Evaluation of skimmed milk flocculation method for virus recovery from tomatoes

Melgaço, Fabiana Gil; Corrêa, Adriana Abreu; Ganime, Ana Carolina; Brandão, Marcelo Luiz Lima; Medeiros, Valéria de Mello; Rosas, Carla de Oliveira; Lopes, Silvia Maria dos Reis; Miagostovich, Marize Pereira

doi:10.1016/j.bjm.2018.04.014

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Table 1. Recovery success rate (%) and recovery efficiency (%) of skimmed flocculation analyzed in 24 qPCR reactions for norovirus genogroup II (NoV GII), murine nororovirus 1 (MNV-1) and human adenovirus type 2 (HAdV-2).

Abstract

This study aimed to evaluate the elution-concentration methodology based on skimmed milk flocculation from three varieties of tomatoes (Solanum lycopersicum L. [globe], Solanum lycopersicum var. cerasiforme [cherry] and hybrid cocktail [grape tomato]) for further monitoring of field samples. Spiking experiments were performed to determine the success rate and efficiency recovery of human norovirus (NoV) genogroup II, norovirus murine-1 (MNV-1) used as sample process control virus and human adenovirus (HAdV). Mean values of 18.8%, 2.8% and 44.0% were observed for NoV GII, MNV-1 and HAdV, respectively with differences according to the types of tomatoes, with lower efficiency for cherry tomatoes. Analysis of 90 samples, obtained at commercial establishments in the metropolitan region of Rio de Janeiro State, revealed 4.5% positivity for HAdV. Bacterial analysis was also performed with no detection of Salmonella spp., L. monocytogenes and fecal coliforms. Data demonstrated that the skimmed milk flocculation method is suitable for recovering HAdV from tomatoes and highlights the need for considering investigation in order to improve food safety.

Keywords:

Adenovirus

Flocculation

Murine norovirus-1

Norovirus

Tomato

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Introduction

Enteric viruses are described as important contaminants of fresh foods as vegetables and fruits, considering the inadequate system of water irrigation or inappropriate food handling as possible routes of contamination.1 Among those, noroviruses (NoV) are the main agent causing acute gastroenteritis (AG) outbreaks associated with consumption of fresh products worldwide.2–7 NoVs are RNA viruses and its genome is composed of RNA single-strand positive-sense, belonging to genus Norovirus, Caliciviridae family and classified into seven different genogroups (G) and more than 35 genotypes.8,9 NoV GI, GII, and GIV can infect human, NoV GII.4 is the most prevalent genotype related to foodborne infection.10

Additionally, other viruses such as human adenoviruses (HAdV) have been also investigated in water and food samples.11,12 Even though they are rarely associated with foodborne illnesses some of them are associated with cases of gastroenteritis.11,13–16 Currently they have been investigated as indicators of human fecal contamination mainly due to their resistance to adverse environmental conditions, absence of seasonality and its high concentration detected in wastewater samples.12,16,17 HAdVs are DNA viruses belonging to the Adenoviridae family and genus Mastadenovirus with 67 types reported.18

The increasing number of viruses foodborne outbreaks have resulted in a growing number of studies that evaluate elution and concentration methods from different food matrices, as well as the use of sample processes control viruses (SPCVs) as murine norovirus-1 (MNV-1), bacteriophage PP7 and others.19–26 In 2013, the International Organization for Standardization (ISO), together with the European Committee for Standardization (CEN), standardized methodologies for recovering NoV and hepatitis A virus from matrix foods27 that were validated recently.28

This study aims to expand previous studies that adapted successfully skimmed milk flocculation method to recover virus from strawberries.29 Here, we assess NoV, MNV-1 and HAdV success rate and efficiency recoveries from three varieties of tomatoes as well as assess their microbiological quality by investigating NoV GI and GII, HAdV, Salmonella spp., Listeria monocytogenes and fecal coliforms from samples obtained at market places at the Great Metropolitan Region of Rio de Janeiro State.

Materials and methodsViruses and food samples

A NoV GII.4 stool sample (GenBank accession number JX975591) was obtained from the Regional Reference Gastroenteritis Laboratory collection, at Oswaldo Cruz Institute, Rio de Janeiro-RJ, Brazil. Murine norovirus-1 (MNV-1) was kindly provided by Dr. Herbert W. Virgin (Washington University School of Medicine) and propagated in RAW 264.7 cells (a macrophage-like Abelson leukemia virus-transformed cell line derived from BALB/c mice; ATCC®TIB-71™), according to de Abreu Corrêa and Miagostovich.24 HAdVs type 2 was propagated in HEK 293 cells (human embryonic kidney cells; ATCC®CRL1573™) obtained from the Regional Reference Gastroenteritis Laboratory collection, at Oswaldo Cruz Institute, Rio de Janeiro, RJ, Brazil.30

Three species of tomatoes as Solanum lycopersicum L. (globe), Solanum lycopersicum var. cerasiforme (cherry) and hybrid cocktail (grape) were obtained from distinct markets in Rio de Janeiro.

For field analysis 90 tomatoes samples (45 globe and 45 grape tomatoes) were randomly obtained from March to September, 2014 (three–five samples per week). All samples were inoculated with MNV-1, used as SPCV.

Spiking experiments for assessing efficiency of virus recovering using skimmed flocculation method.

Artificial contamination was carried out in duplicate in three independent experiments totaling six assays for each virus. The quantitative PCR (qPCR) TaqMan™ system was used to quantify the absolute number of genome copies (gc)/reaction31 used for those experiments.

Twenty-five grams of tomato samples were spiked by direct application of 250μL of NoV GII.4 (1×106gc/reaction), 100μL of MNV-1 (5×105gc/reaction) and 200μL of HAdV (1×106gc/reaction) onto food surfaces for 2h at room temperature. The values of gc/reaction for NoV GII.4 and MNV-1 spikes were obtained according to the formula shown in Eq. (1), where n is the average number of amplified copies, based on the standard curve; D is the dilution of extracted nucleic acid; V (μL) represent the volumes of cDNA produced (VE); of the eluted nucleic acid (VC); the suspension of virus particles inoculated in the sample (VG); of cDNA was added to the TaqMan (VF) reaction; of the template used for cDNA synthesis (VD); and nucleic acid extracted from the viral particle (obtained by cell culture or stool suspension) (VH). For HAdV, the same calculate, excluding VE and VD. One negative control (seeded with 350μL of phosphate saline buffer [PBS] 1×) was included and processed at the same time together with the other samples.

Skimmed milk flocculation method was performed as described by Melgaço et al.29 including the use of cetyltrimethylammonium bromide (CTAB) (Fig. 1).

Fig. 1.

Flow-chart of the viral elution-concentration method.

(0.16MB).

RNA/DNA extraction and viral detection

Viral RNA/DNA was extracted from 140μL of concentrated samples, using QIAamp viral RNA mini kit® (Qiagen, Valencia, CA, USA), according to manufacturer's instructions. Synthesis of complementary DNA (cDNA) was performed for NoV and MNV-1 detection using random primers, pd(N)6 (Amersham Biosciences, UK) for RNA virus detection.

QPCR using TaqMan™ assays were carried out using a set of specific primers and probes described previously.19,32,33 Reactions were performed using TaqMan Universal PCR Master Mix® (Applied Biosystems, California, USA) according to the manufacturer in ABI 7500® (Applied Biosystems).

For all genomic quantification, a standard curve was performed with eight points of serial plasmid dilutions (107–10°gc/reaction). All the standard curves yield a slope of −3.59 and a R2 (reaction efficiency) of 0.90. An ABI PRISM 7500™ real-time PCR system (Applied Biosystems, Foster City, CA, USA) was used. All samples were tested in duplicate using both undiluted and 1:10 diluted RNA, totalizing four qPCR reactions per sample. Samples were considered positive when at least one replica was detected at the cycle threshold (Ct) 40 or lower.

Bacterial analysis

Salmonella spp. analysis was performed using a semi-automated VIDAS® system (BioMérieux, France) kit using VIDAS®Salmonella (SLM) according to manufacturer's instructions. For L. monocytogenes, the culture method by selective enrichment technique was carried out according to standard methodology (Food and Drug Administration's Bacteriological Analytical Manual online (BAM-FDA).34 Fecal coliform was investigated using a Petrifilm™ Coliform Count Plate (3M, USA) according to the manufacturer's instructions.

Data analysis

Recovery of NoV GII, MNV-1 and HAdV from tomatoes samples was qualitatively and quantitatively analyzed according.35 Qualitative analysis of viral recovery was performed to determine recovery success rate, calculated as the number of qPCR reactions with successful NoV GII.4, MNV-1 or HAdV recovery per number of qPCR reactions performed. Quantitative recovery analyses from samples yielded recovery efficiency (%), calculated per individual sample as mean number of recovered viral genomic copies per inoculated number of NoV GII.4, MNV-1 or HAdV, genomic copies.

Statistical analysis of NoV GII.4 and MNV-1 recovery rates was performed using the nonparametric Mann–Whitney (MW-test), and Wilcoxon (t-test) tests followed by a Kolmogorov–Smirnov (KS-test) test. All statistical analyses were performed using GraphPad Prism 5.01 (GraphPad Software, San Diego, CA, USA). Significance levels were set at 0.05.

ResultsEfficiency of virus recovering

Table 1 shows success rate and recovery efficiency obtained from spiking experiments. No viruses were detected in PBS negative controls. For NoV GII.4, the recovery success rate was of 100% in all specimens, except for cherry and recovery efficiency that ranged from 5.2% to 33.4% with better results for globe and grape tomatoes (Table 1). CTAB treatment did not show significant increase in recovery success rate for all specimens. However, when comparing globe with cherry tomatoes CTAB revealed an increase in recovery efficiency for the first one (p=0.0043).

Table 1.

Recovery success rate (%) and recovery efficiency (%) of skimmed flocculation analyzed in 24 qPCR reactions for norovirus genogroup II (NoV GII), murine nororovirus 1 (MNV-1) and human adenovirus type 2 (HAdV-2).

Method	Types of tomatoes	Treatment	NoV GII.4			MNV-1			HAdV-2
			Positive samples (% recovery success)	Recovery efficiency (%) mean range		Positive samples (% recovery success)	Recovery efficiency (%) mean range		Positive samples (% recovery success)	Recovery efficiency (%) mean range
Skimmed milk flocculation	Globe Tomato	CTAB	24 (100.0)	33.4	7.9–66.3	18 (75.0)	4.1	1.7–9.5	24 (100.0)	60.7	9.8–92.7
		No CTAB	22 (91.6)	18.1	5.8–31.6	21 (87.5)	4.1	1.6–5.2	–	–	–
	Cherry tomato	CTAB	20 (83.3)	5.2	0.4–12.9	11 (45.8)	0.6	0.0–1.2	–	–	–
		No CTAB	21 (87.5)	9.8	0.5–27.0	11 (45.8)	1.9	0.0–5.7	–	–	–
	Grape tomato	CTAB	24 (100.0)	16.9	0.3–52.7	18 (75.0)	2.3	0.05–5.2	24 (100.0)	27.4	2.8–53.2
		No CTAB	24 (100.0)	29.6	2.5–110.9	19 (79.2)	4.2	0.2–11.1	–	–	–

(–) Not done.

For MNV-1 recovery success rate ranged from 45.8% to 87.5%, with lowest values results for cherry tomatoes. Recovery efficiency ranged from 0.6 to 4.2, also with lower results for cherry tomatoes.

For HAdV recovery success rate reach 100% for globe and grape tomatoes with efficiency or recovery of 60.7 and 27.4%, respectively.

Field study

HAdV was detected in four samples, three globe and one grape (4.5%) of the 90 samples tested, with concentrations ranging from 105 to 106gc/g in 25g of tomatoes. All samples were negative for NoV GI and NoV GII. MNV-1 used as SPCV was detected in all samples evaluated. No samples showed contamination by Salmonella spp. or L. monocytogenes (absence in 25g). Fecal coliform levels were <10 CFU/g in all samples tested.

Discussion

The use of organic flocculation method for virus recovery from tomatoes showed variable results among viruses and species studied, both for success rate and efficiency recoveries. In general, the method showed higher efficiency recoveries for NoV GII.4 and HAdV from tomato globe, with percentage of 33.4% and 60.7%, respectively. Considering the varieties analyzed the low recovery percentages obtained for cherry tomatoes was remarkable. Due to unsatisfactory results obtained for virus recovery from this variety, cherry tomatoes were not included in the field study. Previously, low virus recovery efficiency of cherry tomatoes was reported by Pan et al.36 suggesting problems of adsorption of virus on the food surface.

Concerning MNV-1, although the average of efficiency recoveries obtained were less than 5%, independently of the variety, its use as SPCV in field study was successful, with 100% detection in samples without dilution. MNV-1 experiments were also performed to evaluate success rate and recovery efficiency using methodology described by ISO 15216:2017 with results lower than those obtained by the organic flocculation method (data not shown). MNV-1 has been used as SPCV in other matrices, showing a good recovery percentage ranging from 7.78% to 75.65%35 and 8.4% to 66.4%.24

In this study CTAB treatment showed no improvement for NoV GII.4 and MNV-1 efficiency recovery. Although for NoV GII.4 CTAB treatment achieved a higher recovery rate when compared to data reported previously obtained for strawberry samples.29 In this study, we considered CTAB treatment once its use was efficient for strawberry samples.29 CTAB is a reagent described to eliminate possible inhibitors of qPCR reaction, as organic compounds, pigments and sugars present in food samples.37

The initial evaluation of the method with NoV GII.4 and MNV-1 focused on experiments performed later with HAdV, carried out only with globe and grape tomatoes and always using CTAB treatment. Another point to consider is detection limit of the method. As values of detection limit was lower for HAdV (102–103 gc/reaction) and for NoV GII (1.8×103gc/reaction), the high recovery rate and detection of the natural contamination of these viruses in samples evidence the importance of using the organic flocculation method (data not shown).

In relation to monitoring the microbiological quality of tomatoes obtained in the markets of the Greater metropolitan area of Rio de Janeiro, it is important to emphasize that detection of HAdV in samples met Brazilian Standards (a maximum of 102g−1 for fecal coliforms and absence of Salmonella spp./25g). Low levels of fecal coliforms found in this study can be attributed to good agriculture practices. In Brazil, cherry and grape tomatoes are cultivated within a closed system and in greenhouses, thus reducing the possibility of contamination.38,39 The absence of Salmonella spp. and L. monocytogenes in tomatoes also corroborated quality standard of this production demonstrated in studies carried out in the country.40 However, it is necessary to observe different possibilities of contamination until this product reaches the consumer, especially food handling.41,42 HAdV resistance to adverse environmental conditions as well as the absence of seasonality of these viruses reinforced their use as indicators of human fecal contamination in environmental samples,12,17,43 unlike NoVs, detected in association with outbreaks.44,45 Virus detection in tomatoes was described previously in Italy when NoV GII contamination was detected in commercially available tomatoes46 and when a consumption of dried tomatoes contaminated with HAV resulted in fulminant hepatitis.47

Concluding, based on our findings, this method has been proved as an alternative for detecting viruses and can be used for improving food safety programs, although further studies need to be performed in order to meet28 standards.

Funding sources

This work was supported by Ministério da Ciência, Tecnologia e Informação/Conselho Nacional de Desenvolvimento Científico e Tecnológico/Agência Nacional de Vigilância Sanitária (MCTI/CNPq/ANVISA – grant number 403264/2012-0). This research study is under the scope of the activities of Oswaldo Cruz Foundation (Fiocruz) as a Collaborating Center of PAHO/WHO of Public and Environmental Health.

Conflicts of interest

The authors declare no conflicts of interest.

Acknowledgment

We would like to thank Claudia P. Kamel for the English review.

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