An approach for differentiating echovirus 30 and Japanese encephalitis virus infections in acute meningitis/encephalitis: a retrospective study of 103 cases in Vietnam

This study was approved by the Institutional Review Board of the National Institute of Hygiene and Epidemiology (NIHE), Vietnam (No: 01 IRB, November 7, 2005, No: 33 IRB, December 15, 2011).

Cerebrospinal fluid (CSF) specimens were collected only from patients who were clinically diagnosed to have acute meningitis/encephalitis at the time of admission and whose clinical records were available. The patients were from the National Hospital of Pediatrics (NHP) in Hanoi, Northern Vietnam and from Bac Giang General Hospital (BGGH) in Bac Giang, Northern Vietnam. The period of collection at the NHP was from 2001–2002, when an E30 outbreak occurred in Hanoi. The period of collection at BGGH was from 1999 to 2008. NIHE collects clinical specimens from BGGH annually because it is located in a JEV endemic area [16].

CSF specimens were sent to the NIHE for laboratory diagnosis. The E30 cases were identified by the neutralization test (NT) using anti-E30 serum [20]. Several samples that were unidentified by the NT were subjected to the virus isolation and gene amplification method as described below. The JEV cases were confirmed by IgM Capture ELISA [16].

Eight unidentified samples were subjected to virus isolation. Each CSF specimen was inoculated in human rhabdomyosarcoma cells (RD cells). The cells were incubated at 37°C with 5% CO₂ until the cytopathic effect (CPE) was observed under a microscope [21, 22]. Then, the infected culture fluids (ICFs) were collected and kept at -80°C prior to use. The viral RNA was isolated from the ICFs by the QIAamp Viral RNA Mini Kit (QIAGEN) according to the manufacturer’s instructions [23]. To amplify the complete VP1 gene of E30, RNA templates were subjected to reverse transcription and polymerase chain reaction (RT-PCR) using the forward primer 5′-GCRTGCAATGAYTTCTCWGT-3′ and the reverse primer 5′-GCICCIGAYTGITGICCRAA-3′ [24]. The amplicons were sequenced using the ABI PRISM 3100-Avant Genetic Analyzer [25].

Phylogenetic analysis of selected strains of human E30 from different geographical origins was performed based on the VP1 gene sequences (Figure 1). Alignment of these sequences was performed by Clustal W version 2.0 [26], and a neighbor-joining tree [27] was generated using MEGA 5.0 software [28]. The prototype strain Farina of Echovirus 21 (GenBank accession number: AY302547) was used as the out-group. The reliability of the phylogenetic tree was determined by a bootstrap resampling test with 1,000 replicates.

The clinical data from E30-confirmed cases (E30 group) and JEV-confirmed cases (JEV group) were included in the statistical analysis. The statistical analysis was conducted using R version 2.15 software [29]. The difference between the E30 and the JEV groups was tested by Chi-squared tests and Fisher Exact tests. The distribution of values between these groups was compared by the F test, and the difference of values between them was assessed by Student’s t-tests or Welch tests. A P value of less than 0.05 was accepted as significant.

Eighty-eight patients from NHP were confirmed to have E30 infection based on NT (80 patients) and virus isolation (8 patients) (Figure 2). One hundred thirty-four patients at BGGH were confirmed to have JEV infection by IgM Capture ELISA (Figure 2).

E30 was isolated from eight CSF specimens. The VP1 gene in these isolates was sequenced. The designated strain name of each isolate and the corresponding GenBank accession number (enclosed in parentheses below) were as follows: 01VN80 (KC999616), 01VN89 (KC999617), 01VN90 (KC999618), 01VN92 (KC999619), 01VN102 (KC999620), 01VN104 (KC999621), 02VN24 (KC999622), and 02VN28 (KC999623).

We constructed the NJ tree of these eight Vietnamese strains together with the 88 E30 strains from GenBank based on the VP1 gene sequence. Based on this tree, our identified strains were relatively close to the Asian strains that caused aseptic meningitis (Figure 1).

Most patients were under 15 years old in both the E30 and the JEV groups. The median age was 7 in the former group and 6 in the latter group. In the E30 group, there were 30 male patients (70%) and 13 female patients (30%), with a male-to-female ratio of 2.3:1. In the JEV group, there were 22 male patients (37%) and 38 female patients (63%), with a male-to-female ratio of 1:1.7. The percentage of JEV-vaccinated patients in the E30 group was significantly higher than that in the JEV group (E30 vs. JEV: 56% vs. 12%, p < 0.001) (Table 1). Fatal (12%) and sequelae (10%) cases were observed in the JEV group only (Table 1). Both E30 and JEV cases occurred more frequently during the summer season from May to July (Figure 3).

The clinical features during admission of the E30 and the JEV patients are shown in Table 2. The vital sign parameters (body temperature, pulse rate, and respiratory rate) on admission day showed no significant difference between the two groups of patients. A longer hospitalization period was observed in the JEV group than in the E30 group (E30 vs. JEV: 7 [range: 3–23] vs. 9 [1–37] days, p = 0.003). More patients in the E30 group complained of headache (95% vs. 50%, p < 0.001), vomiting (98% vs. 33%, p < 0.001), abdominal symptoms (19% vs. 5%, p = 0.048), and neck or back pain (26% vs. 2%, p < 0.001). On the other hand, more patients in the JEV group had a higher maximum body temperature (38.0 [37.0-41.0] vs. 38.8 [37.0-40.0] °C, p = 0.010), altered consciousness (12% vs. 97%, p < 0.001), and seizures (5% vs. 73%, p < 0.001). The periods of altered consciousness (1 [1-3] vs. 3 [1-17] days, p = 0.002), seizures (1 [1] vs. 2 [1-7] days, p < 0.001), Babinski reflex (1 [1-3] vs. 2 [1-7] days, p = 0.001), and focal neurological signs (1 [1] vs. 2.5 [1-13] days, p = 0.037) lasted longer in the JEV group. Both groups had a similar percentage of patients with signs of meningeal irritations, whereas the duration period was longer in the JEV group (1 [1-6] vs. 3 [1-14] days, p = 0.002). More patients in the JEV group experienced Babinski reflex (42% vs. 62%, p = 0.047), and with a longer duration (1 [1-3] vs. 2 [1-7] days, p = 0.001). Hemiplegia was observed only in the JEV group (25%, p < 0.001).

We also focused on the symptoms observed simultaneously. The combined symptoms of headache and vomiting and the triad of symptoms of fever, headache, and vomiting were observed in more patients in the E30 group (19% vs. 0%, p < 0.001 and 74% vs. 27%, p < 0.001, respectively). On the other hand, occurrence of the combined symptoms of fever and headache was observed only in the JEV group (18%, p = 0.002).

The results of the CSF and blood examination are shown in Table 3. CSF leucocytes were significantly increased in the E30 group (80 [1–750] vs. 18 [5–350] cells/μL, p = 0.003). An increased number of both CSF neutrophils and CSF lymphocytes was observed in the E30 group (neutrophils: 26 [2–381] vs. 10 [3–140] cells/μL, p = 0.033, lymphocytes: 56 [3–676] vs. 12 [4–210] cells/μL, p = 0.043). The CSF sugar levels were significantly decreased in the JEV group (58.7 [27–90] vs. 46.9 [25–74] mg/dL, p < 0.001). Other indicators of CSF and blood components showed no significant difference between the E30 and the JEV groups.

The laboratory diagnosis required at least one week to complete, thus medication was given even before the results of the diagnosis became available. The medication histories of the E30 and the JEV groups are shown in Table 4. A history of the use of steroids showed no significant difference between the two groups (E30 vs. JEV: 98% vs. 97%). The duration of steroids use also showed no difference in both groups (3 [2-4] vs. 3 [2-15] days). More patients were prescribed mannitol (47% vs. 95%, p < 0.001) and antibiotics (35% vs. 95%, p < 0.001) in the JEV group. The duration of mannitol use was longer in the JEV group (1 [1-3] vs. 3 [1-7] days, p < 0.001). A history of the use of diazepam showed no significant difference between the two groups. The duration of diazepam use was longer in the E30 group (6 [2-14] vs. 2 [1-11] days, p < 0.001). More patients in the JEV group were prescribed barbiturates (33% vs. 63%, p = 0.002), chlorpromazine (5% vs. 23%, p = 0.012), fentanyl (0% vs. 33%, p < 0.001), and sodium valproate (0% vs. 33%, p < 0.001).