Introduction

Vibrio parahaemolyticus is a Gram-negative, halophilic bacterium, universally found in the coastal and estuarine marine waters. It is an opportunistic foodborne pathogen, often sheltered on marine reservoirs, predominantly in shellfish, serving as a vehicle for transmission of infection to humans, causing gastroenteritis. V. parahaemolyticus possesses different virulence properties, the major ones are thermostable direct hemolysin (TDH), and TDH-related hemolysins (TRH) encoded by tdh and trh genes, respectively [1]. These factors cause hemolysis and cytotoxicity to the host cells resulting in diarrhea. The virulence genes, tdh, and trh are considered to be a marker for detecting pathogenic V. parahaemolyticus [2]. Along with these virulence genes, secretion systems also play a major role in pathogenicity (T3SS2, T3SS6) [3,4,5]. Reports show the involvement of adhesion factors such as VpadF as a virulence marker with the potential to be used as vaccine candidates [6]. Seafood associated disease outbreaks are one of the major threats to public health. Worldwide gastroenteritis caused by V. parahaemolyticus is usually due to the consumption of contaminated shellfishes and other raw or undercooked seafood. According to the epidemiological data, most outbreaks occur after consuming oysters and clams [7]. V. parahaemolyticus is considered to be one of the major foodborne pathogens by the Centers for Disease Control and Prevention (CDC) [8]. V. parahaemolyticus infection has been increased worldwide in the last two decades, including outbreaks caused by pandemic strains [9].

For the detection of V. parahaemolyticus, several methods are available from conventional to the molecular level. In general, conventional culture-based techniques are time-consuming and often require multiple days to achieve the results. Moreover, these assays show less sensitivity when target bacteria are present in lower numbers [10]. The molecular methods include polymerase chain reaction (PCR), real-time (RT)-PCR (RT-PCR), and more advanced droplet digital PCR. However, these sophisticated techniques require expensive equipment, trained personnel, and expensive reagents [11,12,13,14]. Hence developing simple diagnostic tools without compromising simplicity and sensitivity would be very important. The loop-mediated isothermal amplification (LAMP) assay is one such method that has the potential to be a point-of-care (POC) detection tool. Recently LAMP assay has been customized and used worldwide to detect tuberculosis [15]. LAMP is a DNA based amplification method that amplifies the nucleic acid under isothermal conditions. As compared to existing molecular methods like PCR and RT-PCR, LAMP assay can be performed in a simple dry or water bath [16]. LAMP is known for the specificity and simplicity; hence it would be an excellent tool for detecting an important sea-foodborne pathogen viz V. parahaemolyticus. In this study, we have optimized LAMP assay for the sensitive detection of pathogenic strains of V. parahaemolyticus in seafood without enrichment. The assay was validated by detecting the organism from a direct seafood sample and comparing it with existing molecular methods.

Methods

Bacterial strains, culture condition, and genomic DNA

Details of the bacterial strains used in this study are listed in Table ST1, which includes V. parahaemolyticus strains, other Vibrio, and non-Vibrio strains. All these bacterial strains were tested to determine the specificity of the LAMP assay. The strains of V. parahaemolyticus and other bacterial strains were revived from the institutional deep freezer (−80 °C) (Thermo Scientific, USA) into 5 ml of tryptic soy broth (TSB) (HiMedia, Mumbai, India) and incubated at 35 ± 2 °C for 24 h. The overnight grown V. parahaemolyticus culture was streaked onto a selective medium, thiosulfate–citrate–bile salts–sucrose (TCBS) agar (HiMedia, India) obtain a single colony. Other bacterial strains were directly sub-cultured into 5 ml Luria Bertani (LB) broth. Genomic DNA was extracted from all the cultures used in this study as per the protocol described by Ausubel et al. [17] with minor modifications. DNA concentration and purity were checked using a spectrophotometer (BioSpectrometer® basic, Eppendorf, USA).

LAMP primers and assay optimization

The tdh and trh genes of V. parahaemolyticus were retrieved from NCBI GenBank (https://www.ncbi.nlm.nih.gov/genbank/) database. The sequences were further subjected to multiple sequence alignment tools, multi-align (http://multalin.toulouse.inra.fr/multalin/) [18] to find the consensus sequences. The best-matched sequence was chosen for primer designing. LAMP primer designing was done using PrimerExplorer software—V5 (Eiken Chemical Co. Ltd., Japan; http://primerexplorer.jp/e/).

The LAMP assay was optimized for the detection of V. parahaemolyticus targeting the trh and tdh gene. LAMP assay was performed in a 25 μl reaction mixture, containing 1× reaction mixtures (Eiken Chemical, Japan), template DNA (100 ng/μl), 1 μl of Bst DNA polymerase (Eiken Chemical, Japan), and 40 pmol of FIP and BIP, 20 pmol of F3 and B3, for the amplification of tdh gene 5 pmol of LF primer was used. Results were analyzed using LoopAmp real-time turbidimeter (LA-500, Eiken Japan) and 2% agarose gel, stained with ethidium bromide (0.5 μg/ml) and analyzed using a gel documentation system (Bio-Rad, CA, USA). The reaction was carried out using a simple dry bath (Genei, India) and real-time turbidimeter at different temperatures (60, 63, and 65 °C) for 15, 30, and 60 min, followed by inactivation at 80 °C for 5 min. Details of primers used in this study are listed in Table ST2.

Specificity test of trh and tdh LAMP primers

Various bacterial strains were used to test the specificity of LAMP assay. DNA extracted from the bacterial strains were subjected to both LAMP and conventional PCR amplification. The LAMP assay’s specificity was determined by identifying the amplification of trh and tdh genes in all the bacterial strains (Table ST1).

Sensitivity of the LAMP assay

Determination of sensitivity using purified genomic DNA

The sensitivity of LAMP assay was carried out by preparing a ten-fold serial dilution of DNA extracted from V. parahaemolyticus standard cultures (AQ4037 and 81TDH2 for trh+ and tdh+ respectively) concentration ranging from 100 ng to 1 fg. The LAMP outer primers, F3, and B3 were used for PCR amplifications to check the sensitivity.

Determination of sensitivity in spiked clam meat

The sensitivity of LAMP assay was also determined using clam meat spiked with tdh+ and trh+ V. parahaemolyticus. The clam sample was purchased from a local market, Mangalore, India. Initially, the collected clam was pooled and homogenized in a sterile container. One gram of sample was taken and inoculated into 9 ml of alkaline peptone water (APW). After 18 h of incubation, 1 ml of the enriched sample was then taken in the micro-centrifuge tube and centrifuged at 900 × g for 1 min to separate the larger meat particles. The supernatant was transferred in a fresh tube and centrifuged at 10,000 × g for 10 min. The pellet was gently mixed with 100 μl of molecular grade water. The mixture was then heated at 95 °C for 5 min and immediately transferred into ice for 5 min. Finally, centrifugation was performed at 2800 × g for 5 min, and crude cell lysate (CCL) was collected as supernatant in a fresh tube and preserved at −20 °C for future use. The CCL was used as DNA template and tested for the presence of tdh and trh gene using PCR [19], and LAMP assay (protocol described before). Clam sample negative for conventional PCR & LAMP assay was further used for the sensitivity study. The tdh+ and trh+ V. parahaemolyticus cultures (2.88 × 108 and 2.35 × 108 CFU/g respectively) were serially diluted (ten-fold serial dilution). The 25 g of clam meat in 225 ml of APW was homogenized separately using a high-speed blender. Then, 1 ml from each different V. parahaemolyticus dilutions was inoculated to 9 ml of homogenate, mixed, and immediately subjected for CCL preparation (protocol described before). One microliter of CCL was further used for conventional PCR, RT-PCR, and LAMP assay.

LAMP assay to detect pathogenic V. parahaemolyticus in naturally contaminated samples

Clam (n = 31) and shrimp (n = 31) were collected from the local market in March 2018 to February 2019 (Table 1). The samples were brought to the laboratory, cleaned, and homogenized aseptically in the laboratory. The CCL was prepared from the samples and subjected to LAMP assay targeting trh and tdh genes. Similarly, the same CCL was also subjected to conventional PCR and RT-PCR assay.

Table 1 Details of the samples and results of the LAMP, real-time PCR, and conventional PCR assay

Comparison of LAMP assay with conventional PCR and RT-PCR for the detection of pathogenic V. parahaemolyticus

Conventional PCR assay

Conventional PCR was carried out for all the seafood samples targeting trh, and tdh genes. The assay was performed in 30 μl volumes comprising LAMP F3 and B3 primers and Tada et al. [19] primers using CCL. Amplification was done using a T100™ thermal cycler (Bio-Rad, CA, USA) and visualized on 2% agarose gel and documented (described before).

RT-PCR

The RT-PCR assay was performed in a CFX96 real-time system (Bio-Rad, USA) for all the samples collected in the study. Reaction volume (25 μl) (in triplicate) consists of the supermix (Bio-Rad, USA), 2.5 pmol of each forward and reverse primer of trh and tdh genes (F3 and B3 of LAMP primers, Table ST2), and 2 μl of crude DNA template. Amplification was performed with an initial denaturation at 95 °C for 4 min, followed by amplification for 40 cycles at 95 °C for 20 s and 55 °C for 30 s. Melt curve analysis to check the random amplification of untargeted regions from 65 to 95 °C for 5 s with an increase of 0.5 °C in a stepwise manner as compared to a positive control (±0.5). A cycle threshold (Ct) value of less than 35 was considered to be positive. A no-template control and positive control were included in every reaction. The amplification for various samples (Ct values of 24–35) was validated by considering the Ct value of positive control. Representative amplicons were also confirmed by being visualized on 2% agarose gel and documented (described before).

Statistical analysis

The significant difference between two detection methods, i.e., LAMP and conventional PCR and LAMP and RT-PCR for each gene were calculated using two-sample proportion tests with the significance of p < 0.05. Two sample proportion tests are performed using an online software Mathcracker. Graphs were generated using Prism version 5.0 software (Graph Pad, Inc., La Jolla, USA). The percentage of agreement between three diagnostic assays was calculated using Cohen’s Kappa coefficient in SPSS 16.0 software (SPSS Inc., Chicago, IL, USA). The kappa coefficients’ values were interpreted according to the criteria of Viera and Garrett [20].

Result and discussion

Specificity and sensitivity of LAMP assay

In LAMP assay, 63 °C temperatures for 60 min of amplification was found to be optimum for both tdh and trh genes. An increase in the turbidity due to LAMP reaction was measured using LoopAmp real-time turbidimeter as compared to negative controls. The reaction was considered positive when turbidity reached 0.1 within 60 min (Fig. SF1). Specificity assay of LAMP assay was tested using various bacterial strains, including both V. parahaemolyticus and other bacterial strains. Both the designed primers of trh and tdh genes showed good specificity with no false positive and negative results for the tested bacterial isolates (Fig. SF2). In general, the presence of tdh and/or trh is primarily associated with the pathogenic strains of V. parahaemolyticus and is considered a virulence marker [1, 2, 21]. It is also true that the presence of tdh or trh genes have been reported in other non-V. parahaemolyticus vibrionaceae species, including V. mimicus, V. cholerae, V. hollisae, V. diaboilcus, and V. alginolyticus [1]. Hence, further inclusion of these strains harboring tdh or trh can confirm the assay’s high specificity. However, due to these strains’ unavailability, we could not include them during our specificity study.

The sensitivity of LAMP assay was found to be high. In the DNA dilution method, LAMP assay was able to detect 1 pg of DNA (trh and tdh), whereas conventional PCR was able to detect 100 pg of DNA (Fig. SF3). Similarly, when the sensitivity of the assay was tested with spiked clam meat, it was able to detect 102 CFU/g (1 CFU per reaction) and 104 CFU/g (100 CFU per reaction) by LAMP and conventional PCR assay, respectively. The RT-PCR assay showed a similar degree of sensitivity of LAMP assay with a detection limit of 102 CFU/g (Fig. 1). Di et al. [22] developed LAMP assay targeting tlh and tdh, which could able to detect as low as 2 CFU/g of V. parahaemolyticus in seafood. Prompamorn et al. [23] reported the detection limit of 103 CFU/g for V. parahaemolyticus in spiked samples. LAMP assays with both loop primers can detect the target cells at concentration of 10 CFU per reaction [24]. Previously, LAMP assay was developed for tdh and trh to detect pathogenic strains of V. parahaemolyticus however, not been tested using seafood samples [2, 25, 26]. To date, all the LAMP-based assays developed for the detection of pathogenic V. parahaemolyticus targeting trh and tdh was not validated by direct seafood samples, and the studies involved either enrichment or use of pure cultures. The other available isothermal amplification methods for the detection of V. parahaemolyticus require enrichment for detecting 2 CFU/g of cells in the seafood sample [27]. The validation of an assay is important to confirm the sensitivity, specificity, and accuracy of the method. Therefore, in this study, we have tested the optimized LAMP assay using clam and shrimp samples collected from the local market for 1 year.

Fig. 1
figure 1

Determination of sensitivity test by artificial contamination of clam targeting trh+ and tdh+ V. parahaemolyticus culture. (A1, B1) Conventional PCR amplification targeting trh using Tada et al. [19] and F3–B3. Lane M: 100 bp marker, Lane 1: Negative control, Lane 2: Positive control: 2.35 × 107 CFU/ml. Lanes 3–9: Reaction carried out with spiked suspensions containing 106, to 0 CFU/ml cells. (A2, B2) Conventional PCR amplification targeting tdh using Tada et al. [19] and F3–B3. Lane M: 100 bp marker, Lane 1: Negative control, Lane 2: Positive control: 2.88 × 107 CFU/ml. Lanes 3–9: Reaction carried out with spiked suspensions containing 106, to 0 CFU/ml cells. (C1, C2) LAMP amplification targeting trh and tdh. Lane M: 100 bp marker, Lane 1: Positive control (trh: 2.35 × 107 CFU/ml and tdh: 2.88 × 107 CFU/ml), Lane 2: Negative control, Lanes 3–9: Reaction carried out with spiked suspensions containing 106, to 0 CFU/ml cells. (D1, D2) Results of RT-PCR showing sensitivity for trh and tdh (F3 and B3) in the spiked sample

Detection of V. parahaemolyticus in naturally contaminated seafood sample

Reports on the presence of trh and tdh gene in environmental samples are always checked using conventional culture-based methods or standard conventional PCR based assays. The detection limit using these available methods is affected by low amount of template DNA, inhibitory agents present in the sample to perform conventional PCR [28]. Hence, the report of low prevalence may be due to the false-negative results by the tool used to detect the pathogenic strains of V. parahaemolyticus. Malcolm et al. [21] reported better LAMP assay sensitivity for the detection of V. parahaemolyticus over multiplex PCR, even when the targeted contaminant density was low in shellfish.

In this study, out of 62 samples screened (clam and shrimp), eight (12.9%) were positive for trh, and seven (11.29%) samples for tdh gene by LAMP assay (Fig. SF4, Table 1). Five (8.02%) samples were positive for both trh and tdh. However, three (4.83%) samples were positive for trh, and two (3.22%) samples were positive for tdh gene. The increase in the pathogenic strains of V. parahaemolyticus in the food chain is possibly due to cross-contamination in the seafood harvesting, processing and distributing centers, and changing cooking habits. Hence, these issues need to be addressed, and simple detection methods required to be implemented. A similar result was also observed by Raghunath et al. [29] where the number of trh+ V. parahaemolyticus was significantly higher in seafood samples as compared to tdh+ V. parahaemolyticus.

In different types of seafood samples, six (19.35%) clam, and four shrimp (12.9%) samples were carrying pathogenicity associated genes (trh/tdh). Further, LAMP assay detected the presence of trh gene in five (16.12%) clam and three (9.6%) shrimp samples. tdh gene was detected in three (9.6%) clam samples and four (12.9%) shrimp samples. Odeyemi [7] reported a meta-analysis of the incidence of V. parahaemolyticus from 2003 to 2015, which showed that the prevalence of V. parahaemolyticus was 52.9% for clam and 48.3% for shrimp. Besides, other studies also prove the fact that V. parahaemolyticus prevalence is relatively more in shellfish [30, 31].

Comparison of LAMP assay with conventional PCR and RT-PCR

None of the seafood samples were positive for trh gene in conventional PCR assay, and only one sample (1.6%) was positive for tdh gene. This is possibly due to CCL as a template for conventional PCR. Reports suggest that PCR amplification can be affected due to the presence of inhibitors in the reaction mix. However, this is not a major issue for LAMP assay since it is based on bst polymerase enzyme [32, 33]. In the RT-PCR assay, 15 (24.19%) samples were positive for trh, and 14 (22.58%) samples were positive for tdh genes (Fig. 2, Table 1). Results were analyzed using a two-sample proportion test to check the significant difference between the techniques compared in the study. A significant difference (p < 0.05) in the results was observed when samples were subjected to LAMP and conventional PCR for the detection of two different genes (trh and tdh). However, no significant difference was observed when LAMP and RT-PCR were used to detect V. parahaemolyticus using trh and tdh genes. Cao et al. [34] explained the equal sensitivity of LAMP and RT-PCR for the detection of viable but non-culturable (VBNC) V. parahaemolyticus. The agreement between LAMP and RT-PCR analysis was found to be fair with kappa value k ≥ 0.2 for both the genes. There was no agreement between LAMP and PCR with kappa value k ≤ 0. Samples showing positive amplification in LAMP, RT-PCR, and PCR methods are represented in the Venn diagram (Fig. SF5). Even though the RT-PCR (cutoff Ct value ≤35) was able to amplify tdh and trh genes in slightly more samples than LAMP assay, LAMP assay can be considered to be a better practical method to detect pathogenic strains of V. parahaemolyticus due to its simplicity and cost-effectiveness.

Fig. 2
figure 2

Comparison between LAMP, conventional PCR assay, and RT-PCR of trh gene (a) and tdh gene (b). *Significant difference between LAMP and conventional PCR assay (p < 0.05). #No significant difference between LAMP and real-time PCR assay