Outbreak of caliciviruses in the Singapore military, 2015

On 31 August 2015, a military camp in Singapore housing an approximately 5000 military personnel reported a suspected AGE outbreak. In the Singapore military, AGE cases are defined as patients with at least three episodes of watery stool and/or two episodes of vomiting within the 24 h prior to reporting sick. These cases should also have no history of recurrent diarrhea, vomiting, nor abdominal pain. A cluster of 10 or more cases meeting these criteria, linked either by space or a common food source, across 24 h constitutes an AGE outbreak.

Epidemiology teams were sent to conduct investigations and implement control measures. Symptom surveys and hygiene inspections were conducted; and water, food, and stool samples were tested. Water samples were obtained from common water sources at food halls and accommodation areas of the affected soldiers. Food samples were obtained from the food halls in the military camp and these were samples of the food consumed by the military personnel 2 days prior to the AGE outbreak. All the food and water samples were sent to an independent laboratory for culture and testing. Stool samples of cases and food handlers were collected and sent to DSO National Laboratories within 24 h after collection for PCR testing. The number of military personnel reporting sick with AGE was monitored daily by the camp clinic. Control measures were focused on the escalation of personal and environmental hygiene, which included the separation of affected and unaffected soldiers, enforcement of rigorous hand-washing and hygiene practices, and disinfection of communal areas with bleach. We describe here the epidemiological curve, symptoms experienced by the affected soldiers, and results of food, water, and stool tests.

The assays used for detecting 8 bacterial pathogens (i.e., Bacillus cereus, Campylobacter jejuni, Clostridium perfringens, diarrheagenic Escherichia coli, Listeria monocytogenes, Salmonella spp., Shigella spp. and Vibrio spp.) were a mix of those developed in-house and published assays modified into multiplex PCRs and were used routinely during AGE outbreaks [10]. The real-time reverse transcription PCR (RT-PCR) to detect NoV and SaV followed the protocols as previously described [19, 20]. All these assays were validated with test panels from various external quality assessment providers.

Reverse transcription was first performed on samples that were tested positive for both NoV and SaV with oligo(dT)₂₀ primer using the SuperScript® III First-Strand Synthesis System (Thermo Fisher Scientific, Waltham, USA) according to the manufacturer’s instructions. Partial capsid sequence was amplified from NoV- and SaV-positive samples according to Kojima et al. and Hansman et al. [21, 22]. The primer pairs used in this study are shown in Table 1. Primer set G1SKF and G1SKR was used for NoV GI-positive samples while primer set G2SKF and G2SKR was used for NoV GII-positive samples. The expected size of the amplicons generated by both sets of primers is about 330 bp. SaV-specific primers used for the amplification of the partial capsid sequence were SV-F13 and SV-R13 for the first-round PCR and SV-F22 and SV-R2 for the second-round PCR. The expected size of the amplicon generated by this nested PCR is about 430 bp. The PCR products were electrophoresed on 1% agarose in 0.5× Tris-borate-EDTA (TBE) buffer and visualized by Midori Green (Nippon Genetics Europe GmbH, Düren, Germany) staining. Those amplicons of the correct size were sent for Sanger sequencing.

Nucleotide sequences amplified from NoV and SaV detected during the outbreak, together with sequences from reference strains from the NCBI database were aligned with Clustal W method using the MegAlign module of the DNASTAR software package, version 12.2.0 (Lasergene, Madison, USA). A phylogenetic tree from bootstrap analysis with 1000 replicates was generated by the Neighbor–Joining method using the MegAlign module of the DNASTAR software package, version 12.2.0 (Lasergene, Madison, USA). The phylogenetic trees were rooted using a NoV GIII strain (Aba-Z5/GIII.1/HUN/EU360814) and a Porcine SaV GIII strain (Porcine Complete Genome/NC_000940.1) for their respective trees.

From 31 August to 9 September 2015, an AGE outbreak affecting 150 military personnel occurred at a military camp in Singapore (attack rate of approximately 3%). These military personnel typically reside in military camp during the working week and return home on weekends if there are no military activities. Primary healthcare for military personnel is provided by clinics within the military camps, which also serve as on-site surveillance for infectious diseases. The epidemiological curve of this AGE outbreak is shown in Fig. 1. After the surge of AGE cases (n = 37) on the initial day of outbreak (31 August 2015), the number of new cases for the next two days remained high at n = 29 and n = 27 respectively. This is likely due to the spread of the viral pathogens before the implemented control measures can take effect. On day 4 (3 September 2015) of the outbreak, the number of cases decreased to 18, indicating that the implemented control measures are beginning to take effect. On day 5 (4 September 2015), the number cases decreased to 9 and most military personnel returned home for the weekend of 5 and 6 September 2015. Upon their return to the military camp on the 7 September 2015 (Day 8), a higher than average number of 20 AGE cases was further reported. The following day on 8 September 2015 (Day 9), the number of new cases reported was back to baseline at 8 new cases, indicating that the outbreak had been under control. After a period of careful monitoring, the outbreak was declared closed on 9 September (Day 10) with a final tally of 150 affected military personnel.

A symptom survey was conducted among the patients during the outbreak and the most common clinical manifestation was diarrhea affecting 119 patients (79.3%). Other symptoms included vomiting (62.8%), abdominal pain (42.7%), nausea (42.0%) and fever (6.0%).

Food and water samples from the involved food halls were sent for microbiological testing by an independent laboratory. Final results (data not shown) from these tests showed that all the food and water samples met satisfactory standard, suggesting that the food and water supply to the military camp are not the source of the caliciviruses that caused this AGE outbreak.

86 stool specimens collected from 65 AGE cases and 58 stool samples from the food-handlers were sent to DSO National Laboratories for molecular testing. None of the samples from the AGE cases were positive for the 8 bacterial pathogens tested. We detected a total of 21 SaV-positive samples (from 20 patients), 16 NoV GI-positive samples (from 16 patients) and 9 NoV GII-positive specimens (from 8 patients). Specimens obtained from 5 AGE patients were positive for both NoV GI and SaV. The prevalence of patients with double-pathogen infections, single-pathogen infections and non-SaV/NoV infections within these 65 AGE patients was 7.7%, 52.3%, and 40.0%, respectively. None of the stool samples from the food-handlers were tested positive for NoV or SaV, indicating that they were not the source of the caliciviruses that started the AGE outbreak. The epidemiological curve of the outbreak and the distribution of the NoV- and SaV-positive cases are shown in Fig. 1.

Of the 25 NoV-positive samples, we were able to amplify and sequence the partial capsid region sequence from 14 NoV GI-positive samples and 2 NoV GII-positive sample. Sequences from the outbreak and reference strains from the NCBI database were aligned and a phylogenetic tree was constructed (Fig. 2). The phylogenetic tree showed that all but one of the NoV GI sequences were essentially identical to each other and clustered together with a NoV GI.7 isolate detected in stream water in Korea (20150227FL01/GI.7/KR/KT383953.1) (Fig. 2). The remaining NoV GI sequence clustered with a GI.9 isolate detected in sewage in China (Nanning2011/GI.9/CN/KM246907.1), thereby suggesting the environmental origins of the NoV GI isolates detected in this AGE episode (Fig. 2). From the frequency of the NoV GI.7 strain detected in the NoV GI-positive samples (13 out of 14 samples sequenced), it is also suggested that NoV GI.7 is the main NoV GI strain that caused the outbreak.

For NoV GII, both sequences clustered together with a human isolate of NoV GII.17 detected in Japan (Kawasaki308/GII.17/JP/LC037415.1) (Fig. 2). The remaining 7 NoV GII-positive samples failed to amplify for their partial capsid region, and no other strains of NoV GII were identified for this AGE outbreak.

Of the 21 SaV-positive samples, we were able to amplify and sequence the partial capsid region sequence from 11 SaV-positive samples. Sequences from the outbreak and reference strains were aligned and a phylogenetic tree was constructed (Fig. 3). All the SaV sequences amplified were essentially identical to each other and clustered together with two SaV GII.3 human isolates detected in Japan (i.e., Tokyo09-468/GII.3/JP/AB622445.1 and Tokyo10-3233/GII.3/JP/AB622458.1), suggesting the human origin of this SaV strain. Interestingly, one of the SaV GII.3-infected patients was also simultaneously infected with another strain of SaV closely related to a human SaV GI.3 isolate detected in Japan (Tokyo10-1526/GI.3/JP/AB622455.1). From the frequency of the SaV GII.3 strain detected in the SaV-positive samples (11 out of 11 samples sequenced), it is also suggested that SaV GII.3 is the main SaV GII strain that caused the outbreak.

The NoV and SaV sequences amplified for this study were submitted to GenBank under accession numbers KU298647-KU298674.