Transfer and Inactivation of Listeria monocytogenes during Pilot-Scale Dicing and Flume Washing of Onions
Department of Food Science and Human Nutrition, Michigan State University, East Lansing, MI 48824, USA
*
Author to whom correspondence should be addressed.
Appl. Microbiol. 2024, 4(1), 439-452; https://doi.org/10.3390/applmicrobiol4010030
Submission received: 24 January 2024
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Revised: 16 February 2024
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Accepted: 22 February 2024
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Published: 27 February 2024
(This article belongs to the Special Issue Applied Microbiology of Foods 2.0)
Abstract
:This study assessed the extent of L. monocytogenes transfer from onions to the surface of a commercial dicer, from inoculated onions to uninoculated onions, and the efficacy of various sanitizers during the subsequent flume washing of diced onions. Spanish yellow onions (Allium cepa L.) were dip-inoculated in a 3-strain avirulent L. monocytogenes cocktail (5.9 or 4.2 log CFU/50 g) and air-dried. After dicing one 2.2 kg batch of onions inoculated at ~5.9 log CFU/50 g followed by ten uninoculated batches of 2.2 kg each, L. monocytogenes progressively decreased from 4.6 to 2.6 log CFU/50 g in baches 1 through 10, respectively. After onions inoculated at ~4.0 log CFU/g were diced and flume washed for 2 min in tap water, electrolyzed water containing 55 ppm free chlorine, 80 ppm free chlorine from a commercial sanitizer, or 80 ppm peroxyacetic acid and dewatered on a mechanical shaker table, L. monocytogenes populations decreased 0.4, 0.3, 1.4, and 1.0 log, respectively, with populations of ~1.2 log CFU/mL in water for all three sanitizers. These findings should be useful in future risk assessments and aid in the development of improved industry guidelines to better enhance the safety of diced onions.
1. Introduction
Increased consumption of raw, minimally processed, fresh-cut produce is raising many new safety concerns regarding the risk of foodborne illness. After two major recalls in 2007 and 2012, one of which involved ~22,000 kg of diced onions from a single producer, the safety of raw onions continues to be under scrutiny [1,2]. Due to the widespread use of onions as a food ingredient, the 2012 recall led to 11 additional recalls issued across the United States and Canada, all without incident [2]. In follow-up investigations, the implicated strain of L. monocytogenes was recovered from multiple sites within the processing facility, including a chute under an inspection table, a shroud on a peeling machine, and the loading hopper of a peeling machine [3], indicating the pathogen likely entered the facility on the unpeeled onions and then spread to subsequent onions during processing. Interestingly, in 2023, 80 cases of salmonellosis across 23 states were traced to diced onions from this same commercial producer with the outbreak strain also recovered from environmental samples where the onions were grown [4]. While these reports emphasize the potential spread of pathogens during commercial dicing, in other instances, Listeria-contaminated salads containing onions as an ingredient could not be linked to onions as the source of the contamination [5,6,7].
The incidence of Listeria in fresh produce is generally considered to be very low, with multiple studies failing to detect Listeria in whole intact onions at retail [8,9]. However, in 2022, whole Vidalia onions contaminated with L. monocytogenes were recalled by one Georgia grower from six states without incident [10]. Numerous studies have identified and tracked the presence of Listeria and other pathogens in produce packinghouses as well as on product contact surfaces during the processing of fresh-cut produce [11,12,13,14,15,16,17].
Commercial onion processing begins with “topping and tailing” where the root and sprout ends of the onion bulb are simultaneously removed by blades either before or after the outer skin is peeled using a corkscrew-type conveyer. Thereafter, the onions are mechanically diced, flume washed in water containing 50 to 200 ppm chlorine, and then mechanically dewatered for packaging. However, due to the potential spread of Listeria during onion dicing and the limited efficacy of sanitizers, commercially prepared diced onions need to be properly refrigerated to minimize the risk of growth and adverse public health consequences [18,19].
A series of studies have been published on the transfer of L. monocytogenes as well as Escherichia coli O157:H7 and Salmonella during the shredding of leafy greens [20,21], dicing of celery [22], and slicing/dicing of tomatoes [23,24,25,26]. In several reports, log-linear, Weibull, and exponential decay models [27,28,29,30] were used to better describe the trends in bacterial transfer for different processing scenarios.
In a follow up to our previous work demonstrating the spread of L. monocytogenes from one inoculated to twenty uninoculated onions during mechanical slicing [24], this study aimed to assess (1) the ability of L. monocytogenes to transfer from inoculated onions to the components of an industry-scale mechanical dicer and then to sequentially diced uninoculated onions and (2) the efficacy of several commonly used commercial sanitizers during the flume washing of Listeria-inoculated diced onions.
2. Materials and Methods
2.1. Experimental Design
Transfer of three avirulent L. monocytogenes strains (M3, J22F, J29H) from 2.2 kg of whole-surface-inoculated onions to the components of a commercial dicer was assessed. Subsequently, L. monocytogenes transfer from 2.2 kg of surface-inoculated onions to ten 2.2 kg batches of uninoculated onions during mechanical dicing was quantified by direct plating, with these findings then subjected to mathematical modeling to predict the extent of transfer. Finally, Listeria-inoculated diced onions were used to assess the efficacy of flume washing in water alone, and in water containing 55 ppm free chlorine, 80 ppm free chlorine, or 80 ppm peroxyacetic acid.
2.2. L. monocytogenes Strains
Three avirulent L. monocytogenes strains—M3 serotype 1/2a (parent was Mackaness strain), J22F serotype 4b (parent was NCTC 10527), and J29H serotype 4b (parent was NCTC 10527) (obtained from Dr. Sophia Karthariou, North Carolina State University, Raleigh, NC, USA) were used for all experiments. All cultures were stored at −80 °C in trypticase soy broth containing 0.6% (w/v) yeast extract (TSBYE, Becton, Dickinson and Company, Sparks, MD, USA) and 10% (v/v) glycerol. These strains were streaked for isolation to plates of trypticase soy agar containing 0.6% (w/v) yeast extract (TSAYE, Becton, Dickinson and Company) and incubated 24 h at 35 °C. Thereafter, an isolated colony of each strain underwent two consecutive 24 h/35 °C transfers in TSBYE. A cocktail was prepared by combining equal volumes of the three avirulent strains, followed by appropriate dilution to obtain populations of ~7.0 or 5.5 log CFU/mL for onion inoculation, with these levels confirmed by surface plating on Modified Oxford Agar (MOX, Neogen Corp., Lansing, MI, USA).
2.3. Onions
Spanish yellow onions (Allium cepa L.) were purchased from a local supplier (Stan Setas Produce Company, Lansing, MI, USA) and stored at 4 °C for no more than 7 d before use. The root and sprout portions of each whole onion were removed using a sterile knife. After hand peeling the outer skin, the onions were tempered to room temperature (23 °C ± 2 °C) and weighed prior to dicing.
2.4. Onion Dicer
A large-scale commercial dicer (Model H-A, Urschell, Valparaiso, IN, USA) located in the Department of Food Science and Human Nutrition Fruit and Vegetable Processing Laboratory (Michigan State University, East Lansing, MI, USA) was used for all experiments (Figure 1). Eight 100 cm2 product contact areas of the dicer—the side and bottom of the loading drum, front and back of the rotating paddles, slicing blade, cross-cut blade, dicing blade, and the discharge chute were chosen for sampling.
2.5. L. monocytogenes Transfer during Dicing
Whole peeled onions were immersed in the diluted 3-strain avirulent cocktail containing ~7.0 or 5.5 log CFU/mL for 2 min and then air-dried in a biosafety cabinet for 90 min, giving initial populations of ~5.9, or 4.2 log CFU/50 g. Transfer of L. monocytogenes to the commercial dicer was assessed by dicing one 2.2 kg batch of inoculated onions. Eight 100 cm2 areas of the dicer were sampled after disassembly using the 1-ply composite tissue method [31]. One 50 g diced onion sample was collected and assessed for numbers of Listeria to confirm the initial inoculation level.
Transfer of L. monocytogenes was also assessed by dicing one 2.2 kg batch of inoculated onions immediately followed by ten 2.2 kg batches of uninoculated onions. Each of the 11 diced onion batches was collected separately and mixed by hand with one 50 g sample collected at random for quantification of Listeria. After dicing the 10 batches of uninoculated onions, the dicer was disassembled and the same eight 100 cm2 areas were again sampled using the 1-ply composite tissue method. All dicing experiments were conducted in triplicate. After each experiment, the dicer was disassembled, washed with a brush to physically remove debris, and then sanitized with 200 ppm Quorum V (Ecolab, Saint Paul, MN, USA), rinsed with tap water and allowed to dry before reassembly.
2.6. Flume Washing with Various Sanitizers
The processing equipment for washing the diced onions was also located in the Department of Food Science and Human Nutrition Fruit and Vegetable Processing Laboratory. This processing line included a water recirculation tank (~1000-L capacity), 3.6 m-long flume tank (~130-L capacity; Heinzen Manufacturing Inc., Gilroy, CA, USA) and a dewatering shaker table operated by a 1-horsepower washdown duty motor (Baldor Electric Co., Ft. Smith, AR, USA) at 1760 rpm. The water recirculation tank containing 700 L of tap water (~15 °C) with or without a sanitizer was connected by a rigid plastic discharge hose (4.5 m × 0.1 m) to the flume tank by a centrifugal pump (model XB754FHA, Sterling Electric, Inc., Irvine, CA, USA). A custom-made stainless-steel screen was attached to the end of flume tank to retain the diced onions for 2 min of washing (Figure 2). All washing experiments were conducted in triplicate. After each experiment, the disassembled dicer and flume line were rinsed to physically remove debris, and then sanitized with 200 ppm Quorum V (Ecolab, Saint Paul, MN, USA), rinsed with tap water and allowed to air dry.
2.7. Sanitizers
Three different sanitizer treatments were used in this study. A commercial chlorine-based sanitizer (XY-12, Ecolab, St. Paul, MN, USA) was diluted in tap water to contain 80 ppm free chlorine and adjusted to pH of 6.5 with 10% (w/v) citric acid (CA). Electrolyzed water containing ~55 ppm free chlorine was produced on site using a commercial generator (PathoSans®, Spraying Systems Co., Westfield, IN, USA). A peroxyacetic acid-based sanitizer (Tsunami-100, Ecolab, St. Paul, MN, USA) was diluted in tap water to contain to 80 ppm peroxyacetic acid (PAA). Chlorine test kit 321 (Ecolab) was used to measure chlorine levels, and peroxyacetic acid test kit 311 (Ecolab) was used to measure PAA concentrations.
2.8. Evaluation of Sanitizer Efficacy
Whole peeled onions (9.1 kg) were immersed in the diluted 3-strain avirulent cocktail containing ~7.0 log CFU/mL for 2 min and then air-dried in a biosafety cabinet for 90 min, giving a population of ~4.0 log CFU/g. After dicing the 9.1 kg of inoculated onions with the same commercial dicer, seven 50 g samples were weighed into mesh produce bags (pore size < 0.5 cm), which were then placed in the flume tank containing 90 L of sanitizer-free water, 80 ppm free chlorine, 80 ppm PAA, or 55 ppm free chlorine as electrolyzed water, and vigorously agitated by hand for 2 min. During sanitizer exposure, 50 mL water and 50 g onion samples were collected every 20 s. After 2 min of washing, the flume pump was activated, and the screen was raised to flush the diced onions across the shaker table with a final 50 mL water and 50 g onion sample collected after 20 s of dewatering. After onion and water sample collection, the flume tank was emptied, and two surface samples (100 cm2) were taken from the flume tank and the shaker table as shown in Figure 2.
2.9. Microbial Analysis
All samples from the Listeria transfer experiments were added to Whirl-pak® bags containing University of Vermont Medium (UVM, Neogen), homogenized by stomaching (Stomacher 400 Circulator, Seward USA, Davie, FL, USA) for 1 min at 300 rpm, appropriately diluted in phosphate-buffered solution (PBS), and plated, with or without prior filtration through a 0.45 µm filter membrane using a vacuum pump (Model E46046, EMD Millipore Corporation, Billerica, MA, USA), on MOX with the UVM-diluted samples enriched at 35 °C. All plates were examined for typical Listeria colonies after 48 h of incubation at 35 °C. When samples were negative for Listeria by direct plating, the UVM enrichments were streaked to plates of MOX, incubated at 35 °C for 48 h, and then examined for the presence or absence of Listeria. All samples from the sanitizer efficacy studies were added to Whirl-pak® bags containing Neutralizing Buffer (Difco, BD, Franklin Lakes, NJ, USA), homogenized by stomaching for 1 min at 300 rpm, appropriately diluted in PBS, and plated, with or without prior filtration through a 0.45 µm filter membrane on MOX to quantify Listeria.
2.10. Statistical Analysis
All experiments were performed in triplicate. Listeria populations were reported as log CFU/onion ± SE for the inoculated and uninoculated onions or log CFU/100 cm2 ± SE for the dicer surface samples. For subsequent analysis of the Listeria transfer data, samples positive by enrichment were assumed to contain 1 CFU, whereas surface samples negative by enrichment were assumed to contain 0.5 CFU. Onion samples negative by enrichment were not included in the analysis. The Tukey–Kramer Honestly Significant Difference Test was performed using JMP 10 (SAS Institute Inc., Cary, NC, USA). Statistical significance was set at p < 0.05.
2.11. Evaluation of Transfer Model
An exponential decay model from a previous study (Sheen and Hwang, 2010) was used to describe the L. monocytogenes transfer pattern during dicing of onions. The model used to fit the data is shown in Equation (1):
where Y (dependent variable) is the log CFU/onion transferred and X (independent variable) is the number of the specific uninoculated batch of onions that was diced. A and B are the transfer model parameters. The above equation was fitted using the nlinfit algorithm of MATLAB (R2012a, MathWorks, Natick, MA, USA). The estimated parameters, normalized root mean squared errors (NRMSE) of the model, shown in Equation (2), and asymptotic 95% confidence intervals of the parameters were then estimated as follows:
where NRMSE is the normalized root mean squared error, RMSE is the root mean squared error, Ymax is the maximum value taken by Y, and Ymin is the minimum value taken by Y.
Y = A·e X/B
3. Results
3.1. Transfer from Inoculated Onion to Dicer
After dicing one batch of inoculated onions, L. monocytogenes was present on all dicer surfaces sampled with similar trends observed at both inoculation levels (Figure 3). The drum and slicer blade yielded average Listeria populations of 4.0 ± 0.2 and 4.2 ± 0.5, and 2.7 ± 0.4 and 3.6 ± 0.3 log CFU/100 cm2 after dicing a single batch of onions inoculated to contain ~5.9 or 4.2 log CFU/50 g, respectively. Listeria contaminated the remaining surfaces at varying levels, with the paddles and cross-cut blades yielding lower levels than the other components.
At the lower inoculation level, there was no significant (p > 0.05) difference in the Listeria populations retained on the dicer components after dicing 10 batches of uninoculated onions (Figure 4). However, at the higher inoculation level, the drum bottom and circular dicing blades retained significantly (p < 0.05) higher populations of L. monocytogenes than the other components (Figure 5).
3.2. Transfer from Inoculated to Subsequently Diced Uninoculated Onions
After dicing one batch of inoculated onions followed by 10 batches of uninoculated onions, Listeria was detected in at least one of three replicates by enrichment at the low inoculation level. At the higher inoculation level of ~5.9 log CFU/50 g, Listeria populations in batches 1, 5, and 10 averaged 4.6 ± 0.1, 3.0 ± 0.1, and 2.3 ± 0.2 log CFU/50 g, respectively (Figure 6). The exponential model reasonably fit the lower and higher inoculation level transfer data with NRMSEs of 0.17 and 0.20, respectively (Table 1).
3.3. Sanitizer Evaluation
Diced onions yielded Listeria populations of 3.6, 2.6, 3.0, and 3.7 log CFU/g after 2 min of washing in tap water, 80 ppm free chlorine, 80 ppm PAA, and 55 ppm free chlorine followed by shaker table dewatering. The chlorine-based sanitizer was significantly (p < 0.05) better than tap water, yielding a ~1.4 log CFU/g reduction (Figure 7A).
Listeria populations in sanitizer-free water increased to ~1.2 log CFU/mL during washing (Figure 7B). During the first minute of washing with a sanitizer, Listeria was quantifiable in three water samples at or near the limit of detection, which was attributed to the accumulation of onion particulates on the filter membrane during sample processing. Surface samples yielded significantly (p < 0.05) higher Listeria populations when sanitizers were not used (Table 2).
4. Discussion
The Listeria transfer results during onion dicing are consistent with other studies showing the ability of foodborne pathogens to cross-contaminate large quantities of previously uncontaminated celery [22], leafy greens [32], and tomatoes [25,26] during dicing, slicing, and shredding. When 9.1.kg of radicchio was inoculated with E. coli O157:H7 at 6.0 log CFU/g, mechanically shredded, conveyed, flume washed in sanitizer-free water, and centrifugally dried, followed by 907 kg of uninoculated iceberg lettuce, E. coli O157:H7 was recovered from all of the processed lettuce indicating that even a small amount of contaminated product can have serious consequences [32]. When Kaminski, Davidson, and Ryser [22] mechanically hand-diced 250 g of celery inoculated with L. monocytogenes at 5.6 log CFU/g followed by 15 250-g batches of uninoculated celery, Listeria populations progressively decreased from 5.2 log CFU/g in batch 1 to 2.0 log CFU/g in batch 15. In the only other reported study using the same commercial dicer, Wang and Ryser [26] reported a 2.2 log reduction in Salmonella when one 0.9 kg batch of Roma tomatoes was diced followed by ten uninoculated batches compared to the 2.3 log reduction that was for L. monocytogenes in diced onions. Therefore, the extent to which Salmonella and Listeria spread appears to be unaffected by the type of product being diced or sliced as also shown by Alnughaymishi [33].
In our study, areas of the commercial dicer most prone to Listeria contamination after onion dicing included the rolling dicing blades, loading hopper, and slicer blade (Figure 3). Similarly, Buchholz, Davidson, Marks, Todd, and Ryser [32] showed that radicchio buildup was most evident on the cutting wheel and discharge chute of the shredder with statistically similar populations of E. coli O157:H7 recovered from the shredder, flume tank, and shaker table after processing 907 kg of iceberg lettuce. Kaminski, Davidson, and Ryser [22] also recovered 10.8 of 250 g of red Swiss chard from a mechanical hand dicer after dicing 15 250 g baches of celery with the retained Swiss chard expected to spread to additional product over time.
Proper cleaning protocols for both food and non-food contact surfaces in food processing are important to minimize the risk of product contamination by Listeria. Lundén, Autio, and Korkeala, ref. [34] showed that a mechanical dicing machine was the vehicle for a resident Listeria population that moved between three processing plants, with the dicer blades identified as one source of contamination. The 2012 recall prompted actions by the responsible party that included a cleaning and sanitizing protocol to eliminate L. monocytogenes from the facility. However, after actions were taken, the same strain was again identified on various equipment surfaces, demonstrating the difficulty in effectively removing colonized Listeria [1,2,3].
Sanitizers are clearly needed in flume water to minimize cross-contamination from the water during washing [35]. This study supports previous work showing that chlorine-based sanitizers are effective when the organic load is low [36,37,38,39]. Sanitizers are far less effective against Listeria and other bacterial pathogens when the product is contaminated. While the presence of Listeria on diced onions after flume washing raises additional concerns regarding potential migration into the product through cut surfaces, this study did not evaluate the location of Listeria on or in diced onion after dicing. Hence, decreased sanitizer efficacy during the flume tank washing of diced onions may be partly due to the protection of internalized Listeria cells during flume washing.
All studies have their own limitations based on the experimental design employed. In this work, the peeled onions that were first diced were also dip-inoculated to contain levels of L. monocytogenes unlikely to be found in naturally contaminated onions. However, high inoculation levels yielding quantifiable numbers of Listeria by direct plating were necessary for predictive modeling as demonstrated in previous studies. Commercial-type production practices for diced onions were followed as closely as possible using a commercial dicer and pilot-scale flume washing and dewatering line. However, differences in equipment design will affect the extent of bacterial cross-contamination [25]. During extended operation, any build-up of onion particulates would be expected to further extend the transfer of Listeria. In this study, the drum, blade, and chute of the dicer best supported the ongoing spread of Listeria, with these areas in need of more rigorous post-processing cleaning and sanitizing. Designers of such equipment should also pay special attention to cleanability and eliminate any potential harborage sites that may lead to biofilm formation and the long-term spread of microbial contaminants. Increasing levels of organic material in the flume water also dictate the need for continuous monitoring and control of the sanitizer concentration to maintain efficacy [26,36].
To our knowledge, this is the first study to show that Listeria can transfer and survive during the simulated commercial production of diced onions. During washing, the chlorine-based sanitizer used in this study was more effective at inactivating Listeria than peroxyacetic acid or electrolyzed water. However, organic matter commonly present in commercial onion wash water would be expected to decrease the efficacy of chlorine. Therefore, it is imperative that onions be diced and washed under as sanitary conditions as possible to minimize contamination, and then properly refrigerated to maximize end-product safety.
Author Contributions
Conceptualization, E.T.R.; methodology, A.M.S. and H.W.; data collection, A.M.S. and H.W.; formal analysis, A.M.S., H.W. and E.T.R.; writing—original draft preparation, A.M.S., H.W. and E.T.R.; writing—review and editing, A.M.S., H.W. and E.T.R.; project administrator, E.T.R.; funding acquisition, E.T.R.; supervision, E.T.R. All authors have read and agreed to the published version of the manuscript.
Funding
This research was supported by the U.S. Department of Agriculture National Institute for Food and Agriculture under grant number 2011-51110-31027.
Institutional Review Board Statement
Not applicable.
Informed Consent Statement
Not applicable.
Data Availability Statement
Data sharing is not applicable to this article.
Conflicts of Interest
The authors declare no conflicts of interest. The funders had no role in the design of the study; in the collection, analyses, or interpretation of data; in the writing of the manuscript; or in the decision to publish the results.
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Figure 1.
(A) Commercial dicer. (B) Commercial dicer sampling locations: slicer blade (1), paddles (2, 3), and drum (4, 5). (C) Commercial dicer sampling locations: rolling dicer blades (6) and cross-cut blades (7). (D) Commercial dicer sampling location: chute (8).
Figure 1.
(A) Commercial dicer. (B) Commercial dicer sampling locations: slicer blade (1), paddles (2, 3), and drum (4, 5). (C) Commercial dicer sampling locations: rolling dicer blades (6) and cross-cut blades (7). (D) Commercial dicer sampling location: chute (8).
Figure 2.
Processing equipment: (A) 3.6 m flume tank and (B) dewatering shaker table.
Figure 3.
L. monocytogenes transfer from inoculated onions (5.9 or 4.2 log CFU/50 g) to different dicer components. Values were compared between components at the same inoculation level. Bars with different letters are significantly different.
Figure 3.
L. monocytogenes transfer from inoculated onions (5.9 or 4.2 log CFU/50 g) to different dicer components. Values were compared between components at the same inoculation level. Bars with different letters are significantly different.
Figure 4.
Listeria populations remaining on the different dicer surfaces after dicing one inoculated (4.2 log CFU/50 g) followed by 10 uninoculated batches of onions. Populations were compared across the different components after dicing with A denoting no significant difference.
Figure 4.
Listeria populations remaining on the different dicer surfaces after dicing one inoculated (4.2 log CFU/50 g) followed by 10 uninoculated batches of onions. Populations were compared across the different components after dicing with A denoting no significant difference.
Figure 5.
Listeria populations remaining on the different dicer surfaces after dicing one inoculated (5.9 log CFU/50 g) followed by 10 uninoculated batches of onions. After dicing bars with different letters are significantly different.
Figure 5.
Listeria populations remaining on the different dicer surfaces after dicing one inoculated (5.9 log CFU/50 g) followed by 10 uninoculated batches of onions. After dicing bars with different letters are significantly different.
Figure 6.
(A). Predicted L. monocytogenes transfer from one batch of inoculated onions batch (4.2 log CFU/50 g) to 10 batches of uninoculated onions. ypred is the prediction line; yobs is the observed line; CB is the confidence band for the prediction line. (B). Predicted L. monocytogenes transfer from one batch of inoculated onions batch (5.9 log CFU/50 g) to 10 batches of uninoculated onions. ypred is the prediction line; yobs is the observed line; CB is the confidence band for the prediction line.
Figure 6.
(A). Predicted L. monocytogenes transfer from one batch of inoculated onions batch (4.2 log CFU/50 g) to 10 batches of uninoculated onions. ypred is the prediction line; yobs is the observed line; CB is the confidence band for the prediction line. (B). Predicted L. monocytogenes transfer from one batch of inoculated onions batch (5.9 log CFU/50 g) to 10 batches of uninoculated onions. ypred is the prediction line; yobs is the observed line; CB is the confidence band for the prediction line.
Figure 7.
(A). Listeria populations on diced onions during washing and shaker table dewatering. * Denotes significant difference between treatment and water control. (B). Listeria populations in water during washing and shaker table dewatering of diced onion.
Figure 7.
(A). Listeria populations on diced onions during washing and shaker table dewatering. * Denotes significant difference between treatment and water control. (B). Listeria populations in water during washing and shaker table dewatering of diced onion.
Table 1.
Model parameters A and B for L. monocytogenes transfer from one inoculated onion to 10 uninoculated batches of onions during dicing.
Table 1.
Model parameters A and B for L. monocytogenes transfer from one inoculated onion to 10 uninoculated batches of onions during dicing.
| Inoculation Level (log CFU/50 g) | A (95% CI) a | B (95% CI) | NRMSE b (log CFU/50 g) |
|---|---|---|---|
| 4.2 | 2.98 (2.27, 3.68) | −9.23 (−13.96,−4.5) | 0.17 |
| 5.9 | 4.74 (4.37,5.11) | −12.76 (−15.29,−10.23) | 0.20 |
a Coefficient value (95% confidence interval). b Normalized root mean squared error for the transfer model.
Table 2.
Listeria populations (log CFU/100 cm2) on the flume tank and shaker table after onion dicing and dewatering.
Table 2.
Listeria populations (log CFU/100 cm2) on the flume tank and shaker table after onion dicing and dewatering.
| Equipment Surface | Water | Electrolyzed Water | Chlorine + Citric Acid | Peroxyacetic Acid |
|---|---|---|---|---|
| Flume Tank | 1.6 ± 0.3 a * (6/6) | −0.3 ± 0.00 b (0/6) | −0.3 ± 0.0 b (0/6) | −0.1 ± 0.2 b (1/6) |
| Shaker Table | 2.1 ± 0.3 a (6/6) | 0.5 ± 0.3 b (4/6) | 0.6 ± 0.2 b (5/6) | −0.3 ± 0.1 b (1/6) |
* Fraction represents number of quantifiable samples. Populations on equipment surface were compared across sanitizers. Rows with different letters are significantly different.
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MDPI and ACS Style
Scollon, A.M.; Wang, H.; Ryser, E.T. Transfer and Inactivation of Listeria monocytogenes during Pilot-Scale Dicing and Flume Washing of Onions. Appl. Microbiol. 2024, 4, 439-452. https://doi.org/10.3390/applmicrobiol4010030
AMA Style
Scollon AM, Wang H, Ryser ET. Transfer and Inactivation of Listeria monocytogenes during Pilot-Scale Dicing and Flume Washing of Onions. Applied Microbiology. 2024; 4(1):439-452. https://doi.org/10.3390/applmicrobiol4010030
Chicago/Turabian StyleScollon, Andrew M., Haiqiang Wang, and Elliot T. Ryser. 2024. "Transfer and Inactivation of Listeria monocytogenes during Pilot-Scale Dicing and Flume Washing of Onions" Applied Microbiology 4, no. 1: 439-452. https://doi.org/10.3390/applmicrobiol4010030
