Quantifying Yersinia pseudotuberculosis Type III Secretion System Activity Following Iron Starvation and Anaerobic Growth
Summary
Bacteria colonize host tissues that vary in oxygen and iron bioavailability, yet most approaches to studying bacteria use aerated, rich media. This protocol describes culturing the human pathogen Yersinia pseudotuberculosis under varying iron concentrations and oxygen tension, and quantifying activity of the Yersinia type III secretion system, which is an important virulence factor.
Abstract
A key virulence mechanism for many Gram-negative pathogens is the type III secretion system (T3SS), a needle-like appendage that translocates cytotoxic or immunomodulatory effector proteins into host cells. The T3SS is a target for antimicrobial discovery campaigns since it is accessible extracellularly and largely absent from non-pathogenic bacteria. Recent studies demonstrated that the T3SS of Yersinia and Salmonella are regulated by factors responsive to iron and oxygen, which are important niche-specific signals encountered during mammalian infection. Described here is a method for iron starvation of Yersinia pseudotuberculosis, with subsequent optional supplementation of inorganic iron. To assess the impact of oxygen availability, this iron starvation process is demonstrated under both aerobic and anaerobic conditions. Finally, incubating the cultures at the mammalian host temperature of 37 °C induces T3SS expression and allows quantification of Yersinia T3SS activity by visualizing effector proteins released into the supernatant. The steps detailed here offer an advantage over the use of iron chelators in the absence of iron starvation, which is insufficient for inducing robust iron starvation, presumably due to efficient Yersinia iron uptake and scavenging systems. Likewise, acid-washing laboratory glassware is detailed to ensure the removal of residual iron, which is essential for inducing robust iron starvation. Additionally, using a chelating agent is described to remove residual iron from media, and culturing the bacteria for several generations in the absence of iron to deplete bacterial iron stores. By incorporating standard protocols of trichloroacetic acid-induced protein precipitation, SDS-PAGE, and silver staining, this procedure demonstrates accessible ways to measure T3SS activity. While this procedure is optimized for Y. pseudotuberculosis, it offers a framework for studies in pathogens with similar robust iron uptake systems. In the age of antibiotic resistance, these methods can be expanded to assess the efficacy of antimicrobial compounds targeting the T3SS under host-relevant conditions.
Introduction
Many clinically relevant Gram-negative pathogens like Yersinia, Vibrio, Escherichia, Pseudomonas, and Shigella encode the type III secretion system (T3SS) to inject effector proteins into host cells1. In many bacterial species, the T3SS is under strict regulatory control2. For example, translocation of Yersinia T3SS effector proteins into target host cells is critical to subvert host defense mechanisms and enable bacterial colonization of host tissues. However, Yersinia T3SS activity is metabolically burdensome and can trigger recognition by host immune receptors3. Accordingly, regulators that sense specific environmental cues control the expression of T3SS genes in many bacterial species. As pathogens such as Yersinia experience environmental changes during their infection cycle that impact the expression of critical virulence factors, it is important to develop laboratory conditions that mimic salient features of host niches occupied by bacterial pathogens. Specifically, oxygen tension and iron availability differ among various tissue sites in a spatiotemporal manner and impact the expression of virulence genes such as the T3SS4,5,6. Therefore, the goal of this method is to assess how oxygen and iron impact the expression of the Yersinia T3SS. This will provide insight into the dynamics of the host-pathogen interaction.
The method described here details how to culture Yersinia pseudotuberculosis aerobically and anaerobically, as well as how to deplete Yersinia iron stores during aerobic or anaerobic growth. There are a few important considerations highlighted here regarding successfully culturing bacteria under these variable conditions. First, anaerobic culturing requires additional glucose supplementation, a modification that is noted in the media recipe. Second, since Y. pseudotuberculosis employs siderophores and other iron uptake systems that can robustly scavenge iron from the environment, special attention is devoted to ensuring the culture media and laboratory glassware are as free of iron as possible7. Previous studies have used iron chelators such as dipyridyl to deplete iron from rich-media bacterial cultures to mimic iron starvation8,9. However, depleting Yersinia iron stores to induce iron starvation requires the removal of residual iron in glassware and media as well as prolonged growth in the absence of iron. This protocol details how to acid wash glassware and chelate media to remove residual iron, in addition to culturing the bacteria for several generations to ensure thorough iron starvation. Iron starvation can be ensured by measuring relative transcript levels of well-characterized iron-responsive genes across conditions, as demonstrated here with yfeA, and bfd.
The culmination of this protocol demonstrates how to precipitate secreted T3SS effector proteins from each of these conditions by treating the culture supernatant with trichloroacetic acid (TCA) and visualizing secreted proteins through SDS-PAGE. Finally, relative T3SS activity is assessed by visualizing secreted proteins via silver staining and quantifying relative levels of T3SS effector proteins, referred to as Yersinia outer proteins (Yops)10.
T3SS activity assays generally utilize specific antibodies to detect T3SS effector protein levels in the culture supernatant. However, western blotting antibodies for T3SS effector proteins are often not commercially available. Therefore, special attention has been taken to ensure that the final visualization of T3SS activity in this method does not require specific antibodies, and instead can leverage silver staining, which allows for the visualization of all secreted proteins. While this method is specifically tailored and optimized for Y. pseudotuberculosis, it can be adapted to other bacterial species, though the exact media conditions and incubation times will vary.
Protocol
Representative Results
Discussion
The T3SS is an important virulence factor in many pathogenic bacteria; therefore, developing laboratory techniques to study its regulation is important for understanding pathogenesis and developing potential therapeutics1. Iron and oxygen are known to be important host cues sensed by bacterial pathogens to regulate T3SS expression5; therefore, this method presents a strategy for culturing Y. pseudotuberculosis under either anaerobic or aerobic conditions, with iron…
Disclosures
The authors have nothing to disclose.
Acknowledgements
Graphical Images created using BioRender.com. This study was supported by the National Institutes of Health (www.NIH.gov) grant R01AI119082.
Materials
| 10 mL Luer-Lok Tip syringe | BD | 301029 | |
| 10x SDS Running Buffer | Home made | 0.25 M Tris base, 1.92 M Glycine, 1% SDS in 1 L volume | |
| 12.5% SDS-Page Gel | Home made | ||
| 15 mL culture tubes | Falcon | 352059 | For initial overnight |
| 15 mL Falcon tubes | Falcom | 352196 | For supernatant collection |
| 250 mL culture flask | Belco | 251000250 | |
| 500 mL Filter System | Corning | 431097 | |
| 6 N Hydrochloric acid solution | Fisher Scientific | 7732185 | |
| Acetone | Fisher Chemical | A949-4 | 4 L |
| Bio Rad ChemiDoc MP Imaging System | Bio Rad | Model Number: Universal Hood III | |
| Borosilicate glass culture tubes | Fisherbrand | 14-961-34 | For anaerobic culturing |
| Chelex 100 Resin | Bio Rad | 142-1253 | |
| Chelex M9 +0.9% Glucose media | Home made | 6 g/L Na2HPO4, 3 g/L KH2PO4, 0.5 g/L NaCl, 1 g/L NH4Cl, 1% casamino acids, 0.9% dextrose, 0.0005% thiamine, 5 g/L Chelex 100 Resin. Stir media for 18 h at room temp, filter using 500 mL Corning filtration unit, then add MgSO4 for 1 mM MgSO4 final solution | |
| Final Sample Buffer (FSB) | Home made | 0.1 M Tris-HCl, 4% SDS, 20% glycerol, 0.2% of Bromophenol Blue | |
| FSB:DTT solution | Home made | FSB+0.2M DTT | |
| Image Lab Software | Bio Rad | https://www.bio-rad.com/en-us/product/image-lab-software?ID=KRE6P5E8Z | Software |
| Isotemp Heat Block | Fisher Scientific | 88860021 | |
| LB Agar Plates | Home made | 10 g Tryptone, 5 g Yeast extract, 10 g NaCl, 15 g Agar in 1 L total volume. Autoclaved | |
| M9+0.2% Glucose Media | Home made | 6 g/L Na2HPO4, 3 g/L KH2PO4, 0.5 g/L NaCl, 1 g/L NH4Cl, 1 mM MgSO4, 1 mg/L FeSO47H2O, 1% casamino acids, 0.2% dextrose, 0.0005% thiamine | |
| Millex-GP PES 0.22um filter attachment for syringe | Millipore | SLGPR33RS | For FeSO47H2O filtration |
| Millex-GV PVDF 0.22um filter attachment for syringe | Millipore | SLGVR33RS | For supernatant filtration |
| Precision Plus Protein Unstained Standard | Bio Rad | 1610363 | |
| SDS-PAGE Gel Apparatus | Bio Rad | Model Number: Mini PROTEAN Tetra Cell | |
| SilverXpress Silver Staining Kit | Invitrogen | LC6100 | |
| The BellyDancer Shaker | IBI Scientific | BDRAA1155 | |
| Trichloroacetic acid solution 6.1N | Sigma Aldrich | T0699 | |
| Vinyl Anaerobic Chamber | Coy Lab Products | https://coylab.com/products/anaerobic-chambers/vinyl-anaerobic-chambers/#details | |
| qPCR Primer sequences | |||
| yfeA forward – CAC AGT CAG CAG ACC TTA TCT T | |||
| yfeA reverse – GGC AGA CGG GAC ATC TTT AAT A | |||
| bfd forward – ccagcatcagccccatacag | |||
| bfd reverse – tggcttgtcggatgcacttc | |||
| yopE forward – CCATAAACCGGTGGTGAC | |||
| yopE reverse – CTTGGCATTGAGTGATACTG |
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