Aifen Ou
Kan Wang2†
Yanrui Ye
Junyan Liu- 1Department of Food, Guangzhou City Polytechnic, Guangzhou, China
- 2Center for Translational Medicine, The Second Affiliated Hospital of Shantou University Medical College, Shantou, China
- 3School of Biological Science and Engineering, South China University of Technology, Guangzhou, China
- 4School of Food Science and Engineering, Guangdong Province Key Laboratory for Green Processing of Natural Products and Product Safety, South China University of Technology, Guangzhou, China
- 5School of Materials Science and Engineering, South China University of Technology, Guangzhou, China
- 6Department of Civil and Environmental Engineering, University of Maryland, College Park, College Park, MD, United States
Salmonella enterica is a typical foodborne pathogen with multiple toxic effects, including invasiveness, endotoxins, and enterotoxins. Viable but nonculturable (VBNC) is a type of dormant form preserving the vitality of microorganisms, but it cannot be cultured by traditional laboratory techniques. The aim of this study is to develop a propidium monoazide-crossing priming amplification (PMA-CPA) method that can successfully detect S. enterica rapidly with high sensitivity and can identify VBNC cells in food samples. Five primers (4s, 5a, 2a/1s, 2a, and 3a) were specially designed for recognizing the specific invA gene. The specificity of the CPA assay was tested by 20 different bacterial strains, including 2 standard S. enterica and 18 non-S. enterica bacteria strains covering Gram-negative and Gram-positive isolates. Except for the two standard S. enterica ATCC14028 and ATCC29629, all strains showed negative results. Moreover, PMA-CPA can detect the VBNC cells both in pure culture and three types of food samples with significant color change. In conclusion, the PMA-CPA assay was successfully applied on detecting S. enterica in VBNC state from food samples.
Introduction
During food processing, food is frequently contaminated by foodborne bacteria, including Staphylococcus aureus, Salmonella enterica, and Escherichia coli O157 (Kirk et al., 2015; Miao et al., 2017a; Sharma et al., 2019). S. enterica is a typical foodborne pathogen with multiple toxic effects, including invasiveness, endotoxins, and enterotoxins (Eng et al., 2015). Various serotypes of Salmonella are implicated in foodborne infections and contaminate food products, including eggs, milk, poultry, meat, and vegetables. It is the main cause of human gastrointestinal and other related diseases (Bao et al., 2017a, b; Wen et al., 2020). Recently, studies confirmed that S. enterica is capable of entering into the viable but non-culturable state (VBNC) state under an adverse environment, which could include low-temperature, salt stress, and nutrient starvation (Roszak et al., 1984; Chmielewski and Frank, 1995; Gupte et al., 2003; Zeng et al., 2013; Morishige et al., 2017; Highmore et al., 2018). VBNC cells cannot be detected by traditional culture-based methods (Xu et al., 2011a; Lin et al., 2017; Miao et al., 2017a; Xie et al., 2017a). Therefore, it is urgent to develop a rapid and sensitive assay to detect S. enterica, especially in the VBNC state.
The molecular biological method, classified into polymerase chain reaction (PCR) and isothermal amplification, is a new strategy to detect pathogens (Xu et al., 2012; Xu et al., 2012a; Liu et al., 2019). PCR and PCR-based assays have been well developed in the last few decades (You et al., 2012; Zhong et al., 2013; Xu et al., 2016c). However, these assays require complicated procedures that may increase the uncertainty in result determination (Tada et al., 1992; Zhong et al., 2013; Xu et al., 2017a; Xie et al., 2017b; Jia et al., 2018). Quantitative real-time PCR can achieve the result interpretation by digital curve without electrophoresis but with lower detection limits (Xu et al., 2007; Miao et al., 2017b, c). Isothermal amplification assays include loop-mediated isothermal amplification (LAMP), rolling circle amplification (RCA), and strand displacement amplification (SDA) (Fire and Xu, 1995; Zhao et al., 2009; Zhao et al., 2010a, b; Bao et al., 2017c; Xu et al., 2017b). Reverse transcription LAMP (RT-LAMP) or other isothermal amplification assays have been utilized to replace the PCR assay (Parida et al., 2005).
Cross Priming Amplification (CPA) is a novel isothermal method relying on five primers (2a/1s, 2a, 3a, 4s, and 5a) to amply the target nucleotide sequences (Xu et al., 2012). It does not require any special instrumentation and presents high rapidity, specificity, and sensitivity. Recently, CPA assays have been used for the detection of E. coli O157:H7, Listeria monocytogenes, Enterobacter sakazakii, Yersinia enterocolitica, and other pathogens (Wang et al., 2014; Zhang et al., 2015; Wang et al., 2018; Xu et al., 2020). Therefore, CPA is a potentially valuable tool for the rapid detection of foodborne pathogens, and the combination of propidium monoazide (PMA) may achieve the detection of VBNC state (Xu et al., 2010; Wang et al., 2011; Xu et al., 2011c).
Materials and Methods
Bacterial Strains
To standardize and evaluate the reaction system of CPA assay, non-S. enterica bacteria strains, including various species of Gram-negative and Gram-positive non-target strains, were used in this study (Table 1). Two standard S. enterica ATCC14028 and ATCC29629 were used as positive controls. All strains used in this study had been preliminarily identified in the Lab of Clinical Microbiology, Zhongshan Supervision Testing Institute of Quality and Metrology.
Table 1. Reference strains and results of CPA assays.
All bacteria were prepared for genomic DNA isolation after incubation in trypticase soy broth (TSB, Huankai Microbial, China) at 37°C at 200 rpm overnight. The genomic DNA was isolated by Bacterial DNA extraction Kit (Dongsheng Biotech, Guangzhou, China) according to the manufacturer’s protocol. The concentration and quality of the DNA were measured using Nano Drop 2000 (Thermo Fisher Scientific Inc., Waltham, MA, United States) at 260 and 280 nm. The isolated DNA was stored at −20°C for further use.
CPA Detection System Design
As a species specific gene in Salmonella, invA has been selected, and its specificity in Salmonella has been previously confirmed. The CPA primers were specifically designed for invA gene in S. enterica using Primer Premier 5, including five primers recognizing five distinct regions in the gene open reading frame sequence (Table 2). All primers were assessed for specificity by BLAST against the sequences in Genebank.
Table 2. Primers sequence for detection of CPA.
The PCR reaction was conducted to serve as a control in a total 25 μL volume with 12.5 μL 2× Taq PCR Master Mix (Dongsheng Biotech, Guangzhou, China), 3 μM each of forward and reverse primers, 2 μL of DNA template and the total volume was added up to 25 μL with nuclease-free water. The amplification procedure included a 5-min denaturation at 95°C, 32 cycles of amplification at 95°C for 30 s, 52°C 30 s, 72°C for 35 s, and final amplification at 72°C for 5 min. The PCR products were detected by electrophoresis on 1.5% agarose gels.
The CPA reaction system was performed using thermostatic equipment or a water bath in a 26 μL system, containing 20 mM Tris–HCl, 10 mM (NH4)2SO4, 10 mM KCl, 8.0 mM MgSO4, 0.1% Tween 20, 0.7 M betain (sigma), 1.4 mM dNTP (each), 8 U Bst DNA polymerase (NEB, United States), 1.0 μM primer of 2a/1s, 0.5 μM (each) primer of 2a and 3a, 0.6 μM (each) primer of 4s and 5a, 1 μL mixture chromogenic agent (mixture with calcein and Mn2+), 1 μL template DNA, and a volume of up to 26 μL of nuclease-free water. The mixed chromogenic agent consists of 0.13 mM calcein and 15.6 mM MnCl2⋅4H2O. And mixed reaction solution was incubated at 65°C for 60 min and heated at 80°C for 2 min to terminate the reaction. Nuclease-free water substituted target DNA was used as a negative control. Subsequently, the amplified products were analyzed by electrophoresis on 1.5% agarose gels and observed the color change by naked eyes.
CPA Detection System Optimization
The specificity of CPA was evaluated by amplifying the genomic DNA extracted from 2 standard S. enterica strains and 18 non-S. enterica strains.
To determine the sensitivity of the CPA assay, serial 10-fold dilutions of the genomic DNA of S. enterica ATCC14280 were prepared and used in the reaction. The sensitivity of the CPA method was compared with the PCR method. All the tests were performed in triplicate.
Application of CPA Assay in Food Products
The application of CPA assay in the detection of S. enterica was conducted in three rice products (Cantonese rice cake, steamed bread, and rice noodle purchased from Guangzhou Restaurant, Guangzhou, China). Different concentrations (from 108 CFU/mL to 10 CFU/mL) of S. enterica ATCC14028 were applied to contaminate food samples. Subsequently, genomic DNA was extracted from the contaminated food samples and subjected to CPA and PCR methods in triplicate (Xu et al., 2020).
VBNC State Induction
The VBNC state of S. enterica was induced by oligotrophic medium (sterile saline) at a low temperature. The bacterial overnight culture (∼108 CFU/mL) was washed three times and resuspended by sterile saline and then stored at −20°C. The culturable cell number was measured by plate counting method, and viable cells were determined by LIVE/DEAD® BacLight kitTM (ThermoFisher scientific, United States) with a fluorescence microscope after the cells were no longer culturable. The culturable and viable cell enumerations were performed every three days.
PMA-CPA Detection System
The PMA-CPA were developed to detect the VBNC cells of S. enterica with the observation of color change. The PMA-CPA was further applied in the detection of VBNC cells in contaminated rice food products (Cantonese rice cake, steamed bread, and rice noodle from Guangzhou Restaurant, Guangzhou, China).
Results
Development of CPA Assay
The CPA assays for the detection of invA gene were set up using S. enterica ATCC14028. The products were analyzed by 1.5% agarose gel electrophoresis, and the bands were observed under UV light (Figure 1A). The results of electrophoresis revealed that the amplicons of CPA are of various sizes, showing as a ladder pattern on agarose gel instead of a single band. The fluorescent dye (MgCl2 and calcein) changes the reaction system from orange to green in the reaction system (Figure 1B).
Figure 1. Amplification products were visually detected both by 1.5% agarose gel electrophoresis under UV light (A) and observation at the color change by naked eye (B). M, DNA marker; lane 1, positive control; lane NC, negative products (A); tube 1, positive products; tube NC, negative control.
The evaluation of the specificity of CPA assay was performed in 2 S. enterica strains and 18 non-S. enterica reference strains. Results were recorded by 1.5% agarose gel electrophoresis and color change. Ladder pattern bands and orange to yellow color changes were only observed in the 2 S. enterica strains (Figure 2). It indicated that only the target S. enterica strains were detected with positive results, showing the high specificity of the CPA assay.
Figure 2. Specificity of CPA assay for detection S. enterica strains with invA genes by 1.5% agarose gel electrophoresis and observation at the color change by naked eye; M-DNA marker; lane 1–2, S. enterica ATCC 29629 and ATCC 14028; lane 2–20, non-S. enterica strains. NG/21, negative control.
Detection of S. enterica in Food Products
The CPA assays were applied in the detection of S. enterica in three food samples (Cantonese rice cake, steamed bread, and rice noodle). The homogenized rice products (9 mL) were inoculated with 1 mL 10-fold serial dilution of pure S. enterica culture. The concentration of artificial contamination food samples ranging from 108 CFU/mL to 10 CFU/mL with 10-fold series dilutions was applied. All three food samples were included for the application. As expected, the LOD shows an insignificant difference among food samples, and the results are identical. Only the samples with a concentration higher than 103 CFU/mL were able to be detected (Figure 3). Thus, the detection limit of the CPA assay was 103 CFU/mL.
Figure 3. Sensitivity of the CPA assay in food samples of S. enterica with invA genes by 1.5% agarose gel electrophoresis (A) and agent mixture (B); M-DNA marker; lane 1–8, 107 CFU/mL, 106 CFU/mL, 105 CFU/mL, 104 CFU/mL, 103 CFU/mL, 102 CFU/mL, 10 CFU/mL negative control.
Detection of VBNC Cells by PMA-CPA Assay
The PMA-CPA assay was established using VBNC cells of S. enterica. The PMA dye was added to either pure culture or flour samples with a final concentration of 5 μg/mL. After incubation at room temperature for 10 min in dark, the samples were exposed to a 650 W halogen lamp with a distance of 15 cm for 5 min, which inactivates unbinding PMA molecules rather than PMA-DNA molecules. All the dying process was performed in an ice bath to prevent DNA damage. Results showed that PMA-CPA can detect the VBNC cells both in pure culture and food samples with significant color change from orange to yellow (Figure 4). The samples with dead cells remain orange in both pure culture and food samples.
Figure 4. Detection of VBNC state of S. enterica in pure cultures and food samples by PMA-CPA assay with observation at the color change by naked eye. 1 – VBNC cells in pure cultures; 2 – dead cells in pure cultures; 3 – VBNC cells in food samples; 4 – dead cells in food samples.
Discussion
Salmonella enterica is a common foodborne pathogen that may cause serve illness. The generation of S. enterica VBNC state occurs during the chlorination of wastewater or food (Oliver et al., 2005; Zeng et al., 2013). Non-ionic detergents and sanitizers can also induce S. enterica into VBNC state (Morishige et al., 2013; Purevdorj-Gage et al., 2018; Robben et al., 2018). Furthermore, a multi-stress environment in complex components of food and storage conditions may induce the VBNC state formation of foodborne pathogens (Lin et al., 2016; Miao et al., 2016; Xu et al., 2016a,b).
Various molecular techniques have been developed to identify microbes. PCR is a mature method to detect foodborne microbes, but it has low sensitivity and complex variable temperature programs (Kim et al., 1999). RT-PCR has been used to detect microbes compared with the method in ISO 21872-1:2007. RT-PCR achieved higher sensitivity but with long pre-enrichment and 24 h of complicate procedure. Although RT-PCR is able to show results via a digital curve, the sensitivity of this method is limited and the procedure is complicated (Xu et al., 2008a; Miao et al., 2018; Xu et al., 2018; Zhao et al., 2018a,b). RT-LAMP or other isothermal amplification has been used reported to replace RT-PCR to increase the detection limit (Xu et al., 2008b; Xu et al., 2009; Liu et al., 2018a,b; Lv et al., 2020). However, sophisticated equipment with these technologies has brought certain difficulties to rapid on-site testing (Xu et al., 2011b; Xu et al., 2012b). CPA technique is a new strategy to achieve rapid detection and can be performed under constant temperature using a simple water bath. Furthermore, with the improvement of fluorescence dye, results can be identified by the color change in the reaction tube by the naked eye. For VBNC and dead cells, they are both nonculturable. However, VBNC cells differ from dead cells in their intact cell membrane and thus could be differentiated via PMA, which is capable of differentiating viable and dead cells.
Therefore, the developed CPA method can successfully detect the S. enterica with high rapidity and sensitivity and can identify the VBNC cells in food samples when combining with PMA.
Data Availability Statement
The raw data supporting the conclusions of this article will be made available by the authors, without undue reservation.
Author Contributions
JL conceived of the study and participated in its design and coordination. AO and KW performed the experimental work and collected the data. YY and XG organized the database. LC and LQ performed the statistical analysis. AO wrote the manuscripts. All authors contributed to manuscript revision, read, and approved the submitted manuscript.
Funding
This work was supported by the National Key Research and Development Program of China (2016YFD04012021).
Conflict of Interest
The authors declare that the research was conducted in the absence of any commercial or financial relationships that could be construed as a potential conflict of interest.
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Keywords: Salmonella enterica, viable but non-culturable (VBNC), crossing priming amplification (CPA), propidium monoazide (PMA), rapid detection
Citation: Ou A, Wang K, Ye Y, Chen L, Gong X, Qian L and Liu J (2021) Direct Detection of Viable but Non-culturable (VBNC) Salmonella in Real Food System by a Rapid and Accurate PMA-CPA Technique. Front. Microbiol. 12:634555. doi: 10.3389/fmicb.2021.634555
Received: 28 November 2020; Accepted: 19 January 2021;
Published: 18 February 2021.
Edited by:
Yang Deng, College of Food Science and Engineering, Qingdao Agricultural University, ChinaReviewed by:
Wensen Jiang, Cedars Sinai Medical Center, United StatesYanmei Li, University of Maryland, Baltimore, United States
Yuting Tian, School of Food Science, Fujian Agriculture and Forestry University, China
Ying Mu, University of Tennessee Health Science Center (UTHSC), United States
Copyright © 2021 Ou, Wang, Ye, Chen, Gong, Qian and Liu. This is an open-access article distributed under the terms of the Creative Commons Attribution License (CC BY). The use, distribution or reproduction in other forums is permitted, provided the original author(s) and the copyright owner(s) are credited and that the original publication in this journal is cited, in accordance with accepted academic practice. No use, distribution or reproduction is permitted which does not comply with these terms.
*Correspondence: Junyan Liu, jliu81@uthsc.edu; Lu Qian, qianlu@scut.edu.cn
†These authors have contributed equally to this work