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Molecular detection of virulence factors among food and clinical Enterococcus faecalis strains in South Brazil

Abstract

The present report aimed to perform a molecular epidemiological survey by investigating the presence of virulence factors in E. faecalis isolated from different human clinical (n = 57) and food samples (n = 55) in Porto Alegre, Brazil, collected from 2006 to 2009. In addition, the ability to form biofilm in vitro on polystyrene and the β-haemolytic and gelatinase activities were determined. Clinical strains presented a higher prevalence of aggregation substance (agg), enterococcal surface protein (esp) and cytolysin (cylA) genes when compared with food isolates. The esp gene was found only in clinical strains. On the other hand, the gelatinase (gelE) and adherence factor (ace) genes had similar prevalence among the strains, showing the widespread occurrence of these virulence factors among food and clinical E. faecalis strains in South Brazil. More than three virulence factor genes were detected in 77.2% and 18.2% of clinical and food strains, respectively. Gelatinase and β-haemolysin activities were not associated with the presence of gelE and cylA genes. The ability to produce biofilm was detected in 100% of clinical and 94.6% of food isolates, and clinical strains were more able to form biofilm than the food isolates (Student's t-test, p < 0.01). Results from the statistical analysis showed significant associations between strong biofilm formation and ace (p = 0.015) and gelE (p = 0.007) genes in clinical strains. In conclusion, our data indicate that E. faecalis strains isolated from clinical and food samples possess distinctive patterns of virulence factors, with a larger number of genes that encode virulence factors detected in clinical strains.

virulence determinants; clinical enterococci; food enterococci; biofilm formation


Molecular detection of virulence factors among food and clinical Enterococcus faecalis strains in South Brazil

A.W. MedeirosI; R.I. PereiraII; D.V. OliveiraI; P.D. MartinsI; P.A. d'AzevedoIII; S. Van der SandI; J. FrazzonIV; A.P.G FrazzonI

IPrograma de Pós-Graduação em Microbiologia Agrícola e do Ambiente, Universidade Federal do Rio Grande do Sul, Porto Alegre, RS, Brazil

IIInstituto de Ciências Básicas da Saúde, Departamento de Microbiologia, Universidade Federal do Rio Grande do Sul, Porto Alegre, RS, Brazil

IIIDepartamento de Ciências Básicas da Saúde, Universidade Federal de Ciências da Saúde de Porto Alegre, Porto Alegre, RS, Brazil

IVInstituto de Ciência e Tecnologia de Alimentos, Universidade Federal do Rio Grande do Sul, Porto Alegre, RS, Brazil

Send correspondence to Send correspondence to A.P.G. Frazzon Instituto de Ciência e Tecnologia de Alimentos, Universidade Federal do Rio Grande do Sul Rua Sarmento Leite, n. 500, sala 158 90050-170, Porto Alegre, RS, Brazil E-mail: ana.frazzon@ufrgs.br

ABSTRACT

The present report aimed to perform a molecular epidemiological survey by investigating the presence of virulence factors in E. faecalis isolated from different human clinical (n = 57) and food samples (n = 55) in Porto Alegre, Brazil, collected from 2006 to 2009. In addition, the ability to form biofilm in vitro on polystyrene and the β-haemolytic and gelatinase activities were determined. Clinical strains presented a higher prevalence of aggregation substance (agg), enterococcal surface protein (esp) and cytolysin (cylA) genes when compared with food isolates. The esp gene was found only in clinical strains. On the other hand, the gelatinase (gelE) and adherence factor (ace) genes had similar prevalence among the strains, showing the widespread occurrence of these virulence factors among food and clinical E. faecalis strains in South Brazil. More than three virulence factor genes were detected in 77.2% and 18.2% of clinical and food strains, respectively. Gelatinase and β-haemolysin activities were not associated with the presence of gelE and cylA genes. The ability to produce biofilm was detected in 100% of clinical and 94.6% of food isolates, and clinical strains were more able to form biofilm than the food isolates (Student's t-test, p < 0.01). Results from the statistical analysis showed significant associations between strong biofilm formation and ace (p = 0.015) and gelE (p = 0.007) genes in clinical strains. In conclusion, our data indicate that E. faecalis strains isolated from clinical and food samples possess distinctive patterns of virulence factors, with a larger number of genes that encode virulence factors detected in clinical strains.

Key words: virulence determinants, clinical enterococci, food enterococci, biofilm formation.

Introduction

Enterococcus faecalis are common bacteria that inhabit the gastrointestinal tract of humans and animals, being widely distributed in soil, water, plants and food products (Giraffa 2006; Frazzon et al., 2009). These microorganisms have been associated with nosocomial infections, bacteremia, surgical wound infection, endocarditis, and urinary tract infections (Huycke et al., 1998; Samuelsson et al., 2003; d'Azevedo et al., 2006). The enterococcal infection is complicated by the intrinsic resistance to some antimicrobials commonly prescribed for Gram-positive cocci, such as cephalosporin, lincomycin, cotrimoxazole, and low levels of penicillin and aminoglycosides, as well as by the ability to acquire resistance genes via transposons or plasmids (Huycke et al., 1998; Kayser 2003).

Virulence factors of E. faecalis are thought to ease adherence of bacteria to the host cell membranes and to environmental surfaces, where they can obtain nutrients and evade the host immune response. The extracellular surface protein (Esp), encoded by the esp gene, is a cell wallassociated protein which serve as adhesin for the pathogen to host tissue colonization and persistence in urinary tract infections (Fischer and Phillips, 2009). Another cell surface protein present in E. faecalis is adhesion of collagen (Ace), which mediates the association of bacteria to host cell matrix proteins, such as collagen I and IV and laminin. Studies have demonstrated that Ace protein may contribute to the pathogenesis of enterococci in endocarditis (Koch et al., 2004; Lebreton et al., 2009; Upadhyaya et al., 2009). The aggregation substance (Agg) is a pheromone-inducible surface protein of E. faecalis required for cell-to-cell contact during conjugation and for adhesion to eukaryotic cells. This protein eases aggregation of donor and recipient bacteria and aids conjugative plasmid transfer during bacterial conjugation. Studies have revealed that aggregation substance may promote adherence of bacterial proteins to extracellular matrix proteins and also may increase cell surface hydrophobicity (Cariolato et al., 2008; Upadhyaya et al., 2009).

Some extracellular proteins, such as gelatinase and cytolysin, have been classified as virulence factors of enterococci. Gelatinase is a zinc metalloprotease encoded by the chromosomal gelE gene. It hydrolyzes gelatin, casein, hemoglobin, and other bioactive compounds (Walters et al., 2003). The cytolysin, a bacterial toxin with β-haemolytic properties in humans and with bacteriocin activity against other Gram-positive bacteria, is encoded by the cytolysin operon (cylR1, cylR2, cylLL, cylLS, cylM, cylB, cylA, cylI). The proteins encoded by cylLLand cylLSare precursors of two small lantibiotic-like peptides, which are modified by the product of cylM gene. The peptides are transported out of the cell by the product of cylB gene, an ATP-binding cassette transporter. The cylA gene product processes the peptides and activates them, allowing them to combine and then to produce the cytolysin. The mechanism that signals the upregulation of the operon involves two regulator proteins corresponding to the cylR1 and cylR2 gene products from a divergently transcribed operon. An immunity function is present and is provided by a membrane protein encoded by the cylI gene (Gaspar et al., 2009; Singh et al., 2010).

The ambiguous role of Enterococcus has stimulated research in order to determine particular characteristics of enterococci isolated from food and clinical samples and to solve the questions about the risks of using this microorganism in food. In addition, the pathogenesis of these microorganisms remains unclear, but it is proposed that some virulence factors could increase the capacity of Enterococcus to cause infection, facilitating the adhesion and colonization (Franz et al., 2003). So far, in Brazil, there are no studies investigating the prevalence of virulence factors among food and clinical strains of E. faecalis. This study aimed to investigate the prevalence of virulence factors in E. faecalis isolated from diverse human clinical and food samples collected in South Brazil, as well as to access their ability to form biofilm in vitro on polystyrene and to determine their β-haemolytic and gelatinase activities.

Materials and Methods

Enterococcus faecalis isolates

The E. faecalis investigated in the present study were isolated from different human clinical samples (urine, blood and cervical secretion) (n = 57) and foods samples (cassava, beetroot, potato, sweet potato, parsley, cabbage, raw meat, pasteurized milk and dairy products, such colonial cheese type and soft cheese) (n = 55) in Porto Alegre, Brazil, from 2006 to 2009 (d'Azevedo et al., 2006, Riboldi et al., 2009). All strains had already been identified to genus level by PCR with genus-specific primer pairs and to species level using the conventional biochemical tests (Dutka-Mahlen et al., 1995; Facklam et al., 2002).

Detection of virulence factors genes by PCR method

The virulence factors genes gelE (gelatinase), esp (extracellular surface protein), agg (aggregation substance), ace (adhesin of collagen) and cylA (activator of cytolysin) were identified by PCR, using specific primes (Duprè et al., 2003). E.faecalis JH2-2 and MMH594 were used as positive controls.

Detection of β-haemolytic and gelatinase activities

The β-haemolytic activity was determined by streaking the strains on Columbia Agar (Himedia Laboratories Ltd., India) supplemented with 5% defibrinated horse blood (Semedo et al., 2003). The gelatinase activity was performed in tubes containing brain heart infuse on broth (BHI) supplemented with 12% of gelatin substrate (Himedia Laboratories Ltd., India) (Marra et al., 2007).

Biofilm formation in vitro assay

Biofilm formation on polystyrene microplates was quantified by the crystal violet staining method with some improvements (Stepanovic et al., 2000). Briefly, bacteria were cultured at 36ºC in tryptic soy broth (TSB) for 18 h. The wells of sterile 96-well flat-bottomed polystyrene microplates were filled with 180 µL of TSB supplemented with 0.75% glucose (TSBG) and 20 µL of bacterial suspension containing approximately 108 cfu/mL. Subsequently, the plates were incubated for 18 h at 36 ºC. The optical density (O.D.) was measured at 492 nm (O.D.492) in spectrophotometer (Anthos 2010 Microplates Reader) (Vogel et al., 2000). The cut-off O.D. (O.D.c) was defined as three standard deviations above the mean O.D. of the negative control. All strains were separated into categories using the O.D. measurement of bacterial films, as it follows: O.D. < O.D.c= non-adherent, O.D.c < O.D. < (2x O.D.c) = weakly adherent, (2x O.D.c) < O.D. < (4x O.D.c) = moderately adherent and (4x O.D.c) < O.D. = strongly adherent (Christensen et al., 1985). The experiments were performed at least three times for each strain. Staphylococcus epidermidis American Type Culture Collection 35984 classified as a strong adherent was used as the positive control. This strain was selected because it has been used successfully in research of biofilm (Hufnagel et al., 2004; Marinho et al., 2013).

Statistical analysis

The results were analyzed using the Chi-square test and Fischer's exact, followed by residual analysis. All statistical analyses were performed with Statistic Package of the Social Science software (SPSS) 13th edition and a p value < 0.05 was considered significant. Student's t-test was used to compare the absorbance values of biofilm formers among clinical and food isolates. Results were also considered significant when p value was < 0.05.

Results

Prevalence of virulence genes among clinical and food enterococci

The distributions of virulence factor genes among clinical and food E. faecalis are show in Table 1. Clinical strains displayed the highest prevalence of aggregation substance (agg), enterococcal surface protein (esp) and cytolysin (cylA) genes when compared with food isolates, and, in addition, esp gene was found only in clinical strains. On the other hand, the gelatinase (gelE) and adherence factor (ace) genes had similar prevalence among the strains, showing the widespread occurrence of these virulence factors among food and clinical E. faecalis strains in South Brazil.

In a total of 112 E. faecalis, the gelE gene was the most prevalent factor (77.7%), followed by the ace (74.1%), while agg, esp and cylA genes were detected in 38.4%, 34.8% and 31.25% of the isolates, respectively. Forty-four (77.2%) clinical and 10 (18.2%) food strains harbored more than three virulence factor genes (Figure 1).


Relationship between virulence factor gene and corresponding phenotype

Expression of gelatinase and β-haemolysin in vitro was not always correlated with the detection of gelE and cylA genes by PCR (Table 1). Analysis of congruence between gelatinase and gelE pointed out that 24 (54.5%) clinical and 6 (13.9%) gelE-positive food strains were unable to degrade gelatin, and non-haemolytic activity was detected in 23 (74.2%) clinical and two (50%) cylA-positives food strains.

Biofilm formation and virulence factor genes

Table 2 shows the results of the biofilm formation assay of clinical and food E. faecalis strains. All clinical isolates formed biofilm vs. 94.5% of food strains, and 49 of 57 clinical strains (86%) were strong biofilm formers vs. 31 (56.4%) of the food isolates Statistically significant difference between the amount of biofilm formed by the clinical strains and the one formed by food strains was observed (p < 0.001) Results from the statistical analysis showed significant associations between strong biofilm formation and ace (p = 0.015) and gelE (p = 0.007) genes in clinical strains. On the other hand, no correlation between biofilm formation and the presence of agg (p = 0.115) and esp (p = 0.064) genes were observed in clinical E. faecalis.

Discussion

Differences in the distribution of virulence factors among E. faecalis isolated from clinical samples and food in South Brazil were observed, in which clinical strains exhibited more virulence factors determinants when compared with food isolates. This result agrees with Abriouel et al. (2008) and Cariolato et al. (2008), who observed that E. faecalis isolated from vegetables and environment harbored fewer determinants when compared with clinical isolates.

Our results showed a high prevalence (57.9%) of agg gene in clinical strains. Dupont et al. (2008) and Bittencourt and Suzart (2004) also found a similar prevalence of agg gene in E. faecalis isolated from clinical samples. On the other hand, the prevalence of agg (18.2%) in food strains was lower than previously reported by Eaton and Gasson (2001), who encountered a high frequency (67%) of agg in E. faecalis strains isolated from food. The difference observed between the previous study and results showed here may be caused by the lower number (n = 8) of

E. faecalis tested by Eaton and Gasson (2001). Strains harboring agg gene should be clearly undesirable in food, since the product of this gene mediates contact between bacterial cells and host cells, facilitating the acquisition of genes and the colonization ability. No correlation between biofilm formation in vitro on polystyrene microplates and the presence of agg gene in E. faecalis isolated from food and clinical samples was observed in the present study. Aggregation substance plays an important role in mediating efficiently the adhesion between bacteria, thereby easing plasmid exchange. Bacterial adherence appears to be a multifactorial phenomenon involving specific and nonspecific determinants. Studies have shown the relation between adherence or biofilm formation and E. faecalis aggregation substance using renal (VERO) and intestinal (CACO-2) epithelial cells or ex vivo model of cardiac valve colonization, rather than polystyrene microplates (Duprè et al., 2003; Chuang-Smith et al., 2010).

The occurrence of esp only in clinical isolates observed in our study agrees with results obtained by Mannu et al. (2003), which revealed the presence of enterococcal surface protein gene only in clinical strains, although they contrast with previous studies that detected esp gene in isolates from vegetables and water, possibly reflecting differences in the origins of the isolates (Eaton and Gasson 2001; Drahovská et al., 2004; Abriouel et al., 2008). The role of Esp in enterococcal infection is still undetermined, although most of the esp-positive clinical strains were isolated from urinary infection, supporting the function of this protein in tissue colonization (Shankar et al., 2001; Sava et al., 2010). Even though some studies suggest an important role for Esp in enterococcal biofilm formation, in our study, the occurrence of esp gene was not correlated with biofilm formation on polystyrene surface. These results are in accordance with previous findings, which have also demonstrated biofilm formation by esp-negative E. faecalis strains (Duprè et al., 2003; Rosa et al., 2006).

A higher frequency of cylA gene in clinical isolates and a lower one in food strains has also been observed in other studies (Semedo et al., 2003; Drahovská et al., 2004). Analysis of congruence between hemolytic activity and isolates carrying the cylA gene showed a lack of hemolytic activity in 74.2% of clinical and 50% of cylA-positive food isolates. Cosentino et al. (2010) have found clinical strains of enterococci carrying the cly genes and being non-haemolitic. The lack of cytolysin phenotypic/genotypic congruence may suggest missing genes in the cyl operon among cylA-positive/haemolysin-negative strains or the presence of silent cylA gene (Gaspar et al., 2009; Upadhyaya et al., 2009).

In the present study, an equivalent frequency of gelE gene was observed in food and clinical strains. These results are in agreement with data reported by others studies (Mohamed et al., 2004; Abriouel et al., 2008). The presence of the gelE gene and the lack of gelatinase activity in Enterococcus have been associated with manipulation in laboratory, silent genes, and low level expression or downregulation of the gelE gene (Lopes et al., 2006). Our data showed that strong biofilm formation correlated with gelE (p < 0.05) in clinical strains. Hancock and Perego (2004) and Mohamed et al. (2004) encountered a positive relation between gelE and biofilm formation. The gelE gene might directly or indirectly degrade collagen protein or other tissue proteins of host cells, which may further aggravate tissue injury.

The ace gene was distributed equally among clinical and food enterococci. Cariolato et al. (2008) reported similar prevalence of ace gene in enterococci isolated from human samples and dairy products. A positive association was observed between strong biofilm formation and the presence of ace in clinical strains (p < 0.05). Our results are in accordance with Singh et al. (2010), who observed that deletions in the ace gene result in a significant attenuation of the ability of E. faecalis to colonize and to cause aortic valve endocarditis, and they showed that Ace plays an important role in the early stages of colonization, possibly by mediating the adherence of E. faecalis to collagen exposed at the site of vascular injury. The function of ace in Enterococcus from other sources has not yet been elucidated.

Almost all isolates were able to form biofilms in vitro by the technique of adhesion in polyethylene. The correlation between virulence factor genes and biofilm formation is contentious. Some researchers affirm that the biofilm formation is a common characteristic of Enterococccus (Mohamed et al., 2004; Rosa et al., 2006). Enterococci isolated from food showing ability to form biofilms are alarming, since this ability contributes to survival, persistence and dissemination of resistant enterococci and/or resistance genes in diverse environmental conditions. Moreover, they are potential sources of contamination that might lead to food spoilage or transmission of diseases (Franz et al., 2003). In clinical strains, this ability is also remarkable, since biofilms can be formed in medical devices, such as catheter and surgical prostheses, and infections caused by biofilms are often treated by the implant removal, which increases the trauma and the treatment cost (Baldassarri et al., 2001; Rosa et al., 2006).

In conclusion, our data indicate that E. faecalis strains isolated from different clinical samples and foods displays distinctive patterns of virulence factors, since a larger number of genes that encode them were detected predominantly in clinical strains. Silent cylA and gelE genes were frequently detect in both groups. Despite the fact that E. faecalis isolated from food showed a low frequency of virulence genes, they may act as reservoirs of virulence factors, enabling the dissemination of these genes to the human microbiota through the food chain. Additional investigations are needed to evaluate the expression of such factors, which may not be revealed by in vitro phenotypic tests during the course of infection.

Acknowledgments

We thank the Conselho Nacional de Desenvolvimento Científico e Tecnológico (CNPq -#306397/2006-4, #473769/2007-7 and#470291/2010-9) and the Coordenação de Aperfeiçoamento de Pessoal de Nivel Superior (CAPES) of the Brazilian government.

We also thank Prof. Dra. Rosane Rech for statistical analysis.

Submitted: July 2, 2012;

Approved: April 1, 2013.

All the content of the journal, except where otherwise noted, is licensed under a Creative Commons License CC BY-NC.

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  • Send correspondence to

    A.P.G. Frazzon
    Instituto de Ciência e Tecnologia de Alimentos, Universidade Federal do Rio Grande do Sul
    Rua Sarmento Leite, n. 500, sala 158
    90050-170, Porto Alegre, RS, Brazil
    E-mail:
  • Publication Dates

    • Publication in this collection
      18 Apr 2014
    • Date of issue
      2014

    History

    • Received
      02 July 2012
    • Accepted
      01 Apr 2013
    Sociedade Brasileira de Microbiologia USP - ICB III - Dep. de Microbiologia, Sociedade Brasileira de Microbiologia, Av. Prof. Lineu Prestes, 2415, Cidade Universitária, 05508-900 São Paulo, SP - Brasil, Ramal USP 7979, Tel. / Fax: (55 11) 3813-9647 ou 3037-7095 - São Paulo - SP - Brazil
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