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Isolation of Rhodocyclus gelatinosus from poultry slaughterhouse wastewater

Abstracts

Four cultures of photosynthetic bacteria isolated from poultry slaughterhouse wastewater were identified as Rhodocyclus gelatinosus based on the following properties: reddish color of cultures in synthetic medium, presence of motility, slightly curved Gram-negative rods morphology, gelatin liquefying activity, utilization of citrate as carbon source and production of bacteriochlorophyl a and carotenoids of the spirilloxanthin alternative series. R. gelatinosus may represent a source of nutrients and pigments with application in poultry feed.

Photosynthetic bacteria; Rhodocyclus gelatinosus; poultry slaughterhouse wastewater


Quatro culturas de bactérias fotossintetizantes isoladas de águas residuárias de abatedouro de aves foram identificadas como Rhodocyclus gelatinosus com base nas seguintes propriedades: desenvolvimento de cor avermelhada nos cultivos em meio sintético, motilidade positiva, morfologia de bastonetes gram-negativos ligeiramente curvos, atividade de liquefação da gelatina, utilização de citrato como fonte de carbono e produção de bacterioclorofila a e carotenóides da série espiriloxantina alternativa. Esses testes foram também aplicados para uma linhagem de Rhodocyclus gelatinosus de referência para efeito de comparação. A biomassa de R. gelatinosus pode representar uma fonte de nutrientes e de pigmentos na alimentação de aves.


Isolation of Rhodocyclus gelatinosus from poultry slaughterhouse wastewater

Elisa Helena Giglio PonsanoI; Pedro Magalhães LacavaII; Marcos Franke PintoI

IDepartamento de Apoio, Produção e Saúde Animal; Curso de Medicina Veterinária; Universidade Estadual Paulista; C. P. 341; 16050-680; Araçatuba - SP - Brazil

II Departamento de Bioquímica; Instituto de Química; Universidade Estadual Paulista; C. P. 355; 14801-970; Araraquara - SP - Brazil

Correspondence Correspondence to Elisa Helena Giglio Ponsano Universidade Estadual Paulista C. P. 341 16050-680; Araçatuba - SP - Brazil

ABSTRACT

Four cultures of photosynthetic bacteria isolated from poultry slaughterhouse wastewater were identified as Rhodocyclus gelatinosus based on the following properties: reddish color of cultures in synthetic medium, presence of motility, slightly curved Gram-negative rods morphology, gelatin liquefying activity, utilization of citrate as carbon source and production of bacteriochlorophyl a and carotenoids of the spirilloxanthin alternative series. R. gelatinosus may represent a source of nutrients and pigments with application in poultry feed.

Key words: Photosynthetic bacteria, Rhodocyclus gelatinosus, poultry slaughterhouse wastewater

RESUMO

Quatro culturas de bactérias fotossintetizantes isoladas de águas residuárias de abatedouro de aves foram identificadas como Rhodocyclus gelatinosus com base nas seguintes propriedades: desenvolvimento de cor avermelhada nos cultivos em meio sintético, motilidade positiva, morfologia de bastonetes gram-negativos ligeiramente curvos, atividade de liquefação da gelatina, utilização de citrato como fonte de carbono e produção de bacterioclorofila a e carotenóides da série espiriloxantina alternativa. Esses testes foram também aplicados para uma linhagem de Rhodocyclus gelatinosus de referência para efeito de comparação. A biomassa de R. gelatinosus pode representar uma fonte de nutrientes e de pigmentos na alimentação de aves.

INTRODUCTION

Purple non-sulfur bacteria (PNSB) are among the most energetically versatile of all prokaryotes. These phototrophic bacteria have the ability to utilize various organic compounds as substrates to carry out their photoheterotrophic metabolism under anaerobiosis in the presence of light and to grow photoautotrophically using CO2 as carbon source and either sulfur reduced compounds or H2 as electron donors. Some PNSB can also grow anaerobically in the dark using fermentative metabolism but most can grow aerobically in darkness by respiration (Brock et al., 1994). They represent a very heterogeneous group, with different types of metabolism, morphology, composition of photosynthetic pigments and internal membrane structures (Balloni et al., 1982; Imhoff and Trüper, 1989; Brock et al., 1994). Members of this group are widely distributed in nature. They may be found in aquatic environments, either marine or freshwater and in moist soils (Imhoff and Trüper, 1989) and are also associated with many kinds of industrial wastewaters, where they play an important role in the decontamination of pollutants, mainly under sunlight and in sub-surface environments, where anaerobic conditions prevail (Kobayashi and Tchan, 1973; Kobayashi, 1975; Pfennig, 1978; Siefert et al., 1978; Sasikala et al., 1995). Many authors have suggested the use of PNSB for the depuration of industrial wastewaters, with the advantage of biomass production, known to be rich in compounds such as proteins with high amounts of essential amino acids, carotenoids, biological cofactors and vitamins, specially B12 (Kobayashi, 1975; Kobayashi and Kurata, 1978; Noparatnaraporn et al., 1983; Balloni et al., 1986; Balloni et al., 1987). The purpose of this study was to develop a methodology for the isolation of Rhodocyclus gelatinosus from poultry slaughterhouse wastewater and for its characterization.

MATERIALS AND METHODS

Poultry slaughterhouse wastewater: Wastewater generated from poultry slaughter and rinsing, after filtering, decantation and flotation operations was collected in plastic bottles previously disinfected with 100 ppm sodium hypocloride solution and taken to laboratory under anaerobiosis by tight closing of the bottles.

Reference microbial culture:Rhodocyclus gelatinosus wild type strain 52 used as reference for the identification experiments was donated by Centre de Génétique Moléculaire, Gif sur Yvette, France (Jirsakova and Reiss-Husson, 1993).

Culture media: Pfennig's medium (Pfennig, 1974) containing (g/l) KH2PO4 0.5; MgSO4.7H2O 0.4; NaCl 0.4; NH4Cl 0.4; CaCl2.2H2O 0.05; organic compound 1; yeast extract 0.2; ferric citrate 0.005; trace elements solution 10 ml (FeSO4.7H2O 200 mg; ZnSO4.7H2O 10 mg; MnCl2.4H2O 3 mg; H3BO3 30 mg; CoCl2.6H2O 20 mg; CuCl2.2H2O 1 mg; NiCl2.6H2O 2 mg; Na2MoO4.2H2O 3 mg) was used (pH 7.0). It was autoclaved at 121oC for 15 minutes. Nutritive-gelatin agar (Koneman et al., 1989) contained (g/l) meat extract 3; bacteriological peptone 20; gelatin 120, and was autoclaved at 121oC for 15 minutes (pH 6.8). Motility agar (Bier, 1978) contained (g/l) bacteriological peptone 10; yeast extract 3; NaCl 5; gelatin 80; bacteriological agar 4, and was autoclaved at 121oC for 15 minutes (pH 7.4).

Vitamin solutions: Biotin 0.0015% sol.: biotin 1.5 mg; distilled water 100 ml. Membrane filtration on MilliporeÔ 0.22 mm. Thiamine 0.005% sol.: thiamine-HCl 5 mg; distilled water 100 ml. Membrane filtration on MilliporeÔ 0.22 mm.

Isolation of Rhodocyclus gelatinosus: Waste samples were filtered three times (once through a metal sieve and twice through paper filter WhatmanÔ # 3) and left under anaerobiosis in 500 ml glass cylinders supplied with glass stoppers for 7 days at 32 ± 2°C and light intensity of 1400 ± 200 lux, generated by incandescent (40W) and fluorescent (15W) lamps in an oven. After that, waste was transferred (30% v/v) to screw-cap test tubes (15x180mm) completely filled with Pfennig's medium (sodium acetate as organic compound). Tubes were tightly closed to keep anaerobiosis atmosphere and incubated as above. Contents of these tubes were transferred (30% v/v) to new screw-cap test tubes and filled with Pfennig's medium (sodium acetate as organic compound) enriched with biotin 0.0015% (1 ml/l) and thiamine 0.005% (1 ml/l) instead of yeast extract. Vitamin solutions were added after medium autoclaving. Incubation conditions were the same used previously. Enriched cultures were purified by repeated streaking on agar plates (Pfennig's medium enriched with vitamin solutions plus 2% bacteriological agar) until colonies were obtained. Plate dishes were kept in glass jars where anaerobiosis atmosphere was produced with CO2 (AnaerobacÔ/Probac) and incubated at 32 ± 2°C and 1400 ± 200 lux for 10 days.

Identification of R gelatinosus: Each pink or red colony isolated from petri dishes, as well as wild type strain 52 maintained in Pfennig's semi-solid agar (Pfennig's medium plus 1.2% bacteriological agar), were suspended in sterile saline and submitted to the following characterization tests, which were performed in triplicates:

Gelatin hydrolysis. Suspensions were transferred to screw-cap test tubes completely filled with nutritive-gelatin agar and incubated under anaerobiosis, at 32 ± 2°C and 1400 ± 200 lux, during 15 to 20 days.

Motility. Suspensions were transferred to screw-cap test tubes containing motility agar and incubated under anaerobiosis, at 32 ± 2°C and 1400 ± 200 lux, during 7 to 10 days.

Morphology. Morphology was checked through optical microscopy of Gram-stained suspensions (Bier, 1978).

Citrate utilization. Suspensions were transferred to screw-cap test tubes completely filled with liquid Pfennig's medium containing ferric citrate as sole organic compound and incubated under anaerobiosis, at 32 ± 2°C and 1400 ± 200 lux, during 15 to 20 days.

Absorption spectrum of living cells. One loop of each of the four cultures identified as R. gelatinosus on the basis of tests as above, as well as of the wild type strain 52 were transferred to screw-cap test tubes filled with Pfennig's medium enriched with 0.3% yeast extract. After 10 days of incubation under anaerobiosis at 1400 ± 200 lux and 32 ± 2°C, 3.5 ml of each culture were homogenized with 5 g of sucrose and the absorption spectrum was measured in a Varian 634 spectrophotometer using Pfennig's medium enriched with 0.3% yeast extract as the blank (Silva, 1997).

RESULTS AND DISCUSSION

Bergey's Manual of Determinative Bacteriology (Holt et al., 1994) describes the existence of six genera and 26 species in subgroup 3 of the classification of anoxigenic phototrophic bacteria. Among them, Rhodocyclus gelatinosus is characterized as a slightly curved and motile rod that may use a variety of carbon compounds as electron and carbon sources under anaerobic conditions in the light. This microorganism requires biotin and thiamine as growth factors, produces carotenoid pigments of the alternative spirilloxanthin series and is able to hydrolyze gelatin and to utilize citrate as sole carbon source. These features differ this species from the others of the genus (Imhoff and Trüper, 1989; Willens et al., 1991; Holt et al., 1994; Sasikala et al., 1995). According to Imhoff and Trüper (1989), the description of cell morphology, color of the cell suspensions, in vivo absorption spectra and some physiological properties leads to the identification of most species of PNSB.

From characteristics presented in Table 1, four cultures (R1, R2, R3, R4) were identified as Rhodocyclus gelatinosus as compared to Rhodocyclus gelatinosus wild type strain 52. These features agreed with those described for R. gelatinosus in the literature (Balloni et al. 1982; Imhoff and Trüper, 1989; Prasertsan et al., 1993; Holt et al., 1994). On both liquid and solid Pfennig's media, cultures showed red color after incubation period due to interaction among peculiar photosynthetic pigments of Rhodocyclus gelatinosus. Microbial growth occurred along the whole test tubes with liquid medium because these bacteria showed positive-phototaxy and were able to adhere to glassware where they became immobilized because of their flagella interlace and because of the abundant mucus production on liquid media, typical for this organism (Balloni et al., 1982). Slightly curved and rod-shaped morphology, as well as Gram-negative staining and presence of motility were in agreement with literature data (Balloni et al., 1982; Imhoff and Trüper, 1989; Prasertsan et al., 1993). Motility was confirmed by the presence of growth around needle puncture in motility agar. In young cultures, cells of R. gelatinosus are highly motile by means of polar flagella (Imhoff and Trüper, 1989).

Cultures classified as positive-gelatinase appeared deep red after incubation period and showed liquefaction of gelatin agar after 30 minutes at 4°C. The main feature of this organism was the ability to liquefy gelatin by means of an extra-cellular protease activity (Imhoff and Trüper, 1989; Holt et al., 1994). The four cultures grew slowly in Pfennig's medium containing citrate and only developed pink to red color after near 15 days of incubation. R. gelatinosus produces citrate lyase, which enables it to consume citrate and excrete large amounts of acetate to the medium, serving as carbon source after citrate comes exhausted (Imhoff and Trüper, 1989; Holt et al., 1994). Photosynthetic pigments produced by R. gelatinosus were bacteriochlorophyl a and carotenoids of the alternative spirilloxanthin series, with spheroidene, hydroxispheroidene and spirilloxanthin as major compounds (Holt et al., 1994). In vivo absorption spectra for the four isolated strains and for the wild type strain 52 are showed in Fig. 1 and their absorption maxima are showed in Table 2. According to Trüper and Imhoff (1992), absorption maxima of R. gelatinosus cell suspensions are 373-374, 455-460, 476-486, 506-518, 806-810 and 854-865 nm, due to the blend of alternative spirilloxanthin series carotenoids and bacteriochlorophyl a, whose absorption maxima are at 375, 590, 800 - 810 and 830 - 890 nm (Imhoff and Trüper, 1989; Brock et al., 1994). These peaks are in agreement with those found to R1, R2, R3, R4 and to wild type strain 52, used for comparison.


Based on the results found in this experiment about color of cultures, cells morphology and motility, gelatin liquefaction, citrate utilization and absorption spectrum, four cultures (R1, R2, R3, R4) isolated from poultry slaughterhouse wastewater were identified as Rhodocyclus gelatinosus, as compared to a reference R. gelatinosus strain.

ACKNOWLEDGMENTS

E. H. G. P. thanks Alberto Minoru Miyasaka and Frango Sertanejo staff for the cooperation and the supply of the waste.

Received: February 15, 2001

Revised: September 19, 2001

Accepted: November 27, 2001

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  • Correspondence to
    Elisa Helena Giglio Ponsano
    Universidade Estadual Paulista
    C. P. 341
    16050-680; Araçatuba - SP - Brazil
  • Publication Dates

    • Publication in this collection
      29 Apr 2003
    • Date of issue
      Dec 2002

    History

    • Accepted
      27 Nov 2001
    • Reviewed
      19 Sept 2001
    • Received
      15 Feb 2001
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