Identity of a Novel Swine Hepatitis E Virus in Taiwan Forming a Monophyletic Group with Taiwan Isolates of Human Hepatitis E Virus

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Journal of Clinical Microbiology, December 1999, p. 3828-3834, Vol. 37, No. 12
0095-1137/99/$04.00+0
Copyright © 1999, American Society for Microbiology. All rights reserved.

Identity of a Novel Swine Hepatitis E Virus in Taiwan Forming a Monophyletic Group with Taiwan Isolates of Human Hepatitis E Virus

Sen-Yung Hsieh,¹^,²^,^* Xiang-Jin Meng,³^, Ying-Hua Wu,¹^,² Shih-Tung Liu,² Albert W. Tam,⁴ Dneg-Yn Lin,¹ and Yun-Fan Liaw¹

Liver Research Unit, Chang Gung Memorial Hospital,¹ and Department of Microbiology and Immunology, School of Medicine, Chang Gung University,² Taoyuan, Taiwan; Laboratory of Infectious Diseases, National Institute of Allergy and Infectious Diseases, National Institutes of Health, Bethesda, Maryland 20892³; and Molecular Virology Department, Genelabs Technologies, Redwood City, California 94063⁴

Received 18 June 1999/Returned for modification 12 August 1999/Accepted 31 August 1999

	ABSTRACT

Top Abstract Introduction Materials and Methods Results Discussion References

Recently, we found that more than 10% of the cases of acute non-A, non-B, non-C hepatitis in Taiwan were caused by a novelstrain of hepatitis E virus (HEV). Since none of these patientshad a history of travel to areas where HEV is endemic, the sourceof transmission remains unclear. The recent discovery of a swineHEV in herd pigs in the United States has led us to speculatethat HEV may also circulate in herd pigs in Taiwan and may serveas a reservoir for HEV in Taiwan. Of 275 herd pigs obtained from10 pig farms in Taiwan, 102 (37%) were seropositive for serumanti-HEV immunoglobulin G (IgG). A 185-bp genomic sequence withinthe ORF-2 of the HEV genome was amplified and cloned from serumsamples of an anti-HEV positive pig and subsequently from serumsamples of a patient with acute hepatitis E. Sequence comparisonrevealed that the swine and human isolates of HEV share 97.3%identity. Phylogenetic analyses further showed that the Taiwanswine and human isolates of HEV form a distinct branch divergentfrom all other known strains of HEV, including the U.S. swinestrain. To examine the potential risk of cross-species transmissionof swine HEV to humans, the seroprevalences of anti-HEV IgG in30 swine handlers, 20 pork dealers, and 50 control subjects wereassessed and were found to be 26.7, 15, and 8%, respectively (forswine handlers versus controls, P = 0.048). Our findings may helpprovide an understanding of the modes of HEV transmission andmay also raise potential public health concerns for HEVzoonosis.

	INTRODUCTION

Top Abstract Introduction Materials and Methods Results Discussion References

Hepatitis E virus (HEV) is the major causative pathogen of enterically transmitted non-A, non-B hepatitis (3, 4, 17,33). HEV is a nonenveloped RNA virus. Its genome, about 7.5kb in size, contains three partially overlapping open readingframes (ORFs) (18, 40). ORF-1 likely encodes nonstructuralviral proteins (putative RNA helicase, protease, and RNA-dependentRNA polymerase). ORF-2 encodes the putative capsid protein, andORF-3 encodes a cytoskeleton-associated phosphoprotein (14,18, 40, 50).

HEV is transmitted primarily via a fecal-oral route, and hepatitis E occurs predominantly as outbreaks of waterborne epidemicsin developing countries (3, 18). Hepatitis E is rarely diagnosedin developed countries and is usually regarded as imported (1,8, 21, 38, 39). It has, however, long been an enigmathat the seroprevalence of HEV antibodies (anti-HEV) is relativelyhigh in areas where HEV is not endemic compared to the documenteddisease burden (7, 22, 25, 30, 32, 45).

Taiwan, an area of endemicity for viral hepatitis A and B, has never had an epidemic of hepatitis E. However, about 10 to20% of the cases of acute hepatitis identified on this islandare without a defined etiology. Recently, we found that more than10% of our cases of acute non-A, non-B, non-C hepatitis were causedby acute infection with a novel strain of HEV (12). A partialsequence within the ORF-1 of this novel strain of HEV was successfullycloned from four of these patients. Phylogenetic studies indicatedthat all four of these isolates of HEV form a distinct branchdivergent from all previously reported isolates worldwide (12).Since none of our patients had a disease-related history of travelto areas where HEV is endemic, it is quite likely that the transmissionof HEV occurred in Taiwan. Therefore, it is important to determinethe source of transmission of HEV in Taiwan. Recently, a novelstrain of HEV from swine (the U.S. swine HEV strain) was isolatedfrom herd pigs in the midwestern United States (26). Subsequently,two cases of acute hepatitis E reported in the United States werefound to be caused by an HEV strain genetically very similar tothe U.S. swine HEV strain (36). These findings suggest thatswine HEV may be involved in cross-species infection between swineand humans. Since swine HEV and the U.S. human strains of HEVare so similar genetically and since Taiwan has a dense populationof pigs, it was of interest to examine whether pigs in Taiwanare a potential reservoir for HEV transmission to humans. Hereinwe report evidence of HEV circulation in herd pigs in Taiwan andidentification of a Taiwan strain of swine HEV genetically distinctfrom the U.S. swine HEV strain. Interestingly, sequence comparisonand phylogenetic analyses indicated that the Taiwan swine andhuman isolates of HEV were distinct from other known strains ofHEV but were very closely related to eachother.

	MATERIALS AND METHODS

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Swine serum samples. Serum samples were collected from 275 pigs on 10 pig farms in different geographic regions in Taiwan. Almost all the pigstested in this study were older than 3 months. Serum samples from10 specific-pathogen-free (SPF) pigs raised under laboratory conditionswere included as negative controls for the enzyme-linked immunosorbentassay (ELISA) for detection of anti-HEV in swinesera.

ELISA for anti-HEV in swine. The standard ELISA for anti-HEV in swine was performed essentially as described previously (26, 27). Briefly, a purified55-kDa truncated form of the putative capsid protein derived froma human strain of HEV (Sar-55) was used as the antigen for theELISA (42, 43). Peroxidase-labeled goat anti-swine immunoglobulinG (IgG) was used as the secondary antibody. All of the swine serumsamples were assayed in duplicate. Preimmune and hyperimmune anti-HEV-positivesera as well as preinoculation and postinoculation sera from apig experimentally infected with swine HEV were included as negativeand positive controls, respectively (26, 27). In addition,serum samples from 10 SPF pigs were included as negativecontrols.

Human serum samples. To examine the genetic relationship of the Taiwan swine isolate of HEV to the human HEV isolate causing sporadic cases ofacute hepatitis E in Taiwan, acute-phase sera from a patient withacute hepatitis E were used for molecular cloning of a cognateregion within the ORF-2 of the HEV genome. We had used the sameserum sample to clone a partial sequence within the ORF-1 of HEVin a previous study (patient T821) (12). To assess the seroprevalenceof anti-HEV IgG in pig handlers, serum samples were obtained from30 individuals who had worked on swine farms for at least 5 years.Twenty individuals who had worked in pork companies and 50 age-and sex-matched (to the swine handlers) healthy individuals wereincluded as controlgroups.

ELISA for anti-HEV IgG and anti-HEV IgM in human. Serum was assayed for anti-HEV IgG and anti-HEV IgM in humans by using commercial diagnostic kits according to the manufacturer'sinstructions (Genelabs Diagnostica, Singapore) (48).

RNA extraction and reverse transcription-PCR (RT-PCR). RNA was extracted from 100 µl of each serum sample by the single-step acid-phenol method and was converted to cDNA by a randomprimer method as described previously (11). The cDNA templateswere subjected to amplification by a PCR standardized to detectHEV RNA. Two sets of primers derived from the putative capsidgene of the U.S. swine HEV strain (26) were used for the nestedPCR. The first-round and second-round PCRs were performed similarlywith 25 and 35 cycles, respectively, and the PCR parameters includeddenaturation for 40 s at 94°C, annealing for 1 min at 55°C, andextension for 1 min at 72°C. The amplified DNA products were analyzedby gel electrophoresis and were subsequently cloned into the pGEM-Tvector according to the manufacturer's instructions (Promega,Madison, Wis.). The cloned PCR products were sequenced with anAutomatic Sequencer Kit (ABI PRISM 337 DNA sequencer PRISM 337Collection; Sequence Analysis 3.0; Perkin-Elmer). The primer sequencesfor the first-round PCR were as follows: sense primer, 5'-AACACACCTTACACTGGTGCAT-3',and antisense primer, 5'-TGCCCTTGTCCTGCTGCGCATTCT-3'. Those forthe second-round PCR were as follows: sense primer, 5'-CGTGTTTCCCGGTACACCAGCACA-3',and antisense primer, 5'-CAGTTGGCCCCCGGCCGACGAA-3'.

Sequence analyses. Pairwise sequence comparison and phylogenetic analyses were carried out with the aid of computer software (Clustal) with aweighted residue weight table (DNAstar, Inc., Madison, Wis.).

Nucleotide sequence accession numbers. The GenBank accession numbers for the Taiwan swine and human isolates of HEV reported herein are AF077004 and AF077005,respectively.

	RESULTS

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Serological evidence that HEV is circulating in herd pigs in Taiwan. Two hundred seventy-five serum samples obtained from pigs on 10 pig farms were assayed for the presence of anti-HEV IgG. Asshown in Table 1, about 37.1% of the pigs tested were seropositivefor anti-HEV IgG. However, the percentage of pigs seropositivefor anti-HEV IgG varied among different farms: from as low as0% (0 of 6 pigs) and 4.8% (2 of 42 pigs) to as high as 61.5% (16of 26 pigs) and 66.7% (20 of 30 pigs). The variations were notconsidered to be a result of age differences, since almost allthe pigs tested were older than 3 months. The specificity of theELISA for assaying anti-HEV IgG in swine sera had been validatedpreviously (26) and was further supported by seronegativityfor anti-HEV in 10 SPF pigs raised under laboratory conditions(data not shown).

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TABLE 1. Prevalence of antibodies to HEV in herd pigs in Taiwan

Identification of a novel sequence of HEV from a pig serum sample positive for anti-HEV. Fifty-six serum samples obtained from farms 9 and 10 were subjected to RT-PCR amplification to attempt to identify the sequencewithin the conserved ORF-2 region of HEV. Only 1 of the 38 anti-HEV-positiveserum samples was positive by RT-PCR for HEV RNA, while all 18anti-HEV-negative serum samples remained RT-PCR negative (datanot shown). Cloning and sequencing analysis confirmed that theamplified PCR product was derived from the genome of a novel HEVstrain. The nucleotide sequence of this novel strain of HEV (strainswT74) from swine was compared to the sequences of the correspondingregions of the U.S. swine HEV and other strains of human HEV (Fig.1).

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FIG. 1. Nucleotide sequence alignments of a 185-bp genomic sequence within the ORF-2 region of HEV. Ch.1, Ch.2, Ch.3, CHb, and CXj are five isolates from China (GenBank accession nos., D11092, L25547, L25595, M94177, and L08816, respectively); Pk, Ind532, Np, Br, Ind, MY, Egy, and Chad are the isolates from Pakistan (accession no. M80581), India (accession no. U62621), Nepal (accession no. AF020607), Myanmar (accession no. M73218), India (accession no. X99441), Myanmar (accession no. D10330), Egypt (accession no. AF051351), and Chad (accession no. U62121), respectively; swUS and USP-1 are swine and human isolates, respectively, from the United States (accession nos. AF011921 and AF035437, respectively); swT74 (accession no. AF077004) is the swine isolate from Taiwan; T821 (accession no. AF077005) is the isolate from patient T821 (this report); Mx (accession no. M74506) is an isolate from Mexico. The nucleotide position is relative to the numbering system for the Burmese isolate (40). The nucleotide sequence of isolate Ch.1 is shown on top, and only nucleotide substitutions are indicated (uppercase) for other isolates.

Comparison of Taiwan swine HEV to Taiwan human HEV. We have previously reported the identification of a novel strain of HEV from patients with acute non-A, non-B, non-C hepatitisin Taiwan (12). The cDNA fragments cloned from these human strainsof HEV were within the ORF-1. In order to determine the geneticrelationship between strains of swine HEV and human HEV in Taiwan,a patient with acute hepatitis E was selected. The patient wasa 72-year-old retired farmer who had lived beside a pig farm inthe northern region of Taiwan for decades. The patient had nohistory of travel abroad before the episode of acute hepatitis.The patient was admitted to the Chang Gung Memorial Hospital presentingwith a typical clinical course of acute viral hepatitis. The peaklevels of serum alanine aminotransferase (ALT) and total bilirubinwere 1,126 U/liter and 22.5 mg%, respectively. The diagnosis ofacute hepatitis E was based on elevated levels of ALT and totalbilirubin along with the following findings: (i) negative resultsof testing for serum hepatitis A virus IgM antibodies, hepatitisB virus IgM core antibodies, hepatitis B virus surface antigen,hepatitis C virus antibodies, and hepatitis C virus RNA as determinedby RT-PCR; (ii) seropositivity for HEV IgM and IgG antibodies;and (iii) positivity for HEV RNA in serum by an RT-PCR as describedpreviously (12). Serum samples collected on day 10 after theonset of jaundice were used for the molecular cloning of a partialgenomic fragment within the ORF-2 of HEV (Fig. 1). We had usedthe same serum sample to clone a partial sequence within the ORF-1of HEV in a previous report (patient T821) (12). Comparisonof the sequence of this ORF-2 region revealed that this Taiwanisolate of human HEV (T821) shared 97.3 and 98.4% sequence identitieswith the Taiwan swine HEV isolate (swT74) at the nucleotide leveland the amino acid level, respectively (Table 2).

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TABLE 2. Identities of nucleotide sequences and amino acid sequences shown in Fig. 1

Phylogenetic analyses of the swine and human strains of HEV isolated in Taiwan and other available strains of HEV worldwide. A pairwise comparison based on a 185-bp sequence within the ORF-2 was performed (Table 2). The Taiwan swine HEV strain (swT74),the Taiwan human HEV strain (T821), the U.S. swine HEV strain(swUS), a strain of HEV identified from a patient in the UnitedStates (US-1), and other strains of HEV isolated from other regionsof the world were included in the comparison. As shown in Table2, the nucleotide sequence identity between the U.S. swine isolateand US-1 was 92.4%, whereas the identity between the Taiwan swineisolate and the U.S. swine isolate was 80.0%, and that betweenthe Taiwan swine isolate and US-1 was 77.3%. Clearly, the twoswine strains of HEV isolated in different geographic regionswere genetically distinct. The nucleotide sequences of the Taiwanswine and human isolates of HEV were 97.3% identical to each other,while they shared only about 70% nucleotide sequence identitieswith HEV strains isolated from China, Pakistan, India, Nepal,Burma, Egypt, and Chad. Phylogenetic analysis, as shown in Fig.2, indicated that the Taiwan swine and Taiwan human isolates ofHEV were clustered into a single branch, while the U.S. swineisolate and the U.S. human isolate (US-1) formed another distinctbranch. The isolates from Asia including China, Pakistan, India,Nepal, and Myanmar formed the third branch, and the Mexican isolatealone represented the fourth branch (Fig. 2). The isolates fromAfrica (Egypt and Chad) were clustered with each other and wererelatively related to the isolates from Asia, but they were quitedivergent from the Taiwan, U.S., and Mexican isolates. As a result,both of the isolates from Egypt and Chad might be classified asa subbranch of the Asian strains. The phylogenetic tree basedon the partial sequence within ORF-2 is very similar to the treebased on the partial sequence within ORF-1 presented in our previousreport (12). However, the sequence within ORF-1 of the Taiwanswine isolate was not available for analysis in our previous study.

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FIG. 2. Phylogenetic tree based on a 185-bp sequence within the ORF-2 region of the HEV genome. The sources of these isolates are described in the text as well as in the legend to Fig. 1. The phylogenetic tree was constructed with the computer software Clustal with the weighted residue weight table (DNAstar) grounded on the sequence divergence. The length of each pair of branches represents the distance between sequence pairs. The scale beneath the tree measures the distance between sequences. Units indicate the number of substitution events.

Prevalence of serum anti-HEV IgG in pig handlers and in general population in Taiwan. To examine whether pig handlers are at higher risk for HEV infection, 30 individuals who had been handling pigs for more than5 years were assayed for the presence of anti-HEV. Anti-HEV IgGwas detected in 26.7% (8 of 30) of these pig handlers. In comparison,20 individuals who worked in pork companies but who had no directcontact with pigs were included, and 15% (3 of 20) were foundto be positive for serum anti-HEV IgG. In addition, 50 age- andsex-matched (to the group of pig handlers) individuals were alsoselected as controls, and 8% (4 of 50) were found to be positivefor serum anti-HEV IgG. As shown in Table 3, the differencesin the seroprevalence rates among the three groups are not statisticallysignificant, while the difference between the pig handlers andthe controls was marginally significant (P = 0.048 by Fisher'sexact test).

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TABLE 3. Rates of serum antibodies against HEV in persons handing pig or not handling pigs

	DISCUSSION

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It has long been an enigma that the seroprevalence of anti-HEV is relatively high in countries where HEV is not endemic (7,22, 25, 30, 41). Recently, an increasing number of patientswith sporadic acute hepatitis E but with no history of travelto areas where HEV is endemic have been reported in industrializedcountries (15, 16, 20, 37, 49, 51), suggesting thatHEV infection in those patients is acquired domestically. Theneed to explain domestic infection of HEV in areas where HEV isnot endemic has led to a hypothesis that animals may serve asreservoirs for the transmission of human hepatitis E (34). Thishypothesis is further supported by the findings that anti-HEVhas been detected in a number of wild animals including pigs,sheep, and rats in areas where HEV is endemic (5, 6) andthat domestic pigs, monkeys, rats, and sheep were reportedly susceptibleto infection with HEV (2, 13, 24, 45). Balayan et al.(2) reported that Russian domestic swine were susceptible toexperimental infection with a Central Asian strain of HEV isolatedfrom a human. However, the identity of the virus infecting pigsin that study was not known since the virus recovered from thepigs was not sequenced. Others have failed to experimentally infectpigs with two well-characterized epidemic strains of human HEV,including an Asian strain of human HEV (27, 31). Recently,a U.S. strain of human HEV isolated from a U.S. resident was shownto infect pigs, but this U.S. strain of human HEV is geneticallyvery closely related to the U.S. strain of swine HEV (28). Itis possible that the genetic makeup of a particular HEV strainmay determine the host range. Experimental infections of rhesusmonkeys and chimpanzees with swine HEV and of pigs with a humanstrain of HEV (28) provided experimental and genetic evidencefor cross-species HEV infection. However, further experimentsare needed to confirm that swine serve as a natural reservoirfor transmission of humanHEV.

We report herein on another isolate of swine HEV identified from a pig in Taiwan. The Taiwan swine HEV strain is geneticallydistinct from the swine HEV strain reported in the United States(26) and other known strains of HEV, but it is very closelyrelated to the HEV strain isolated from humans with sporadic acutehepatitis E in Taiwan (12). Several lines of evidence suggestthat the Taiwan swine isolate of HEV and the human strains ofHEV causing sporadic acute hepatitis E in Taiwan may be variantsof the same virus. (i) On the basis of a 185-bp sequence withinthe ORF-2 of the HEV genome, the Taiwan swine and human isolatesof HEV are genetically very similar to each other (97.3 and 98.4%sequence identities at the nucleotide and amino acid levels, respectively).(ii) The phylogenetic tree based on the partial ORF-2 sequence(Fig. 2) is very similar to the one generated previously witha partial ORF-1 sequence, the sequence of which has not been determinedfor the Taiwan swine isolate (12). The similar genetic relationshipamong different isolates of HEV was obtained by separate phylogeneticanalyses of the entire genome and of each of the putative viralgenes, as well as the respective peptides of HEV (10), whichfurther support our hypothesis. (iii) The human isolate of HEVfrom which the partial ORF-2 sequence was determined in this studyemanated from the same serum sample (T821) that was used to clonethe partial sequence within ORF-1 in our previous study (12).Therefore, the Taiwan swine isolate of HEV very likely forms amonophyletic group with the four human isolates of HEV describedin our previous report (12). Further studies are warranted tocharacterize genetically and experimentally the novel swine HEVstrain identified in Taiwan and to determine definitively thephylogenetic relationships among these novel HEVstrains.

Since the identification of novel strains of HEV from two U.S. residents without a history of travel to areas where HEV isendemic, numerous HEV variants have recently been identified inareas where the disease is not endemic (9, 12, 20, 36,37, 46, 47, 51). Novel HEV variants which are geneticallydistinct from the Burmese, Mexican, and U.S. genotypes have beenidentified from Taiwan (12), Italy (37, 51), Greece (37),Egypt (44), and China (46). However, the sequences of thenew Chinese isolates that have been reported were not in the sameregion as those of the Taiwan isolates of human and swine HEVwhose sequences have been reported (46), and the sequences ofthe Italian and Greek isolates are not yet available in the database(37, 51) to permit us to perform a phylogenetic analysis.Recently, by using bootstrap resampling of the multiple-sequencealignment, Schlauder et al. (37) reported a phylogenetic treebased on a partial sequence within ORF-1. They showed that theisolates from Taiwan were relatively more closely related to theisolates from Liaoning Province of China (namely, the new Chinesegenotype) but were divergent from Burmese-like group (includingisolates from Burma, Pakistan, India, Nepal, and western China),the Mexican isolate, the U.S. group (including two human isolatesand one swine isolate from the United States), or the novel isolatesfrom Europe (including two the Italian isolates and one Greekisolate). However, a definitive genetic relationship between theTaiwan swine HEV strain and the human isolates of HEV from LiaoningProvince of China remains to bedetermined.

The seroprevalence of anti-HEV in swine in Taiwan was found to be relatively high, suggesting that HEV is widespread in theswine population in Taiwan. Similar results were reported forpigs in the United States (26). Therefore, it is reasonableto speculate that HEV may circulate in the swine population worldwide.This may pose a potential public health concern as a zoonosisfor pig handlers as well as for the general population, sinceHEV is transmitted by the fecal-oral route. In addition, consideringthe immense interest in xenotransplantation of pig organs, swineHEV may also pose a potential risk forxenozoonosis.

As a first step toward addressing the question of whether swine HEV can be transmitted to humans, we assessed the prevalenceof serum anti-HEV IgG in pig handlers, pork dealers, and the generalpopulation. Similar to previous reports (22), the prevalenceof serum anti-HEV was relatively high even in the control groups(8% of the general population and 15% of pork dealers). Althoughthe prevalence of serum anti-HEV was higher in pig handlers (26.7%),the difference in prevalence between pig handlers and the generalpopulation group is only marginally significant (for pig handlersversus the general population group, P = 0.048 by Fisher's exacttest). These findings indicate (i) that HEV infection occasionallyoccurs in the general population. (ii) Transmission of swine HEVto humans does occur, but not frequently. In fact, only a fewcases of acute hepatitis E have been identified in the UnitedStates, although most of the pigs there were infected with HEV.Considering that pigs usually become infected at an early ageand the majority of adult pigs are seropositive for anti-HEV (26)and considering that shedding of virus in feces occurs only duringthe acute stage of infection, anti-HEV-positive adult pigs veryunlikely shed virus in their feces or sera. In addition, becausethe virus is transmitted by the fecal-oral route, transmissionof HEV is greatly dependent on the sanitary conditions under whichthe pig handlers work, which have been much improved in recentyears in industrialized countries. These factors should significantlyreduce the risk for transmission of HEV from swine to humans.(iii) Swine may not be the only animal reservoir for HEV. Thathepatitis E has been reported in countries that do not traditionallyraise pigs and that the high rate of seroprevalence of anti-HEVin the general population in areas where HEV is not endemic indicatethe presence of other animal reservoirs for HEV. In fact, serumanti-HEV has been found in wild rats, monkeys, and sheep in areaswhere HEV is endemic (6). Domestic animals such as dogs, cats,and rats may also serve as reservoirs for transmission of humanhepatitis E. Clearly, the natural history of HEV must be determinedin order to effectively prevent HEVzoonosis.

Overt hepatitis E is usually associated with a higher serum bilirubin level (17, 29, 47) and a higher mortality ratethan acute hepatitis caused by hepatitis A or B virus (18).However, most of the individuals positive for serum anti-HEV IgGdo not have a history of overt hepatitis, suggesting that subclinicalinfection with HEV exists and occurs more frequently than overthepatitis. Indeed, in pigs naturally infected with HEV and inpigs experimentally infected with swine HEV, only mild histologicalevidence of hepatitis was observed (26, 28). Similarly, onlymild biochemical and histological evidence of hepatitis was observedin nonhuman primates experimentally infected with swine HEV (27).Variations in the clinical manifestations of viral hepatitis areusually dependent on multiple factors, such as the age of thepatients and the immune response of the host. The genetic heterogeneityof the virus may also be an important determining factor. Forexample, infection with genotype 1b of the hepatitis C virus usuallyruns a graver course and has a poorer response to interferon therapythan infection with other genotypes (19, 23, 35). It is,therefore, very important to determine whether an avirulent strainof HEV is causing a subclinical infection or whether a virulentstrain of HEV is causing severe hepatitis in humans. The Taiwanswine HEV strain does not appear to cause any clinical symptomsin swine (data not shown). However, a strain of HEV very similarto the Taiwan swine HEV strain caused overt hepatitis in humansin Taiwan (for example, patient T821). Furthermore, pigs inoculatedwith the US-2 human strain of HEV remained clinically normal (28).Nevertheless, these findings do not exclude the possibility thatclinically divergent presentations of human HEV infection area result of the genetic heterogeneity of the virus. Comparisonof the sequences of HEV isolates from patients with or withoutovert hepatitis is necessary to address this question. However,it is almost impossible to isolate HEV from individuals withoutovert hepatitis, since HEV infection is transient and subclinicalhepatitis goesunattended.

	ACKNOWLEDGMENTS

We thank Suzanne U. Emerson and Robert H. Purcell for providing the purified HEV antigen for detection of swine anti-HEV.We also thank Pei-Ying Yang for excellent technical assistanceand Su-Chen Chi for help in preparation of themanuscript.

This work was supported in part by a fund from the Chang Gung Memorial Hospital and a grant (DOH89-TD-1027) from the Departmentof Health, Executive Yuan,Taiwan.

	FOOTNOTES

^* Corresponding author. Mailing address: Liver Research Unit, Chang Gung Memorial Hospital, 199 Tung Hua North Rd., Taipei,Taiwan 155. Phone: 886-3-3281200, ext. 8107. Fax: 886-3-3272236and 886-3-3282824. E-mail: siming{at}adm.cgmh.com.tw.

Present address: Department of Biomedical Sciences and Pathobiology, Center for Molecular Medicine and Infectious Diseases,Virginia Polytechnic Institute and State University, Blacksburg,VA 24061-0342.

REFERENCES

Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References

1. Bader, T., K. Krawczynski, L. Polish, and M. Favorov. 1991. Hepatitis E in a U.S. traveler to Mexico. N. Engl. J. Med. 325:1659[Medline]. (Letter.)

2. Balayan, M. S., P. K. Usmanov, N. A. Zamayatina, D. I. Djumalieva, and F. R. Karas. 1990. Brief report: experimental hepatitis E infection in domestic pigs. J. Med. Virol. 32:58-59[Medline].

3. Bradley, D. W., K. Krawczynski, E. H. Cook, Jr., K. McCaustaland, C. D. Humphrey, J. E. Spelbring, H. Myint, and J. E. Maynard. 1987. Enterically transmitted non-A, non-B hepatitis: serial passages of disease in cynomolgus macaques and tamarines and recovery of disease-associated 27- to 34-nm virus-like particles. Proc. Natl. Acad. Sci. USA 84:6277-6281[Abstract/Free Full Text].

4. Bradley, D. W. 1990. Enterically-transmitted non-A, non-B hepatitis. Br. Med. Bull. 46:442-461[Abstract/Free Full Text].

5. Clayson, E. T., B. L. Innis, K. S. A. Myint, S. Narupiti, D. W. Vaughn, S. Giril, P. Ranabhat, and M. P. Shrestha. 1995. Detection of hepatitis E virus infections among domestic swine in the Kathmandu Valley of Nepal. Am. J. Trop. Med. Hyg. 53:228-232.

6. Clayson, E. T., R. Snitbhan, M. Ngarmpochana, D. W. Vaughn, and M. P. Shresth. 1996. Evidence of the hepatitis E virus (HEV) is a zoonotic virus: detection of natural infections among swine, rats and chickens in an area endemic for human disease, p. 329-335. In Y. Busson, P. Coursaget, and M. Kane (ed.), Enterically transmitted hepatitis viruses. La Simarre, Joué-lès-Tours, France.

7. Dawson, G. J., K. H. Chau, C. M. Cabal, P. O. Yarbough, G. R. Reye, and I. K. Mushahwar. 1992. Solid-phase enzyme-linked immunosorbent assay for hepatitis E virus IgG and IgM antibodies utilizing recombinant antigens and synthetic peptides. J. Virol. Methods 38:175-186[Medline].

8. Dawson, G. J., I. K. Mushahwar, and K. H. Chau. 1992. Detection of long-lasting antibody to hepatitis E virus in an U.S. traveler to Pakistan. Lancet 340:426-427[Medline].

9. Erker, J. C., S. M. Desai, G. G. Schlauder, G. J. Dawsone, and I. K. Mushahwa. 1999. A hepatitis virus variant from the United States: molecular characterization and transmission in cynomolgus macaques. J. Gen. Virol. 80:681-690[Abstract].

10. Gouvea, V., N. Snellings, M. J. Popek, C. F. Longer, and B. L. Innis. 1998. Hepatitis E virus: complete genome sequence and phylogenetic analysis of a Nepali isolate. Virus Res. 57:21-26[Medline].

11. Hsieh, S. Y., P. Y. Yang, H. C. Chen, and Y. F. Liaw. 1997. Cloning and characterization of the 5' terminal sequences of the RNA genome of GB virus C/hepatitis G virus. Proc. Natl. Acad. Sci. USA 94:3206-3210[Abstract/Free Full Text].

12. Hsieh, S. Y., Y. P. Yang, Y. P. Ho, C. M. Chu, and Y. F. Liaw. 1998. Identification of a novel strain of hepatitis E virus responsible for sporadic acute hepatitis in Taiwan. J. Med. Virol. 55:300-304[Medline].

13. Jameel, S., H. Durgapal, C. M. Habibullah, M. S. Khuroo, and S. K. Panda. 1992. Enteric non-A, non-B hepatitis: epidemics, animal transmission, and hepatitis E virus detection by the polymerase chain reaction. J. Med. Virol. 37:263-270[Medline].

14. Jameel, S., M. Zafrullah, M. H. Ozdener, and S. K. Panda. 1996. Expression in animal cells and characterization of the hepatitis E virus structural proteins. J. Virol. 70:207-216[Abstract].

15. Jardi, R., M. Buti, F. Rodriguez-Frias, and R. Esteban. 1993. Hepatitis E infection in acute sporadic hepatitis in Spain. Lancet 341:1355-1356[Medline].

16. Johansson, P. J., I. K. Mushahwar, G. Norkrans, O. Weiland, and E. Nordenfelt. 1995. Hepatitis E infection in patients with acute hepatitis non-A-D in Sweden. Scand. J. Infect. Dis. 27:543-546[Medline].

17. Khuroo, M. S. 1980. Study of an epidemic of non-A, non-B hepatitis: possibility of another human hepatitis virus distinct from post-transfusion non-A, non-B type. Am. J. Med. 68:818-823[Medline].

18. Krawczynski, K. 1993. Hepatitis E. Hepatology 17:932-941[Medline].

19. Kurosaki, M., N. Enomoto, T. Murakami, I. Sakuma, Y. Ashina, C. Yamamoto, T. Ikeda, S. Tozuda, N. Izumi, F. Marumo, and C. Sato. 1997. Analysis of genotype and amino acid residues 2209 to 2248 of the NS5A region of hepatitis C virus in relation to the response to interferon-beta therapy. Hepatology 25:750-753[Medline].

20. Kwo, P. Y., G. G. Schlauder, H. A. Carpenter, P. J. Murphy, J. E. Rosenblatt, G. J. Dawson, E. E. Mase, K. Krawczynski, and V. Balan. 1997. Acute hepatitis E by a new isolate acquired in the United States. Mayo Clin. Proc. 72:1133-1136[Medline].

21. Lau, J. Y., R. Sallie, J. W. Fang, P. O. Yarbough, G. R. Reyes, B. C. Portmann, G. Mieli-Vergani, and R. Willian. 1995. Detection of hepatitis E virus genome and gene products in two patients with fulminant hepatitis E. J. Hepatol. 22:605-610[Medline].

22. Lee, S. D., Y. J. Wang, R. H. Lu, C. Y. Chan, K. J. Lo, and R. Moeckli. 1994. Seroprevalence of antibody to hepatitis E virus among Chinese subjects in Taiwan. Hepatology 19:866-870[Medline].

23. Le Guen, B., G. Squadrito, B. Nalpas, P. Berthelot, S. Pol, and C. Berchot. 1997. Hepatitis C virus genome complexity correlates with response to interferon therapy: a study in French patients with chronic hepatitis C. Hepatology 25:1250-1254[Medline].

24. Maneerat, Y., E. T. Clayson, K. S. A. Myint, G. D. Young, and B. L. Innis. 1996. Experimental infection of the laboratory rat with the hepatitis E virus. J. Med. Virol. 48:121-128[Medline].

25. Mast, E. E., I. K. Kuramoto, M. O. Favorov, V. R. Sehocning, B. T. Burkholder, C. N. Shapirs, and P. V. Holland. 1997. Prevalence of risk factors for antibodies to hepatitis E virus seroreactivity among blood donors in northern California. J. Infect. Dis. 176:34-40[Medline].

26. Meng, X. J., R. H. Purcell, P. G. Halbur, J. R. Lehman, D. M. Webb, T. S. Tsareva, J. S. Haynes, B. J. Thacker, and S. U. Emerson. 1997. A novel virus in swine in closely related to the human hepatitis E virus. Proc. Natl. Acad. Sci. USA 94:9860-9865[Abstract/Free Full Text].

27. Meng, X. J., P. G. Halbur, J. S. Haynes, T. S. Tsareva, J. D. Bruna, P. L. Royer, R. H. Purcell, and S. U. Emerson. 1998. Experimental infection of pigs with the newly identified swine hepatitis E virus (swine HEV), but not with human strains of HEV. Arch. Virol. 143:1405-1415[Medline].

28. Meng, X. J., P. G. Halbur, M. S. Shapiro, S. Govindarajan, I. D. Bruna, I. K. Mushahwar, R. H. Purcell, and S. U. Emerson. 1998. Genetic and experimental evidence for cross-species infection by swine hepatitis E virus. J. Virol. 72:9714-9721[Abstract/Free Full Text].

29. Morrow, R. H., H. F. Smetana, F. T. Sai, and J. H. Edgcomb. 1968. Unusual features of viral hepatitis in Accra, Ghana. Ann. Intern. Med. 68:1250-1264.

30. Paul, D. A., M. F. Knigge, A. Ritter, R. Gutierrez, T. Pilo-Matia, K. H. Chau, and J. G. Dawson. 1994. Determination of hepatitis E virus seroprevalence by using recombinant fusion proteins and synthetic peptides. J. Infect. Dis. 169:801-806[Medline].

31. Platt, K. B., K. J. Yoon, and S. Zimmerman. 1998. Susceptibility of swine to hepatitis E virus and its significance to human health, p. 125-126. In Swine research report. Iowa State University, Ames.

32. Quiroga, J. A., T. Cotonat, I. Castillo, and V. Carreno. 1996. Hepatitis E virus seroprevalence in acute viral hepatitis in a developed country confirmed by a supplemental assay. J. Med. Virol. 50:16-19[Medline].

33. Reyes, G. R., M. A. Purdy, J. P. Kim, K. C. Luk, L. M. Young, K. E. Fry, and D. W. Bradley. 1990. Isolation of a cDNA from the virus responsible for enterically transmitted non-A, non-B hepatitis. Science 247:1335-1339[Abstract/Free Full Text].

34. Reyes, G. R. 1997. Overview of the epidemiology and biology of the hepatitis E virus, p. 239-258. In R. A. Willsen (ed.), Viral Hepatitis. Marcel Dekker, Inc., New York, N.Y.

35. Romeo, R., M. G. Rumi, E. Del Ninno, and M. Colombo. 1997. Hepatitis C genotype 1b and risk of hepatocellular carcinoma. Hepatology 26:1077-1081[Medline].

36. Schlauder, G. G., G. J. Dawson, J. C. Erker, P. Y. Kwo, M. F. Knigge, D. L. Smalley, J. E. Rosenblatt, S. M. Desai, and I. K. Mushahwar. 1998. The sequence and phylogenetic analysis of a novel hepatitis E virus isolated from a patient with acute hepatitis reported in the United States. J. Gen. Virol. 79:447-456[Abstract].

37. Schlauder, G. G., S. M. Desai, A. R. Zanetti, N. C. Tassopoulos, and I. K. Mushahwar. 1999. Novel hepatitis E virus (HEV) isolates from Europe: evidence for additional genotypes of HEV. J. Med. Virol. 57:243-251[Medline].

38. Skidmore, S. J., P. O. Yarbough, K. A. Gabor, A. W. Tam, and G. R. Reyes. 1991. Imported hepatitis E in UK. Lancet 337:1541[Medline].

39. Smalley, D. L., S. C. Brewer, G. J. Dawson, C. Kyrk, and B. Waters. 1996. Hepatitis E virus infection in an immigrant to the United States. South. Med. J. 89:993-996.

40. Tam, A. W., M. M. Smith, M. E. Guerra, C. C. Huang, D. W. Bradley, K. E. Fry, and G. R. Reyes. 1991. Hepatitis E virus (HEV): molecular cloning and sequencing of the full-length viral genome. Virology 185:120-131[Medline].

41. Thomas, D. L., P. O. Yarbough, D. Vlahov, S. A. Tsarev, K. E. Nelson, A. J. Saah, and R. H. Purcell. 1997. Seroreactivity to hepatitis E virus in areas where the disease is not endemic. J. Clin. Microbiol. 35:1244-1247[Abstract].

42. Tsareva, S. A., S. U. Emerson, G. R. Reyes, T. S. Tsareva, L. J. Legters, I. A. Malik, M. Iqbal, and R. H. Purcell. 1992. Characterization of a prototype strain of hepatitis E virus. Proc. Natl. Acad. Sci. USA 89:559-563[Abstract/Free Full Text].

43. Tsareva, S. A., T. S. Tsareva, S. U. Emerson, A. Z. Kapikian, J. Ticehurst, W. London, and R. H. Purcell. 1993. ELISA for antibody to hepatitis E virus (HEV) based on complete open-reading frame-2 protein expressed in inset cells: identification of HEV infection in primates. J. Infect. Dis. 168:369-378[Medline].

44. Tsareva, S. A., L. N. Binn, P. J. Gomatos, R. R. Arthure, M. K. Monier, H. van Cuyck-Gandr, C. F. Longer, and B. L. Innis. 1999. Phylogenetic analysis of hepatitis E virus isolates from Egypt. J. Med. Virol. 57:68-74[Medline].

45. Usmanov, R. K., M. S. Balayan, O. V. Dvoinkova, D. B. Alymbaeva, N. A. Zamiatina, I. A. Kazachkov, and V. I. Belov. 1994. An experimental infection in lambs by the hepatitis E virus. Vopr. Virusol. 9:165-168.

46. Wang, Y., R. Ling, J. C. Erker, H. Zhang, H. Li, S. Desai, I. K. Mushahwar, and T. I. Harrison. 1999. A divergent genotype of hepatitis E virus in Chinese patients with acute hepatitis. J. Gen. Virol. 80:169-177[Abstract].

47. Wu, J. C., I. J. Sheen, T. Y. Chiang, W. Y. Sheng, Y. J. Wand, C. Y. Chan, and S. D. Lee. 1998. The impact of traveling to endemic areas on the spread of hepatitis E virus infection: epidemiological and molecular analyses. Hepatology 27:1415-1420[Medline].

48. Yarbough, P. O., A. W. Tam, K. E. Fry, I. K. Krawczynski, K. A. McCaustland, D. W. Bradley, and G. R. Reyes. 1991. Hepatitis E virus: identification of type-common epitopes. J. Virol. 65:5790-5797[Abstract/Free Full Text].

49. Zaaijer, H. L., F. P. Mauser-Bunschoten, J. H. ten Veen, H. P. Kapprell, M. Kok, H. M. van den Berg, and P. N. Lelie. 1995. Hepatitis E virus antibodies among patients with hemophilia, blood donors, and hepatitis patients. J. Med. Virol. 46:244-246[Medline].

50. Zafrullah, M., M. H. Ozadener, S. K. Panda, and S. Jameel. 1997. The ORF3 protein of hepatitis E virus is a phosphoprotein that associates with the cytoskeleton. J. Virol. 71:9045-9053[Abstract].

51. Zanetti, A. R., G. G. Schlauder, L. Romano, E. Tanzi, P. Fabris, G. J. Dawson, and I. K. Mushahwar. 1999. Identification of a novel variant of hepatitis E virus in Italy. J. Med. Virol. 57:356-360[Medline].

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1.	Bader, T., K. Krawczynski, L. Polish, and M. Favorov. 1991. Hepatitis E in a U.S. traveler to Mexico. N. Engl. J. Med. 325:1659[Medline]. (Letter.)
2.	Balayan, M. S., P. K. Usmanov, N. A. Zamayatina, D. I. Djumalieva, and F. R. Karas. 1990. Brief report: experimental hepatitis E infection in domestic pigs. J. Med. Virol. 32:58-59[Medline].
3.	Bradley, D. W., K. Krawczynski, E. H. Cook, Jr., K. McCaustaland, C. D. Humphrey, J. E. Spelbring, H. Myint, and J. E. Maynard. 1987. Enterically transmitted non-A, non-B hepatitis: serial passages of disease in cynomolgus macaques and tamarines and recovery of disease-associated 27- to 34-nm virus-like particles. Proc. Natl. Acad. Sci. USA 84:6277-6281[Abstract/Free Full Text].
4.	Bradley, D. W. 1990. Enterically-transmitted non-A, non-B hepatitis. Br. Med. Bull. 46:442-461[Abstract/Free Full Text].
5.	Clayson, E. T., B. L. Innis, K. S. A. Myint, S. Narupiti, D. W. Vaughn, S. Giril, P. Ranabhat, and M. P. Shrestha. 1995. Detection of hepatitis E virus infections among domestic swine in the Kathmandu Valley of Nepal. Am. J. Trop. Med. Hyg. 53:228-232.
6.	Clayson, E. T., R. Snitbhan, M. Ngarmpochana, D. W. Vaughn, and M. P. Shresth. 1996. Evidence of the hepatitis E virus (HEV) is a zoonotic virus: detection of natural infections among swine, rats and chickens in an area endemic for human disease, p. 329-335. In Y. Busson, P. Coursaget, and M. Kane (ed.), Enterically transmitted hepatitis viruses. La Simarre, Joué-lès-Tours, France.
7.	Dawson, G. J., K. H. Chau, C. M. Cabal, P. O. Yarbough, G. R. Reye, and I. K. Mushahwar. 1992. Solid-phase enzyme-linked immunosorbent assay for hepatitis E virus IgG and IgM antibodies utilizing recombinant antigens and synthetic peptides. J. Virol. Methods 38:175-186[Medline].
8.	Dawson, G. J., I. K. Mushahwar, and K. H. Chau. 1992. Detection of long-lasting antibody to hepatitis E virus in an U.S. traveler to Pakistan. Lancet 340:426-427[Medline].
9.	Erker, J. C., S. M. Desai, G. G. Schlauder, G. J. Dawsone, and I. K. Mushahwa. 1999. A hepatitis virus variant from the United States: molecular characterization and transmission in cynomolgus macaques. J. Gen. Virol. 80:681-690[Abstract].
10.	Gouvea, V., N. Snellings, M. J. Popek, C. F. Longer, and B. L. Innis. 1998. Hepatitis E virus: complete genome sequence and phylogenetic analysis of a Nepali isolate. Virus Res. 57:21-26[Medline].
11.	Hsieh, S. Y., P. Y. Yang, H. C. Chen, and Y. F. Liaw. 1997. Cloning and characterization of the 5' terminal sequences of the RNA genome of GB virus C/hepatitis G virus. Proc. Natl. Acad. Sci. USA 94:3206-3210[Abstract/Free Full Text].
12.	Hsieh, S. Y., Y. P. Yang, Y. P. Ho, C. M. Chu, and Y. F. Liaw. 1998. Identification of a novel strain of hepatitis E virus responsible for sporadic acute hepatitis in Taiwan. J. Med. Virol. 55:300-304[Medline].
13.	Jameel, S., H. Durgapal, C. M. Habibullah, M. S. Khuroo, and S. K. Panda. 1992. Enteric non-A, non-B hepatitis: epidemics, animal transmission, and hepatitis E virus detection by the polymerase chain reaction. J. Med. Virol. 37:263-270[Medline].
14.	Jameel, S., M. Zafrullah, M. H. Ozdener, and S. K. Panda. 1996. Expression in animal cells and characterization of the hepatitis E virus structural proteins. J. Virol. 70:207-216[Abstract].
15.	Jardi, R., M. Buti, F. Rodriguez-Frias, and R. Esteban. 1993. Hepatitis E infection in acute sporadic hepatitis in Spain. Lancet 341:1355-1356[Medline].
16.	Johansson, P. J., I. K. Mushahwar, G. Norkrans, O. Weiland, and E. Nordenfelt. 1995. Hepatitis E infection in patients with acute hepatitis non-A-D in Sweden. Scand. J. Infect. Dis. 27:543-546[Medline].
17.	Khuroo, M. S. 1980. Study of an epidemic of non-A, non-B hepatitis: possibility of another human hepatitis virus distinct from post-transfusion non-A, non-B type. Am. J. Med. 68:818-823[Medline].
18.	Krawczynski, K. 1993. Hepatitis E. Hepatology 17:932-941[Medline].
19.	Kurosaki, M., N. Enomoto, T. Murakami, I. Sakuma, Y. Ashina, C. Yamamoto, T. Ikeda, S. Tozuda, N. Izumi, F. Marumo, and C. Sato. 1997. Analysis of genotype and amino acid residues 2209 to 2248 of the NS5A region of hepatitis C virus in relation to the response to interferon-beta therapy. Hepatology 25:750-753[Medline].
20.	Kwo, P. Y., G. G. Schlauder, H. A. Carpenter, P. J. Murphy, J. E. Rosenblatt, G. J. Dawson, E. E. Mase, K. Krawczynski, and V. Balan. 1997. Acute hepatitis E by a new isolate acquired in the United States. Mayo Clin. Proc. 72:1133-1136[Medline].
21.	Lau, J. Y., R. Sallie, J. W. Fang, P. O. Yarbough, G. R. Reyes, B. C. Portmann, G. Mieli-Vergani, and R. Willian. 1995. Detection of hepatitis E virus genome and gene products in two patients with fulminant hepatitis E. J. Hepatol. 22:605-610[Medline].
22.	Lee, S. D., Y. J. Wang, R. H. Lu, C. Y. Chan, K. J. Lo, and R. Moeckli. 1994. Seroprevalence of antibody to hepatitis E virus among Chinese subjects in Taiwan. Hepatology 19:866-870[Medline].
23.	Le Guen, B., G. Squadrito, B. Nalpas, P. Berthelot, S. Pol, and C. Berchot. 1997. Hepatitis C virus genome complexity correlates with response to interferon therapy: a study in French patients with chronic hepatitis C. Hepatology 25:1250-1254[Medline].
24.	Maneerat, Y., E. T. Clayson, K. S. A. Myint, G. D. Young, and B. L. Innis. 1996. Experimental infection of the laboratory rat with the hepatitis E virus. J. Med. Virol. 48:121-128[Medline].
25.	Mast, E. E., I. K. Kuramoto, M. O. Favorov, V. R. Sehocning, B. T. Burkholder, C. N. Shapirs, and P. V. Holland. 1997. Prevalence of risk factors for antibodies to hepatitis E virus seroreactivity among blood donors in northern California. J. Infect. Dis. 176:34-40[Medline].
26.	Meng, X. J., R. H. Purcell, P. G. Halbur, J. R. Lehman, D. M. Webb, T. S. Tsareva, J. S. Haynes, B. J. Thacker, and S. U. Emerson. 1997. A novel virus in swine in closely related to the human hepatitis E virus. Proc. Natl. Acad. Sci. USA 94:9860-9865[Abstract/Free Full Text].
27.	Meng, X. J., P. G. Halbur, J. S. Haynes, T. S. Tsareva, J. D. Bruna, P. L. Royer, R. H. Purcell, and S. U. Emerson. 1998. Experimental infection of pigs with the newly identified swine hepatitis E virus (swine HEV), but not with human strains of HEV. Arch. Virol. 143:1405-1415[Medline].
28.	Meng, X. J., P. G. Halbur, M. S. Shapiro, S. Govindarajan, I. D. Bruna, I. K. Mushahwar, R. H. Purcell, and S. U. Emerson. 1998. Genetic and experimental evidence for cross-species infection by swine hepatitis E virus. J. Virol. 72:9714-9721[Abstract/Free Full Text].
29.	Morrow, R. H., H. F. Smetana, F. T. Sai, and J. H. Edgcomb. 1968. Unusual features of viral hepatitis in Accra, Ghana. Ann. Intern. Med. 68:1250-1264.
30.	Paul, D. A., M. F. Knigge, A. Ritter, R. Gutierrez, T. Pilo-Matia, K. H. Chau, and J. G. Dawson. 1994. Determination of hepatitis E virus seroprevalence by using recombinant fusion proteins and synthetic peptides. J. Infect. Dis. 169:801-806[Medline].
31.	Platt, K. B., K. J. Yoon, and S. Zimmerman. 1998. Susceptibility of swine to hepatitis E virus and its significance to human health, p. 125-126. In Swine research report. Iowa State University, Ames.
32.	Quiroga, J. A., T. Cotonat, I. Castillo, and V. Carreno. 1996. Hepatitis E virus seroprevalence in acute viral hepatitis in a developed country confirmed by a supplemental assay. J. Med. Virol. 50:16-19[Medline].
33.	Reyes, G. R., M. A. Purdy, J. P. Kim, K. C. Luk, L. M. Young, K. E. Fry, and D. W. Bradley. 1990. Isolation of a cDNA from the virus responsible for enterically transmitted non-A, non-B hepatitis. Science 247:1335-1339[Abstract/Free Full Text].
34.	Reyes, G. R. 1997. Overview of the epidemiology and biology of the hepatitis E virus, p. 239-258. In R. A. Willsen (ed.), Viral Hepatitis. Marcel Dekker, Inc., New York, N.Y.
35.	Romeo, R., M. G. Rumi, E. Del Ninno, and M. Colombo. 1997. Hepatitis C genotype 1b and risk of hepatocellular carcinoma. Hepatology 26:1077-1081[Medline].
36.	Schlauder, G. G., G. J. Dawson, J. C. Erker, P. Y. Kwo, M. F. Knigge, D. L. Smalley, J. E. Rosenblatt, S. M. Desai, and I. K. Mushahwar. 1998. The sequence and phylogenetic analysis of a novel hepatitis E virus isolated from a patient with acute hepatitis reported in the United States. J. Gen. Virol. 79:447-456[Abstract].
37.	Schlauder, G. G., S. M. Desai, A. R. Zanetti, N. C. Tassopoulos, and I. K. Mushahwar. 1999. Novel hepatitis E virus (HEV) isolates from Europe: evidence for additional genotypes of HEV. J. Med. Virol. 57:243-251[Medline].
38.	Skidmore, S. J., P. O. Yarbough, K. A. Gabor, A. W. Tam, and G. R. Reyes. 1991. Imported hepatitis E in UK. Lancet 337:1541[Medline].
39.	Smalley, D. L., S. C. Brewer, G. J. Dawson, C. Kyrk, and B. Waters. 1996. Hepatitis E virus infection in an immigrant to the United States. South. Med. J. 89:993-996.
40.	Tam, A. W., M. M. Smith, M. E. Guerra, C. C. Huang, D. W. Bradley, K. E. Fry, and G. R. Reyes. 1991. Hepatitis E virus (HEV): molecular cloning and sequencing of the full-length viral genome. Virology 185:120-131[Medline].
41.	Thomas, D. L., P. O. Yarbough, D. Vlahov, S. A. Tsarev, K. E. Nelson, A. J. Saah, and R. H. Purcell. 1997. Seroreactivity to hepatitis E virus in areas where the disease is not endemic. J. Clin. Microbiol. 35:1244-1247[Abstract].
42.	Tsareva, S. A., S. U. Emerson, G. R. Reyes, T. S. Tsareva, L. J. Legters, I. A. Malik, M. Iqbal, and R. H. Purcell. 1992. Characterization of a prototype strain of hepatitis E virus. Proc. Natl. Acad. Sci. USA 89:559-563[Abstract/Free Full Text].
43.	Tsareva, S. A., T. S. Tsareva, S. U. Emerson, A. Z. Kapikian, J. Ticehurst, W. London, and R. H. Purcell. 1993. ELISA for antibody to hepatitis E virus (HEV) based on complete open-reading frame-2 protein expressed in inset cells: identification of HEV infection in primates. J. Infect. Dis. 168:369-378[Medline].
44.	Tsareva, S. A., L. N. Binn, P. J. Gomatos, R. R. Arthure, M. K. Monier, H. van Cuyck-Gandr, C. F. Longer, and B. L. Innis. 1999. Phylogenetic analysis of hepatitis E virus isolates from Egypt. J. Med. Virol. 57:68-74[Medline].
45.	Usmanov, R. K., M. S. Balayan, O. V. Dvoinkova, D. B. Alymbaeva, N. A. Zamiatina, I. A. Kazachkov, and V. I. Belov. 1994. An experimental infection in lambs by the hepatitis E virus. Vopr. Virusol. 9:165-168.
46.	Wang, Y., R. Ling, J. C. Erker, H. Zhang, H. Li, S. Desai, I. K. Mushahwar, and T. I. Harrison. 1999. A divergent genotype of hepatitis E virus in Chinese patients with acute hepatitis. J. Gen. Virol. 80:169-177[Abstract].
47.	Wu, J. C., I. J. Sheen, T. Y. Chiang, W. Y. Sheng, Y. J. Wand, C. Y. Chan, and S. D. Lee. 1998. The impact of traveling to endemic areas on the spread of hepatitis E virus infection: epidemiological and molecular analyses. Hepatology 27:1415-1420[Medline].
48.	Yarbough, P. O., A. W. Tam, K. E. Fry, I. K. Krawczynski, K. A. McCaustland, D. W. Bradley, and G. R. Reyes. 1991. Hepatitis E virus: identification of type-common epitopes. J. Virol. 65:5790-5797[Abstract/Free Full Text].
49.	Zaaijer, H. L., F. P. Mauser-Bunschoten, J. H. ten Veen, H. P. Kapprell, M. Kok, H. M. van den Berg, and P. N. Lelie. 1995. Hepatitis E virus antibodies among patients with hemophilia, blood donors, and hepatitis patients. J. Med. Virol. 46:244-246[Medline].
50.	Zafrullah, M., M. H. Ozadener, S. K. Panda, and S. Jameel. 1997. The ORF3 protein of hepatitis E virus is a phosphoprotein that associates with the cytoskeleton. J. Virol. 71:9045-9053[Abstract].
51.	Zanetti, A. R., G. G. Schlauder, L. Romano, E. Tanzi, P. Fabris, G. J. Dawson, and I. K. Mushahwar. 1999. Identification of a novel variant of hepatitis E virus in Italy. J. Med. Virol. 57:356-360[Medline].