Abstract
The quorum sensing signals—acyl homoserine lactones (AHLs) were directly detected in 1-9-day-old subtidal biofilms developed in a coastal fish farm by using AHL reporter strains and gas chromatography–mass spectrometry. Both methods showed that the AHL molecules and/or AHL-producing bacterial community were dynamic during biofilm development, with dominant AHLs changed from short-chain to long-chain AHLs. Terminal restriction fragment length polymorphism analysis of the bacterial 16S rRNA genes derived from subtidal biofilms of different ages was compared to that of the 21 AHL-producing bacteria isolated from the same batch of subtidal biofilms. All terminal restriction fragments (TRFs) generated from AHL-producing bacteria matched with the dominant TRFs derived from the biofilm bacterial community samples. Particularly, the TRFs of all AHL-producing Vibrio spp. matched with the TRFs that were dominant only in 1-day-old biofilm, suggesting that AHL-producing vibrios were one of the pioneer groups during subtidal biofilm formation. We reported here for the first time the dynamics of AHLs and AHL-producing bacteria during the formation of a subtidal biofilm.
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Introduction
Surfaces submerged in seawater are readily colonized by marine microorganisms including bacteria, diatoms, protozoa, fungi and so on. The assemblage of these attached microorganisms on a surface is referred to as a marine biofilm (Cooksey and Wigglesworth-Cooksey, 1995; Costerton et al., 1995). Marine biofilms play important roles in various biological processes, such as the biofouling development, nitrogen fixation, sulfate reduction and so on, therefore are important topics in marine ecological study (Costerton et al., 1995; Qian, 1999; Decho, 2000; Huang et al., 2007b).
Bacteria are dominant and active members of marine biofilms. In laboratory bacterial biofilms are inextricably linked with bacterial quorum sensing (QS), the density-dependent cell–cell communication (Parsek and Greenberg, 2005). QS allows bacteria to alter their behavior on a population-wide scale in response to changes in the number and/or species present in a community (Waters and Bassler, 2005). Several phenotypes beneficial for bacterial surface colonization, including motility, exopolysaccharide production, biofilm formation and toxin production, are often regulated by QS (Davies et al., 1998; Stoodley et al., 2002; Parsek and Greenberg, 2005; Waters and Bassler, 2005).
N-acyl homoserine lactones (AHLs) are the best-studied QS signals among Gram-negative bacteria. AHL-based QS system was firstly discovered from marine Vibrio fischeri (Milton, 2006). Recently, AHL-producing bacteria were isolated from ‘marine snow’ (Gram et al., 2002), marine sponges (Taylor et al., 2004; Mohamed et al., 2008), marine water column, eukaryotic algae (Wagner-Dobler et al., 2005) and marine subtidal biofilms (Huang et al., 2007a), suggesting the potential impacts of AHLs in marine bacterial communities. It was proposed that bacteria might use QS as a weapon to compete for survival or to dominate in a natural niche (Waters and Bassler, 2005; Defoirdt et al., 2008). Indeed, in the laboratory, AHL was shown to mediate the interaction between Pseudomonas aeruginosa and Agrobacterium tumefaciens in biofilm cocultures (An et al., 2006), whereas AHL-QS blockers and the presence of AHLs were found to change bacterial community composition and function in natural environments and activated sludge (Valle et al., 2004; McLean et al., 2005; Dobretsov et al., 2007).
Marine natural biofilms are unique ecological niches where multiple species of bacteria attach and grow on a surface in a dynamic process (Costerton et al., 1995; Decho, 2000). Although molecular mechanisms of AHL-regulated biofilm formation had been extensively studied in the laboratory (Davies et al., 1998; Parsek and Greenberg, 2005; Waters and Bassler, 2005); little is known about the ecological roles of AHLs in natural biofilm formation (Manefield and Turner, 2002; Parsek and Greenberg, 2005). In our parallel study, 21 AHL-producing bacteria were isolated from subtidal biofilms of different ages (Huang et al., 2008). In this study, we provided evidence that bacterial AHL signals were prevalent and variable in situ in subtidal biofilms; and the composition of AHL-producing bacteria was dynamics during biofilm development.
Materials and methods
Development of subtidal biofilms
Subtidal biofilms were developed during 12th–21st October 2006 at Yung Shue Au fish farm, Hong Kong (22° 25′ 35N, 114° 16′ 46E). During the sampling period, the weather was stable and the average water parameters were: temperature 27.4 °C, salinity 31.7 p.p.t., dissolved oxygen 6.7 mg l−1, and the pH value 8.0 (Hong Kong Environmental Protection Department).
Polystyrene Petri dishes for different experimental purposes were held in fishnets and submerged 2 m below the seawater level. Petri dishes were retrieved from the field after 1, 3, 5, 7 and 9 days of submersion and transported immediately back to the laboratory in a heat-proof container filled with in situ seawater.
Detection of AHLs in subtidal biofilms by AHL reporter strain
The AHL reporter strains A. tumefaciens strain A136 (pCF218) (pCF372) and Chromobacterium violaceum strain CV026 (obtained from Prof. McLean, Texas State University) were used to detect AHLs in subtidal biofilms. The strain A136 produces a blue color in the presence of 5-bromo-4-chloro-3-indolyl-β-D-galactopyranoside (X-Gal) in response to a wide range of AHLs (McLean et al., 1997), whereas the strain CV026 produces a purple pigment when induced by short- to medium-chain AHLs, such as C4-, C6-, C8-HSL and 3-oxo-C6-, C8-HSL (McClean et al., 1997).
The AHL reporter strain was streaked on the Luria Broth agar plate (diameter=90 mm, Sterilin, UK). For A136 bioassay, 50 μl X-Gal (20 mg ml−1) were spread on each plate before bioassay was performed. Then the smaller Petri dish (diameter=50 mm Falcon #1006, USA) with subtidal biofilm developed on it was placed approximately 1 cm apart from the streak, with biofilms directly in contact with agar (Figure 1). Five replicates were performed for each day biofilm. Experimental plates were then incubated at 28 °C for 48 h. If AHLs are present, they diffuse through the agar and activate the coloration of the reporter strains. Assays with A. tumefaciens A136 vs A. tumefaciens KYC6 and C. violaceum CV026 vs C. violaceum ATCC 31532 served as positive controls. Assays with the reporter strain vs itself and vs clean dish served as negative controls.
Profiling of AHLs in subtidal biofilms by gas chromatography—mass spectrometry
On each sampling day, subtidal biofilms were harvested by swabbing both sides of 100 Petri dishes (diameter=90 mm) with sterile cotton buds. Biofilms were extracted three times with 300 ml of ethyl acetate (EA) containing 0.2% (v/v) glacial acetic acid. The EA extracts were combined and the solvent was removed by evaporation under reduced pressure; the extracts were freeze dried, redissolved in 1 ml of dichloromethane and then subjected to gas chromatography—mass spectrometry (GC-MS) analysis.
Gas chromatography—mass spectrometry (Varian/CP-3800 and Varian/Saturn 2200) was incorporated with a relatively nonpolar capillary column (CP-Sil 8 CB-MS, 30-m length, 0.25 μm film thickness, 0.25 mm internal diameter). The injection port and the interface were held at 220 and 300 °C, respectively. The temperature was programmed from 120 to 275 °C at 10 °C per minute, followed by a 15 °C per minute ramp to 300 °C and a hold at 300 °C for 5 min with helium as the carrier gas.
AHLs in the samples were identified by comparing to standard AHLs and also to specific fragment patterns reported in (Cataldi et al., 2004). Standard AHLs included N-butyryl-, hexanoyl-, octanoyl-, decanoyl-, dodecanoyl-, tetradecanoyl-homoserine lactone (C4-, C6-, C8-, C10-, C12-, C14-HSL) and N-3-oxo-butyryl-, hexanoyl-, octanoyl-, decanoyl-, dodecanoyl-homoserine lactone (3-oxo-C4-, C6-, C8-, C10-, C12-, C14-HSL), and N-3-OH-butyryl-, hexanoyl-, octanoyl-, decanoyl-homoserine lactone (3-OH-C4-, C6-, C8-, C10-HSL), which were purchased from the laboratory of Prof. Paul Williams, UK. AHLs with C4- and C6- side chain were grouped into short-chain AHLs. AHLs with C8- and C10- side chain were grouped into medium-chain AHLs. AHLs with C12- and C14- side chain were grouped into long-chain AHLs.
Collection and extraction of genomic DNA from biofilms and water column
On each sampling day, biofilms from five Petri dishes (diameter=90 mm) were rinsed with artificial seawater and swabbed with sterile cotton buds to collect the bacterial community. On the first sampling day, 3 l (for three replicates) of seawater were collected at the biofilm sampling site. Seawater was filtered first through a 100-μm-pore-size polycarbonate membrane (Millipore, Bedford, MA, USA) and subsequently through a 0.22-μm-pore-size membrane (Millipore). Each 0.22-μm membrane or cotton bud was immediately frozen in 0.8 ml of extraction buffer (100 mM Tris-HCl, 100 mM Na2–EDTA, 100 mM Na2HPO4, 1.5 M NaCl, 1% cetyl trimethylammonium bromide; pH 8). Bacterial cells in the samples were lysed in two freeze-thaw cycles, using liquid nitrogen and a 65 °C water bath. Total DNA was extracted and purified according to the SDS-based method described in Zhou et al. (1996). Purified DNA was dissolved in 50 μl of sterile H2O and kept at −20 °C until use.
Amplification of the 16S rRNA gene by PCR
The 16S rRNA genes in the DNA samples were amplified by PCR using the primers 341F (5′-CCTACGGGAGGCAGCAG-3′) and 926R-fluorescein (Fam; 5′-CCGTCAATTCCTTTRAGTTT-3′; Liu et al., 1997). The latter was labeled at the 5′ end with 6-carboxy Fam. Each PCR mixture contained 3 μl of DNA sample, 1.25 U of Taq polymerase (Amersham Biosciences, Piscataway, NJ, USA), 0.25 mM of dNTPs, 0.1 μM of each primer, 1.5 mM of MgCl2 and 2.5 μl of 10 × PCR buffer in a total volume of 25 μl. PCR was performed in the following thermal cycles: 95 °C for 5 min; 30 cycles of 95 °C for 30 s, 55 °C for 40 s, 72 °C for 1 min and 72 °C for 10 min. PCR products were checked on 1% agarose gel. Desired PCR products were purified using a PCR Purification Mini Kit (Watson, China) according to the manufacturer's instructions. For each sample, PCR was performed with three replicates for later on terminal restriction fragment length polymorphism (TRFLP) analysis.
Terminal restriction fragment length polymorphism
PCR products were cleaved with 10 U of the restriction enzyme MspI at 37 °C for 6 h. Digested products were precipitated with three volumes of cold absolute ethanol, centrifuged (12 000 r.p.m.) at 4 °C for 20 min and washed with 100 μl of 75% cold ethanol. Purified products (10 μl) together with 0.5 μl of the internal size standard (ET550-R, Amersham Biosciences) were denatured at 95 °C for 2 min, snap cooled on ice and subjected to electrophoresis on a MegaBACE genetic analyzer (Amersham Biosciences) operated in the genotyping mode.
Analysis of TRFs in AHL-producing bacteria
A total of 21 AHL-producing bacteria were isolated from the same batch of subtidal biofilms in a parallel study (Huang et al., 2008) and subjected to TRFLP analysis. Genomic DNA was extracted from pure colonies of each isolate using a bacterial genomic DNA extraction kit (TaKaRa, China), whereas the primers, restriction enzyme and PCR conditions to obtain TRFs from each isolate were the same as mentioned above.
Statistical analysis
All analyses of the TRFs generated from TRFLP analysis were performed using Genetic Profiler in the MegaBACE software package (Amersham Biosciences). For each sample, TRFs that were <50 fluorescence units in intensity, <50 bp in size, and >550 bp in size were excluded from statistical analysis to screen off background noise, to avoid pseudo-TRFs derived from primers and to avoid inaccurate size determination, respectively (Moesender et al., 1999). The Bray–Curtis similarity matrix was constructed based on the total number of TRFs observed in all samples and the presence or absence of TRFs in individual samples. Agglomerative hierarchical clustering was performed by the ‘group average’ method to display a dendrogram using PRIMER statistical software (Plymouth Marine Laboratory, Plymouth, UK). In all cases, the threshold level for significance was 5%.
Results
Presence of AHLs in subtidal biofilms over time
Representative results of the AHL reporter strain bioassays were shown in Figure 1. Among the five replicates, four of the 1-day biofilms and three of the 3-day biofilms could induce coloration of C. violaceum CV026, none of the 5-, 7- and 9-day biofilms induced coloration of C. violaceum CV026. Moreover, four out of five 1-day biofilms and all of the other biofilms induced a blue coloration of A. tumefaciens A136, although maximal induction was observed at 7- and 9-day biofilms (Figure 1). As the two reporter strains respond to different ranges of AHLs, the differential induction of the reporter strains suggested that dominant AHLs and/or AHL-producing bacterial communities changed in subtidal biofilms over time. No coloration was induced in the negative controls (that is, clean dishes or reporter strains themselves), whereas AHL overproducing strains (strain 31532 and KYC6) induced coloration of reporter strains in the positive controls.
Profiling of AHLs in biofilm extracts
Acyl homoserine lactones in the biofilm extracts were identified by comparing their gas-chromatographic retention times and mass spectra with those of the standard AHLs. Figure 2 shows the identification of C10-HSL in the 9-day biofilm extract by GC-MS analysis. AHL profiles in the biofilm extracts were summarized in Table 1. Diverse AHLs including C6∼C14-HSL and 3-oxo-C4∼C14-HSL (see Supplementary Figure 1 for example of 3-oxo-C8-HSL) were detected in biofilms of different ages. In the 1-day biofilms, long-chain AHLs such as C14-HSL and 3-oxo-C12, C14-HSL were absent, whereas in the 7- and 9-day biofilms, short-chain AHLs such as 3-oxo-C4, C6-HSL were absent.
TRFLP analysis of bacterial communities in subtidal biofilms and water column
With the combination of primers and restriction enzyme used in this study, the mean numbers of TRFs derived from biofilms of different ages ranged from 13 to 22, with the most abundant in the 1- and 5-day biofilms and least abundant in the 9-day biofilm (Figure 3). The average number of TRFs in water samples was 20 (Figure 3).
Electropherograms of TRFs for bacterial community derived from 1–9-day biofilms and water column were shown in Figure 4. The bacterial community composition was dynamic in biofilms and some peaks were unique compared to the water column (Figure 4). The TRFs of 312, 313 and 423 bp, were dominant in all samples. However, some TRFs were specifically dominant in certain samples, such as TRFs of 150 bp, 204 bp, 470 pb in the 1-day biofilm; 110 bp in the 7-day biofilm and 245 bp in water sample, respectively.
Cluster analysis showed that three replicates from each sample shared >75% similarity (Figure 5). The bacterial communities derived from the 3-, 5- and 7-day biofilms could be further grouped into a larger cluster sharing >60% similarity. The bacterial communities derived from the water column were distinct and shared less than 50% similarity with those derived from biofilms, indicating that the planktonic bacterial community was quite different from the attached bacterial communities. The bacterial communities derived from 9-day biofilms shared less than 20% similarity with the rest (Figure 5), suggesting that bacterial community became more distinct as the biofilm developed.
TRFs of AHL-producing bacteria
In total, 11 TRFs with sizes ranged from 71 to 423 bp were generated from the 21 AHL-producing bacteria (Table 2). With the exception of sf24, which generated two TRFs, all other bacterial isolates generated single TRFs upon MspI digestion of PCR-amplified 16S rRNA gene. All of these TRFs could be matched with the TRFs derived from the biofilm bacterial community samples, and most of them contributed to the dominant peaks in the biofilms, such as TRFs of 127, 204, 300, 312, 313, 370 and 423 bp (Figure 4).
Within the sample size of this study, TRFs generated by Vibrio spp., the TRF of 150 and 204 bp, were unique to this group and only dominant in the 1-day biofilm community samples (Figure 4), indicating that AHL-producing vibrios attached readily to a surface and were one of the pioneer groups during biofilm formation. The bacteroidetes also generated three distinguishable TRFs at 71, 125 and 375 bp. Although for AHL-producing Pseudoalteromonas spp. and α-proteobacteria, diverse TRFs were generated and most of the TRFs were shared in these two groups, such as TRFs of 127, 300, 313 and 423 bp.
Discussion
Dynamics of AHLs during subtidal biofilm formation
The observation that only the 1- and 3-day subtidal biofilms could induce coloration of the reporter strain CV026 was similar with that in our previous study, which was carried out at the university pier, a quite different costal marine environment (Huang et al., 2007a). These consistent results suggest that dynamics of AHLs in subtidal biofilms over time may follow similar pattern in coastal marine environments. As coloration of the strain CV026 is induced only by short- to medium-chain AHLs, although inhibited by long-chain AHLs (McClean et al., 1997), together with the results from the strain A136 bioassay, we propose that dominant AHLs produced by bacteria in subtidal biofilms changed from short-chain to long-chain over time. This proposal was further supported by direct profiling of AHL molecules by GC-MS analysis, which revealed that long-chain AHLs were absent in the 1-day-old biofilms, whereas short-chain AHLs were absent in the 7- and 9-day-old biofilms (Table 1). Changes in dominant AHLs could be due to the shift in AHL profiles produced by bacteria or the succession of AHL-producing bacterial community over time. Indeed, the AHL-producing bacterial community could be as dynamic as the whole bacterial community during subtidal biofilm formation. The presence of diverse AHL molecules suggests the complexity of AHL-based QS in subtidal biofilm communities.
Dynamics of AHL-producing bacteria during subtidal biofilm formation
Previous studies showed that succession of bacterial community in biofilms could happen within 3 days (Dang and Lovell, 2000), and might become stable after 6 days (Qian et al., 2003). However, the dynamic pattern of a biofilm varies under different environmental conditions (Qian et al., 2003; Webster and Negri, 2006). In this study, the number of TRFs in 9-day-old biofilms was less than the younger biofilms (Figure 3), whereas the major peaks in 9-day biofilms showed stronger signals than those in the younger biofilms (Figure 4), suggesting a decrease in bacterial diversity and an increase in dominance of certain bacteria in the biofilm community. Our data showed that the subtidal biofilm developed in a fish farm remained highly dynamic within 9 days of sampling period, and the bacterial community in the biofilm became more distinct from that in water column (Figure 5).
There are no specific probes or primers available to detect the AHL-producing bacteria using a PCR approach (Zhou et al., 1996), thus detecting the presence of AHL-producing bacteria in their original community relies on the cultivable isolates. DNA fingerprinting methods such as TRFLP offer rapid analysis and comparison of bacterial community structures among samples (Massol-Deya et al., 1995). However, relating these community profiles to species composition is not straightforward because of the fact that different species may result in one single TRF in TRFLP analysis (Kent et al., 2003). This could be complemented somehow by determination of TRFs derived from individual isolates (Lee et al., 2006).
Relating the TRFs of AHL-producing isolates to biofilms community is in good agreement with the AHL reporter bioassay results and our isolating records (see Supplementary Table 1). For example, the three isolates sf28, sf41 and sf47, which were the only strains that induced coloration of CV026 (Huang et al., 2008), generated TRFs of 127, 204 and 312 bp that were specifically abundant in the 1- and 3-day-old biofilms (Figure 4), which also induced coloration of CV026 (Figure 1). Moreover, AHL-producing vibrios generated TRFs of 150 and 204 bp that were only dominant in the 1-day-old biofilms but not in other biofilms (Figure 4), which coincided with our isolation records that all Vibrio spp. were isolated from the 1-day-old biofilms. Moreover, AHL-producing Pseudoalteromonas spp., α-proteobacteria and bacteroidetes were isolated throughout the sampling time; their TRFs were also dominant in TRFLP profiles over time. For example, the TRFs at 300, 312, 313, 375 and 423 bp.
Changes in the dominance of TRFs generated by AHL-producing bacteria over time were visible in TRFLP; however, other bacterial group could also contribute to these TRFs. Online analysis of possible matches to these TRFs may give us some idea about who are they (Lee et al., 2006); however, the real dynamics of these groups along biofilms development requires further study and more advanced methods, such as High-Density Universal 16S rRNA Microarray Analysis method (DeSantis et al., 2007).
Potential roles of AHLs in marine biofilms formation
Bacteria in natural environments tend to attach and grow on surfaces, living as biofilms (Stoodley et al., 2002; Parsek and Greenberg, 2005). Interactions between members in the community are undoubtedly linked with bacterial metabolic activity (Moller et al., 1998). For several species, QS has been shown to influence bacterial surface attachment and biofilm development in laboratory (Davies et al., 1998; An et al., 2006). Studies on natural biofilms have mainly focused on the comparison of bacterial community compositions in biofilms from contrasting environments (Qian et al., 2003; Lee et al., 2006), and phylogenetic identification of major bacteria constituting biofilms (Dang and Lovell, 2000). Few studies have been conducted to address the biological forces that drive the succession of bacterial community composition during biofilm development. The question remains open whether QS contribute to the dominance of certain bacteria in a multi-species natural biofilms.
In this study, all of the TRFs generated by AHL-producing bacteria belonged to the dominant peaks in the TRFLP of different biofilm samples. This is not surprising because most AHL-producing bacteria belonged to Vibrio spp., Pseudoalteromonas spp. and Rhodobacteraceae family (Huang et al., 2008) that were frequently found to be dominant in early marine biofilm communities (Acinas et al., 1999; Dang and Lovell, 2000; Lau et al., 2002; Buchan et al., 2005). The ability to use QS may be part of the genetic machinery that enables these bacteria to dominate in the subtidal biofilm community.
We observed that TRFs for AHL-producing Vibrio spp. only dominated in the TRFLP of the first day biofilm. This result suggests that vibrios in the seawater tend to attach to a surface and are one of the pioneer groups in the biofilm community. The nondominance of Vibrio spp. in the later time biofilms does not preclude their existence in the biofilms, but rather indicates the succession in the bacterial community composition. It had been reported that some Vibrio spp. employed biofilm formation to survive in the marine environments, and QS played an important role in this process (Bartlett and Azam, 2005; Milton, 2006; Mueller et al., 2007). No clear succession was found in this study for other two major AHL-producing groups, the Pseudoalteromonas spp. and the Rhodobacteraceae family. Their TRFs and isolation records suggested that these bacteria were rather persistent throughout the sampling time. The importance of Pseudoalteromonas spp. and Rhodobacteraceae family in marine environments is becoming more and more significant (Holmstrom and Kjelleberg, 1999; Buchan et al., 2005); the roles of QS and biofilm formation in the survival and the dominance of these two groups of bacteria also deserve more attention in the future.
As a global regulation signals for bacterial activities, AHLs may affect not only the biofilm composition, but also the consequence of biofilm activities in environment such as biofouling development, nitrogen fixation, sulfate reduction, the degradation of organic matter and, moreover, provide shelter for certain bacteria (Costerton et al., 1995; Qian, 1999; Decho, 2000; Valle et al., 2004; Queck et al., 2006; Huang et al., 2007b; Case et al., 2008). For examples, the cross-domain communication by AHLs between bacteria in biofilms and spores of green alga Ulva indicated a direct function of AHLs in biofouling development (Joint et al., 2002). Furthermore, it was reported that QS mediated developmental traits in the resistance of Serratia marcescens biofilms against protozoan grazing (Queck et al., 2006). The potential roles of AHLs in marine environments remain to be explored.
In conclusion, we reported here for the first time the dynamics of AHLs and AHL-producing bacteria during a 9-day subtidal biofilm formation. We proposed that bacterial QS signals AHLs have great implications in the ecological functions of marine natural biofilms.
References
Acinas SG, Anton J, Rodriguez-Valera F . (1999). Diversity of free-living and attached bacteria in offshore western Mediterranean waters as depicted by analysis of genes encoding 16 rRNA. Appl Environ Microbiol 65: 514–522.
An D, Danhorn T, Fuqua C, Parsek MR . (2006). Quorum sensing and motility mediate interactions between Pseudomonas aeruginosa and Agrobacterium tumefaciens in biofilm co-cultures. Proc Natl Acad Sci USA 103: 3828–3833.
Bartlett DH, Azam F . (2005). Chitin, cholera, and competence. Science 310: 1775–1777.
Buchan A, Gonzalez JM, Moran MA . (2005). Overview of the marine Roseobacter lineage. Appl Environ Microbiol 71: 5665–5677.
Case RJ, Labbate M, Kjelleberg S . (2008). AHL-driven quorum-sensing circuits: their frequency and function among the Proteobacteria. ISMEJ 2: 345–349.
Cataldi TRI, Bianco G, Frommberger M, Schmitt-Kopplin PH . (2004). Direct analysis of selected N-acyl-L-homoserine lactones by gas chromatography/mass spectrometry. Rapid Commun Mass Spectrom 18: 1341–1344.
Cooksey KE, Wigglesworth-Cooksey B . (1995). Adhesion of bacteria and diatoms to surfaces in the sea—a review. Aquat Microb Ecol 9: 87–96.
Costerton JW, Lewandowski Z, Caldwell DE, Korber DR, Lappin-Scott HM . (1995). Microbial biofilms. Annu Rev Microbiol 49: 711–745.
Dang H, Lovell CR . (2000). Bacterial primary colonization and early succession on surfaces in marine waters as determined by amplified rRNA gene restriction analysis and sequence analysis of 16S rRNA genes. Appl Environ Microbiol 66: 467–475.
Davies DG, Parsek MR, Pearson JP, Iglewski BH, Costerton JW, Greenberg EP . (1998). The involvement of cell-to-cell signals in the development of a bacterial biofilm. Science 280: 295–298.
Decho AW . (2000). Microbial biofilms in intertidal systems: an overview. Contin Shelf Res 20: 1257–1273.
Defoirdt T, Boon N, Sorgeloos P, Verstraete W, Bossier P . (2008). Quorum sensing and quorum quenching in Vibrio harveyi: lessons learned from in vivo work. ISMEJ 2: 19–26.
DeSantis TZ, Brodie EL, Moberg JP, Zubieta IX, Piceno YM, Andersen GL . (2007). High-density universal 16S rRNA microarray analysis reveals broader diversity than typical clone library when sampling the environment. Microb Ecol 53: 371–383.
Dobretsov S, Dahms HU, Huang YL, Wahl M, Qian PY . (2007). The effect of quorum sensing blockers on formation of marine microbial communities and larval attachment. FEMS Microbiol Ecol 60: 177–188.
Gram L, Grossart HP, Schlingloff A, Kiorboe T . (2002). Possible quorum sensing in marine snow bacteria: production of acylated homoserine lactones by Roseobacter strains isolated from marine snow. Appl Environ Microbiol 68: 4111–4116.
Holmstrom C, Kjelleberg S . (1999). Marine Pseudoalteromonas species are associated with higher organisms and produce biologically active extracellular agents. FEMS Microbiol Ecol 30: 285–293.
Huang YL, Ki JS, Case R, Qian PY . (2008). Diversity and acyl-homoserine lactone production among subtidal biofilm forming bacteria. Aquat Microb Ecol 52: 185–193.
Huang YL, Dobretsov S, Ki JS, Yang LH, Qian PY . (2007a). Presence of acyl-homoserine lactone in subtidal biofilm and the implication in larval behavioral response in the polychaete Hydroides elegans. Microb Ecol 54: 384–392.
Huang YL, Dobretsov S, Xiong H, Qian PY . (2007b). Relevance of biofilm formation of Pseudoalteromonas spongiae for its inductiveness to larval settlement of the polychaete Hydroides elegans. Appl Environ Microbiol 73: 6284–6288.
Joint I, Tait K, Callow ME, Callow JA, Milton D, Williams P et al. (2002). Cell-to-cell communication across the prokaryote-eukaryote boundary. Science 298: 1207.
Kent AD, Smith DJ, Benson BJ, Triplett EW . (2003). Web-based phylogenetic assignment tool for analysis of terminal restriction fragment length polymorphism profiles of microbial communities. Appl Environ Microbiol 69: 6768–6776.
Lau SCK, Mak KKW, Chen F, Qian PY . (2002). Bioactivity of bacterial strains isolated from marine biofilms in Hong Kong waters for the induction of larval settlement in the marine polychaete Hydroides elegans. Mar. Ecol Prog Ser 226: 301–310.
Lee OO, Lau SCK, Qian PY . (2006). Consistent bacterial community structure associated with the surface of the sponge Mycale adhaerens. Microb Ecol 52: 693–707.
Liu WT, Marsh TL, Cheng K, Forney LJ . (1997). Characterization of microbial diversity by determining terminal restriction fragment length polymorphisms of genes encoding 16S rRNA. Appl Environ Microbiol 63: 4516–4522.
Manefield M, Turner SL . (2002). Quorum sensing in context: out of molecular biology and into microbial ecology. Microbiology 148: 3762–3764.
Massol-Deya AA, Odelson DA, Hickey RF, Tiedje JM . (1995). Bacterial community fingerprinting of amplified 16S and 16–23S ribosomal DNA gene sequences and restriction endonuclease analysis (ARDRA). In: Akkermans ADL, van Elsas JD, de Bruijn FJ (eds). Molecular Microbial Ecology Manual, vol. 2. Kluwer Academic Publishers: Boston, pp 1–8.
McClean KH, Winson MK, Fish L, Taylor A, Chhabra SR, Camara M et al. (1997). Quorum sensing in Chromobacterium violaceum: exploitation of violacein production and inhibition for the detection of N-acylhomoserine lactones. Microbiology 143: 3703–3711.
McLean RJC, Barnes MB, Windham MK, Merchant M, Forstner MRJ, Fuqua C . (2005). Cell–cell influences on bacterial community development in aquatic biofilms. Appl Environ Microbiol 71: 8987–8990.
McLean RJC, Whiteley M, Stickler DJ, Fuqua WC . (1997). Evidence of autoinducer activity in naturally occurring biofilms. FEMS Microbiol Lett 154: 259–263.
Milton DL . (2006). Quorum sensing in vibrios: complexity for diversification. Int J Med Microbiol 296: 61–71.
Moesender MM, Arrieta JM, Muyzer G, Winter C, Herndl GJ . (1999). Optimization of terminal-restriction fragment length polymorphism analysis for complex marine bacterioplankton communities and comparison with denaturing gradient gel electrophoresis. Appl Environ Microbiol 65: 3518–3525.
Mohamed NM, Cicirelli EM, Kan J, Chen F, Fuqua C, Hill RT . (2008). Diversity and quorum-sensing signal production of Proteobacteria associated with marine sponges. Environ Microbiol 10: 75–86.
Moller S, Sternberg C, Andersen JB, Christensen BB, Ramos JL, Givskov M et al. (1998). In situ gene expression in mixed-culture biofilms: evidence of metabolic interactions between community members. Appl Environ Microbiol 64: 721–732.
Mueller RS, McDougald D, Cusumano D, Sodhi N, Kjelleberg S, Azam F et al. (2007). Vibrio cholerae strains possess multiple strategies for abiotic and biotic surface colonization. J Bacteriol 189: 5348–5360.
Parsek MR, Greenberg EP . (2005). Sociomicrobiology: the connections between quorum sensing and biofilms. Trends Microbiol 13: 27–33.
Qian PY . (1999). Larval settlement of polychaetes. Hydrobiologia 402: 239–253.
Qian PY, Thiyagarajan V, Lau SCK, Cheung SCK . (2003). Relationship between bacterial community profile in biofilm and attachment of the acorn barnacle Balanus amphitrite. Aquat Microb Ecol 33: 225–237.
Queck SY, Weitere M, Moreno AM, Rice SA, Kjelleberg S . (2006). The role of quorum sensing mediated developmental traits in the resistance of Serratia marcescens biofilms against protozoan grazing. Environ Microbiol 8: 1017–1025.
Stoodley P, Sauer K, Davies DG, Costerton JW . (2002). Biofilms as complex differentiated communities. Annu Rev Microbiol 56: 187–209.
Taylor MW, Schupp PJ, Baillie HJ, Charlton TS, de Nys R, Kjelleberg S et al. (2004). Evidence for acyl homoserine lactone signal production in bacteria associated with marine sponges. Appl Environ Microbiol 70: 4387–4389.
Valle A, Bailey MJ, Whiteley AS, Manefield M . (2004). N-acyl-L-homoserine lactones (AHLs) affect microbial community composition and function in activated sludge. Environ Microbiol 6: 424–433.
Wagner-Dobler I, Thiel V, Eberl L, Allgaier M, Bodor A, Meyer S et al. (2005). Discovery of complex mixtures of novel long-chain quorum sensing signals in free-living and host-associated marine alpha proteobacteria. Chem Biochem 6: 2195–2206.
Waters CM, Bassler BL . (2005). Quorum sensing: cell-to-cell communication in bacteria. Annu Rev Cell Dev Biol 21: 319–346.
Webster NS, Negri AP . (2006). Site-specific variation in Antarctic marine biofilms established on artificial surfaces. Environ Microbiol 8: 1177–1190.
Zhou J, Bruns MA, Tiedje JM . (1996). DNA recovery from soils of diverse composition. Appl Environ Microbiol 62: 316–322.
Acknowledgements
We thank Professor R McLean (Department of Biology, Texas State University) for his kind gifts of the AHL reporter strains. We also thank Ms MMY Tsoi and Dr R Zhang for their consultant in TRFLP analysis; Dr Z Yu for his help in PCR optimization and laboratory mates from the Kolter laboratory for their valuable comments on paper writing. This study was supported by an RGC grant (CA04/05.Sc01, HKUST6402/05M) and a Croucher Foundation Research grant (CF-CAS03/04.Sc01) to PY Qian.
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Supplementary Information accompanies the paper on The ISME Journal website (http://www.nature.com/ismej)
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Huang, YL., Ki, JS., Lee, O. et al. Evidence for the dynamics of Acyl homoserine lactone and AHL-producing bacteria during subtidal biofilm formation. ISME J 3, 296–304 (2009). https://doi.org/10.1038/ismej.2008.105
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DOI: https://doi.org/10.1038/ismej.2008.105
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