Prevalence and serotype distribution of <i>Listeria monocytogenes</i> isolated from foods in Montevideo-Uruguay

Braga, Valeria; Vázquez, Sylvia; Vico, Victoria; Pastorino, Valeria; Mota, María Inés; Legnani, Marcela; Schelotto, Felipe; Lancibidad, Gustavo; Varela, Gustavo

doi:10.1016/j.bjm.2017.01.010

ABSTRACT

The aim of this work was to study the prevalence of Listeria monocytogenes in foods obtained in retail shops and food industries located in Montevideo-Uruguay, and to identify the serogroups of the obtained isolates. Three-thousand one-hundred and seventy-five food samples (frozen, deli meats, ready-to-eat and cheese) were analyzed. The obtained isolates were serogrouped by multiplex PCR and serotyped by conventional procedure. Genetic comparisons were performed using pulsed-field gel electrophoresis on a sub-set of isolates belonging to the same serotype successively recovered from the same establishment. L. monocytogenes was isolated from 11.2% of samples. The highest prevalence was observed in frozen foods (38%), followed by cheese (10%). 1/2b and 4b were the most frequently identified serotypes. In six of 236 analyzed establishments we successively recovered L. monocytogenes isolates belonging to the same serotype. Most of them corresponded to serotype 1/2b. Pulsed-field gel electrophoresis profiles suggest that at least 33% of L. monocytogenes 1/2b isolates are genetically related and that may remain viable for prolonged periods. The observed prevalence of L. monocytogenes was lower than reported in neighboring countries. Our findings highlight the role that frozen foods may play in the spread of this pathogen, and the relevance of serotypes 1/2b and 4b.

Keywords:
Food-borne diseases; Listeriosis; Serotyping; Pulsed-field gel electrophoresis

Introduction

Listeria monocytogenes is a bacterial pathogen that causes a potentially severe disease both in people and animals, called listeriosis. Worldwide, it has been estimated that almost 90% of human cases occur after consumption of contaminated food. The most frequently implicated foodstuffs both in outbreaks and sporadic cases are soft cheese, frankfurters, unpasteurized milk, deli meats, smoked fish, dairy products, salads and refrigerated ready-to-eat products (RTE).¹1 Cartwright E, Jackson K, Johnson S, Graves L, Silk B. Listeriosis outbreaks and associated food vehicles United States, 1998-2008. Emerg Infect Dis. 2013;19:1-10.

2 Centers for Disease Control. Update: multistate outbreak of Listeriosis in United States, 1998-1999. Morb Mortal Wkly Rep. 1999;47:1117-1118.

3 Centers for Disease Control. Preliminary FoodNet data on the incidence of foodborne illnesses selected sites, United States 2002. Morb Mortal Wkly Rep. 2003;52:340-343.

4 Vazquez-Boland J, Kuhn M, Berche P, et al. Listeria pathogenesis and molecular virulence determinants. Clin Microbiol Rev. 2001;14:584-640.^-⁵5 Cossart P. Illuminating the landscape of host-pathogen interactions with the bacterium Listeria monocytogenes. Proc Natl Acad Sci U S A. 2011;108:19484-19491.

Listeriosis may occur as a mild febrile gastroenteritis or as a more severe invasive disease such as meningoencephalitis or sepsis. L. monocytogenes is capable of producing serious illness in pregnant women, newborns, elderly people and immunocompromised individuals (e.g. transplant recipients, patients receiving antineoplastic drugs or immunosuppressive therapy). In this high-risk group, listeriosis has a high lethality rate of 20-30%.⁴4 Vazquez-Boland J, Kuhn M, Berche P, et al. Listeria pathogenesis and molecular virulence determinants. Clin Microbiol Rev. 2001;14:584-640.

5 Cossart P. Illuminating the landscape of host-pathogen interactions with the bacterium Listeria monocytogenes. Proc Natl Acad Sci U S A. 2011;108:19484-19491.

6 Todd E, Notermans S. Surveillance of listeriosis and its causative pathogen, Listeria monocytogenes. Food Control. 2011;22:1484-1490.^-⁷7 Torres K, Sierra S, Poutou R, Carrascal A, Mercado M. Patogénesis de Listeria monocytogenes, microorganismo zoonótico emergente. Rev MVZ Cordoba. 2005;10:511-543.

This bacterium is widely disseminated in different food production environments, including manufacturing and packing plants, distribution and storage facilities. It develops biofilms on equipment, walk-in freezers, drains, etc.⁸8 Hassan A, Birt D, Frank J. Behavior of Listeria monocytogenesin a Pseudomonas putida biofilm on a condensate forming surface. J Food Prot. 2004;67:322-327.

9 Kalmokoff M, Austin J, Wan X, Sanders G, Banerjee S. Adsorption, attachment and biofilm formation among isolates of Listeria monocytogenes using model conditions. J Appl Microbiol. 2001;91:725-734.^-¹⁰10 Swaminathan B, Gerner-Smidt P. The epidemiology of human listeriosis. Microbes Infect. 2007;9:1236-1243. This feature, added to its capacity for growth at cooling temperatures and survival through long freezing-thawing periods¹¹11 Hain T, Chatterjee SS, Ghai R, et al. Pathogenomics of Listeria spp. Int J Med Microbiol. 2007;297:541-557. are responsible for the increasing risks of food contamination with this bacterium.

Since 1980s, L. monocytogenes has emerged as a major public health burden. Nevertheless, its importance as a food-borne pathogen is not always recognized, due to a very long incubation period between consumption of the contaminated food and onset of illness as well as sporadic exposure. Nowadays L. monocytogenes represents a serious challenge to food safety and it is one of the microorganisms of significant concern the food industry.¹²12 López V, Suárez M, Chico-Calero I, Navas J, Martínez-Suárez J. Foodborne Listeria monocytogenes: are all the isolates equally virulent? Rev Argent Microbiol. 2006;38:224-234.

13 Montero D, Bodero M, Riveros G, et al. Molecular epidemiology and genetic diversity of Listeria monocytogenes isolates from a wide variety of ready-to-eat foods and their relationship to clinical strains from listeriosis outbreaks in Chile. Front Microbiol. 2015;6:1-9.^-¹⁴14 O’Connor L, O’Leary M, Leonard N, et al. The characterization of Listeria spp. isolated from food products and the food-processing environment. Lett Appl Microbiol. 2010;51:490-498.

While several phenotypic and genotypic methods have been described and applied to the study of L. monocytogenes isolates, the most frequently used are serotyping and DNA macro-restriction digest followed by pulsed-field gel electrophoresis (PFGE).¹⁵15 Cardozo A, Ramón L, Poutou R, Carrascal A, Zambrano D. Electroforesis en Gel de Campo Pulsado (PFGE) para la diferenciación molecular de Listeria monocytogenes. Univ Sci. 2013;18:203-222.

16 Chenal-Francisque V, Diancourt L, Cantinelli T, et al. Optimized multilocus variable-number tandem-repeat analysis assay and its complementarity with pulsed-field gel electrophoresis and multilocus sequence typing for Listeria monocytogenes clone identification and surveillance. J Clin Microbiol. 2013;51:1868-1880.

17 Kérouanton A, Marault M, Petit L, Grout J, Dao TT. Evaluation of a multiplex PCR assay as an alternative method for Listeria monocytogenes serotyping. J Microbiol Methods. 2010;80:134-137.

18 Lepe J, Torres M, Liró J, Luque R, Aznar J. Caracterización microbiológica de los aislados de Listeria monocytogenes procedentes de casos humanos en Andalucía. Enf Inf Microbiol Clin. 2012;30:602-607.

19 Liu D. Identification, subtyping, and virulence determination of Listeria monocyotgenes an important foodborne pathogen. J Med Microbiol. 2006;55:645-659.

20 Gerner-Smith P, Hise K, Kincaid J, et al. PulseNet USA: a five-year update. Foodborne Pathog Dis. 2006;3:9-19.

21 Graves L, Swaminathan B. PulseNet standardized protocol for subtyping Listeria monocytogenes by macro-restriction and pulsed-field gel electrophoresis. Int J Food Microbiol. 2001;65:55-62.

22 Neves E, Lourenço A, Silva A, Coutinho R, Brito L. Pulsed-field gel electrophoresis (PFGE) analysis of Listeria monocytogenes isolates from different sources and geographical origins and representative of the twelve serovars. Syst Appl Microbiol. 2008;31:387-392.^-²³23 Doumith M, Buchrieser C, Glaser P, Jacquet C, Martin P. Differentiation of the major Listeria monocytogenes Serovars by multiplex PCR. J Clin Microbiol. 2004;42:3819-3822. PFGE remains as the gold standard method applied to the study of listeriosis outbreaks.¹⁹19 Liu D. Identification, subtyping, and virulence determination of Listeria monocyotgenes an important foodborne pathogen. J Med Microbiol. 2006;55:645-659.

20 Gerner-Smith P, Hise K, Kincaid J, et al. PulseNet USA: a five-year update. Foodborne Pathog Dis. 2006;3:9-19.

21 Graves L, Swaminathan B. PulseNet standardized protocol for subtyping Listeria monocytogenes by macro-restriction and pulsed-field gel electrophoresis. Int J Food Microbiol. 2001;65:55-62.^-²²22 Neves E, Lourenço A, Silva A, Coutinho R, Brito L. Pulsed-field gel electrophoresis (PFGE) analysis of Listeria monocytogenes isolates from different sources and geographical origins and representative of the twelve serovars. Syst Appl Microbiol. 2008;31:387-392.^,²⁴24 Foerster C, Gonzalez-Hein G, Troncoso M, Figueroa G. Pulsed-field gel electrophoresis pattern similarities between Listeria monocytogenes isolated from human patients and poultry in Chile. CyTA - J Food. 2013;11:14-18.. Serotyping is an additional tool to characterize L. monocytogenes isolates.²³23 Doumith M, Buchrieser C, Glaser P, Jacquet C, Martin P. Differentiation of the major Listeria monocytogenes Serovars by multiplex PCR. J Clin Microbiol. 2004;42:3819-3822. To date, 13 serotypes have been defined for L. monocytogenes. More than 90% of the recovered strains from food, animal and human samples typically belong to serotypes 1/2a, 1/2b, 1/2c and 4b. The multiplex PCR assay previously described by Doumith et al.,²³23 Doumith M, Buchrieser C, Glaser P, Jacquet C, Martin P. Differentiation of the major Listeria monocytogenes Serovars by multiplex PCR. J Clin Microbiol. 2004;42:3819-3822. appears as practical screening procedure to identify these serotypes.

PFGE remain as the gold standard method applied to the study of listeriosis outbreaks.¹⁹19 Liu D. Identification, subtyping, and virulence determination of Listeria monocyotgenes an important foodborne pathogen. J Med Microbiol. 2006;55:645-659.

20 Gerner-Smith P, Hise K, Kincaid J, et al. PulseNet USA: a five-year update. Foodborne Pathog Dis. 2006;3:9-19.

21 Graves L, Swaminathan B. PulseNet standardized protocol for subtyping Listeria monocytogenes by macro-restriction and pulsed-field gel electrophoresis. Int J Food Microbiol. 2001;65:55-62.^-²²22 Neves E, Lourenço A, Silva A, Coutinho R, Brito L. Pulsed-field gel electrophoresis (PFGE) analysis of Listeria monocytogenes isolates from different sources and geographical origins and representative of the twelve serovars. Syst Appl Microbiol. 2008;31:387-392.^,²⁴24 Foerster C, Gonzalez-Hein G, Troncoso M, Figueroa G. Pulsed-field gel electrophoresis pattern similarities between Listeria monocytogenes isolated from human patients and poultry in Chile. CyTA - J Food. 2013;11:14-18.

The purposes of this work were to study the prevalence of L. monocytogenes contamination in various food samples obtained from retail store and food industries located in Montevideo city, Uruguay and to identify the main serotypes of the obtained isolates.

Materials and methods

Processing of food samples

Between October 2011 and August 2013, 3175 food samples were analyzed (220 were frozen products, both from animal and vegetable source; 2180 ready-to-eat foods, from animal and vegetable origin; 580 deli meats; and 195 cheese) at the Bromatological Laboratory (Intendencia de Montevideo). Samples were taken from 236 establishments (retail shops and food industries) located in Montevideo city, Uruguay as part of a food safety surveillance program.

For microbiological studies, pools of five products from the same establishment and food category were prepared (44 of frozen products, 436 of ready-to-eat foods, 116 of deli meats, and 39 of cheese, respectively) and were analyzed according to ISO 11290-1-1996 and ISO 11290-1:1996/Amd 1:2004 guide²⁵25 ISO (International Organization for Standardization) 11290-1. Microbiology of food and animal feeding stuffs. In: Horizontal Method for the Detection and Enumeration of Listeria monocytogenes. Part 1: Detection method. Geneva: International Organization for Standardization, International Electrotechnical Committee; 1996.^,²⁶26 ISO (International Organization for Standardization) 11290-1:1996/Amd 1. Modification of the Isolation Media and the Haemolysis Test, and Inclusion of Precision Data. Geneva: International Organization for Standardization, International Electrotechnical Committee; 2004. using a real-time PCR DuPont Qualicon BAX^® System (DuPont Qualicon, Wilmington, DE, USA) following the manufacturer's instructions.

L. monocytogenes isolation and identification

Positive samples according to real-time PCR results were streaked onto two selective media plates: Oxford medium base with Modified Oxford Antimicrobic Supplement (BD - Becton, Dickinson and Company, Franklin Lakes, NJ, USA) and BBL™ CHROMagar™Listeria (BD), both incubated for 24-48 h at 35-37 °C. Suspect colonies (small, convex and surrounded by a black halo; blue colonies less than 3 mm in diameter and surrounded by a white halo, respectively) were identified using API Listeria kit (bioMérieux, Marcy l’Etoile, France) and additional standard biochemical assays that included: β-Hemolysis halo production on Trypticase Soy Agar (BD) supplemented with sheep blood (5%) plates, catalase reaction, bile esculin; and Christie-Atkins-Munch-Petersen (CAMP) tests with control strains of Staphylococcus aureus and Rhodococcus equi.²⁷27 Wellinghausen N. Listeria and erysipelothrix. In: Versalovics J, Carrol KC, Funke G, Jorgensen JH, Landry ML, Warnok DW, eds. Manual of Clinical Microbiology. 10th ed. Washington, DC: ASM Press; 2011:461-471.

When food samples from retail shop or factory displayed positive results to L. monocytogenes, it was visited again and samples of the same food types were taken and analyzed according to the above described procedure.

Confirmed L. monocytogenes isolates were conserved in 10% reconstituted skim milk at -20 °C and also in 20% glycerol at -80 °C for further assays.

Serotyping

Multiplex PCR was used to determine L. monocytogenes serogroup as described previosly.²³23 Doumith M, Buchrieser C, Glaser P, Jacquet C, Martin P. Differentiation of the major Listeria monocytogenes Serovars by multiplex PCR. J Clin Microbiol. 2004;42:3819-3822. Briefly, DNA was extracted from colonies grown overnight in Trypticase Soy Agar plates (BD) supplemented with sheep blood (5%). Colonies (4-5) were suspended in 50 µL of lysis buffer (SDS 0.25%, NaOH 0.05 N) and boiled for 15 min. Then, 100 µL of ultra-purified water was added to each tube and centrifuged at 15 000 × g for 15 min. Supernatant (2 µL) was used in each PCR reaction.

The amplification reactions were carried out in a Gene Amp PCR System 2700 thermocycler (Applied Biosystems^®, Foster City, CA, USA). PCR products were run in 2% agarose gel and visualized by staining with ethidium bromide. L. monocytogenes serotype 1/2a (CIP 89381), L. monocytogenes serotype 1/2b (CIP 90602), L. monocytogenes serotype 1/2c (CIP 89756) and L. monocytogenes serotype 4b (CIP 88868) strains were used as positive controls and ultra purified water as negative control. Classical serotyping for L. monocytogenes 1 and 4 somatic antigens was carried out using commercially available Listeria Antisera (BD) according to manufacturer's instructions for strains belonging to PCR serogroups IIa, IIb, IIc and IVb.

Pulsed-field gel electrophoresis (PFGE)

PFGE was performed according to CDC procedure for L. monocytogenes using only the ApaI restriction enzyme.²⁸28 Centers for Disease Control and Prevention. Standard Operating Procedure for PulseNet PFGE of Listeria monocytogenes. Atlanta, GA: CDC; 2013 (PNL04 Last Updated April 2013). This procedure was applied only to isolates belonging to the same serotype recovered from the same establishment. Briefly, bacterial suspensions were adjusted to an optical density of 1.4 at 610 nm, mixed with equal volume of 1.2% pulsed-field grade certified agarose (Bio-Rad, Hercules, CA, USA) solution preheated to 55 °C, and then placed into suitable molds. Plugs were washed six times with wash solution, cut in thick pieces (height ca. 2 mm) and digested for 2 h at 30 °C with 25 U of ApaI restriction enzyme (New England Biolabs Inc., Ipswich, MA, USA).

The separation of DNA fragments was performed by using a CHEF DR-II system (Bio-Rad). Salmonella enterica serotype Braenderup (CDCH9812) was included as molecular mass control. We also included one isolate belonging to serotype 1/2c, recovered in this study.

The bands were visualized by gel staining with 100 µg/mL ethidium bromide, and the image was captured with the FOTO/Analyst™ Investigator Eclipse FOTODYNE system (Thermo Fischer Scientific, Waltham, MA, US). PFGE patterns were analyzed using the BioNumerics software, 6.1 version (Applied Maths NV, Sint-Martens-Latem, Belgium). The Dice correlation coefficient was used to determine the similarity levels.²⁹29 Dice L. Measures of the amount of ecologic association between species. Ecology. 1945;26:297-302. For the cluster patterns analysis the UPGMA (unweighted-pair group matching algorithm)²⁴24 Foerster C, Gonzalez-Hein G, Troncoso M, Figueroa G. Pulsed-field gel electrophoresis pattern similarities between Listeria monocytogenes isolated from human patients and poultry in Chile. CyTA - J Food. 2013;11:14-18.^,³⁰30 Jain A, Murty M, Flynn P. Data clustering: a review. ACM Compt Sur. 2000;31:264-323. was used with a tolerance and optimization of 1.5%. Strains that showed ≥80% similarity were considered as belonging to the same pulsogroup.¹³13 Montero D, Bodero M, Riveros G, et al. Molecular epidemiology and genetic diversity of Listeria monocytogenes isolates from a wide variety of ready-to-eat foods and their relationship to clinical strains from listeriosis outbreaks in Chile. Front Microbiol. 2015;6:1-9.

Results

Occurrence of L. monocytogenes in different types of food

We isolated L. monocytogenes from 71 out of 635 (11.2%; 95% CI 8.75-13.65%) pooled food samples. The distribution of 71 L. monocytogenes isolates included frozen foods (17), ready-to-eat (42), deli meats (8), and cheese (4). The highest prevalence of L. monocytogenes contamination was observed in frozen foods (38%; 95% CI 24-52%), followed by cheese (10%; 95% CI 0.6-19.4%), RTE samples (9%; 95% CI 6.3-11.7%) and deli meat (7%; 95% CI 2.4-11.6).

Serotype determination and distribution in food

All isolates identified as serogroup IIa, IIb and IIc by multiplex PCR showed positive agglutination with serotype 1 antiserum; and were considered serotypes 1/2a, 1/2b and 1/2c, respectively. Because the serotypes 4d and 4e are rare both in food and human samples,²³23 Doumith M, Buchrieser C, Glaser P, Jacquet C, Martin P. Differentiation of the major Listeria monocytogenes Serovars by multiplex PCR. J Clin Microbiol. 2004;42:3819-3822. all the isolates that were PCR-positive for serogroup IVb were considered serotype 4b. In the present study 1/2b and 4b were the most frequently identified serotypes: 33 strains (45.83%) and 30 strains (41.67%), respectively; followed by 1/2a, 5 strains (6.94%) and 1/2c, 3 strains (4.17%). Table 1 shows the serotype distribution of L. monocytogenes isolated from food samples analyzed in this study.

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Table 1
Serotype distribution of Listeria monocytogenes in different analyzed food samples.

PFGE profiles

In 41 out of 236 (17.4%) establishments we recovered L. monocytogenes, and in 27 (68%) of them this agent was again isolated in later visits. In only six cases (15%) we repeatedly recovered L. monocytogenes belonging to the same serotype (Fig. 1). Most of these isolates (12 out of 16) corresponded to serotype 1/2b and were recovered from food samples taken from five out of six establishments. In four out of five (#1, #4, #5 and #6) we identified 1/2b isolates with an identical PFGE pattern in successive visits (Fig. 1). The analyzed isolates from the sixth establishment (#3) corresponded to serotype 4b.

Fig. 1
Dendrogram of L. monocytogenes isolates belonging to the same serotype and recovered from the same company. One isolate belonging to 1/2c serotype from this study is also included as control. Most 1/2b isolates analyzed by ApaI PFGE were in the same pulsogroup (similarity > 80%). RTE, ready-to-eat food (sandwiches, vegetable salads).

In four establishments (#1, #4, #5 and #6) we recovered successive 1/2b isolates that had an identical ApaI PFGE pattern to the first isolate (Fig. 1). Also, in two different companies (#1 and #2) we recovered two isolates (IM 257 and IM 171, respectively) belonging to serotype 1/2b that showed identical ApaI PFGE profile. In company #3, we detected four isolates belonging to serotype 4b in successive visits. Isolates IM 228 and IM 230 showed a 90% > similarity; whereas isolates IM 224 and IM 288, had a similarity of 63% (Fig. 1).

Discussion

The overall prevalence of L. monocytogenes contamination found in this set of analyzed foods (11.2%) is lower than that previously reported in Chile (25%)¹³13 Montero D, Bodero M, Riveros G, et al. Molecular epidemiology and genetic diversity of Listeria monocytogenes isolates from a wide variety of ready-to-eat foods and their relationship to clinical strains from listeriosis outbreaks in Chile. Front Microbiol. 2015;6:1-9. or in China (22%).³¹31 Chen M, Wu Q, Zhang J, Wu S, Guo W. Prevalence, enumeration, and pheno- and genotypic characteristics of Listeria monocytogenes isolated from raw foods in South China. Front Microbiol. 2015;6:1026, eCollection 2015. Differences in prevalence may be due to the types of analyzed food in our investigation. We did not analyze pâté; instead, Montero et al. included 62 samples of this food category and they found that 55% were contaminated with L. monocytogenes.¹³13 Montero D, Bodero M, Riveros G, et al. Molecular epidemiology and genetic diversity of Listeria monocytogenes isolates from a wide variety of ready-to-eat foods and their relationship to clinical strains from listeriosis outbreaks in Chile. Front Microbiol. 2015;6:1-9. Likewise, prevalence figures lower than those found by us have been reported. In India, examining other food types involved in the spread of L. monocytogens as milk, ice cream, fruit salad, meat and fish, Nayak et al. found an overall prevalence of 1.5%.³²32 Nayak DN, Savalia CV, Kalyani IH, Kumar R, Kshirsagar DP. Isolation, identification, and characterization of Listeria spp. from various animal origin foods. Vet World. 2015;8:695-701.

As was previously reported in China by Chen et al.,³¹31 Chen M, Wu Q, Zhang J, Wu S, Guo W. Prevalence, enumeration, and pheno- and genotypic characteristics of Listeria monocytogenes isolated from raw foods in South China. Front Microbiol. 2015;6:1026, eCollection 2015. in the present study the highest prevalence of L. monocytogenes contamination was observed in frozen foods (38%) such as pizza, fish fillets, lasagna, ravioli, chicken, and meat; followed by cheese (10%) and RTE samples (9%) (sandwiches, vegetable salads, chicken salads, Bolognese sauce, cheesecake and apple pie). These findings highlight the potential role that these food categories may play in the spread of this bacterium and alert to health personnel about the need to proper handling and cooking in individuals that have known high-risk of developing severe illness as pregnant women, elderly people and immunocompromised patients.⁴4 Vazquez-Boland J, Kuhn M, Berche P, et al. Listeria pathogenesis and molecular virulence determinants. Clin Microbiol Rev. 2001;14:584-640.^,⁵5 Cossart P. Illuminating the landscape of host-pathogen interactions with the bacterium Listeria monocytogenes. Proc Natl Acad Sci U S A. 2011;108:19484-19491.

In our study, 1/2b and 4b were the most frequently recovered serotypes, followed by 1/2a and 1/2c. In Chile, Montero et al.,¹³13 Montero D, Bodero M, Riveros G, et al. Molecular epidemiology and genetic diversity of Listeria monocytogenes isolates from a wide variety of ready-to-eat foods and their relationship to clinical strains from listeriosis outbreaks in Chile. Front Microbiol. 2015;6:1-9. found a slightly different distribution; with 4b serotype (46%) being the most prevalent, followed by 1/2a (32%) and 1/2b (13%). The observed variation may be due to differences in the types of food included in each investigation. Likewise, in Colombia, Muñoz³³33 Muñoz A. Distribución de serotipos de Listeria monocytogenes aislados de alimentos, Colombia, 2000-2009. Biomédica. 2012;32:408-417. found that the most prevalent serotypes isolated from 1424 food samples taken between 2000 and 2009 were 4b, 1/2b, 1/2a, with an evident predominance of strains belonging to 4b regarding the other serotypes (ratio of 5 to 1). In contrast, the most common serotypes isolated from RTE food (including natural cheese, meat products, seafood and pickled vegetables) in Japan were 1/2a (47.6%), 1/2b (20.6%) and 4b (14.3%).³⁴34 Shimojima Y, Ida M, Nakama A, et al. Prevalence and contamination levels of Listeria monocytogenes in ready-to-eat foods in Tokyo, Japan. J Vet Med Sci. 2016;78:1183-1187. Similar findings were reported in other countries of the northern hemisphere. In Poland, Korsak et al.,³⁵35 Korsak D, Borek A, Daniluk S, Grabowska A, Pappelbaum K. Antimicrobial susceptibilities of Listeria monocytogenes strains isolated from food and food processing environment in Poland. Int J Food Microbiol. 2012;158:203-208. analyzed 471 L. monocytogenes strains isolated from different foods and found the following serotype distribution: 1/2a, 54.4%; 1/2c, 25.5%; 1/2b, 12.5% and 4b 7.6%. In Ireland, O’Connor et al.¹⁴14 O’Connor L, O’Leary M, Leonard N, et al. The characterization of Listeria spp. isolated from food products and the food-processing environment. Lett Appl Microbiol. 2010;51:490-498. found that the most common serotype present in different food categories was 1/2a followed by 4b. Also in China, Chen et al. found that the most prevalent isolates from raw foods corresponded to serotypes 1/2a and 1/2b.³¹31 Chen M, Wu Q, Zhang J, Wu S, Guo W. Prevalence, enumeration, and pheno- and genotypic characteristics of Listeria monocytogenes isolated from raw foods in South China. Front Microbiol. 2015;6:1026, eCollection 2015. In the present study, 87% of the analyzed L. monocytogenes isolates belong to lineage I (1/2b and 4b); the remaining cultures belong to lineage II (1/2a and 1/2c). Both lineages include the most commonly recovered serotypes from human listeriosis cases. Our results contrast with other reports showed that strains belonging to lineage II are more prevalent in foods.¹⁵15 Cardozo A, Ramón L, Poutou R, Carrascal A, Zambrano D. Electroforesis en Gel de Campo Pulsado (PFGE) para la diferenciación molecular de Listeria monocytogenes. Univ Sci. 2013;18:203-222.^,³⁶36 Orsi RH, den Bakker HC, Wiedmann M. Listeria monocytogenes lineages: genomics, evolution, ecology and phenotypic characteristics. Int J Med Microbiol. 2011;301:79-96.^,³⁷37 Shen J, Rump L, Zhang Y, Chen Y, Wang X, Meng J. Molecular subtyping and virulence gene analysis of Listeria monocytogenes isolates from food. Food Microbiol. 2013;35:58-64. These authors suggest that the higher genetic variation seen in lineage II strains is consistent with adaptation to more diverse environments.

As occurs in Chile, Colombia, Ireland, Japan, and other countries, serotypes recovered in the present study are responsible for human listeriosis cases.¹⁰10 Swaminathan B, Gerner-Smidt P. The epidemiology of human listeriosis. Microbes Infect. 2007;9:1236-1243.^,¹¹11 Hain T, Chatterjee SS, Ghai R, et al. Pathogenomics of Listeria spp. Int J Med Microbiol. 2007;297:541-557.^,¹³13 Montero D, Bodero M, Riveros G, et al. Molecular epidemiology and genetic diversity of Listeria monocytogenes isolates from a wide variety of ready-to-eat foods and their relationship to clinical strains from listeriosis outbreaks in Chile. Front Microbiol. 2015;6:1-9.^,¹⁴14 O’Connor L, O’Leary M, Leonard N, et al. The characterization of Listeria spp. isolated from food products and the food-processing environment. Lett Appl Microbiol. 2010;51:490-498.^,¹⁹19 Liu D. Identification, subtyping, and virulence determination of Listeria monocyotgenes an important foodborne pathogen. J Med Microbiol. 2006;55:645-659.^,³³33 Muñoz A. Distribución de serotipos de Listeria monocytogenes aislados de alimentos, Colombia, 2000-2009. Biomédica. 2012;32:408-417.^,³⁸38 Kalekar S, Rodrigues J, D’ Costa D, et al. Genotypic characterization of Listeria monocytogenes isolated from humans in India. Ann Trop Med Parasitol. 2011;105:351-358.^,³⁹39 Leong D, Alvarez-Ordoñez A, Jordan K. Monitoring occurrence and persistence of Listeria monocytogenes in foods and food processing environments in the Republic of Ireland. Front Microbiol. 2014;5:1-8. In Uruguay severe cases of listeriosis in people have been attributed to serotypes 1/2a, 1/2b and 4b isolates. In the same period in which this study was conducted, we received at the Department of Bacteriology and Virology laboratory 26 isolates of L. monocytogenes recovered from human samples; 14 of them belonged to serotype 1/2b, 9 to 4b and 3 to 1/2a (unpublished results).

Unlike what occurs in some northern hemisphere countries, L. monocytogenes belonging to serotype 4b appears to be prevalent in foods from several South American countries including Uruguay.¹³13 Montero D, Bodero M, Riveros G, et al. Molecular epidemiology and genetic diversity of Listeria monocytogenes isolates from a wide variety of ready-to-eat foods and their relationship to clinical strains from listeriosis outbreaks in Chile. Front Microbiol. 2015;6:1-9.^,³³33 Muñoz A. Distribución de serotipos de Listeria monocytogenes aislados de alimentos, Colombia, 2000-2009. Biomédica. 2012;32:408-417.^,⁴⁰40 De Vasconcelos Byrne V, Hofer E, Vallim D, de Castro Almeida RC. Occurrence and antimicrobial resistance patterns of Listeria monocytogenes isolated from vegetables. Braz J Microbiol. 2016;47:438-443. Therefore, it would be interesting to perform other studies to test for a possible hemispheric correlation with L. monocytogenes serotypes. Especially taking into account the ability of this serotype to produce severe illnesses and also considering that some investigators suggest that 4b serotype strains may have a higher tendency to cause outbreaks when they are present in foods.³³33 Muñoz A. Distribución de serotipos de Listeria monocytogenes aislados de alimentos, Colombia, 2000-2009. Biomédica. 2012;32:408-417.^,⁴¹41 Kanki M, Naruse H, Taguchi M, Kumeda Y. Characterization of specific alleles in InlA and PrfA of Listeria monocytogenes isolated from foods in Osaka, Japan and their ability to invade Caco-2 cells. Int J Food Microbiol. 2015;211:18-22.

Apart from the deli meat samples, in the remaining analyzed food samples (frozen foods, ready-to-eat and cheese) 1/2b and 4b isolates accounted for over 90% of the isolates. This result suggest the role of these food categories in the spread of L. monocytogenes strains belonging to serotypes frequently recovered from human cases of listeriosis.

The PFGE results suggest that isolates belonging to serotype 1/2b have a capacity to survive for prolonged periods in the environment and/or food. In this regard, 19 months after the first visit at establishment #5 we recovered one isolate 1/2b that showed an identical ApaI PFGE pattern to the first one. Similar observations were made at premises #1, #4 and #6, although in these cases the time elapsed between visits was lower (3 months, 27 and 15 days, respectively). These results agree with that previously suggested by Orsi et al. about the higher genetic stability of L. monocytogenes strains belonging to lineage I.³⁶36 Orsi RH, den Bakker HC, Wiedmann M. Listeria monocytogenes lineages: genomics, evolution, ecology and phenotypic characteristics. Int J Med Microbiol. 2011;301:79-96.

In two different companies (#1 and #2) and in different periods (10 month apart), we recovered two isolates (IM 257 and IM 171, respectively) belonging to serotype 1/2b with identical ApaI PFGE profile. It could be because both establishments share product suppliers. On the other hand, in company #3, we recovered four isolates of serotype 4b from frozen food. Isolates IM 228 and IM 230 were recovered eight months apart and showed a similarity of 93%. Instead, isolates IM 224 and IM 288 were recovered one year apart and showed a 63% similarity. It is difficult to establish by PFGE whether these last pair it is the same isolate that suffered genetic modifications or they are two different isolates.⁴²42 Tenover FC, Arbeit RD, Goering RV, et al. Interpreting chromosomal DNA restriction patterns produced by pulsed-field gel electrophoresis: criteria for bacterial strain typing. J Clin Microbiol. 1995;33:2233-2239. We must analyze them by PFGE using another restriction enzyme or with other procedures such as MLST or WGS, among other typing methods, for proper characterization.¹⁶16 Chenal-Francisque V, Diancourt L, Cantinelli T, et al. Optimized multilocus variable-number tandem-repeat analysis assay and its complementarity with pulsed-field gel electrophoresis and multilocus sequence typing for Listeria monocytogenes clone identification and surveillance. J Clin Microbiol. 2013;51:1868-1880.^,⁴³43 Holch A, Webb K, Lukjancenko O, Ussery D, Rosenthal B, Grame L. Genome sequencing identifies two nearly unchanged strains of persistent Listeria monocytogenes isolated at two different fish processing plants sampled 6 years apart. Appl Environ Microbiol. 2013;79:2944-2951. They could even correspond to different serotypes, taking into account the aforementioned limitations of serotyping procedure used. The overall PFGE results obtained in the present study suggest that at least 11 out of 33 1/2b isolates recovered from different foods are part of a single pulsogroup (similarity ≥ 80%).

Conclusions

The present study provided the first data about food prevalence and serotype distribution of L. monocytogenes in foods in Uruguay. The highest prevalence was observed in frozen foods followed by cheese and RTE samples. Our results highlight the potential role that these food categories may play in the spread of this food-borne pathogen and alert to health personnel about the need to proper handling and cooking in individuals that have known high-risk of developing severe. 1/2b and 4b were the most frequently identified serotypes. The ApaI PFGE results suggest that most 1/2b strains recovered from different foods are genetically related and that they may remain viable for prolonged periods in frozen food and/or food production, storage and distribution environments. These findings highlight the need to apply standardized sanitary and control practices to reduce the contamination with this pathogen in the food production chains.

Funding

This work was supported by Comisión Sectorial de Investigación Científica-UdelaR, programa CSIC-Grupos, ID 290 to GV and FS.
Funding

This work was supported by Comisión Sectorial de Investigación Científica-UdelaR, programa CSIC-Grupos, ID 290 to GV and FS.

Acknowledgements

We thank PhD. Teresa Camou for providing the reference strains of L. monocytogenes and Mrs. Clara Menéndez for critically reading the manuscript.

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⁴¹
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Publication Dates

Publication in this collection
Oct-Dec 2017

History

Received
12 Sept 2016
Accepted
12 Jan 2017

This is an Open Access article distributed under the terms of the Creative Commons Attribution Non-Commercial No Derivative License, which permits unrestricted non-commercial use, distribution, and reproduction in any medium provided the original work is properly cited and the work is not changed in any way.

[1] Funding

This work was supported by Comisión Sectorial de Investigación Científica-UdelaR, programa CSIC-Grupos, ID 290 to GV and FS.

[2] Funding

This work was supported by Comisión Sectorial de Investigación Científica-UdelaR, programa CSIC-Grupos, ID 290 to GV and FS.

Food category (number of analyzed pools)
	Frozen (44)	Ready to eat (436)	Deli meat (116)	Cheese (39)
Serotype	Number of products (%) positive for a particular serotype
1/2a	2 (11.76)	3 (7.14)	0 (0)	0 (0)
1/2b	6 (35.29)	19 (45.24)	6 (75)	2 (50)
1/2c	1 (5.88)	0 (0)	2 (25)	0 (0)
4b	8 (47.08)	20 (47.62)	0 (0)	2 (50)

Total	17 (100)	42 (100)	8 (100)	4 (100)

Brasil