JoVE Logo
Authors
Contact Us

Sign In

A subscription to JoVE is required to view this content. Sign in or start your free trial.

In This Article

  • Summary
  • Abstract
  • Introduction
  • Protocol
  • Results
  • Discussion
  • Disclosures
  • Acknowledgements
  • Materials
  • References
  • Reprints and Permissions

Summary

This protocol describes the visualization of biofilm development following exposure to host-factors using a slide chamber model. This model allows for direct visualization of biofilm development as well as analysis of biofilm parameters using computer software programs.

Abstract

Biofilms consist of groups of bacteria encased in a self-secreted matrix. They play an important role in industrial contamination as well as in the development and persistence of many health related infections. One of the most well described and studied biofilms in human disease occurs in chronic pulmonary infection of cystic fibrosis patients. When studying biofilms in the context of the host, many factors can impact biofilm formation and development. In order to identify how host factors may affect biofilm formation and development, we used a static chambered coverglass method to grow biofilms in the presence of host-derived factors in the form of sputum supernatants. Bacteria are seeded into chambers and exposed to sputum filtrates. Following 48 hr of growth, biofilms are stained with a commercial biofilm viability kit prior to confocal microscopy and analysis. Following image acquisition, biofilm properties can be assessed using different software platforms. This method allows us to visualize key properties of biofilm growth in presence of different substances including antibiotics.

Introduction

Bacterial biofilms are groups of microorganisms that are attached to one another and encased in a self-secreted matrix.1,2 Classically, they represent bacteria physically attached to an abiotic or biotic surface formed under conditions of flow. Biofilms have also been shown to grow in static conditions (absence of flow) and distal from surfaces, such as at the air-liquid interface of thermal pools or pellicles formed in test tubes. These biofilms have long been recognized in the environment and are a major detriment to industrial processes, as they can form in water reservoirs or in pipes, resulting in biofouling, corrosion and blockages.3,4

Biofilms are also critical in healthcare settings, as they have been shown be involved in catheter related infections, pulmonary infections in cystic fibrosis patients, as well as in numerous other infections.5,6 One of the hallmarks of biofilm infections is the decreased susceptibility of bacteria to antibiotics and impaired clearance by the innate immune system.7-9 The most well studied, clinically relevant scenarios involving biofilm-based infection occurs in patients with cystic fibrosis (CF), who are chronically infected with Pseudomonas aeruginosa biofilms. P. aeruginosa can undergo a number of changes during establishment of chronic infection that make it very difficult to treat.10,11 Biofilms can differentially activate innate immunity and drive inflammation.12-14 As these infections lead to increased morbidity and mortality in CF patients, it is crucial to understand factors that can affect biofilm development in this context.

A recent study suggests that host-factors are critical in the formation of P. aeruginosa biofilm aggregates.15 These biofilms contribute to reduced susceptibility to antibiotics and host defense mechanisms. The presence of host-derived factors, such as neutrophil elastase, as well as secreted products from microorganisms present in the CF lung, have the potential to greatly modulate biofilm formation and development.16 Additionally, biofilms interact with the host to modulate expression of numerous pathways and initiate inflammation. While high throughput methods, such as the standard crystal violet assay, can provide some information with regards to the biofilm process, visualization of the biofilm in response to these factors provide more in-depth information.

In this manuscript we describe a method for using factors from the sputum of patients with CF to study the development of biofilms in vitro. This method allows for rapid visualization of biofilms exposed to sputum containing host factors using a commercial biofilm viability kit. This technique can be used to visually identify changes that occur during biofilm growth in the presence of exogenous products, and represents an improved method to analyze the changes in biofilm development under various conditions.

Protocol

Note that Research Ethics Board (REB) is required to collect and store sputum samples from human subjects. These studies were approved by the Hospital for Sick Children REB#1000019444.

1. Preparing CF Sputum Samples

  1. Collect sputum sample from patients during routine visits to the cystic fibrosis clinic and keep on ice.
  2. Transport sputum sample on ice within the first hour of collection, to the research laboratory, to undergo processing.

2. Sputum Processing

  1. Record the volume of the sputum sample obtained. Add phosphate buffered saline (PBS) to 2x the volume of the sample (i.e., 2 parts PBS, 1 part sample).
  2. Mix the sample well with a transfer pipette. Vortex the sample on the highest setting for 1 min to mix completely.
  3. Aliquot 1 ml of the above mixture into the appropriate number 1.5 ml microcentrifuge tubes and spin down at 5,000 x g for 20 min at 4 °C.
  4. Following centrifugation, remove the supernatant and discard the pellet.
  5. Filter sterilize the supernatant through a 0.22 µm filter and collect in a clean microcentrifuge tube.
    NOTE: Sterility of filtrate is tested by plating on LB agar and inoculating liquid media.
  6. Store sputum supernatant at -80 °C for future use.
    NOTE: Sputum from multiple patients can also be pooled following filtration.
  7. Prior to use, dilute sputum filtrate 1/10 v/v (100 μl of sputum, 900 μl of media) in desired media.
    NOTE: Here, standard lysogeny broth (LB) media was used.

3. Chambered Coverglass Method for Biofilm Formation

  1. Grow bacterial isolate of interest overnight in desired media at 37 °C with shaking (200 rpm).
    Note: A number of different bacteria were used, including clinical isolates Pseudomonas aeruginosa, Staphylococcus aureus, Burkholderia cepacia complex and Achromobacter xylosoxidans. Choice of media depends on strains and conditions of interest, however LB media can be used for initial experiments.
  2. From overnight culture, place 40 μl of culture into 4 ml of fresh media and grow for 3-4 hr at 37 °C with shaking (200 RPM) to obtain a culture with an optical density at 600 nm (OD600) of approximately 0.5-0.6.
  3. Dilute the culture from step 3.2 to 1/5 in desired media with 10% sputum filtrate or without sputum filtrate (as control). Other concentration of sputum filtrate can be tested (i.e., 50% or 100%).
  4. Use 200 μl of the dilution to seed wells of slide chambers.
  5. Allow bacteria to attach for 4 hr at 37 °C without shaking.
  6. After 4 hr, remove the media and gently wash the biofilm with 1x fresh media. Replace with 200 μl fresh media.
    NOTE: To study the effects of sputum on the biofilm, the fresh media should contain sputum supernatant.
  7. Allow biofilms to grow for desired amount of time at 37 °C without shaking, replacing media every 12 hr, without washing until the time for microscopy.
    NOTE: To study the effect of sputum supernatants on biofilm antibiotic susceptibility, antibiotics are added to the media following 24 hr of biofilm growth and are maintained in the media until staining and imaging of biofilms.

4. Staining Biofilms and Confocal Microscopy

  1. Following desired growth time (24-48 hr works best), remove media from chamber wells and gently wash each chamber twice with 300 μl of sterile PBS.
  2. Prepare staining mixture for biofilm by mixing 1 µl of each dye (provided in the viability kit) for each ml of solution needed. Make dye in water or media solution.
    NOTE: Water is recommended by the manufacturer.
  3. Add 200 µl of dye mixture to each well of chambered coverglass and incubate at room temperature, in the dark for 45 min.
  4. Remove staining mixture from chambers and wash each well with 300 μl of sterile PBS. Remove PBS and replace with fresh water or media.
  5. Proceed with visualization of biofilms via confocal microscopy.

5. Visualizing Biofilms with Confocal Microscopy

  1. Read stained biofilms in chambers immediately after staining (within 1 hr). Minimize delay in visualization of the slides by staining 1 to 2 8-well chambers at a time.
  2. Perform imaging using confocal microscope with lasers for excitation and filter sets for acquisition.
    NOTE: Here, the spinning disk confocal system with spectral borealis lasers (Green: 491nm, Red: 561 nm) were used for excitation. Emission filter sets of 515/40 and 624/40 were used to visualize the stains from the biofilm viability kit.
  3. Take images using a 25X water objective on confocal microscope with camera.
  4. Use Z-Stacks to model the biofilm. Take images every 0.5-1 μm starting from the first in-focus plane to the last in-focus frame of the biofilm (typically spanning 30-80 μm for 48 hr biofilms)
  5. Take 3-5 images from each well.
    NOTE: Thus for an 8 well chambered coverglass, 24-40 images will be generated.
  6. Save images for analysis.
    NOTE: Images should be saved as OME-TIFF files to be analyzed using COMSTAT18,19. Instructions for biofilm image analysis can be found at http://www.comstat.dk/. Once images are imported, parameters such as average thickness, biomass and surface coverage for each channel (red and green) can be analyzed.

Results

The overall design of the experiment is represented in Figure 1. The use of this protocol provides a convenient method to visualize the changes in biofilms grown for different periods of time (e.g., 24, 48 or 72 hr). Importantly, exogenous signals, such as sputum filtrates, can be added to visualize the changes in biofilm development. As seen in Figure 2, the presence of 10% sputum filtrates can change the architecture of the biofilm (Fig...

Discussion

The methods described herein allow for visualization of bacterial biofilms grown in the presence of exogenous products. Not surprisingly, the production of the exoproducts is of importance when using this type of system. For instance, Dithiothreitol (DTT), is often used on human sputum samples to help liquefy the samples. However, the effect of DTT alone can decrease biofilm development and viability (data not shown). Thus, proper controls for all conditions are necessary. Furthermore, the addition of human sputum produc...

Disclosures

None.

Acknowledgements

TB acknowledges a research fellowship from Cystic Fibrosis Canada.

Materials

NameCompanyCatalog NumberComments
Lab-Tek II Chambered coverglass, #1.5 borosilicate, 8-wellThermo Sicher Scientific155409
Filmtracer Live/Dead Biofilm Viabilty KitThermo Fisher ScientificL10316
Blood agar platesThermo Fisher ScientificR10215Confirming viability via CFU counts or selecting colonies for innoculation
COMSTATAvailble software onlineCOMSTAT is software to analyze biofilm images. Available www.comstat.dk 
Millers LB BrothThermo Fisher Scientific12780-052Standard media for overnight gowth/biofilm growth
Millex-GV Syringe FiltersMilliporeSLGV013SLFiltering of sputum supernants
Phosphate Buffered Saline (Dulbecco A)OxoidBR0014GWashing of biofilm chambers after media removal
Zeiss AxioVert 200MCarl Zeiss
Hamamatsu C9100-13 EM-CCDQS Technologies Inc.
Spectral BorealisQs Technologies Inc.
Perkin Elmer VolocityQS Technologies Inc.Instructions for this software can be found at: http://cellularimaging.perkinelmer.com/pdfs/manuals/VolocityuserGuide.pdf

References

  1. Beaudoin, T., Waters, V. Infections with biofilm formation: selection of antimicrobials and role of prolonged antibiotic therapy. Pediatr.Infect.Dis.J. , (2016).
  2. Donlan, R. M. Biofilms: microbial life on surfaces. Emerg.Infect.Dis. 8 (9), 881-890 (2002).
  3. Hobley, L., Harkins, C., MacPhee, C. E., Stanley-Wall, N. R. Giving structure to the biofilm matrix: an overview of individual strategies and emerging common themes. FEMS Microbiol.Rev. 39 (5), 649-669 (2015).
  4. Katharios-Lanwermeyer, S., Xi, C., Jakubovics, N. S., Rickard, A. H. Mini-review: Microbial coaggregation: ubiquity and implications for biofilm development. Biofouling. 30 (10), 1235-1251 (2014).
  5. Donlan, R. M. Biofilm formation: a clinically relevant microbiological process. Clin.Infect.Dis. 33 (8), 1387-1392 (2001).
  6. Bjarnsholt, T., et al. The in vivo biofilm. Trends Microbiol. 21 (9), 466-474 (2013).
  7. Mah, T. F., Pitts, B., Pellock, B., Walker, G. C., Stewart, P. S., O'Toole, G. A. A genetic basis for Pseudomonas aeruginosa biofilm antibiotic resistance. Nature. 426 (6964), 306-310 (2003).
  8. Mah, T. F. Biofilm-specific antibiotic resistance. Future Microbiol. 7 (9), 1061-1072 (2012).
  9. Beaudoin, T., Zhang, L., Hinz, A. J., Parr, C. J., Mah, T. F. The biofilm-specific antibiotic resistance gene ndvB is important for expression of ethanol oxidation genes in Pseudomonas aeruginosa biofilms. J. Bacteriol. 194 (12), 3128-3136 (2012).
  10. Beaudoin, T., Aaron, S. D., Giesbrecht-Lewis, T., Vandemheen, K., Mah, T. F. Characterization of clonal strains of Pseudomonas aeruginosa isolated from cystic fibrosis patients in Ontario, Canada. Can. J. Microbiol. 56 (7), 548-557 (2010).
  11. Vidya, P., et al. Chronic infection phenotypes of Pseudomonas aeruginosa are associated with failure of eradication in children with cystic fibrosis. Eur.J.Clin.Microbiol.Infect.Dis. , (2015).
  12. Beaudoin, T., Lafayette, S., Nguyen, D., Rousseau, S. Mucoid Pseudomonas aeruginosa caused by mucA mutations result in activation of TLR2 in addition to TLR5 in airway epithelial cells. Biochem.Biophys.Res.Commun. 428 (1), 150-154 (2012).
  13. Beaudoin, T., et al. The level of p38alpha mitogen-activated protein kinase activation in airway epithelial cells determines the onset of innate immune responses to planktonic and biofilm Pseudomonas aeruginosa. J.Infect.Dis. 207 (10), 1544-1555 (2013).
  14. LaFayette, S. L., et al. Cystic fibrosis-adapted quorum sensing mutants cause hyperinflammatory responses. Sci.Adv. 1 (6), e1500199 (2015).
  15. Staudinger, B. J., et al. Conditions associated with the cystic fibrosis defect promote chronic Pseudomonas aeruginosa infection. Am.J.Respir.Crit.Care Med. 189 (7), 812-824 (2014).
  16. Kennedy, S., et al. Activity of Tobramycin against Cystic Fibrosis Isolates of Burkholderia cepacia Complex Grown as Biofilms. Antimicrob.Agents Chemother. 60 (1), 348-355 (2015).
  17. Tom, S. K., Yau, Y. C., Beaudoin, T., LiPuma, J. J., Waters, V. Effect of High-Dose Antimicrobials on Biofilm Growth of Achromobacter Species Isolated from Cystic Fibrosis Patients. Antimicrob.Agents Chemother. 60 (1), 650-652 (2015).
  18. Heydorn, A., et al. Quantification of biofilm structures by the novel computer program COMSTAT. Microbiology. 146 (Pt 10), 2395-2407 (2000).
  19. Vorregaard, M. . Informatics and Mathematical Modelling. , (2008).
  20. Jurcisek, J. A., Dickson, A. C., Bruggeman, M. E., Bakaletz, L. O. In vitro Biofilm Formation in an 8-well Chamber Slide. J. Vis. Exp. (47), e2481 (2011).

Reprints and Permissions

Request permission to reuse the text or figures of this JoVE article

Request Permission

Explore More Articles

BiofilmSputumAntibioticsBacterial BiofilmsBiofilm DevelopmentChambered CoverglassMicroscopyViability StainingLuria BrothOptical DensityCentrifugationFiltrationPBS

This article has been published

Video Coming Soon

JoVE Logo

Privacy

Terms of Use

Policies

Contact Us

Recommend to library

JoVE NEWSLETTERS

Research

Education

Authors

Librarians

ABOUT JoVE

Copyright © 2025 MyJoVE Corporation. All rights reserved