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Characterizing Multidrug Efflux Systems in Acinetobacter baumannii Using an Efflux-Deficient Bacterial Strain and a Single-Copy Gene Expression System
In This Article
Summary
We describe a facile procedure for the single-copy chromosomal complementation of an efflux pump gene using a mini-Tn7-based expression system into an engineered efflux-deficient strain of Acinetobacter baumannii. This precise genetic tool allows for controlled gene expression, which is key for the characterization of efflux pumps in multidrug resistant pathogens.
Abstract
Acinetobacter baumannii is recognized as a challenging Gram-negative pathogen due to its widespread resistance to antibiotics. It is crucial to comprehend the mechanisms behind this resistance to design new and effective therapeutic options. Unfortunately, our ability to investigate these mechanisms in A. baumannii is hindered by the paucity of suitable genetic manipulation tools. Here, we describe methods for utilizing a chromosomal mini-Tn7-based system to achieve single-copy gene expression in an A. baumannii strain that lacks functional RND-type efflux mechanisms. Single-copy insertion and inducible efflux pump expression are quite advantageous, as the presence of RND efflux operons on high-copy number plasmids is often poorly tolerated by bacterial cells. Moreover, incorporating recombinant mini-Tn7 expression vectors into the chromosome of a surrogate A. baumannii host with increased efflux sensitivity helps circumvent interference from other efflux pumps. This system is valuable not only for investigating uncharacterized bacterial efflux pumps but also for assessing the effectiveness of potential inhibitors targeting these pumps.
Introduction
Acinetobacter baumannii is a World Health Organization top priority pathogen due to its encompassing resistance to all classes of antibiotics1. It is an opportunistic pathogen mostly affecting hospitalized, injured, or immunocompromised people. A. baumannii largely evades antibiotics via efflux pumps, the most relevant being the Resistance-Nodulation-Division (RND) family of exporters2. Understanding how these efflux pumps work mechanistically will allow one to develop targeted therapeutic options.
One common way that cellular processes can be specifically distinguis....
Protocol
1. Experimental preparation
- Purify the plasmid pUC18T-mini-Tn7T-LAC-Gm9 (insertion plasmid, Figure 2A) with the gene of interest.
NOTE: Here, the gene of interest is adeIJK. The final plasmid concentration should be ≥100 ng/µL. - Purify the helper plasmid (pTNS2)9 and the excision plasmid (pFLP2ab)6 (Figure 2B.......
Representative Results
The chromosomal insertion procedure takes only 2 h total across 3 days to see a result-colonies growing on a selective agar plate (Figure 1A-C). The expected number of colonies on the transformation plate is strain dependent: one may see 20-30 or even hundreds of colonies as insertion of Tn7 at attTn7 sites is specific and efficient9. Patching transformation plate colonies onto selective media (Figure 4A<.......
Discussion
Even though this procedure for the chromosomal insertion of an inducible single-copy gene expression system in A. baumannii is technically straightforward and not labor-intensive, there are a few important steps that need to be emphasized. First, preparation of the competent cells needs to be done on ice as much as possible as the cells become fragile during the replacement of the media with ice-cold water. Ideally, the centrifugation steps are performed at 4 °C, but centrifugation at room temperature is ac.......
Acknowledgements
This work was supported by a Discovery Grant from the Natural Science and Engineering Council of Canada to AK. The schematics used in the figures are created with BioRender.com.
....Materials
| Name | Company | Catalog Number | Comments |
| 0.2 mL PCR tube | VWR | 20170-012 | For colony boil preparations and PCR reactions |
| 1.5 mL microfuge tubes | Sarstedt | 72-690-301 | General use |
| 13-mL culture tubes, Pyrex | Fisher | 14-957K | Liquid culture vessels |
| 6x DNA loading buffer | Froggabio | LD010 | Agarose gel electrophoresis sample loading dye |
| Acetic acid, glacial | Fisher | 351271-212 | Agarose gel running buffer component |
| Agar | Bioshop | AGR003 | Solid growth media |
| Agarose | BioBasic | D0012 | Electrophoretic separation of PCR reaction products; used at a concentration of 0.8–2% |
| Agarose gel electrophoresis unit | Fisher | 29-237-54 | Agarose gel electrophoresis; separation of PCR reaction products |
| Carbenicillin | Fisher | 50841231 | Selective media |
| Culture tube closures | Fisher | 13-684-138 | Stainless steel closure for 13-mL culture tubes |
| Deoxynucleotide triphosphate (dNTP) set | Biobasic | DD0058 | PCR reaction component; supplied as 100 mM each dATP, dCTP, dGTP, dTTP; mixed and diluted for 10 mM each dNTP |
| Dry bath/block heater | Fisher | 88860023 | Isotemp digital dry bath for boil preparations |
| Electroporation cuvettes | VWR | 89047-208 | 2 mm electroporation cuvettes with round cap |
| Electroporator | Cole Parmer | 940000009 | 110 VAC, 60 Hz electroporator |
| Ethidium bromide | Fisher | BP102-1 | Visualization of PCR reaction products and DNA marker in agarose gel |
| Ethylenediaminetetraacetic acid (EDTA) | VWR | CA-EM4050 | Agarose gel running buffer component |
| Gentamicin | Biobasic | GB0217 | For the preparation of selective media |
| Glycerol | Fisher | G33 | Preparation of bacterial stocks for long-term storage in an ultra-low freezer |
| Incubator (shaking) | New Brunswick Scientific | M1352-0000 | Excella E24 Incubator Shaker for liquid culture growth |
| Incubator (static) | Fisher | 11-690-550D | Isotemp Incubator Oven Model 550D for solid (LB agar) culture growth |
| Inoculation loop | Sarstedt | 86.1562.050 | Streaking colonies onto agar plates |
| Inoculation spreader | Sarstedt | 86.1569.005 | Spreading of culture onto agar plates |
| Lysogeny broth (LB) broth, Lennox | Fisher | BP1427 | Liquid growth media (20 g/L: 5 g/L sodium chloride, 10 g/L tryptone, 5 g/L yeast extract) |
| Microfuge | Fisher | 75002431 | Sorvall Legend Micro 17 for centrifugation of samples |
| Mini-centrifuge | Fisher | S67601B | Centrifugation of 0.2 mL PCR tubes |
| Petri dishes | SPL Life Sciences | 10090 | For solid growth media (agar plates): 90 x 15 mm |
| Pipettes | Mandel | Various | Gilson single channel pipettes (P10, P20, P200, P1000) |
| Power supply | Biorad | 1645050 | PowerPac Basic power supply for electrophoresis |
| Primers | IDT | NA | PCR reaction component; specific to gene of interest; prepared at 100 μM as directed on the product specification sheet |
| Sucrose | BioBasic | SB0498 | For the preparation of counterselective media for removal of the pFLP2ab plasmid from transformed A. baumannii |
| Taq DNA polymerase | FroggaBio | T-500 | PCR reaction component; polymerase supplied with a 10x buffer |
| Thermal cycler | Biorad | 1861096 | Model T100 for PCR |
| Toothpicks | Fisher | S24559 | For patching colonies onto agar plates |
| Trizma base | Sigma | T1503 | Agarose gel running buffer component |
| Ultrapure water | Millipore Sigma | ZLXLSD51040 | MilliQ water purification system: ultra pure water for media and solution preparation, and cell washing |
| Wide range DNA marker | Biobasic | M103R-2 | Size determination of PCR products on an agarose gel |
| Wooden inoculating sticks | Fisher | 29-801-02 | Inoculating cultures with colonies from agar plates |
References
- Prioritization of pathogens to guide research, discovery, research and development of new antibiotics for drug-resistant bacterial infections, including tuberculosis. World Health Organization Available from: https://www.who.int/publications/i/item/WHO-EMP-IAU-2017.12 (2017)
- Kornelsen, V., Kumar, A. Update on multidrug resistance efflux pumps in Acinetobacter spp.
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