Your search keyword '"Emily R, Forster"' showing total 6 results

1. The CspC pseudoprotease regulates germination of Clostridioides difficile spores in response to multiple environmental signals.

Author

Amy E Rohlfing, Brian E Eckenroth, Emily R Forster, Yuzo Kevorkian, M Lauren Donnelly, Hector Benito de la Puebla, Sylvie Doublié, and Aimee Shen

Subjects

Genetics, QH426-470

Abstract

The gastrointestinal pathogen, Clostridioides difficile, initiates infection when its metabolically dormant spore form germinates in the mammalian gut. While most spore-forming bacteria use transmembrane germinant receptors to sense nutrient germinants, C. difficile is thought to use the soluble pseudoprotease, CspC, to detect bile acid germinants. To gain insight into CspC's unique mechanism of action, we solved its crystal structure. Guided by this structure, we identified CspC mutations that confer either hypo- or hyper-sensitivity to bile acid germinant. Surprisingly, hyper-sensitive CspC variants exhibited bile acid-independent germination as well as increased sensitivity to amino acid and/or calcium co-germinants. Since mutations in specific residues altered CspC's responsiveness to these different signals, CspC plays a critical role in regulating C. difficile spore germination in response to multiple environmental signals. Taken together, these studies implicate CspC as being intimately involved in the detection of distinct classes of co-germinants in addition to bile acids and thus raises the possibility that CspC functions as a signaling node rather than a ligand-binding receptor.

Published

2019

2. The Listeria monocytogenes PASTA Kinase PrkA and Its Substrate YvcK Are Required for Cell Wall Homeostasis, Metabolism, and Virulence.

Author

Daniel A Pensinger, Kyle M Boldon, Grischa Y Chen, William J B Vincent, Kyle Sherman, Meng Xiong, Adam J Schaenzer, Emily R Forster, Jörn Coers, Rob Striker, and John-Demian Sauer

Subjects

Immunologic diseases. Allergy, RC581-607, Biology (General), QH301-705.5

Abstract

Obstacles to bacterial survival and replication in the cytosol of host cells, and the mechanisms used by bacterial pathogens to adapt to this niche are not well understood. Listeria monocytogenes is a well-studied Gram-positive foodborne pathogen that has evolved to invade and replicate within the host cell cytosol; yet the mechanisms by which it senses and responds to stress to survive in the cytosol are largely unknown. To assess the role of the L. monocytogenes penicillin-binding-protein and serine/threonine associated (PASTA) kinase PrkA in stress responses, cytosolic survival and virulence, we constructed a ΔprkA deletion mutant. PrkA was required for resistance to cell wall stress, growth on cytosolic carbon sources, intracellular replication, cytosolic survival, inflammasome avoidance and ultimately virulence in a murine model of Listeriosis. In Bacillus subtilis and Mycobacterium tuberculosis, homologues of PrkA phosphorylate a highly conserved protein of unknown function, YvcK. We found that, similar to PrkA, YvcK is also required for cell wall stress responses, metabolism of glycerol, cytosolic survival, inflammasome avoidance and virulence. We further demonstrate that similar to other organisms, YvcK is directly phosphorylated by PrkA, although the specific site(s) of phosphorylation are not highly conserved. Finally, analysis of phosphoablative and phosphomimetic mutants of YvcK in vitro and in vivo demonstrate that while phosphorylation of YvcK is irrelevant to metabolism and cell wall stress responses, surprisingly, a phosphomimetic, nonreversible negative charge of YvcK is detrimental to cytosolic survival and virulence in vivo. Taken together our data identify two novel virulence factors essential for cytosolic survival and virulence of L. monocytogenes. Furthermore, our data demonstrate that regulation of YvcK phosphorylation is tightly controlled and is critical for virulence. Finally, our data suggest that yet to be identified substrates of PrkA are essential for cytosolic survival and virulence of L. monocytogenes and illustrate the importance of studying protein phosphorylation in the context of infection.

Published

2016

3. Differential effects of ‘resurrecting' Csp pseudoproteases during Clostridioides difficile spore germination

Author

Aimee Shen, Emily R. Forster, Amy E. Rohlfing, and M. Lauren Donnelly

Subjects

medicine.medical_treatment, Microbiology, Biochemistry, Catalysis, 03 medical and health sciences, Bacterial Proteins, subtilisin-like serine protease, Catalytic triad, Spore germination, medicine, Molecular Biology, Pathogen, Research Articles, 030304 developmental biology, Spores, Bacterial, Genetics, Serine protease, 0303 health sciences, Protease, biology, Clostridioides difficile, 030306 microbiology, Chemistry, Gene Expression Regulation, Developmental, pseudoprotease, Gene Expression Regulation, Bacterial, Clostridium difficile, Cell Biology, Differential effects, Signaling, 3. Good health, spore germination, pseudoenzyme, Enzymology, biology.protein, Carrier Proteins, Function (biology), Clostridioides

Abstract

Clostridioides difficile is a spore-forming bacterial pathogen that is the leading cause of hospital-acquired gastroenteritis. C. difficile infections begin when its spore form germinates in the vertebrate gut upon sensing bile acids. These germinants induce a proteolytic signaling cascade controlled by three members of the subtilisin-like serine protease family, CspA, CspB, and CspC. Notably, even though CspC and CspA are both pseudoproteases, they are nevertheless required to sense germinants and activate the protease, CspB. Thus, CspC and CspA are part of a growing list of pseudoenzymes that play important roles in regulating cellular processes. However, despite their importance, the structural properties of pseudoenzymes that allow them to function as regulators remain poorly understood. Our recently determined crystal structure of CspC revealed that its degenerate site residues align closely with the catalytic triad of CspB, so in this study we tested whether the ancestral protease activity of the CspC and CspA pseudoproteases could be “resurrected.” Restoring the catalytic triad to these pseudoproteases failed to resurrect their protease activity, although the mutations differentially affected the stability and function of these pseudoproteases. Degenerate site mutations destabilized CspC and impaired spore germination without impacting CspA stability or function. Thus, our results surprisingly reveal that the presence of a catalytic triad does not necessarily predict protease activity. Since close homologs of C. difficile CspA occasionally carry an intact catalytic triad, our results imply that bioinformatics predictions of enzyme activity may overlook pseudoenzymes in some cases.

Published

2020

4. A microbial transporter of the dietary antioxidant ergothioneine

Author

Daniel G. Dumitrescu, Elizabeth M. Gordon, Yekaterina Kovalyova, Anna B. Seminara, Brianna Duncan-Lowey, Emily R. Forster, Wen Zhou, Carmen J. Booth, Aimee Shen, Philip J. Kranzusch, and Stavroula K. Hatzios

Subjects

Molecular Weight, Humans, Ergothioneine, Sulfhydryl Compounds, Oxidation-Reduction, General Biochemistry, Genetics and Molecular Biology, Antioxidants

Abstract

Low-molecular-weight (LMW) thiols are small-molecule antioxidants required for the maintenance of intracellular redox homeostasis. However, many host-associated microbes, including the gastric pathogen Helicobacter pylori, unexpectedly lack LMW-thiol biosynthetic pathways. Using reactivity-guided metabolomics, we identified the unusual LMW thiol ergothioneine (EGT) in H. pylori. Dietary EGT accumulates to millimolar levels in human tissues and has been broadly implicated in mitigating disease risk. Although certain microorganisms synthesize EGT, we discovered that H. pylori acquires this LMW thiol from the host environment using a highly selective ATP-binding cassette transporter-EgtUV. EgtUV confers a competitive colonization advantage in vivo and is widely conserved in gastrointestinal microbes. Furthermore, we found that human fecal bacteria metabolize EGT, which may contribute to production of the disease-associated metabolite trimethylamine N-oxide. Collectively, our findings illustrate a previously unappreciated mechanism of microbial redox regulation in the gut and suggest that inter-kingdom competition for dietary EGT may broadly impact human health.

Published

2022

5. The CspC pseudoprotease regulates germination of Clostridioides difficile spores in response to multiple environmental signals

Author

Sylvie Doublié, Emily R. Forster, M. Lauren Donnelly, Yuzo Kevorkian, Brian E. Eckenroth, Aimee Shen, Amy E. Rohlfing, and Hector Benito de la Puebla

Subjects

Models, Molecular, Cancer Research, Physiology, Protein Conformation, QH426-470, Crystallography, X-Ray, Biochemistry, Microbial Physiology, Medicine and Health Sciences, Electrochemistry, Bile, Salt Bridges, Bacterial Physiology, Amino Acids, Receptor, Pathogen, Genetics (clinical), Spores, Bacterial, chemistry.chemical_classification, 0303 health sciences, Crystallography, biology, Organic Compounds, Chemistry, Physics, Condensed Matter Physics, Transmembrane protein, Body Fluids, Amino acid, Germination, Physical Sciences, Crystal Structure, Anatomy, Basic Amino Acids, medicine.symptom, Research Article, Substitution Mutation, Clostridium Difficile, Glycine, Arginine, Microbiology, Bile Acids and Salts, 03 medical and health sciences, Bacterial Proteins, Stress, Physiological, medicine, Genetics, Solid State Physics, Bacterial Spores, Molecular Biology, Ecology, Evolution, Behavior and Systematics, 030304 developmental biology, Bacteria, Clostridioides difficile, 030306 microbiology, Gut Bacteria, Organic Chemistry, Organisms, Chemical Compounds, Biology and Life Sciences, Proteins, Bacteriology, Gene Expression Regulation, Bacterial, biology.organism_classification, Spore, Aliphatic Amino Acids, Mechanism of action, Mutation, Carrier Proteins

Abstract

The gastrointestinal pathogen, Clostridioides difficile, initiates infection when its metabolically dormant spore form germinates in the mammalian gut. While most spore-forming bacteria use transmembrane germinant receptors to sense nutrient germinants, C. difficile is thought to use the soluble pseudoprotease, CspC, to detect bile acid germinants. To gain insight into CspC’s unique mechanism of action, we solved its crystal structure. Guided by this structure, we identified CspC mutations that confer either hypo- or hyper-sensitivity to bile acid germinant. Surprisingly, hyper-sensitive CspC variants exhibited bile acid-independent germination as well as increased sensitivity to amino acid and/or calcium co-germinants. Since mutations in specific residues altered CspC’s responsiveness to these different signals, CspC plays a critical role in regulating C. difficile spore germination in response to multiple environmental signals. Taken together, these studies implicate CspC as being intimately involved in the detection of distinct classes of co-germinants in addition to bile acids and thus raises the possibility that CspC functions as a signaling node rather than a ligand-binding receptor., Author summary The major nosocomial pathogen Clostridioides difficile depends on spore germination to initiate infection. Interestingly, C. difficile’s germinant sensing mechanism differs markedly from other spore-forming bacteria, since it uses bile acids to induce germination and lacks the transmembrane germinant receptors conserved in almost all spore-forming organisms. Instead, C. difficile is thought to use CspC, a soluble pseudoprotease, to sense these unique bile acid germinants. To gain insight into how a pseudoprotease senses germinant and propagates this signal, we solved the crystal structure of C. difficile CspC. Guided by this structure, we identified mutations that alter the sensitivity of C. difficile spores to not only bile acid germinant but also to amino acid and calcium co-germinants. Taken together, our study implicates CspC in either directly or indirectly sensing these diverse small molecules and thus raises new questions regarding how C. difficile spores physically detect bile acid germinants and co-germinants.

Published

2018

6. The Listeria monocytogenes PASTA Kinase PrkA and Its Substrate YvcK Are Required for Cell Wall Homeostasis, Metabolism, and Virulence

Author

Daniel A. Pensinger, Rob Striker, Grischa Y. Chen, Kyle Sherman, Jörn Coers, Emily R. Forster, William J.B. Vincent, Kyle Boldon, John-Demian Sauer, Adam J. Schaenzer, and Meng Xiong

Subjects

0301 basic medicine, Glycerol, Inflammasomes, medicine.disease_cause, Pathology and Laboratory Medicine, Biochemistry, Mass Spectrometry, Mice, White Blood Cells, Cytosol, Cell Wall, Animal Cells, Medicine and Health Sciences, Homeostasis, Protein phosphorylation, Listeriosis, Biology (General), Post-Translational Modification, Phosphorylation, Host cell cytosol, Immune System Proteins, Virulence, Kinase, Cell biology, Bacterial Pathogens, Physical sciences, Chemistry, Medical Microbiology, Pathogens, Cellular Structures and Organelles, Cellular Types, Intracellular, Research Article, Cell Physiology, QH301-705.5, Virulence Factors, Immune Cells, 030106 microbiology, Blotting, Western, Immunology, Microbial Sensitivity Tests, Monomers (Chemistry), Biology, Microbiology, 03 medical and health sciences, Cell Walls, Listeria monocytogenes, Virology, Genetics, medicine, Animals, Polymer chemistry, Molecular Biology, Microbial Pathogens, Blood Cells, Macrophages, Biology and Life Sciences, Proteins, Cell Biology, RC581-607, Listeria Monocytogenes, Cyclic AMP-Dependent Protein Kinases, Cell Metabolism, Mice, Inbred C57BL, Disease Models, Animal, Parasitology, Immunologic diseases. Allergy

Abstract

Obstacles to bacterial survival and replication in the cytosol of host cells, and the mechanisms used by bacterial pathogens to adapt to this niche are not well understood. Listeria monocytogenes is a well-studied Gram-positive foodborne pathogen that has evolved to invade and replicate within the host cell cytosol; yet the mechanisms by which it senses and responds to stress to survive in the cytosol are largely unknown. To assess the role of the L. monocytogenes penicillin-binding-protein and serine/threonine associated (PASTA) kinase PrkA in stress responses, cytosolic survival and virulence, we constructed a ΔprkA deletion mutant. PrkA was required for resistance to cell wall stress, growth on cytosolic carbon sources, intracellular replication, cytosolic survival, inflammasome avoidance and ultimately virulence in a murine model of Listeriosis. In Bacillus subtilis and Mycobacterium tuberculosis, homologues of PrkA phosphorylate a highly conserved protein of unknown function, YvcK. We found that, similar to PrkA, YvcK is also required for cell wall stress responses, metabolism of glycerol, cytosolic survival, inflammasome avoidance and virulence. We further demonstrate that similar to other organisms, YvcK is directly phosphorylated by PrkA, although the specific site(s) of phosphorylation are not highly conserved. Finally, analysis of phosphoablative and phosphomimetic mutants of YvcK in vitro and in vivo demonstrate that while phosphorylation of YvcK is irrelevant to metabolism and cell wall stress responses, surprisingly, a phosphomimetic, nonreversible negative charge of YvcK is detrimental to cytosolic survival and virulence in vivo. Taken together our data identify two novel virulence factors essential for cytosolic survival and virulence of L. monocytogenes. Furthermore, our data demonstrate that regulation of YvcK phosphorylation is tightly controlled and is critical for virulence. Finally, our data suggest that yet to be identified substrates of PrkA are essential for cytosolic survival and virulence of L. monocytogenes and illustrate the importance of studying protein phosphorylation in the context of infection., Author Summary Infection with intracellular pathogens causes a majority of the global infectious disease associated mortality. A number of intracellular pathogens must directly access the host cytosol in order to cause disease; however, non-cytosol adapted bacteria do not survive or replicate upon access to the cytosol. The mechanisms cytosolic pathogens use to adapt to this niche are largely unknown. The model cytosolic bacterial pathogen Listeria monocytogenes contains a single penicillin-binding-protein and serine/threonine associated (PASTA) kinase, PrkA. In other bacteria, PASTA kinases bind cell wall fragments and phosphorylate downstream effectors involved in cell wall synthesis, central metabolism, virulence, cell division, and biofilm formation. We demonstrate that in L. monocytogenes, PrkA is required for cell wall homeostasis, growth under nutrient limiting conditions, survival and replication in host cells, and virulence in vivo. Furthermore, we identify a highly conserved protein of unknown function, YvcK, as a PrkA substrate. We demonstrate that L. monocytogenes YvcK is similarly required for cell wall stress responses, growth on glycerol, cytosolic survival and virulence in vivo. Surprisingly, a phosphomimetic, nonreversible negative charge at the phosphorylation sites on YvcK inactivates functions of the protein related to intracellular survival and virulence, suggesting that the identification of PASTA kinase substrates phosphorylated during infection will be critical to our understanding of this central regulator metabolism, cell wall homeostasis and ultimately virulence.

Published

2015