The EPS matrix: the "house of biofilm cells".
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J Bacteriol 189(22): 7945-7947

The EPS Matrix: The “House of Biofilm Cells”<sup><a href="#fn1" rid="fn1" class=" fn">▿</a></sup>

Biofilm Centre, University of Duisburg-Essen, Geibelstrasse 41, D-47057 Duisburg, Helmholtz Centre for Environmental Research—UFZ, Brueckstr. 3a, D-39114 Magdeburg, Germany, Wake Forest University, School of Medicine, Winston-Salem, North Carolina 271573
Corresponding author. Mailing address: Wake Forest University School of Medicine, Microbiology and Immunology, Medical Center Boulevard, Winston-Salem, NC 27157. Phone: (336) 716-2016. Fax: (336) 716-9928. E-mail: ude.cmbufw@kainzowd

In response to a suggestion by the Biofilms 2007 organizing committee to hold an evening session on biofilm extracellular polymeric substances (EPS), an exceptionally inspiring event followed contributions by Ken Bayles, Alan Decho, Martina Hausner, Jan Kreft, Thomas Neu, Per Nielsen, Ute Römling, Sarah Schooling, Ulrich Szewzyk, Gideon Wolfaardt, and Liang Yang. The essence of the evening's discussion, moderated by Hans-Curt Flemming and Daniel J. Wozniak, is summarized below.

If biofilms can be metaphorically called a “city of microbes” (24), the EPS represent the “house of the biofilm cells.” The EPS determine the immediate conditions of life of biofilm cells living in this microenvironment by affecting porosity, density, water content, charge, sorption properties, hydrophobicity, and mechanical stability (6).

EPS are biopolymers of microbial origin in which biofilm microorganisms are embedded. In fact, archaeal, bacterial, and eukaryotic microbes produce the biopolymers. Contrary to common belief, EPS are certainly more than only polysaccharides. They comprise, in addition, a wide variety of proteins, glycoproteins, and glycolipids, and in some cases, surprising amounts of extracellular DNA (e-DNA). In environmental biofilms, polysaccharides are frequently only a minor component (7). Unfortunately, it remains a substantial challenge to provide a complete biochemical profile of most EPS samples. It is often difficult to purify EPS matrix constituents apart from other components such as cells or other macromolecules transiently associated with the EPS (16). In addition, carbohydrate chemical analyses remain difficult, due to the diversity in sugar monomers, linkages, and unique structures present in the carbohydrate fraction of the EPS matrix material. Nonetheless, all EPS biopolymers are highly hydrated and form a matrix, which keeps the biofilm cells together and retains water. This matrix interacts with the environment, e.g., by attaching biofilms to surfaces and through its sorption properties, which allow for sequestering of dissolved and particulate substances from the environment, providing nutrients for biofilm organisms. The EPS influence predator-prey interactions, as demonstrated in a system consisting of a predatory ciliate and yeast cells, in which grazing led to an increase in biofilm mass and viability, with EPS as the preferred food source (9).

Some EPS components deserve particular attention. Alginate, a polyanion polysaccharide, is the best-investigated component of mucoid Pseudomonas aeruginosa biofilms. However, several recent reports have shown that other polysaccharides contribute to biofilms formed by nonmucoid P. aeruginosa strains, which are believed to be the first to colonize cystic fibrosis patients. A recent example is the expression of the psl operon, which is required in order to maintain the biofilm structure after attachment. Overproduction of the Psl polysaccharide led to enhanced cell surface and intercellular adhesion of P. aeruginosa, which translated into significant changes in the architecture of the biofilm (14). Nevertheless, other polysaccharides produced by Pseudomonas spp., such as levan, may have a role in biofilm formation (13). P. aeruginosa has been widely used by many biofilm researchers; it is, metaphorically speaking, the Escherichia coli of biofilm research. However, during this session, it was clearly pointed out that this perspective is limited and that extrapolation from P. aeruginosa biofilm results to biofilms in general, while tempting, is not suitable. Environmental biofilms contain surprisingly low levels of alginate. Even charged polysaccharides seem to be relatively rare in nature, as determined by uronic acid analysis. In environmental biofilms, it is extremely difficult to isolate and characterize specific polysaccharides in detail, as Alan Decho pointed out, expressing the experience of many researchers. The production of EPS in natural biofilms is dynamic and can follow cyclic patterns, as demonstrated in marine stromatolites (5). Currently the only in situ approach to EPS glycoconjugates is the use of fluorescently labeled lectins (15). An interesting role in influencing biofilm structure may be that of cellulose, formed by a variety of organisms. Cellulose is also important in infectious processes when coexpressed with curli fimbriae in E. coli (23). Curli as proteinaceous fibrils have attracted interest beyond infection, because curli-like fibrils have also been found to play an important role in natural biofilms produced by a variety of microorganisms. Larsen et al. (12) have found an abundance of amyloid adhesins in natural biofilms, which may contribute considerably to their mechanical properties. Strengthening of the biofilm structure is crucial for the stability of the “house” and the continuation of synergistic interactions based on the spatial proximity of various biofilm organisms. Cellulose has been found to be a component of EPS in amoebae, algae, and bacteria. In agrobacteria, cellulose is involved in attachment. It appears that cellulose plays an underestimated role in environmental EPS.

Biofilms are also an ideal place for exchanging genetic material and maintaining a large and accessible gene pool. Horizontal gene transfer is facilitated, since the cells are maintained in close proximity to each other, are not fully immobilized, and can exchange genetic information. In 1999, Hausner and Wuertz reported significantly higher rates of conjugation in bacterial biofilms than in planktonic populations (8). Recently, however, nucleic acids have attracted more attention. A focus of particular interest during the evening session was the observation of e-DNA within biofilms. Although e-DNA has been reported as a component of biofilms for quite some time, it is commonly considered a remnant of lysed cells. However, e-DNA occurs in sufficiently high quantities to raise some doubt. In fact, Palmgren and Nielsen reported in 1996 the accumulation of DNA in the EPS matrix of activated sludge and pure cultures of Pseudomonas putida (17). Allesen-Holm et al. (1) found that in P. aeruginosa biofilms, the e-DNA is likely derived from whole genomic DNA. Surprisingly, e-DNA was organized in distinct patterns in the biofilms of this organism, forming grid-like structures, suggesting a structural role for e-DNA. The observations of Böckelmann et al. (3), who report the formation of e-DNA as a spatial structure forming a filamentous network in biofilms of an aquatic bacterium, strongly support and differentiate such considerations. The e-DNA had similarities to genomic DNA but also distinct differences. It seemed as if the cells could move along these filaments, using them as nanowires. In the discussion session, speculations were welcome; one was that the cells might use the filaments for electron transfer and even for communication. Yang et al. (25) also found that e-DNA was one of the major matrix components in P. aeruginosa biofilms, functioning as an intercellular connector; they supported the concept of the stabilizing role of e-DNA for the biofilm matrix. In P. aeruginosa, the release of e-DNA is under the control of quorum-sensing systems as well as iron regulation (1, 25). In Staphylococcus aureus biofilms, cidA-controlled cell lysis plays a significant role during biofilm development and releases genomic DNA, which serves as an important structural component of S. aureus biofilms (18). A very interesting question is the mobility of DNA in the matrix. After all, from an energetic point of view, DNA is an expensive molecule, and Matt Parsek put the very justified question of what advantage makes such an effort affordable for the cells.

Not only is the EPS matrix composed of a variety of components, but these components are able to interact. One example is the retention of extracellular proteins such as lipase by alginate (6). Such mechanisms are crucial for preventing the washout of enzymes, keeping them close to the cells that produced them and allowing for effective degradation of polymeric and particulate material. This leads to the concept of an “activated matrix.” Activation is made even more dynamic and versatile by the release of membrane vesicles (MV). These highly ordered nanostructures act as “parcels” containing enzymes and nucleic acids, sent into the depth of the EPS matrix (20). Such MV, along with phages and viruses, which are similar in size, can serve as carriers for genetic material, thereby enhancing gene exchange. Through their chemistry, the MV may bind extraneous components; their enzymes may help degrade polymers, provide nutrients, and permit enhanced resistance to certain inimical agents by inactivating them. Furthermore, MV seem to be part of “biological warfare” within biofilms, occurring as predatory vesicles containing lytic enzymes. This biological warfare is also long-range; in common with other matrix material, MV are shed from the biofilm and thus may deliver, among other things, virulence factors and cell-to-cell signals.

The composition, architecture, and function of the EPS matrix, as discussed in this evening session, revealed a very complex, dynamic, and biologically exciting view. The matrix is a network providing sufficient mechanical stability to maintain a spatial arrangement for microconsortia over a prolonged period. This stability is provided by hydrophobic interactions, cross-linking by multivalent cations, and entanglements of the biopolymers (6, 10), with e-DNA as a newly appreciated structural component. Thomas Neu and John Lawrence tried to systematically arrange the information on EPS components and functions (Table (Table11).

TABLE 1.

EPS functionalitya

Effect of EPS componentNature of EPS componentRole in biofilm
ConstructiveNeutral polysaccharidesStructural component
AmyloidsStructural component
SorptiveCharged or hydrophobic polysaccharidesIon exchange, sorption
ActiveExtracellular enzymesPolymer degradation
Surface-activeAmphiphilicInterface interactions
Membrane vesiclesExport from cell, sorption
InformativeLectinsSpecificity, recognition
Nucleic acidsGenetic information, structure
Redox activeBacterial refractory polymersElectron donor or acceptor?
NutritiveVarious polymersSource of C, N, P
Discussion contribution of T. Neu, based on a prior version published by Allison et al. (2) and completed by the results of the discussion.

While Table Table11 is not complete, it reflects the variety of functions of EPS in the matrix. The discussion section revealed that many aspects of EPS remain to be addressed. An example is their function in biocide resistance (21). Also, the manifold ways in which the biofilm cells can modify their matrix, including production of EPS by various organisms, extracellular enzymatic EPS turnover and modification, and the resulting spatial and temporal heterogeneity, have not been addressed. In this context, species dynamics is crucial, since different species produce different EPS.

In the context of this complexity, modeling of EPS seems to be an almost impossible task, although it would be extremely helpful in predicting and controlling biofilm processes. Consequently, Jan Kreft asked for EPS research to provide more data, which would help to establish and optimize the existing models (11). Determining the rate of EPS production would be a useful task providing such data and giving information about parameters such as the creation of more biovolume. Some of the methods developed by EPS research, such as the use of fluorescent biomarkers, may contribute to the data demanded by modelers.

In conclusion, it appears that “slime” has been very much underestimated. It may turn out that the EPS matrix is considerably more than simply the glue for biofilms. Rather, it appears to be a highly sophisticated system, which endows the biofilm mode of life with particular, successful features. More information about the specific components of the biofilm EPS, as well as their localization and stability, will likely support Costerton and Irvin's visionary concept of “biofilm as a tissue” in 1981, when EPS still was called the “glycocalyx” (4). In this regard, there exciting evidence is emerging that in several microbial communities, EPS often has a defined macromolecular “honeycomb” structure (19, 22).

We are only beginning to understand the construction principles, functions, and dynamics of the “house of the cells.” Further understanding requires more-sensitive and less-destructive new methods, which will allow for the investigation of biofilm processes in situ over time. Then we can better understand what the “house of biofilm cells” is built of and what its functions are.

Notes

The views expressed in this Commentary do not necessarily reflect the views of the journal or of ASM.

Notes
The views expressed in this Commentary do not necessarily reflect the views of the journal or of ASM.

Footnotes

Published ahead of print on 3 August 2007.

Footnotes

REFERENCES

REFERENCES

References

  • 1. Allesen-Holm, M., K. B. Barken, L. Yang, M. Klausen, J. S. Webb, S. Kjelleberg, S. Molin, M. Givskov, and T. Tolker-Nielsen. 2006. A characterization of DNA release in Pseudomonas aeruginosa cultures and biofilms. Mol. Microbiol.59:1114-1128. [[PubMed]
  • 2. Allison, D. G., I. W. Sutherland, and T. R. Neu. 2003. EPS: what's an acronym? p. 381-387. In A. McBain, D. Allison, M. Brading, A. Rickard, J. Verran, and J. Walker (ed.), Biofilm communities: order from chaos? BioLine, Cardiff, United Kingdom.
  • 3. Böckelmann, U., A. Janke, R. Kuhn, T. R. Neu, J. Wecke, J. R. Lawrence, and U. Szewzyk. 2006. Bacterial extracellular DNA forming a defined network-like structure. FEMS Microbiol. Lett.262:31-38. [[PubMed]
  • 4. Costerton, J. W., and R. T. Irvin. 1981. The bacterial glycocalyx in nature and disease. Annu. Rev. Microbiol.35:299-324. [[PubMed]
  • 5. Decho, A. W., P. T. Visscher, and P. P. Reid. 2005. Production and cycling of natural microbial extracellular polymers (EPS) within a marine stromatolite. Paleogeogr. Paleoclimat. Paleoecol.219:71-88. [PubMed]
  • 6. Flemming, H.-C., and JWingender. 2002. Extracellular polymeric substances: structure, ecological functions, technical relevance, p. 1223-1231. In G. Bitton (ed.), Encyclopedia of environmental microbiology, vol. 3. Wiley, New York, NY. [PubMed][Google Scholar]
  • 7. Frølund, B., R. Palmgren, K. Keiding, and P. H. Nielsen. 1996. Extraction of extracellular polymers from activated sludge using a cation exchange resin. Water Res.30:1749-1758. [PubMed]
  • 8. Hausner, M., and SWuertz. 1999. High rates of conjugation in bacterial biofilms as determined by quantitative in-situ analysis. Appl. Environ. Microbiol.65:3710-3713. [Google Scholar]
  • 9. Joubert, L.-M., G. M. Wolfaardt, and A. Botha. 2006. Microbial exopolymers link predator and prey in a biofilm system. Microb. Ecol.52:187-197. [[PubMed]
  • 10. Klausen, M. M., T. R. Thomsen, J. L. Nielsen, L. H. Mikkelsen, and P. H. Nielsen. 2004. Variations in microcolony strength of probe-defined bacteria in activated sludge flocs. FEMS Microbiol. Ecol.50:123-132. [[PubMed]
  • 11. Kreft, J.-U., and J. W. T. Wimpenny. 2001. Effect of EPS on biofilm structure and function as revealed by an individual-based model of biofilm growth. Water Sci. Technol.43:135-141. [[PubMed]
  • 12. Larsen, P., J. L. Nielsen, M. S. Dueholm, R. Wetzel, D. Otzen, and P. H. Nielsen. Amyloid adhesins are abundant in natural biofilms. Environ. Microbiol. [Epub ahead of print.] doi:10.1111/j.1462-2920.2007.01418.x. [] [[PubMed]
  • 13. Laue, H., A. Schenk, L. Hongqiao, L. Lambertsen, T. R. Neu, S. Molin, and M. Ullrich. 2006. Contribution of alginate and levan to biofilm formation by Pseudomonas syringae. Microbiology152:2909-2918. [[PubMed]
  • 14. Ma, L., K. D. Jackson, R. M. Landry, M. R. Parsek, and D. J. Wozniak. 2006. Analysis of Pseudomonas aeruginosa conditional Psl variant reveals roles for the Psl polysaccharide in adhesion and maintaining biofilm structure postattachment. J. Bacteriol.188:8213-8221.
  • 15. Neu, T. R., and J. R. Lawrence. 1999. Lectin-binding-analysis in biofilm systems. Methods Enzymol.310:145-152. [[PubMed]
  • 16. Nielsen, P. H., and A. Jahn. 1999. Extraction of EPS, p. 49-72. In J. Wingender, T. R. Neu, and H.-C. Flemming (ed.), Microbial extracellular polymeric substances. Springer, Berlin, Germany.
  • 17. M. Palmgren, R., and P. H. Nielsen. 1996. Accumulation of DNA in the exopolymeric matrix of activated sludge and bacterial cultures. Water Sci. Technol.34:233-240. [PubMed]
  • 18. Rice, K. C., E. E. Mann, J. L. Endres, E. C. Weiss, J. E. Cassat, M. S. Smeltzer, and K. W. Bayles. 2007. The cidA murein hydrolase regulator contributes to DNA release and biofilm development in Staphylococcus aureus. Proc. Natl. Acad. Sci. USA104:8113-8118.
  • 19. Schaudinn, C., P. Stoodley, A. Kainovic, T. O'Keefe, B. Costerton, D. Robinson, M. Baum, G. Erlich, and P. Webster. 2007. Bacterial biofilms, other structures seen as mainstream concepts. Microbe2:231-237. [PubMed]
  • 20. Schooling, S. R., and T. J. Beveridge. 2006. Membrane vesicles: an overlooked component of the matrices of biofilms. J. Bacteriol.188:5945-5947.
  • 21. Schulte, S., J. Wingender, and H.-C. Flemming. 2005. Efficacy of biocides against biofilms, p 90-120. In W. Paulus (ed.), Directory of microbicides for the protection of materials and processes. Kluwer Academic Publishers, Dordrecht, The Netherlands.
  • 22. Thar, R., and MKuhl. 2002. Conspicuous veils formed by vibrioid bacteria on sulfidic marine sediment. Appl. Environ. Microbiol.68:6310-6320. [Google Scholar]
  • 23. Wang, X., M. Rochon, A. Lamprokostopoulou, H. Lünsdorf, M. Nimtz, and U. Römling. 2006. Impact of biofilm matrix components on interaction of commensal Escherichia coli with the gastrointestinal cell line HT-29. Cell. Mol. Life Sci.63:2352-2363. [[PubMed]
  • 24. Watnick, P., and RKolter. 2000. Biofilm, city of microbes. J. Bacteriol.182:2675-2679. [Google Scholar]
  • 25. Yang, L., K. B. Barken, M. E. Skindersoe, A. B. Christensen, M. Givskov, and T. Tolker-Nielsen. 2007. Effects of iron on DNA release and biofilm development by Pseudomonas aeruginosa. Microbiology153:1318-1328. [[PubMed]
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