflected in properties of their structural proteomes.

Author

Mih, Nathan, Mih, Nathan, Monk, Jonathan M, Fang, Xin, Catoiu, Edward, Heckmann, David, Yang, Laurence, Palsson, Bernhard O, Mih, Nathan, Mih, Nathan, Monk, Jonathan M, Fang, Xin, Catoiu, Edward, Heckmann, David, Yang, Laurence, and Palsson, Bernhard O

Abstract

BACKGROUND:The reconstruction of metabolic networks and the three-dimensional coverage of protein structures have reached the genome-scale in the widely studied Escherichia coli K-12 MG1655 strain. The combination of the two leads to the formation of a structural systems biology framework, which we have used to analyze differences between the reactive oxygen species (ROS) sensitivity of the proteomes of sequenced strains of E. coli. As proteins are one of the main targets of oxidative damage, understanding how the genetic changes of different strains of a species relates to its oxidative environment can reveal hypotheses as to why these variations arise and suggest directions of future experimental work. RESULTS:Creating a reference structural proteome for E. coli allows us to comprehensively map genetic changes in 1764 different strains to their locations on 4118 3D protein structures. We use metabolic modeling to predict basal ROS production levels (ROStype) for 695 of these strains, finding that strains with both higher and lower basal levels tend to enrich their proteomes with antioxidative properties, and speculate as to why that is. We computationally assess a strain's sensitivity to an oxidative environment, based on known chemical mechanisms of oxidative damage to protein groups, defined by their localization and functionality. Two general groups - metalloproteins and periplasmic proteins - show enrichment of their antioxidative properties between the 695 strains with a predicted ROStype as well as 116 strains with an assigned pathotype. Specifically, proteins that a) utilize a molybdenum ion as a cofactor and b) are involved in the biogenesis of fimbriae show intriguing protective properties to resist oxidative damage. Overall, these findings indicate that a strain's sensitivity to oxidative damage can be elucidated from the structural proteome, though future experimental work is needed to validate our model assumptions and findings. CONCLUSION:We thus demo

Published

2020

20. The Exploration of Novel Regulatory Relationships Drives Haloarchaeal Operon-Like Structural Dynamics over Short Evolutionary Distances.

Author

Seitzer, Phillip, Seitzer, Phillip, Yao, Andrew I, Cisneros, Ariana, Facciotti, Marc T, Seitzer, Phillip, Seitzer, Phillip, Yao, Andrew I, Cisneros, Ariana, and Facciotti, Marc T

Abstract

Operons are a dominant feature of bacterial and archaeal genome organization. Numerous investigations have related aspects of operon structure to operon function, making operons exemplars for studies aimed at deciphering Nature's design principles for genomic organization at a local scale. We consider this understanding to be both fundamentally important and ultimately useful in the de novo design of increasingly complex synthetic circuits. Here we analyze the evolution of the genomic context of operon-like structures in a set of 76 sequenced and annotated species of halophilic archaea. The phylogenetic depth and breadth of this dataset allows insight into changes in operon-like structures over shorter evolutionary time scales than have been studied in previous cross-species analysis of operon evolution. Our analysis, implemented in the updated software package JContextExplorer finds that operon-like context as measured by changes in structure frequently differs from a sequence divergence model of whole-species phylogeny and that changes seem to be dominated by the exploration of novel regulatory relationships.

Published

2020

21. Genomic characterization of a diazotrophic microbiota associated with maize aerial root mucilage.

Author

Higdon, Shawn M, Higdon, Shawn M, Pozzo, Tania, Kong, Nguyet, Huang, Bihua C, Yang, Mai Lee, Jeannotte, Richard, Brown, C Titus, Bennett, Alan B, Weimer, Bart C, Higdon, Shawn M, Higdon, Shawn M, Pozzo, Tania, Kong, Nguyet, Huang, Bihua C, Yang, Mai Lee, Jeannotte, Richard, Brown, C Titus, Bennett, Alan B, and Weimer, Bart C

Abstract

A geographically isolated maize landrace cultivated on nitrogen-depleted fields without synthetic fertilizer in the Sierra Mixe region of Oaxaca, Mexico utilizes nitrogen derived from the atmosphere and develops an extensive network of mucilage-secreting aerial roots that harbors a diazotrophic (N2-fixing) microbiota. Targeting these diazotrophs, we selected nearly 600 microbes of a collection obtained from mucilage and confirmed their ability to incorporate heavy nitrogen (15N2) metabolites in vitro. Sequencing their genomes and conducting comparative bioinformatic analyses showed that these genomes had substantial phylogenetic diversity. We examined each diazotroph genome for the presence of nif genes essential to nitrogen fixation (nifHDKENB) and carbohydrate utilization genes relevant to the mucilage polysaccharide digestion. These analyses identified diazotrophs that possessed the canonical nif gene operons, as well as many other operon configurations with concomitant fixation and release of >700 different 15N labeled metabolites. We further demonstrated that many diazotrophs possessed alternative nif gene operons and confirmed their genomic potential to derive chemical energy from mucilage polysaccharide to fuel nitrogen fixation. These results confirm that some diazotrophic bacteria associated with Sierra Mixe maize were capable of incorporating atmospheric nitrogen into their small molecule extracellular metabolites through multiple nif gene configurations while others were able to fix nitrogen without the canonical (nifHDKENB) genes.

Published

2020

22. hipBA toxin-antitoxin systems mediate persistence in Caulobacter crescentus.

Author

Huang, Charlie Y, Huang, Charlie Y, Gonzalez-Lopez, Carlos, Henry, Céline, Mijakovic, Ivan, Ryan, Kathleen R, Huang, Charlie Y, Huang, Charlie Y, Gonzalez-Lopez, Carlos, Henry, Céline, Mijakovic, Ivan, and Ryan, Kathleen R

Abstract

Antibiotic persistence is a transient phenotypic state during which a bacterium can withstand otherwise lethal antibiotic exposure or environmental stresses. In Escherichia coli, persistence is promoted by the HipBA toxin-antitoxin system. The HipA toxin functions as a serine/threonine kinase that inhibits cell growth, while the HipB antitoxin neutralizes the toxin. E. coli HipA inactivates the glutamyl-tRNA synthetase GltX, which inhibits translation and triggers the highly conserved stringent response. Although hipBA operons are widespread in bacterial genomes, it is unknown if this mechanism is conserved in other species. Here we describe the functions of three hipBA modules in the alpha-proteobacterium Caulobacter crescentus. The HipA toxins have different effects on growth and macromolecular syntheses, and they phosphorylate distinct substrates. HipA1 and HipA2 contribute to antibiotic persistence during stationary phase by phosphorylating the aminoacyl-tRNA synthetases GltX and TrpS. The stringent response regulator SpoT is required for HipA-mediated antibiotic persistence, but persister cells can form in the absence of all hipBA operons or spoT, indicating that multiple pathways lead to persister cell formation in C. crescentus.

Published

2020

23. Restoration and Modification of Magnetosome Biosynthesis by Internal Gene Acquisition in a Magnetotactic Bacterium.

Author

Arakaki, Atsushi, Arakaki, Atsushi, Goto, Mayu, Maruyama, Mina, Yoda, Takuto, Tanaka, Masayoshi, Yamagishi, Ayana, Yoshikuni, Yasuo, Matsunaga, Tadashi, Arakaki, Atsushi, Arakaki, Atsushi, Goto, Mayu, Maruyama, Mina, Yoda, Takuto, Tanaka, Masayoshi, Yamagishi, Ayana, Yoshikuni, Yasuo, and Matsunaga, Tadashi

Abstract

Integration of a large-sized DNA fragment into a chromosome is an important strategy for characterization of cellular functions in microorganisms. Magnetotactic bacteria synthesize intracellular organelles comprising membrane-bound single crystalline magnetite, also referred to as magnetosomes. Magnetosomes have gained interest in both scientific and engineering sectors as they can be utilized as a material for biomedical and nanotechnological applications. Although genetic engineering of magnetosome biosynthesis mechanism has been investigated, the current method requires cumbersome gene preparation processes. Here, the chromosomal integration of a plasmid containing ≈27 magnetosome genes (≈26 kbp region) in a non-magnetic mutant of Magnetospirillum magneticum AMB-1 using a broad-host-range plasmid is shown. The genome sequencing of gene-complemented strains reveals the chromosomal integration of the plasmid with magnetosome genes at a specific site, most likely by catalysis of an endogenous transposase. Magnetosome production is successfully enhanced by integrating a variation of magnetosome gene operons in the chromosome. This chromosomal integration mechanism will allow the design of functional magnetosomes de novo and M. magneticum AMB-1 may be used as a chassis for the designed magnetosome production.

Published

2020

24. hipBA toxin-antitoxin systems mediate persistence in Caulobacter crescentus.

Author

Huang, Charlie Y, Huang, Charlie Y, Gonzalez-Lopez, Carlos, Henry, Céline, Mijakovic, Ivan, Ryan, Kathleen R, Huang, Charlie Y, Huang, Charlie Y, Gonzalez-Lopez, Carlos, Henry, Céline, Mijakovic, Ivan, and Ryan, Kathleen R

Abstract

Antibiotic persistence is a transient phenotypic state during which a bacterium can withstand otherwise lethal antibiotic exposure or environmental stresses. In Escherichia coli, persistence is promoted by the HipBA toxin-antitoxin system. The HipA toxin functions as a serine/threonine kinase that inhibits cell growth, while the HipB antitoxin neutralizes the toxin. E. coli HipA inactivates the glutamyl-tRNA synthetase GltX, which inhibits translation and triggers the highly conserved stringent response. Although hipBA operons are widespread in bacterial genomes, it is unknown if this mechanism is conserved in other species. Here we describe the functions of three hipBA modules in the alpha-proteobacterium Caulobacter crescentus. The HipA toxins have different effects on growth and macromolecular syntheses, and they phosphorylate distinct substrates. HipA1 and HipA2 contribute to antibiotic persistence during stationary phase by phosphorylating the aminoacyl-tRNA synthetases GltX and TrpS. The stringent response regulator SpoT is required for HipA-mediated antibiotic persistence, but persister cells can form in the absence of all hipBA operons or spoT, indicating that multiple pathways lead to persister cell formation in C. crescentus.

Published

2020

25. Adaptations of Escherichia coli strains to oxidative stress are reflected in properties of their structural proteomes.

Author

Mih, Nathan, Mih, Nathan, Monk, Jonathan M, Fang, Xin, Catoiu, Edward, Heckmann, David, Yang, Laurence, Palsson, Bernhard O, Mih, Nathan, Mih, Nathan, Monk, Jonathan M, Fang, Xin, Catoiu, Edward, Heckmann, David, Yang, Laurence, and Palsson, Bernhard O

Abstract

BACKGROUND:The reconstruction of metabolic networks and the three-dimensional coverage of protein structures have reached the genome-scale in the widely studied Escherichia coli K-12 MG1655 strain. The combination of the two leads to the formation of a structural systems biology framework, which we have used to analyze differences between the reactive oxygen species (ROS) sensitivity of the proteomes of sequenced strains of E. coli. As proteins are one of the main targets of oxidative damage, understanding how the genetic changes of different strains of a species relates to its oxidative environment can reveal hypotheses as to why these variations arise and suggest directions of future experimental work. RESULTS:Creating a reference structural proteome for E. coli allows us to comprehensively map genetic changes in 1764 different strains to their locations on 4118 3D protein structures. We use metabolic modeling to predict basal ROS production levels (ROStype) for 695 of these strains, finding that strains with both higher and lower basal levels tend to enrich their proteomes with antioxidative properties, and speculate as to why that is. We computationally assess a strain's sensitivity to an oxidative environment, based on known chemical mechanisms of oxidative damage to protein groups, defined by their localization and functionality. Two general groups - metalloproteins and periplasmic proteins - show enrichment of their antioxidative properties between the 695 strains with a predicted ROStype as well as 116 strains with an assigned pathotype. Specifically, proteins that a) utilize a molybdenum ion as a cofactor and b) are involved in the biogenesis of fimbriae show intriguing protective properties to resist oxidative damage. Overall, these findings indicate that a strain's sensitivity to oxidative damage can be elucidated from the structural proteome, though future experimental work is needed to validate our model assumptions and findings. CONCLUSION:We thus demo

Published

2020

26. Stochastic ordering of complexoform protein assembly by genetic circuits.

Author

Jensen, Mikkel Herholdt, Faeder, James R1, Jensen, Mikkel Herholdt, Morris, Eliza J, Tran, Hai, Nash, Michael A, Tan, Cheemeng, Jensen, Mikkel Herholdt, Faeder, James R1, Jensen, Mikkel Herholdt, Morris, Eliza J, Tran, Hai, Nash, Michael A, and Tan, Cheemeng

Abstract

Top-down proteomics has enabled the elucidation of heterogeneous protein complexes with different cofactors, post-translational modifications, and protein membership. This heterogeneity is believed to play a previously unknown role in cellular processes. The different molecular forms of a protein complex have come to be called "complex isoform" or "complexoform". Despite the elucidation of the complexoform, it remains unclear how and whether cellular circuits control the distribution of a complexoform. To help address this issue, we first simulate a generic three-protein complexoform to reveal the control of its distribution by the timing of gene transcription, mRNA translation, and protein transport. Overall, we ran 265 computational experiments: each averaged over 1,000 stochastic simulations. Based on the experiments, we show that genes arranged in a single operon, a cascade, or as two operons all give rise to the different protein composition of complexoform because of timing differences in protein-synthesis order. We also show that changes in the kinetics of expression, protein transport, or protein binding dramatically alter the distribution of the complexoform. Furthermore, both stochastic and transient kinetics control the assembly of the complexoform when the expression and assembly occur concurrently. We test our model against the biological cellulosome system. With biologically relevant rates, we find that the genetic circuitry controls the average final complexoform assembly and the variation in the assembly structure. Our results highlight the importance of both the genetic circuit architecture and kinetics in determining the distribution of a complexoform. Our work has a broad impact on our understanding of non-equilibrium processes in both living and synthetic biological systems.

Published

2020

27. Restoration and Modification of Magnetosome Biosynthesis by Internal Gene Acquisition in a Magnetotactic Bacterium.

Author

Arakaki, Atsushi, Arakaki, Atsushi, Goto, Mayu, Maruyama, Mina, Yoda, Takuto, Tanaka, Masayoshi, Yamagishi, Ayana, Yoshikuni, Yasuo, Matsunaga, Tadashi, Arakaki, Atsushi, Arakaki, Atsushi, Goto, Mayu, Maruyama, Mina, Yoda, Takuto, Tanaka, Masayoshi, Yamagishi, Ayana, Yoshikuni, Yasuo, and Matsunaga, Tadashi

Abstract

Integration of a large-sized DNA fragment into a chromosome is an important strategy for characterization of cellular functions in microorganisms. Magnetotactic bacteria synthesize intracellular organelles comprising membrane-bound single crystalline magnetite, also referred to as magnetosomes. Magnetosomes have gained interest in both scientific and engineering sectors as they can be utilized as a material for biomedical and nanotechnological applications. Although genetic engineering of magnetosome biosynthesis mechanism has been investigated, the current method requires cumbersome gene preparation processes. Here, the chromosomal integration of a plasmid containing ≈27 magnetosome genes (≈26 kbp region) in a non-magnetic mutant of Magnetospirillum magneticum AMB-1 using a broad-host-range plasmid is shown. The genome sequencing of gene-complemented strains reveals the chromosomal integration of the plasmid with magnetosome genes at a specific site, most likely by catalysis of an endogenous transposase. Magnetosome production is successfully enhanced by integrating a variation of magnetosome gene operons in the chromosome. This chromosomal integration mechanism will allow the design of functional magnetosomes de novo and M. magneticum AMB-1 may be used as a chassis for the designed magnetosome production.

Published

2020

28. Genomic characterization of a diazotrophic microbiota associated with maize aerial root mucilage.

Author

Higdon, Shawn M, Chen, Jen-Tsung1, Higdon, Shawn M, Pozzo, Tania, Kong, Nguyet, Huang, Bihua C, Yang, Mai Lee, Jeannotte, Richard, Brown, C Titus, Bennett, Alan B, Weimer, Bart C, Higdon, Shawn M, Chen, Jen-Tsung1, Higdon, Shawn M, Pozzo, Tania, Kong, Nguyet, Huang, Bihua C, Yang, Mai Lee, Jeannotte, Richard, Brown, C Titus, Bennett, Alan B, and Weimer, Bart C

Abstract

A geographically isolated maize landrace cultivated on nitrogen-depleted fields without synthetic fertilizer in the Sierra Mixe region of Oaxaca, Mexico utilizes nitrogen derived from the atmosphere and develops an extensive network of mucilage-secreting aerial roots that harbors a diazotrophic (N2-fixing) microbiota. Targeting these diazotrophs, we selected nearly 600 microbes of a collection obtained from mucilage and confirmed their ability to incorporate heavy nitrogen (15N2) metabolites in vitro. Sequencing their genomes and conducting comparative bioinformatic analyses showed that these genomes had substantial phylogenetic diversity. We examined each diazotroph genome for the presence of nif genes essential to nitrogen fixation (nifHDKENB) and carbohydrate utilization genes relevant to the mucilage polysaccharide digestion. These analyses identified diazotrophs that possessed the canonical nif gene operons, as well as many other operon configurations with concomitant fixation and release of >700 different 15N labeled metabolites. We further demonstrated that many diazotrophs possessed alternative nif gene operons and confirmed their genomic potential to derive chemical energy from mucilage polysaccharide to fuel nitrogen fixation. These results confirm that some diazotrophic bacteria associated with Sierra Mixe maize were capable of incorporating atmospheric nitrogen into their small molecule extracellular metabolites through multiple nif gene configurations while others were able to fix nitrogen without the canonical (nifHDKENB) genes.

Published

2020

29. The Exploration of Novel Regulatory Relationships Drives Haloarchaeal Operon-Like Structural Dynamics over Short Evolutionary Distances.

Author

Seitzer, Phillip, Seitzer, Phillip, Yao, Andrew I, Cisneros, Ariana, Facciotti, Marc T, Seitzer, Phillip, Seitzer, Phillip, Yao, Andrew I, Cisneros, Ariana, and Facciotti, Marc T

Abstract

Operons are a dominant feature of bacterial and archaeal genome organization. Numerous investigations have related aspects of operon structure to operon function, making operons exemplars for studies aimed at deciphering Nature's design principles for genomic organization at a local scale. We consider this understanding to be both fundamentally important and ultimately useful in the de novo design of increasingly complex synthetic circuits. Here we analyze the evolution of the genomic context of operon-like structures in a set of 76 sequenced and annotated species of halophilic archaea. The phylogenetic depth and breadth of this dataset allows insight into changes in operon-like structures over shorter evolutionary time scales than have been studied in previous cross-species analysis of operon evolution. Our analysis, implemented in the updated software package JContextExplorer finds that operon-like context as measured by changes in structure frequently differs from a sequence divergence model of whole-species phylogeny and that changes seem to be dominated by the exploration of novel regulatory relationships.

Published

2020

30. Whole-genome sequences of two new caballeronia strains isolated from cryoturbated peat circles of the permafrost-affected eastern european tundra

Author

Hetz, Stefanie A., Poehlein, Anja, Horn, Marcus A., Hetz, Stefanie A., Poehlein, Anja, and Horn, Marcus A.

Abstract

Annotated genomes of Caballeronia strains SBC1 and SBC2 from acidic permafrost suggest a new species with a facultative lifestyle via oxygen and nitrate respiration. Thus, a contribution to nitrogen cycling in cold and low-pH environments is anticipated. © 2020 Hetz et al. This is an open-access article distributed under the terms of the Creative Commons Attribution 4.0 International license.

Published

2020

31. Pervasive functional translation of noncanonical human open reading frames.

Author

Chen, Jin, Chen, Jin, Brunner, Andreas-David, Cogan, J Zachery, Nuñez, James K, Fields, Alexander P, Adamson, Britt, Itzhak, Daniel N, Li, Jason Y, Mann, Matthias, Leonetti, Manuel D, Weissman, Jonathan S, Chen, Jin, Chen, Jin, Brunner, Andreas-David, Cogan, J Zachery, Nuñez, James K, Fields, Alexander P, Adamson, Britt, Itzhak, Daniel N, Li, Jason Y, Mann, Matthias, Leonetti, Manuel D, and Weissman, Jonathan S

Abstract

Ribosome profiling has revealed pervasive but largely uncharacterized translation outside of canonical coding sequences (CDSs). In this work, we exploit a systematic CRISPR-based screening strategy to identify hundreds of noncanonical CDSs that are essential for cellular growth and whose disruption elicits specific, robust transcriptomic and phenotypic changes in human cells. Functional characterization of the encoded microproteins reveals distinct cellular localizations, specific protein binding partners, and hundreds of microproteins that are presented by the human leukocyte antigen system. We find multiple microproteins encoded in upstream open reading frames, which form stable complexes with the main, canonical protein encoded on the same messenger RNA, thereby revealing the use of functional bicistronic operons in mammals. Together, our results point to a family of functional human microproteins that play critical and diverse cellular roles.

Published

2020

32. Redefining fundamental concepts of transcription initiation in bacteria.

Author

Mejía-Almonte, Citlalli, Mejía-Almonte, Citlalli, Busby, Stephen JW, Wade, Joseph T, van Helden, Jacques, Arkin, Adam P, Stormo, Gary D, Eilbeck, Karen, Palsson, Bernhard O, Galagan, James E, Collado-Vides, Julio, Mejía-Almonte, Citlalli, Mejía-Almonte, Citlalli, Busby, Stephen JW, Wade, Joseph T, van Helden, Jacques, Arkin, Adam P, Stormo, Gary D, Eilbeck, Karen, Palsson, Bernhard O, Galagan, James E, and Collado-Vides, Julio

Abstract

Despite enormous progress in understanding the fundamentals of bacterial gene regulation, our knowledge remains limited when compared with the number of bacterial genomes and regulatory systems to be discovered. Derived from a small number of initial studies, classic definitions for concepts of gene regulation have evolved as the number of characterized promoters has increased. Together with discoveries made using new technologies, this knowledge has led to revised generalizations and principles. In this Expert Recommendation, we suggest precise, updated definitions that support a logical, consistent conceptual framework of bacterial gene regulation, focusing on transcription initiation. The resulting concepts can be formalized by ontologies for computational modelling, laying the foundation for improved bioinformatics tools, knowledge-based resources and scientific communication. Thus, this work will help researchers construct better predictive models, with different formalisms, that will be useful in engineering, synthetic biology, microbiology and genetics.

Published

2020

33. The structure of the endogenous ESX-3 secretion system.

Author

Poweleit, Nicole, Poweleit, Nicole, Czudnochowski, Nadine, Nakagawa, Rachel, Trinidad, Donovan D, Murphy, Kenan C, Sassetti, Christopher M, Rosenberg, Oren S, Poweleit, Nicole, Poweleit, Nicole, Czudnochowski, Nadine, Nakagawa, Rachel, Trinidad, Donovan D, Murphy, Kenan C, Sassetti, Christopher M, and Rosenberg, Oren S

Abstract

The ESX (or Type VII) secretion systems are protein export systems in mycobacteria and many Gram-positive bacteria that mediate a broad range of functions including virulence, conjugation, and metabolic regulation. These systems translocate folded dimers of WXG100-superfamily protein substrates across the cytoplasmic membrane. We report the cryo-electron microscopy structure of an ESX-3 system, purified using an epitope tag inserted with recombineering into the chromosome of the model organism Mycobacterium smegmatis. The structure reveals a stacked architecture that extends above and below the inner membrane of the bacterium. The ESX-3 protomer complex is assembled from a single copy of the EccB3, EccC3, and EccE3 and two copies of the EccD3 protein. In the structure, the protomers form a stable dimer that is consistent with assembly into a larger oligomer. The ESX-3 structure provides a framework for further study of these important bacterial transporters.

Published

2019

34. LurR is a regulator of the central lactate oxidation pathway in sulfate-reducing Desulfovibrio species.

Author

Rajeev, Lara, Rajeev, Lara, Luning, Eric G, Zane, Grant M, Juba, Thomas R, Kazakov, Alexey E, Novichkov, Pavel S, Wall, Judy D, Mukhopadhyay, Aindrila, Rajeev, Lara, Rajeev, Lara, Luning, Eric G, Zane, Grant M, Juba, Thomas R, Kazakov, Alexey E, Novichkov, Pavel S, Wall, Judy D, and Mukhopadhyay, Aindrila

Abstract

The central carbon/lactate utilization pathway in the model sulfate-reducing bacterium, Desulfovibrio vulgaris Hildenborough, is encoded by the highly conserved operon DVU3025-3033. Our earlier in vitro genome-wide study had suggested a network of four two-component system regulators that target this large operon; however, how these four regulators control this operon was not known. Here, we probe the regulation of the lactate utilization operon with mutant strains and DNA-protein binding assays. We show that the LurR response regulator is required for optimal growth and complete lactate utilization, and that it activates the DVU3025-3033 lactate oxidation operon as well as DVU2451, a lactate permease gene, in the presence of lactate. We show by electrophoretic mobility shift assays that LurR binds to three sites in the upstream region of DVU3025, the first gene of the operon. NrfR, a response regulator that is activated under nitrite stress, and LurR share similar binding site motifs and bind the same sites upstream of DVU3025. The DVU3025 promoter also has a binding site motif (Pho box) that is bound by PhoB, a two-component response regulator activated under phosphate limitation. The lactate utilization operon, the regulator LurR, and LurR binding sites are conserved across the order Desulfovibrionales whereas possible modulation of the lactate utilization genes by additional regulators such as NrfR and PhoB appears to be limited to D. vulgaris.

Published

2019

35. Microfluidic-based transcriptomics reveal force-independent bacterial rheosensing.

Author

Sanfilippo, Joseph E, Sanfilippo, Joseph E, Lorestani, Alexander, Koch, Matthias D, Bratton, Benjamin P, Siryaporn, Albert, Stone, Howard A, Gitai, Zemer, Sanfilippo, Joseph E, Sanfilippo, Joseph E, Lorestani, Alexander, Koch, Matthias D, Bratton, Benjamin P, Siryaporn, Albert, Stone, Howard A, and Gitai, Zemer

Abstract

Multiple cell types sense fluid flow as an environmental cue. Flow can exert shear force (or stress) on cells, and the prevailing model is that biological flow sensing involves the measurement of shear force1,2. Here, we provide evidence for force-independent flow sensing in the bacterium Pseudomonas aeruginosa. A microfluidic-based transcriptomic approach enabled us to discover an operon of P. aeruginosa that is rapidly and robustly upregulated in response to flow. Using a single-cell reporter of this operon, which we name the flow-regulated operon (fro), we establish that P. aeruginosa dynamically tunes gene expression to flow intensity through a process we call rheosensing (as rheo- is Greek for flow). We further show that rheosensing occurs in multicellular biofilms, involves signalling through the alternative sigma factor FroR, and does not require known surface sensors. To directly test whether rheosensing measures force, we independently altered the two parameters that contribute to shear stress: shear rate and solution viscosity. Surprisingly, we discovered that rheosensing is sensitive to shear rate but not viscosity, indicating that rheosensing is a kinematic (force-independent) form of mechanosensing. Thus, our findings challenge the dominant belief that biological mechanosensing requires the measurement of forces.

Published

2019

36. LurR is a regulator of the central lactate oxidation pathway in sulfate-reducing Desulfovibrio species.

Author

Rajeev, Lara, Rajeev, Lara, Luning, Eric G, Zane, Grant M, Juba, Thomas R, Kazakov, Alexey E, Novichkov, Pavel S, Wall, Judy D, Mukhopadhyay, Aindrila, Rajeev, Lara, Rajeev, Lara, Luning, Eric G, Zane, Grant M, Juba, Thomas R, Kazakov, Alexey E, Novichkov, Pavel S, Wall, Judy D, and Mukhopadhyay, Aindrila

Abstract

The central carbon/lactate utilization pathway in the model sulfate-reducing bacterium, Desulfovibrio vulgaris Hildenborough, is encoded by the highly conserved operon DVU3025-3033. Our earlier in vitro genome-wide study had suggested a network of four two-component system regulators that target this large operon; however, how these four regulators control this operon was not known. Here, we probe the regulation of the lactate utilization operon with mutant strains and DNA-protein binding assays. We show that the LurR response regulator is required for optimal growth and complete lactate utilization, and that it activates the DVU3025-3033 lactate oxidation operon as well as DVU2451, a lactate permease gene, in the presence of lactate. We show by electrophoretic mobility shift assays that LurR binds to three sites in the upstream region of DVU3025, the first gene of the operon. NrfR, a response regulator that is activated under nitrite stress, and LurR share similar binding site motifs and bind the same sites upstream of DVU3025. The DVU3025 promoter also has a binding site motif (Pho box) that is bound by PhoB, a two-component response regulator activated under phosphate limitation. The lactate utilization operon, the regulator LurR, and LurR binding sites are conserved across the order Desulfovibrionales whereas possible modulation of the lactate utilization genes by additional regulators such as NrfR and PhoB appears to be limited to D. vulgaris.

Published

2019

37. Genome sequence and characterization of the bcs clusters for the production of nanocellulose from the low pH resistant strain Komagataeibacter medellinensis ID13488

Author

Ingeniería química y del medio ambiente, Ingeniaritza kimikoa eta ingurumenaren ingeniaritza, Hernández‐Arriaga, Ana M., Del Cerro, Carlos, Urbina Moreno, Leire, Eceiza Mendiguren, María Aranzazu, Corcuera Maeso, María Ángeles, Retegui Miner, Aloña, Prieto, M. Auxiliadora, Ingeniería química y del medio ambiente, Ingeniaritza kimikoa eta ingurumenaren ingeniaritza, Hernández‐Arriaga, Ana M., Del Cerro, Carlos, Urbina Moreno, Leire, Eceiza Mendiguren, María Aranzazu, Corcuera Maeso, María Ángeles, Retegui Miner, Aloña, and Prieto, M. Auxiliadora

Abstract

Komagataeibacter medellinensis ID13488 (formerly Gluconacetobacter medellinensis ID13488) is able to produce crystalline bacterial cellulose (BC) under high acidic growth conditions. These abilities make this strain desirable for industrial BC production from acidic residues (e.g. wastes generated from cider production). To explore the molecular bases of the BC biosynthesis in this bacterium, the genome has been sequenced revealing a sequence of 3.4Mb containing three putative plasmids of 38.1kb (pKM01), 4.3kb (pKM02) and 3.3 Kb (pKM03). Genome comparison analyses of K.medellinensis ID13488 with other cellulose-producing related strains resulted in the identification of the bcs genes involved in the cellulose biosynthesis. Genes arrangement and composition of four bcs clusters (bcs1, bcs2, bcs3 and bcs4) was studied by RT-PCR, and their organization in four operons transcribed as four independent polycistronic mRNAs was determined. qRT-PCR experiments demonstrated that mostly bcs1 and bcs4 are expressed under BC production conditions, suggesting that these operons direct the synthesis of BC. Genomic differences with the close related strain K.medellinensis NBRC 3288 unable to produce BC were also described and discussed. © 2019 The Authors. Microbial Biotechnology published by John Wiley & Sons Ltd and Society for Applied Microbiology.

Published

2019

38. Eukaryotic Acquisition of a Bacterial Operon

Author

Kominek, Jacek, Doering, Drew T., Opulente, Dana A., Shen, Xing-Xing, Zhou, Xiaofan, DeVirgilio, Jeremy, Hulfachor, Amanda B., Groenewald, Marizeth, Mcgee, Mcsean A., Karlen, Steven D., Kurtzman, Cletus P., Rokas, Antonis, Hittinger, Chris Todd, Kominek, Jacek, Doering, Drew T., Opulente, Dana A., Shen, Xing-Xing, Zhou, Xiaofan, DeVirgilio, Jeremy, Hulfachor, Amanda B., Groenewald, Marizeth, Mcgee, Mcsean A., Karlen, Steven D., Kurtzman, Cletus P., Rokas, Antonis, and Hittinger, Chris Todd

Published

2019

39. Genome sequence and characterization of the bcs clusters for the production of nanocellulose from the low pH resistant strain Komagataeibacter medellinensis ID13488

Author

Ingeniería química y del medio ambiente, Ingeniaritza kimikoa eta ingurumenaren ingeniaritza, Hernández‐Arriaga, Ana M., Del Cerro, Carlos, Urbina Moreno, Leire, Eceiza Mendiguren, María Aranzazu, Corcuera Maeso, María Ángeles, Retegui Miner, Aloña, Prieto, M. Auxiliadora, Ingeniería química y del medio ambiente, Ingeniaritza kimikoa eta ingurumenaren ingeniaritza, Hernández‐Arriaga, Ana M., Del Cerro, Carlos, Urbina Moreno, Leire, Eceiza Mendiguren, María Aranzazu, Corcuera Maeso, María Ángeles, Retegui Miner, Aloña, and Prieto, M. Auxiliadora

Abstract

Komagataeibacter medellinensis ID13488 (formerly Gluconacetobacter medellinensis ID13488) is able to produce crystalline bacterial cellulose (BC) under high acidic growth conditions. These abilities make this strain desirable for industrial BC production from acidic residues (e.g. wastes generated from cider production). To explore the molecular bases of the BC biosynthesis in this bacterium, the genome has been sequenced revealing a sequence of 3.4Mb containing three putative plasmids of 38.1kb (pKM01), 4.3kb (pKM02) and 3.3 Kb (pKM03). Genome comparison analyses of K.medellinensis ID13488 with other cellulose-producing related strains resulted in the identification of the bcs genes involved in the cellulose biosynthesis. Genes arrangement and composition of four bcs clusters (bcs1, bcs2, bcs3 and bcs4) was studied by RT-PCR, and their organization in four operons transcribed as four independent polycistronic mRNAs was determined. qRT-PCR experiments demonstrated that mostly bcs1 and bcs4 are expressed under BC production conditions, suggesting that these operons direct the synthesis of BC. Genomic differences with the close related strain K.medellinensis NBRC 3288 unable to produce BC were also described and discussed. © 2019 The Authors. Microbial Biotechnology published by John Wiley & Sons Ltd and Society for Applied Microbiology.

Published

2019

40. LurR is a regulator of the central lactate oxidation pathway in sulfate-reducing Desulfovibrio species.

Author

Rajeev, Lara, Wen, Z Tom1, Rajeev, Lara, Luning, Eric G, Zane, Grant M, Juba, Thomas R, Kazakov, Alexey E, Novichkov, Pavel S, Wall, Judy D, Mukhopadhyay, Aindrila, Rajeev, Lara, Wen, Z Tom1, Rajeev, Lara, Luning, Eric G, Zane, Grant M, Juba, Thomas R, Kazakov, Alexey E, Novichkov, Pavel S, Wall, Judy D, and Mukhopadhyay, Aindrila

Abstract

The central carbon/lactate utilization pathway in the model sulfate-reducing bacterium, Desulfovibrio vulgaris Hildenborough, is encoded by the highly conserved operon DVU3025-3033. Our earlier in vitro genome-wide study had suggested a network of four two-component system regulators that target this large operon; however, how these four regulators control this operon was not known. Here, we probe the regulation of the lactate utilization operon with mutant strains and DNA-protein binding assays. We show that the LurR response regulator is required for optimal growth and complete lactate utilization, and that it activates the DVU3025-3033 lactate oxidation operon as well as DVU2451, a lactate permease gene, in the presence of lactate. We show by electrophoretic mobility shift assays that LurR binds to three sites in the upstream region of DVU3025, the first gene of the operon. NrfR, a response regulator that is activated under nitrite stress, and LurR share similar binding site motifs and bind the same sites upstream of DVU3025. The DVU3025 promoter also has a binding site motif (Pho box) that is bound by PhoB, a two-component response regulator activated under phosphate limitation. The lactate utilization operon, the regulator LurR, and LurR binding sites are conserved across the order Desulfovibrionales whereas possible modulation of the lactate utilization genes by additional regulators such as NrfR and PhoB appears to be limited to D. vulgaris.

Published

2019

41. The structure of the endogenous ESX-3 secretion system.

Author

Poweleit, Nicole, Poweleit, Nicole, Czudnochowski, Nadine, Nakagawa, Rachel, Trinidad, Donovan D, Murphy, Kenan C, Sassetti, Christopher M, Rosenberg, Oren S, Poweleit, Nicole, Poweleit, Nicole, Czudnochowski, Nadine, Nakagawa, Rachel, Trinidad, Donovan D, Murphy, Kenan C, Sassetti, Christopher M, and Rosenberg, Oren S

Abstract

The ESX (or Type VII) secretion systems are protein export systems in mycobacteria and many Gram-positive bacteria that mediate a broad range of functions including virulence, conjugation, and metabolic regulation. These systems translocate folded dimers of WXG100-superfamily protein substrates across the cytoplasmic membrane. We report the cryo-electron microscopy structure of an ESX-3 system, purified using an epitope tag inserted with recombineering into the chromosome of the model organism Mycobacterium smegmatis. The structure reveals a stacked architecture that extends above and below the inner membrane of the bacterium. The ESX-3 protomer complex is assembled from a single copy of the EccB3, EccC3, and EccE3 and two copies of the EccD3 protein. In the structure, the protomers form a stable dimer that is consistent with assembly into a larger oligomer. The ESX-3 structure provides a framework for further study of these important bacterial transporters.

Published

2019

42. Microfluidic-based transcriptomics reveal force-independent bacterial rheosensing.

Author

Sanfilippo, Joseph E, Sanfilippo, Joseph E, Lorestani, Alexander, Koch, Matthias D, Bratton, Benjamin P, Siryaporn, Albert, Stone, Howard A, Gitai, Zemer, Sanfilippo, Joseph E, Sanfilippo, Joseph E, Lorestani, Alexander, Koch, Matthias D, Bratton, Benjamin P, Siryaporn, Albert, Stone, Howard A, and Gitai, Zemer

Abstract

Multiple cell types sense fluid flow as an environmental cue. Flow can exert shear force (or stress) on cells, and the prevailing model is that biological flow sensing involves the measurement of shear force1,2. Here, we provide evidence for force-independent flow sensing in the bacterium Pseudomonas aeruginosa. A microfluidic-based transcriptomic approach enabled us to discover an operon of P. aeruginosa that is rapidly and robustly upregulated in response to flow. Using a single-cell reporter of this operon, which we name the flow-regulated operon (fro), we establish that P. aeruginosa dynamically tunes gene expression to flow intensity through a process we call rheosensing (as rheo- is Greek for flow). We further show that rheosensing occurs in multicellular biofilms, involves signalling through the alternative sigma factor FroR, and does not require known surface sensors. To directly test whether rheosensing measures force, we independently altered the two parameters that contribute to shear stress: shear rate and solution viscosity. Surprisingly, we discovered that rheosensing is sensitive to shear rate but not viscosity, indicating that rheosensing is a kinematic (force-independent) form of mechanosensing. Thus, our findings challenge the dominant belief that biological mechanosensing requires the measurement of forces.

Published

2019

43. Cellular responses to reactive oxygen species are predicted from molecular mechanisms.

Author

Yang, Laurence, Yang, Laurence, Mih, Nathan, Anand, Amitesh, Park, Joon Ho, Tan, Justin, Yurkovich, James T, Monk, Jonathan M, Lloyd, Colton J, Sandberg, Troy E, Seo, Sang Woo, Kim, Donghyuk, Sastry, Anand V, Phaneuf, Patrick, Gao, Ye, Broddrick, Jared T, Chen, Ke, Heckmann, David, Szubin, Richard, Hefner, Ying, Feist, Adam M, Palsson, Bernhard O, Yang, Laurence, Yang, Laurence, Mih, Nathan, Anand, Amitesh, Park, Joon Ho, Tan, Justin, Yurkovich, James T, Monk, Jonathan M, Lloyd, Colton J, Sandberg, Troy E, Seo, Sang Woo, Kim, Donghyuk, Sastry, Anand V, Phaneuf, Patrick, Gao, Ye, Broddrick, Jared T, Chen, Ke, Heckmann, David, Szubin, Richard, Hefner, Ying, Feist, Adam M, and Palsson, Bernhard O

Abstract

Catalysis using iron-sulfur clusters and transition metals can be traced back to the last universal common ancestor. The damage to metalloproteins caused by reactive oxygen species (ROS) can prevent cell growth and survival when unmanaged, thus eliciting an essential stress response that is universal and fundamental in biology. Here we develop a computable multiscale description of the ROS stress response in Escherichia coli, called OxidizeME. We use OxidizeME to explain four key responses to oxidative stress: 1) ROS-induced auxotrophy for branched-chain, aromatic, and sulfurous amino acids; 2) nutrient-dependent sensitivity of growth rate to ROS; 3) ROS-specific differential gene expression separate from global growth-associated differential expression; and 4) coordinated expression of iron-sulfur cluster (ISC) and sulfur assimilation (SUF) systems for iron-sulfur cluster biosynthesis. These results show that we can now develop fundamental and quantitative genotype-phenotype relationships for stress responses on a genome-wide basis.

Published

2019

44. Disruption of transcription-translation coordination in Escherichia coli leads to premature transcriptional termination.

Author

Zhu, Manlu, Zhu, Manlu, Mori, Matteo, Hwa, Terence, Dai, Xiongfeng, Zhu, Manlu, Zhu, Manlu, Mori, Matteo, Hwa, Terence, and Dai, Xiongfeng

Abstract

Tight coordination between transcription and translation is crucial to maintaining the integrity of gene expression in bacteria, yet how bacteria manage to coordinate these two processes remains unclear. Possible direct physical coupling between the RNA polymerase and ribosome has been thoroughly investigated in recent years. Here, we quantitatively characterize the transcriptional kinetics of Escherichia coli under different growth conditions. Transcriptional and translational elongation remain coordinated under various nutrient conditions, as previously reported. However, transcriptional elongation was not affected under antibiotics that slowed down translational elongation. This result was also found by introducing nonsense mutation that completely dissociated transcription from translation. Our data thus provide direct evidence that translation is not required to maintain the speed of transcriptional elongation. In cases where transcription and translation are dissociated, our study provides quantitative characterization of the resulting process of premature transcriptional termination (PTT). PTT-mediated polarity caused by translation-targeting antibiotics substantially affected the coordinated expression of genes in several long operons, contributing to the key physiological effects of these antibiotics. Our results also suggest a model in which the coordination between transcriptional and translational elongation under normal growth conditions is implemented by guanosine tetraphosphate.

Published

2019

45. Eukaryotic Acquisition of a Bacterial Operon

Author

Kominek, Jacek, Doering, Drew T., Opulente, Dana A., Shen, Xing-Xing, Zhou, Xiaofan, DeVirgilio, Jeremy, Hulfachor, Amanda B., Groenewald, Marizeth, Mcgee, Mcsean A., Karlen, Steven D., Kurtzman, Cletus P., Rokas, Antonis, Hittinger, Chris Todd, Kominek, Jacek, Doering, Drew T., Opulente, Dana A., Shen, Xing-Xing, Zhou, Xiaofan, DeVirgilio, Jeremy, Hulfachor, Amanda B., Groenewald, Marizeth, Mcgee, Mcsean A., Karlen, Steven D., Kurtzman, Cletus P., Rokas, Antonis, and Hittinger, Chris Todd

Published

2019

46. Genome sequence and characterization of the bcs clusters for the production of nanocellulose from the low pH resistant strain Komagataeibacter medellinensis ID13488

Author

Ingeniería química y del medio ambiente, Ingeniaritza kimikoa eta ingurumenaren ingeniaritza, Hernández‐Arriaga, Ana M., Del Cerro, Carlos, Urbina Moreno, Leire, Eceiza Mendiguren, María Aranzazu, Corcuera Maeso, María Ángeles, Retegui Miner, Aloña, Prieto, M. Auxiliadora, Ingeniería química y del medio ambiente, Ingeniaritza kimikoa eta ingurumenaren ingeniaritza, Hernández‐Arriaga, Ana M., Del Cerro, Carlos, Urbina Moreno, Leire, Eceiza Mendiguren, María Aranzazu, Corcuera Maeso, María Ángeles, Retegui Miner, Aloña, and Prieto, M. Auxiliadora

Abstract

Komagataeibacter medellinensis ID13488 (formerly Gluconacetobacter medellinensis ID13488) is able to produce crystalline bacterial cellulose (BC) under high acidic growth conditions. These abilities make this strain desirable for industrial BC production from acidic residues (e.g. wastes generated from cider production). To explore the molecular bases of the BC biosynthesis in this bacterium, the genome has been sequenced revealing a sequence of 3.4Mb containing three putative plasmids of 38.1kb (pKM01), 4.3kb (pKM02) and 3.3 Kb (pKM03). Genome comparison analyses of K.medellinensis ID13488 with other cellulose-producing related strains resulted in the identification of the bcs genes involved in the cellulose biosynthesis. Genes arrangement and composition of four bcs clusters (bcs1, bcs2, bcs3 and bcs4) was studied by RT-PCR, and their organization in four operons transcribed as four independent polycistronic mRNAs was determined. qRT-PCR experiments demonstrated that mostly bcs1 and bcs4 are expressed under BC production conditions, suggesting that these operons direct the synthesis of BC. Genomic differences with the close related strain K.medellinensis NBRC 3288 unable to produce BC were also described and discussed. © 2019 The Authors. Microbial Biotechnology published by John Wiley & Sons Ltd and Society for Applied Microbiology.

Published

2019

47. The effect of modulating the quantity of enzymes in a model ethanol pathway on metabolic flux in Synechocystis sp. PCC 6803

Author

Bartasun, Paulina, Prandi, Nicole, Storch, Marko, Aknin, Yarin, Bennett, Mark, Palma, Arianna, Baldwin, Geoff, Sakuragi, Yumiko, Jones, Patrik R., Rowland, John, Bartasun, Paulina, Prandi, Nicole, Storch, Marko, Aknin, Yarin, Bennett, Mark, Palma, Arianna, Baldwin, Geoff, Sakuragi, Yumiko, Jones, Patrik R., and Rowland, John

Abstract

Synthetic metabolism allows new metabolic capabilities to be introduced into strains for biotechnology applications. Such engineered metabolic pathways are unlikely to function optimally as initially designed and native metabolism may not efficiently support the introduced pathway without further intervention. To develop our understanding of optimal metabolic engineering strategies, a two-enzyme ethanol pathway consisting of pyruvate decarboxylase and acetaldehyde reductase was introduced into Synechocystis sp. PCC 6803. We characteriseda new set of ribosome binding site sequences in Synechocystis sp. PCC 6803 providing a range of translation strengths for different genes under test. The effect of ribosome-bindingsite sequence, operon design and modifications to native metabolism on pathway flux was analysed by HPLC. The accumulation of all introduced proteins was also quantified using selected reaction monitoring mass spectrometry. Pathway productivity was more strongly dependent on the accumulation of pyruvate decarboxylase than acetaldehyde reductase. In fact, abolishment of reductase over-expression resulted in the greatest ethanol productivity, most likely because strains harbouringsingle-gene constructs accumulated more pyruvate decarboxylase than strains carrying any of the multi-gene constructs. Overall, several lessons were learned. Firstly, the expression level of the first gene in anyoperon influenced the expression level of subsequent genes, demonstrating that translational coupling can also occur in cyanobacteria. Longer operons resulted in lower protein abundance for proximally-encoded cistrons. And, implementation of metabolic engineering strategies that have previously been shown to enhance the growth or yield of pyruvate dependent products, through co-expression with pyruvate kinase and/or fructose-1,6-bisphosphatase/sedoheptulose-1,7-bisphosphatase, indicated that other factors had greater control over growth and metabolic flux under the tested

Published

2019

48. Noncontiguous operon is a genetic organization for coordinating bacterial gene expression

Author

Ministerio de Economía y Competitividad (España), European Commission, European Research Council, Solano Goñi, Cristina [0000-0002-6207-1766], Toledo-Arana, Alejandro [0000-0001-8148-6281], Lasa, Íñigo [0000-0002-6625-9221], Sáenz, Sonia, Bitarte, Nerea, García, Begoña, Burgui, Saioa, Vergara-Irigaray, Marta, Valle Turrillas, Jaione, Solano Goñi, Cristina, Toledo-Arana, Alejandro, Lasa, Íñigo, Ministerio de Economía y Competitividad (España), European Commission, European Research Council, Solano Goñi, Cristina [0000-0002-6207-1766], Toledo-Arana, Alejandro [0000-0001-8148-6281], Lasa, Íñigo [0000-0002-6625-9221], Sáenz, Sonia, Bitarte, Nerea, García, Begoña, Burgui, Saioa, Vergara-Irigaray, Marta, Valle Turrillas, Jaione, Solano Goñi, Cristina, Toledo-Arana, Alejandro, and Lasa, Íñigo

Abstract

Bacterial genes are typically grouped into operons defined as clusters of adjacent genes encoding for proteins that fill related roles and are transcribed into a single polycistronic mRNA molecule. This simple organization provides an efficient mechanism to coordinate the expression of neighboring genes and is at the basis of gene regulation in bacteria. Here, we report the existence of a higher level of organization in operon structure that we named noncontiguous operon and consists in an operon containing a gene(s) that is transcribed in the opposite direction to the rest of the operon. This transcriptional architecture is exemplified by the genes menE-menC-MW1733-ytkD-MW1731 involved in menaquinone synthesis in the major human pathogen Staphylococcus aureus. We show that menE-menC-ytkD-MW1731 genes are transcribed as a single transcription unit, whereas the MW1733 gene, located between menC and ytkD, is transcribed in the opposite direction. This genomic organization generates overlapping transcripts whose expression is mutually regulated by transcriptional interference and RNase III processing at the overlapping region. In light of our results, the canonical view of operon structure should be revisited by including this operon arrangement in which cotranscription and overlapping transcription are combined to coordinate functionally related gene expression.

Published

2019

49. The effect of modulating the quantity of enzymes in a model ethanol pathway on metabolic flux in Synechocystis sp. PCC 6803

Author

Bartasun, Paulina, Prandi, Nicole, Storch, Marko, Aknin, Yarin, Bennett, Mark, Palma, Arianna, Baldwin, Geoff, Sakuragi, Yumiko, Jones, Patrik R., Rowland, John, Bartasun, Paulina, Prandi, Nicole, Storch, Marko, Aknin, Yarin, Bennett, Mark, Palma, Arianna, Baldwin, Geoff, Sakuragi, Yumiko, Jones, Patrik R., and Rowland, John

Abstract

Synthetic metabolism allows new metabolic capabilities to be introduced into strains for biotechnology applications. Such engineered metabolic pathways are unlikely to function optimally as initially designed and native metabolism may not efficiently support the introduced pathway without further intervention. To develop our understanding of optimal metabolic engineering strategies, a two-enzyme ethanol pathway consisting of pyruvate decarboxylase and acetaldehyde reductase was introduced into Synechocystis sp. PCC 6803. We characteriseda new set of ribosome binding site sequences in Synechocystis sp. PCC 6803 providing a range of translation strengths for different genes under test. The effect of ribosome-bindingsite sequence, operon design and modifications to native metabolism on pathway flux was analysed by HPLC. The accumulation of all introduced proteins was also quantified using selected reaction monitoring mass spectrometry. Pathway productivity was more strongly dependent on the accumulation of pyruvate decarboxylase than acetaldehyde reductase. In fact, abolishment of reductase over-expression resulted in the greatest ethanol productivity, most likely because strains harbouringsingle-gene constructs accumulated more pyruvate decarboxylase than strains carrying any of the multi-gene constructs. Overall, several lessons were learned. Firstly, the expression level of the first gene in anyoperon influenced the expression level of subsequent genes, demonstrating that translational coupling can also occur in cyanobacteria. Longer operons resulted in lower protein abundance for proximally-encoded cistrons. And, implementation of metabolic engineering strategies that have previously been shown to enhance the growth or yield of pyruvate dependent products, through co-expression with pyruvate kinase and/or fructose-1,6-bisphosphatase/sedoheptulose-1,7-bisphosphatase, indicated that other factors had greater control over growth and metabolic flux under the tested

Published

2019

50. Systematic overexpression study to find target enzymes enhancing production of terpenes in Synechocystis PCC 6803, using isoprene as a model compound

Author

Englund, Elias, Shabestary, Kiyan, Hudson, Elton P., Lindberg, P., Englund, Elias, Shabestary, Kiyan, Hudson, Elton P., and Lindberg, P.

Abstract

Of the two natural metabolic pathways for making terpenoids, biotechnological utilization of the mevalonate (MVA) pathway has enabled commercial production of valuable compounds, while the more recently discovered but stoichiometrically more efficient methylerythritol phosphate (MEP) pathway is underdeveloped. We conducted a study on the overexpression of each enzyme in the MEP pathway in the unicellular cyanobacterium Synechocystis sp. PCC 6803, to identify potential targets for increasing flux towards terpenoid production, using isoprene as a reporter molecule. Results showed that the enzymes Ipi, Dxs and IspD had the biggest impact on isoprene production. By combining and creating operons out of those genes, isoprene production was increased 2-fold compared to the base strain. A genome-scale model was used to identify targets upstream of the MEP pathway that could redirect flux towards terpenoids. A total of ten reactions from the Calvin-Benson-Bassham cycle, lower glycolysis and co-factor synthesis pathways were probed for their effect on isoprene synthesis by co-expressing them with the MEP enzymes, resulting in a 60% increase in production from the best strain. Lastly, we studied two isoprene synthases with the highest reported catalytic rates. Only by expressing them together with Dxs and Ipi could we get stable strains that produced 2.8 mg/g isoprene per dry cell weight, a 40-fold improvement compared to the initial strain., Export Date: 22 October 2018; Article; CODEN: MEENF; Correspondence Address: Lindberg, P.; Department of Chemistry – Ångström, Uppsala University, Box 523, Sweden; email: pia.lindberg@kemi.uu.se; QC 20181106

Published

2018