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Brazilian Journal of Biology

versión impresa ISSN 1519-6984versión On-line ISSN 1678-4375

Braz. J. Biol. v.67 n.1 São Carlos feb. 2007

http://dx.doi.org/10.1590/S1519-69842007000100016 

BIOLOGY

 

Alternative methodology for isolation of biosurfactant-producing bacteria

 

Metodologia alternativa para isolamento de bactérias produtoras de biossurfactante

 

 

Krepsky, N.I, II; Da Silva, FS.I, II; Fontana, LF.I, II; Crapez, MAC.I, *

IPrograma de Pós-Graduação em Biologia Marinha, Universidade Federal Fluminense, Instituto de Biologia, Outeiro de São João Batista, s/n, CEP 24020-140, Campus do Valonguinho, Niterói, Brazil
IIDepartamento de Geologia, Universidade Federal Fluminense, Av. Litorânea s/n, 4° andar, CEP 24210-340, Gragoatá, Niterói, RJ, Brazil

 

 


ABSTRACT

Wide biosurfactant application on biorremediation is limited by its high production cost. The search for cheaper biossurfactant production alternatives has guided our study. The use of selective media containing sucrose (10 g.L-1) and Arabian Light oil (2 g.L-1) as carbon sources showed to be effective to screen and maintain biosurfactant-producing consortia isolated from mangrove hydrocarbon-contaminated sediment. The biosurfactant production was assayed by kerosene, gasoline and Arabian Light Emulsification activity and the bacterial growth curve was determined by bacterial quantification. The parameters analyzed for biosurfactant production were the growth curve, salinity concentration, flask shape and oxygenation. All bacteria consortia screened were able to emulsify the petroleum derivatives tested. Biosurfactant production increased according to the incubation time; however the type of emulsification (non-aqueous phase or aqueous phase) did not change with time but with the compound tested. The methodology was able to isolate biosurfactant-producing consortia from superficial mangrove sediment contaminated by petroleum hydrocarbons and was recommended for selection of biosurfactant producing bacteria in tropical countries with low financial resources.

Keywords: bacteria consortia, bioremediation, petroleum, sediment.


RESUMO

A ampla aplicação de biossurfactantes em biorremediação é limitada pelo seu alto custo de produção. A procura de alternativas de produção mais baratas motivou nosso estudo. O uso de meio seletivo, contendo sacarose (10 g.L-1) e óleo Árabe Leve (2 g.L-1), mostrou-se eficiente na triagem e manutenção de consórcios bacterianos isolados de sedimento de mangue contaminado com hidrocarboneto. A produção de biossurfactante foi avaliada pela Atividade Emulsificante do querosene, gasolina e Árabe Leve e a curva de crescimento foi determinada pela quantificação bacteriana. Os parâmetros analisados para a produção de biossurfactante foram: curva de crescimento, concentração da salinidade, forma do frasco e oxigenação. Todos os consórcios bacterianos pesquisados foram capazes de emulsificar os derivados de petróleo testados. A produção de biossurfactante aumentou de acordo com o tempo de incubação, entretanto, o tipo de emulsificação aquosa e não-aquosa não mudou com o tempo, mas com o composto testado. A metodologia permitiu o isolamento de consórcios bacterianos produtores de biossurfactante de sedimento superficial de mangue contaminado com hidrocarbonetos do petróleo, sendo indicada para seleção de bactéria produtora de biossurfactante em países tropicais com baixos recursos financeiros.

Palavras-chave: consórcio bacteriano, biorremediação, petróleo, sedimento.


 

 

1. Introduction

Marine contamination with petroleum hydrocarbons has caused critical environmental and health problems (Rahman et al., 2002). A spill of over 300,000 gal of marine fuel oil occurred on 18 of January 2000 at Guanabara Bay, Rio de Janeiro, Brazil reaching Guapimirim Environmental Protection Area mangroves. Mangrove sediments are rich in organic matter because of their high biodiversity and low hydrodynamics. Petroleum hydrocarbons tend to adsorb organic matter rich surfaces, such as mangrove sediments, due to their high molecular weight, hydrophobicity and solid state (Sikkema et al., 1995). Consequently, these environments are very sensitive to hydrocarbon contamination.

Only dissolved molecules can be metabolized by microorganisms. Its adsorption to mangrove sediments limits bioavailability of hydrophobic compounds to indigenous microorganisms and reduces the effectiveness of the bioremediation process (Francy et al., 1991, Southam et al., 2001; Paraszkiewicz et al., 2002). The persistence of oil on muddy sediments such as mangrove can cause long term impacts to their highly oil sensitive biota, mainly at intertidal habitats and their associated communities (Michel, 2000).

Fortunately, some indigenous bacteria from chronically contaminated sediment may produce biosurfactant. Biosurfactants produced by hydrocarbon-degrading bacteria can emulsify hydrocarbon-water mixtures, which enables them to grow on the oil droplets. These emulsification properties have also been demonstrated to enhance hydrocarbon degradation in the environment, making them potential tools for oil spill pollution-control (Banat, 1995).

Since the last decade, increasing attention has been paid to the development and implementation of biotechnology for cleaning up this sort of contamination. However, the high production costs associated caused by low strain productivities and high recovery expenses, limit its wide application (Davis et al., 1999). With this scope, the present study proposes an effective methodology to search for biosurfactant-producing bacteria at chronically hydrocarbon-contaminated sediments with low cost.

 

2. Material and Methods

2.1. Site characterization and sampling

Mangrove sediment samples (5 cm of depth) were collected at Guapimirim Environmental Protection Area (from -22° 40’ to -22° 46’ S and from -42° 57’ to -43° 07’ W), Rio de Janeiro, Brazil two years after the January, 2000 oil spill at Guanabara Bay. The samples were transported to a laboratory in a temperature isolated box.

2.2. Chemicals

Kerosene, Gasoline type C and Arabian Light oil used in emulsification activity assays were supplied by the PETROBRAS Oil Company. The hydrocarbon specifications are listed in Table 1 according to Jokuty et al. (2000). Mineral oil applied to create an oxygen-limited environment for the bacteria growth was purchased by Johnson & Johnson (São Paulo, BR).

 

 

2.3. Microbial cultures

Media were prepared with sea water collected from the Itacoatiara beach (-2° 54’ S and -43° 12’ W), Niterói, Brazil filtered through a 0.45 µm pore membrane and diluted with de-ionized water to the desired salt concentration. The growth media prepared for this work are listed in Table 2.

 

 

Arabian Light-degrading bacteria were selected from the sediment samples as follows. The collected sediment (1 g) were inoculated into 50 mL of medium 1 (Table 2) and the flasks were incubated for 30 days at room temperature.

After 30 days of growth, the bacteria were plated for 21 days in medium 2 (Table 2) for mucous bacteria screening. Reddish-pink colonies were selected and then inoculated into 10 mL of medium 3 (Table 2). After 15 days of incubation, 5 mL were transferred to 50 mL of medium 3 for biomass increase and bacteria maintenance. This growth provided the bacteria for the assays.

2.4. Parameters for biosurfactant production

2.4.1. Salinity concentration

Bacteria (1 mL) were inoculated in triplicate into 9 mL of media 4 (Table 2) with salt water concentration of 8 g.L-1, 16 g.L-1 or 24 g.L-1 (Table 2). After 30 days of incubation in tubes, the salt water concentration with the best bacterial growth and mucous formation were transferred into 50 mL of media 4 and incubated for more than 30 days to confirm this observation. This salt-water concentration was then used to prepare the media for emulsification activity and bacterial quantification assays.

2.4.2. Bacterial growth curve

The bacteria cultures were incubated on 100 mL of media 5 (Table 2) for 70 days on Wheaton flask. Emulsification activity and bacteria quantification (BQ) were performed every 72 hours over 30 days of incubation. Another reading was repeated at day 70. Due to bacterial adherence at the bottom of the Wheaton flask (as will be discussed later), the flask shape and oxygenation on Emulsification activity and bacterial quantification were tested.

2.4.3. Flask shape

Erlenmeyer and Wheaton flasks with equal volumes (250 mL) but with different shapes were compared for Emulsification activity and BQ. Readings were performed at days 0, 6, 15, 18 and 30. Assays were done in triplicate.

2.4.4. Oxygenation

A layer of mineral oil was added to both flasks after bacteria inoculation creating an oxygen-limited environment. Emulsification activity and bacterial quantification (BQ) were assayed on days 0, 6, 15, 18 and 30. Results were compared to flasks with no mineral oil addition. Assays were done in triplicate.

2.5. Bacterial Quantification (BQ)

Quantification was performed following Carlucci et al. (1986) and Kepner and Pratt (1994). Each bacterial sample was filtered through a 0.22 µm Black Polycarbonate membrane (Isopore Membrane Filters, Millipore). The stained bacteria were counted at 1000x magnification using epifluorescence microscopy, ten fold in triplicate (Axioskop 50, Zeiss).

2.6. Emulsification activity

Emulsification activity was performed according to Paraszkiewicz et al. (2002). Kerosene, gasoline or Arabian Light was added to bacterial broth in a ratio of 3:2 and then vortexed for 1 minute. After 24 hours rest the height of the emulsified compound was measured and compared with the total height of the hydrocarbon added multiplied by 100 (non-aqueous phase emulsification A). Emulsification of aqueous phase (B) was calculated by dividing the total height of hydrocarbon in the emulsion phase by the total height of the culture media multiplied by 100. The emulsification index (E24) was estimated by the height of the emulsification layer, divided by the total height of the system multiplied by 100. All assays were performed in triplicate for each compound. A control with no bacteria growth was performed for each compound.

2.7. Statistical analysis

The growth curve was compared by the t-Student test with Emulsification activity, the prevalent phase (A or B) for each compound at both flasks and with mineral oil addition. Bacteria quantification (BQ) and E24 of each compound were correlated by Statistics for Windows (StatSoft, Inc., 2000). Only significant values were considered for discussion (p <0.05).

 

3. Results

The bacteria were isolated from the mangrove sediment contaminated with petroleum hydrocarbons. Red Congo Agar distinguished reddish-pink colonies from white ones. Only 3 large reddish-pink mucous colonies with well-defined boundaries were selected for assays, characteristics that may be associated with biossurfactant production. Though plating in Petri dishes are useful to isolate pure colonies, the bacteria remained as consortia which was noticed by epifluorescence microscopy observation (data not shown). These bacteria were unable to grow as pure culture under the growth condition created, as will be discussed later. Consequently, the consortia were labeled as M1, M2 and M3. They grew at 8, 16 and 24 g.L-1 salt-water concentration, however consortia growths at 16 g.L-1 were more intense and viscous (unpublished data). As a result, this concentration was selected to prepare media for emulsification and bacterial quantification assays.

The growth curve of bacteria consortia M1, M2 e M3 are shown in Figure 1. Growth decreased over 70 days of incubation. BQ reduced from 0.60 to 0.15 µgC.cm-3 for M1 (Figure 1a), 0.26 to 0.05 µgC.cm-3 for M2 (Figure 1b) and from 0.55 to 0.10 µgC.cm-3 for M3 (Figure 1c). However, a growth peak was detected on day 6 for M2 (0.16 µgC.cm-3) and on day 21 for M1 (0.47 µgC.cm-3) and M3 (0.23 µgC.cm-3).

 



 

Both Erlenmeyer and Wheaton flasks showed a reduction in bacterial growth in incubation time (Figure 2). Erlenmeyer biomass reduced from 0.66 (M1)/ 0.27 (M2)/ 0.39 (M3) to 0.08 µgC.cm-3 (M1) and 0.0 µgC.cm-3 (M2 and M3) as shown in Figure 2a. This profile was also observed in the Wheaton flasks (Figure 2b). Biomass decreased from 0.60 µgC.cm-3 to 0.12 µgC.cm-3 (M1), 0.26 to 0 µgC.cm-3 (M2) and from 0.55 to 0.17 (M3). However, M2 (at Erlenmeyer) presented a growth peak on day 15 with a biomass of 0.39 µgC.cm-3 (Figure 2a). Therefore, according to the t-student test, Elenmeyer flasks presented a higher biomass than Wheaton flasks (p <0.05).

 




 

Mineral oil addition influenced bacterial growth negatively in both flasks. Biomass reduced from 0.66/0.27 and 0.39 µgC.cm-3 for M1, M2 and M3, respectively, to 0 for M1 and M2, and 0.06 µgC.cm-3 for M3 in Erlenmeyer (Figure 2c) and in Wheaton to 0.12 µgC.cm-3 for M1 and 0 µgC.cm-3 for M2 and M3 (Figure 2d). However, there was a growth peak at day 30 (BQ of 0.12 µgC.cm-3) for M1 grown in the Wheaton flask with mineral oil.

Emulsification index (E24) varied with the bacterial growth phase, the bacteria consortia, the type of flask used for bacterial incubation, the addition of mineral oil and the compound tested. There was no emulsification when biosurfactant-free medium was mixed with hydrocarbons. Kerosene, gasoline and Arabian Light emulsification were detected from the first day of incubation for all bacterial consortia (Figure 1). E24 ranged from 46.51 to 99.56% for kerosene, 23.19% to 100.00% for gasoline and from 40.00 to 95.33% for Arabian Light. The highest emulsification values of kerosene (p <0.05) were detected on day 70 for M1 when BQ was 0.15 µgC.cm-3 (Figure 1a) and on day 15 for M2 (Figure 1b) and M3 (Figure 1c) with E24 of 94.20 and 90.68% and a biomass of 0.01 and 0.12 µgC.cm-3, respectively. The same profile was maintained for gasoline although M3 did not show a significant increase in emulsification rates for this compound (p >0.05). Arabian Light emulsification was higher on days 24 for M2 and M3 and 27 for M1. On day 24, bacterial biomasses were, respectively, 0 and 0.12 µgC.cm-3 and on day 27 it was 0.18 µgC.cm-3. When compared with the t-student test, higher kerosene and Arabian Light E24 for M3 was followed, respectively, by lower BQ on days 15 and 18 (p <0.05).

The range of Emulsification (E24) values for Erlenmeyer and Wheaton flasks are shown in Table 2. Concerning Erlenmeyer, the highest kerosene E24 values (100%) were detected when BQ was 0.09 µgC.cm-3 and in Wheaton (94.20%) when BQ was 0.01 µgC.cm-3. For gasoline, the highest E24 (100%) were found on days 6, 15 and 18 in Erlenmeyer. On these days, biomasses were 0.07, 0.09 and 0 µgC.cm-3, respectively. In the Wheaton flask, the highest gasoline E24 (98.08%) was found on day 18 for M2 with BQ of 0.01 µgC.cm-3. For Arabian Light E24, day 18 presented the highest rates. In Erlenmeyer, E24 was 86.12% when BQ was 0.07 µgC.cm-3 and in Wheaton, 95.33% on day 15 when BQ was 0.12 µgC.cm-3. However, according to the t-Student test, for Erlenmeyer flasks there was no correlation between E24 and BQ values for any of the compounds tested. For Wheaton flasks, E24 of M3 were negatively correlated with BQ on day 15 for kerosene (E24 of 90.68%; BQ 0.12 µgC.cm-3) and on day 18 (E24 66.09% and BQ 0.12 µgC.cm-3) for Arabian Light oil (r = -1.0, p <0.05). There was no correlation of gasoline E24 with BQ.

When mineral oil was added, the highest kerosene E24 (100%) was on day 6 for M3 (BQ of 0.07 µgC.cm-3) in Erlenmeyer and on day 15 for M2 in Wheaton (93.33% and 0 µgC.cm-3). For gasoline, the highest E24 (100%) was on day 18 for M2 and M3, with BQ of 0.09 µgC.cm-3 in Erlenmeyer and Wheaton. However, BQ of M3 in Wheaton was 0.04 µgC.cm-3. The highest (80.32%) Arabian Light E24 was for M3 on day 18 with BQ of 0.09 µgC.cm-3 in Erlenmeyer and 84.37% for M2 in Wheaton with BQ of 0.09 µgC.cm-3 (p <0.05).

The type of emulsification also varied with the compound tested (Figure 3). Non-aqueous (A) emulsification of kerosene ranged from 62.70 to 100% and aqueous emulsification (B) ranged from 21.44 to 100%. For gasoline, the A index ranged from 3.16 to 100% and B index from 15.38 to 100%. Arabian light showed values ranging from 20 to 100% (A) and from 55 to 100% (B). As represented in Figure 3, 58% of the Arabian Light highest emulsification values were in the B phase compared to only 2.8% of emulsification in phase A (p <0.05). However, 11% of kerosene and 5% of gasoline highest emulsification was in phase A (p <0.05).

 

 

The emulsification type ranges for Erlenmeyer and Wheaton flasks are shown in Table 3. Fifty-three percent (53%) of Arabian Light emulsification was in phase B, whilst 33 and 6% of the Erlenmeyer cultured consortia emulsified respectively, kerosene and gasoline in phase A (Figure 4a). Concerning Wheaton (Figure 4b), 67% of Arabian Light emulsification and 6% of gasoline emulsification was in phase B, though 6% of kerosene was in phase A (p <0.05).

 

 

 




 

When bacterial consortia were cultured in Erlenmeyer in the presence of mineral oil (Figure 4c), 67% of Arabian Light emulsification was also in phase B (p <0.05). Kerosene presented 20% of emulsification in phase A, but only 6% of phase B emulsification (p <0.05). The bacterial consortia cultured in the Wheaton flasks with mineral oil (Figure 4d) presented the following emulsification profile: 73% of Arabian Light emulsification in phase B compared to 20% of kerosene emulsification and 13% of gasoline emulsification in phase A (p <0.05).

 

4. Discussion

Our methodology was able to isolate surfactant-producing bacteria from superficial mangrove sediment contaminated with petroleum hydrocarbons. The use of selective media loaded with carbon sources (sucrose – 10 g.L-1 and Arabian Light – 2 g.L-1) showed it was useful in terms of screening and maintenance of biosurfactant-producing bacteria from a highly eutrophic environment. Guanabara Bay and its mangrove protection areas are constantly subject to a multiple source of petroleum arrival (Michel, 2000). This chronicle contamination allows for the natural selection of hydrocarbon-degrading bacteria communities at the sediment.

As others have observed, high biosurfactant production is found to be characteristic under certain qualitative and quantitative environmental conditions depending on nutritional and environmental factors. Many studies have shown that hydrocarbon substrates are preferable for biosurfactant production. There is a growth in biosurfactant production whenever microorganisms such as Candida tropicalis, Candida lipolytica, Corynebacterium lepus and other species grow at the expense of water immiscible substrates. Other bacteria (e.g. Bacillus subtilis, Pseudomonas aeruginosa and Pseudomonas fluorescens) can produce biosurfactants when grown on carbohydrates such as solely carbon sources. However, Arthrobacter paraffeinus, Torulopsis petrophilum and Torulopsis bombicola produce higher amounts of biosurfactants when grown on carbohydrate and hydrocarbon supplemented mediums (Shafi and Khanna, 1995).

The bacteria were able to grow at a wide salinity range - 8, 16 and 24 g.L-1. However the best results of growth and media viscosity were noticed at 16 g.L-1 of salt water. This salinity is 1.5 times lower than the minimal salinity range of mangroves, which range from 25 to 45 g.L-1 according to precipitation and river dynamics of the area. As these bacteria were isolated from mangrove sediment, the growth at wide range salinity was expected. The high mangrove salinity fluctuation linked to the sediment contamination with hydrocarbons selects bacteria able to cope with harsh conditions.

Even after Congo Agar plating and single colony pick, epifluorescence microscopy showed coccus and bacillus coexisting in the same colony (unpublished data). Later the predominant cell of each consortia was identified as Micrococcus spp., Alcanivorax spp. and Hydrococcus spp. by RNAr 16S (data not shown). This indicates the presence of heterogeneous bacteria acting on degradation of hydrocarbons and biosurfactant production. Heterogeneous bacteria communities have broad enzymatic capacities making degradation of hydrocarbon substrates more efficient than single bacteria degradation. According to Knackmuss (1996), biodegradation of compounds such as hydrocarbons, can only be done when the catabolic activities present in the microbial communities complement each other. In short, the metabolic by-products of one microorganism might serve as a nutrient support for the others (Crapez et al. 2000 and Dunne 2002).

Agar Congo is useful to investigate capsules and microcapsules in microorganisms such as a Staphylococcus biofilm producer and invasive Shiguella. Bacterial cells precipitate on their surface staining the colonies from pink to darkish red (Wenneras et al. 2000 and Arciola et al., 2001). We believe that biosurfactant may be produced under the same circumstances of capsule/microcapsule production.

In our experiments, we noticed a reduction in the bacterial growth curve (Figure 2) as bacteria adhered to the bottom of the incubation flasks, producing a biofilm layer. Mineral oil added to the flasks also functioned as a surface for bacterial adherence. Adherence reduced the numbers of free bacteria on the solution, consequently, interfering with bacterial cell quantification. Because our bacteria consortia were isolated from the mangrove sediments, they tended to search for immobilized growth. According to Bonin et al. (2001), the majority of benthic bacteria are not suspended in interstitial water but attached to sediment particles. The hydrophobicity/ hydrophilicity properties of the compounds used as a carbon source can have a marked impact onbacterial immobilization. They also defend that benthic bacterial immobilization changes its physiology in the presence of a solid support, when compared with its planktonic counterparts.

The stable emulsion produced when hydrophobic compounds (kerosene, gasoline or Arabian Light) were mixed with bacteria growth indicates the presence of surfactants in our system. According to Adamson (1990) the presence of a surfactant is necessary to obtain a stable emulsion between two immiscible pure liquids. Once vigorous mixing stops, both phases will separate if there is no surfactant present in the system.

The E24 peaks (>90%) of our bacteria consortia were found from days 15 to 70. These index values are compatible with those found by Paraszkiewicz et al. (2002) for the biosurfactant producer fungus Curvularia lunata. However, they found the maximum E24 peaks (93.0 ± 5.94% and 81.0 ± 9.42%) at 24 and 56 hours. Gram-positive bacteria biosurfactant producer grown on oil diesel as a carbon source showed only 12% of emulsification (Cassidy and Hudack 2001).

The flask shape and the presence of mineral oil influenced E24. For gasoline, there was no difference of E24 between the control and mineral oil for both Erlenmeyer and Wheaton flasks (p <0.05). However, for kerosene and Arabian Light, E24 was higher in the Erlenmeyer flask without mineral oil. We noticed that mineral oil reduces microbial growth and surfactant production in vitro, possibly by oxygen limitation (p <0.05). In accordance, Sikkema et al. (1995) affirm that mineral oil reduces microbial environmental activity.

Although the bacterial growth curve reduced with time due to bacterial adhesion, biosurfactant production increased as noticed by E24 assays. For this reason, this adhesion seemed to be essential in terms of enhancing biosurfactant production. In accordance, Morton and Surman (1994) believe that biosurfactant-producing microorganisms will be often found forming a dense film on the oil-water interface and consume the emulsified hydrocarbon. However, this film developed on the interface should be regarded as a true biofilm. Furthermore, Shafi and Khanna (1995) believe that there is a surge in production of surfactant after the culture has reached an exponential growth and Nadarajah et al. (2002) showed that de-emulsification depends on bacterial density rather than inoculum age, once the latter interferes with cell surface hydrophobicity.

The emulsification type depends on the hydrocarbon composition rather than on the growth phase, flask shape or mineral oil addition. Contrary to this, Paraszkiewicz et al. (2002) related the variation of type of emulsion depending on the growth phase. In our experiments, the growth phase did not influence the type of emulsification, which varied according to the chemical character of each compound. Gasoline and kerosene have a similar density. However, Arabian light has a higher density than the previous one. This may explain the non-aqueous (A) emulsification preference of gasoline and kerosene and the aqueous phase (B) preference of Arabian Light.

This methodology proved to be cheap and effective for the screening, maintenance and quantification of biosurfactant-producing bacteria consortia and was recommended for tropical countries with low founding resources. Although microscopy presented biomass quantification problems, due to bacterial bottom adherence, this observation allowed for the characterization of our samples such as bacteria consortia and cell viability determination at the same time. Marine bacteria tended to form biofilm on surfaces after reaching a population density. This biofilm formation may be fundamental for biosurfactant production and was unlike the shape of the flask used. Biossurfactant production may be governed by harsh conditions assembling capsule and micro-capsule production and depends on heterogeneous bacterial population for effective site decontamination. The aqueous and non-aqueous emulsification property of our biosurfactant allows for its use in hydrocarbon contaminated water and sediment. Isolation and chemical characterization of the biossurfactant produced is the next step of the research.

Acknowledgments — The authors are grateful to PhD Ana Carla Mesquita, PhD Maria das Graças Bispo and M.Sc. Rosana Barreto Ferreira and an anonymous reviewer for suggestions. We would also like to thank Professor Luiz Sérgio Randino Lamego (Universidade Federal Fluminense, Departamento de Físico-Química) and Lucy Seldin (Universidade Federal do Rio de Janeiro, Instituto de Microbiologia Professor Paulo de Goés) for help and advice on data presentation. This work was supported by the Agência Nacional de Petróleo (ANP) under PRH 11 and Capacitação de Auxílio a Pesquisa (CAPES).

 

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Received November 19, 2004
Accepted November 16, 2005
Distributed February 28, 2007

 

 

* e-mail: mirian@vm.uff.br

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