Comparative Pathogenesis of Infection of Pigs with Hepatitis E Viruses Recovered from a Pig and a Human

doi:10.1128/JCM.39.3.918-923.2001

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Journal of Clinical Microbiology, March 2001, p. 918-923, Vol. 39, No. 3
0095-1137/01/$04.00+0 DOI: 10.1128/JCM.39.3.918-923.2001
Copyright © 2001, American Society for Microbiology. All rights reserved.

Comparative Pathogenesis of Infection of Pigs with Hepatitis E Viruses Recovered from a Pig and a Human

P. G. Halbur,¹^,^* C. Kasorndorkbua,¹ C. Gilbert,² D. Guenette,² M. B. Potters,² R. H. Purcell,³ S. U. Emerson,³ T. E. Toth,² and X. J. Meng²

Veterinary Diagnostic and Production Animal Medicine, College of Veterinary Medicine, Iowa State University, Ames, Iowa 50011¹; Center for Molecular Medicine and Infectious Diseases, Department of Biomedical Sciences and Pathobiology, College of Veterinary Medicine, Virginia Polytechnic Institute and State University, Blacksburg, Virginia 24061²; and Laboratory of Infectious Diseases, National Institute of Allergy and Infectious Diseases, National Institutes of Health, Bethesda, Maryland 20892³

Received 11 August 2000/Returned for modification 15 December 2000/Accepted 1 January 2001

	ABSTRACT

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Specific-pathogen-free pigs were inoculated with one of two hepatitis E viruses (HEV) (one recovered from a pig and the otherfrom a human) to study the relative pathogenesis of the two virusesin swine. Fifty-four pigs were randomly assigned to three groups.Seventeen pigs in group 1 served as uninoculated controls, 18pigs in group 2 were intravenously inoculated with the swine HEVrecovered from a pig in the United States, and 19 pigs in group3 were intravenously inoculated with the US-2 strain of humanHEV recovered from a hepatitis patient in the United States. Twoto four pigs from each group were necropsied at 3, 7, 14, 20,27, or 55 days postinoculation (DPI). Evidence of clinical diseaseor elevation of liver enzymes or bilirubin was not found in pigsfrom any of the three groups. Enlarged hepatic and mesentericlymph nodes were observed in both HEV-inoculated groups. Multifocallymphoplasmacytic hepatitis was observed in 9 of 17, 15 of 18,and 16 of 19 pigs in groups 1 to 3, respectively. Focal hepatocellularnecrosis was observed in 5 of 17, 10 of 18, and 13 of 19 pigsin groups 1 to 3, respectively. Hepatitis lesions were very mildin group 1 pigs, mild to moderate in group 2 pigs, and moderateto severe in group 3 pigs. Hepatic inflammation and hepatocellularnecrosis peaked in severity at 20 DPI and were still moderatelysevere at 55 DPI in the group inoculated with human HEV. Hepatitislesions were absent or nearly resolved by 55 DPI in the swine-HEV-inoculatedpigs. All HEV-inoculated pigs seroconverted to anti-HEV immunoglobulinG. HEV RNA was detected by reverse transcriptase PCR in feces,liver tissue, and bile of pigs in both HEV-inoculated groups from3 to 27 DPI. Based on evaluation of microscopic lesions, the US-2strain of human HEV induced more severe and persistent hepaticlesions in pigs than did swine HEV. Pig livers or cells from thelivers of HEV-infected pigs may represent a risk for transmissionof HEV from pigs to human xenograft recipients. Since HEV wasshed in the feces of infected pigs, exposure to feces from infectedpigs represents a risk for transmission of HEV, and pigs shouldbe considered a reservoir forHEV.

	INTRODUCTION

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Hepatitis E virus (HEV) is the leading cause of enterically transmitted non-A, non-B hepatitis in people in many developingcountries (21, 28, 30). Transmission is thought to be primarilyby the fecal-oral route, and waterborne epidemics are characteristicof hepatitis E (1, 28, 30). Clinical disease due to HEVinfection is rarely diagnosed in industrialized countries, andmost cases of HEV infection in industrialized countries occurin people who have traveled to regions where the disease is endemic(10, 21, 28, 30). Clinical cases occur predominantly indeveloping countries in Asia, Africa, and Mexico (1, 2,28, 30). However, sporadic cases of acute hepatitis E in peoplein the United States and other industrialized countries have recentlybeen reported (7, 8, 11, 18, 20, 22, 31, 32,42). Hepatitis E generally affects young adults and usuallyis not fatal, although mortality rates of up to 20% have beenreported for pregnant women (28, 30). In industrialized countries,where hepatitis E was thought to be nonendemic, anti-HEV antibodieshave also been found in a significant proportion of healthy individuals(12, 16, 19, 21, 29, 33). Diagnosis of HEV infectionis based on detection of the virus by reverse transcriptase PCR(RT-PCR) and/or detection of anti-HEV antibodies by serology.HEV was recently declassified from the Caliciviridae family andremains unclassified (14, 17, 27).

In 1997, a novel virus closely related to human HEV was discovered in pigs, characterized, and designated swine HEV (23).Subsequently, two strains of human HEV (US-1 and US-2) isolatedfrom U.S. patients with acute hepatitis were characterized (7,8, 31). The two U.S. strains of HEV share $>=$ 97% amino acididentity with swine HEV in open reading frames 1 and 2 (ORF1 andORF2, respectively) but are genetically distinct from other knownstrains of HEV worldwide. In Taiwan, Hsieh et al. (12) isolatedanother new strain of swine HEV from a pig. This Taiwanese strainof swine HEV shares 97.3% nucleotide sequence identity with ahuman strain of HEV isolated from a retired farmer in Taiwan butis distinct from the U.S. strain of swine HEV. More recently,Wang et al. (40) found that a Chinese strain (T1) of HEV recoveredfrom a patient in mainland China is related to the Taiwanese swineHEV and human HEV strains reported by Hsieh et al. (12) andthat they form a distinct genotype. Also in Taiwan, Wu et al.(41) identified yet another strain of swine HEV isolated fromTaiwanese pigs. This strain of swine HEV shares 84 to 95% nucleotidesequence identity with Taiwanese human strains of HEV (41) whichare related to the G9 and G20 Chinese strains of HEV (40).

The exact role of swine in the transmission of HEV among humans remains unclear. Serologic surveys done to date suggest thatswine HEV is widespread in the midwestern U.S. swine populationas well as in other regions of the world (5, 6, 12, 23,26, 34, 41). Recently, we experimentally infected pigs withswine HEV (24) or with the US-2 strain of human HEV (25).The limited scope of that study did not allow us to define thetemporal pathogenesis of infection of swine with these HEV strains,but clinical disease was not seen. In a reciprocal experiment,we experimentally infected nonhuman primates with the swine HEV(25) or the US-2 strain of human HEV (R. H. Purcell et al.,unpublished data). The HEV-infected primates developed mild hepatitisand slightly elevated liver enzymes. The present comparative pathogenesisstudy was designed to gain a better understanding of the pathogenesisof HEV infection in pigs and to evaluate the usefulness of swineas an animal model of hepatitisE.

	MATERIALS AND METHODS

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Virus inocula. The swine HEV used in this study was originally recovered from a pig in Illinois (23). An infectious pool of swine HEV wassubsequently prepared as a 10% suspension of feces collected froma specific-pathogen-free (SPF) pig experimentally infected withswine HEV. This infectious pool was titrated in SPF pigs and wasfound to have a titer of 10^4.5 50% pig infectious doses (PID₅₀) per ml (25). This standardinfectious pool of swine HEV was used as one inoculum in thisstudy. The US-2 strain of human HEV (kindly provided by Isa Mushahwar,Abbott Laboratories, North Chicago, Ill.) used in this study wasoriginally recovered from a hepatitis patient in Tennessee andtransmitted to cynomolgus monkeys (8, 31). An infectiouspool of the US-2 strain of human HEV was prepared as a 10% suspensionof feces collected from a rhesus monkey experimentally infectedwith the US-2 strain (Purcell et al., unpublished data). Thisinfectious pool was titrated in rhesus monkeys and was found tohave an infectious titer of 10⁵ 50% monkey infectious doses (MID₅₀) per 0.5 ml (Purcell et al.,unpublished data). This standard pool of the US-2 strain of humanHEV was diluted to an infectious titer of 10^4.5 MID₅₀/ml (equivalent to that of the swine-HEV inoculum) and usedas the other inoculum in thisstudy.

Animals. Fifty-four crossbred, 3- to 4-week-old, SPF pigs (Sus scrofa domestica) were randomly assigned to three groups. All animalswere confirmed to be negative for anti-HEV antibodies by an enzyme-linkedimmunosorbent assay (ELISA) (23, 26) prior to inoculation.Seventeen pigs in group 1 served as uninoculated controls. Eighteenpigs in group 2 were each intravenously (i.v.) inoculated with10^4.5 PID₅₀ of swine HEV. Nineteen pigs in group 3 were each i.v. inoculatedwith 10^4.5 MID₅₀ of the US-2 strain of human HEV. Groups 1 and 2 were housedin a BL-2 facility, and group 3 was housed in a BL-3 facility.All pigs were allowed access to food and drinking water adlibitum.

Clinical signs and serum chemistry profiles. Clinical signs and rectal temperature were recorded every 2 to 3 days through 55 days postinoculation (DPI). Blood was collectedprior to inoculation and weekly thereafter for serum liver chemistryprofiles (aspartate aminotransferase, gamma-glutamyl transferase,sorbital dehydrogenase, and bilirubin) on all pigs throughoutthe 55 days of the experiment. Feces and blood were also collectedfrom all pigs at 0, 3, and 7 DPI and weekly thereafter through55 DPI for detection of HEV RNA by RT-PCR and of anti-HEV immunoglobulinG (IgG) by ELISA. Fecal samples were collected directly from therectum with a Dacron fiber tipped swab and then suspended in phosphate-bufferedsaline buffer and stored at $-$ 80°C untiluse.

Evaluation of gross and microscopic lesions. Two to four randomly selected pigs from each group were necropsied at 3, 7, 14, 20, 27, or 55 DPI. Tissues examined grosslyand collected for microscopic examination included brain, tonsil,mandibular salivary gland, lung, heart, stomach, liver, gall bladder,pancreas, duodenum, jejunum, ileum, colon, kidney, adrenal gland,urinary bladder, and skeletal muscle. One section each of theright lateral lobe, right medial lobe, left medial lobe, quadratelobe, and caudate process of the liver was collected and processedfor histologic examination. Two sections of the left lateral lobewere collected and examined. Tissues for histologic examinationwere fixed in 10% neutral buffered formalin, routinely processed,sectioned at a thickness of 6 µm, and stained with hematoxylinandeosin.

Liver sections were blindly examined microscopically and assigned a score for severity of lymphoplasmacytic hepatic lesions.Scores ranged from 0 to 4, where 0 is no inflammation, 1 is 1to 2 focal lymphoplasmacytic infiltrates/10 hepatic lobules, 2is 2 to 5 focal infiltrates/10 hepatic lobules, 3 is 6 to 10 focalinfiltrates/10 hepatic lobules, and 4 is >10 focal infiltrates/10hepaticlobules.

Detection of HEV RNA by RT-PCR. RT-PCR was performed essentially as previously described (24, 25) to detect viral RNA in feces, serum, liver tissue, andbile samples. Total RNA was extracted from 100 µl of each sample(serum, 10% fecal suspension, 10% liver homogenate, or bile) withTriZol reagent (GIBCO/BRL, Gaithersburg, Md.). All samples weretested by a nested PCR with primers located in the putative capsidgene (ORF2) region (24, 25). The first-round PCR producedan expected fragment of 404 bp with the forward primer F1 (5'-AGCTCCTGTACCTGATGTTGACTC-3')and the reverse primer R1 (5'-CTACAGAGCGCCAGCCTTGATTGC-3'). Forthe second-round PCR, the forward primer F2 (5'-GCTCACGTCATCTGTCGCTGCTGG-3')and the reverse primer R2 (5'-GGGCTGAACCAAAATCCTGACATC-3') producedan expected fragment of 266 bp. These two sets of primers weredesigned to amplify both swine HEV and the US-2 strain of humanHEV (24, 25). Total RNA was reverse transcribed with the R1reverse primer and SuperScript II reverse transcriptase (GIBCO/BRL)at 42°C for 1 h. The resulting cDNA was amplified by PCR withAmpliTaq Gold DNA polymerase. The PCR was carried out for 39 cyclesof denaturation at 94°C for 1 min, annealing at 52°C for 1 min,and extension at 72°C for 1.5 min, followed by a final incubationat 72°C for 7 min. The second-round PCRs were performed with parameterssimilar to those described above with 10 µl of the first-roundPCR mixture as the template. The amplified PCR products were examinedby gelelectrophoresis.

Detection of anti-HEV antibodies. The standard ELISA for anti-HEV antibody in pigs was performed essentially as previously described (23, 24, 26). Weused a purified 55-kDa truncated recombinant capsid protein derivedfrom ORF2 of the human HEV strain Sar-55 as the antigen. Peroxidase-labeledgoat anti-swine IgG (Kirkegaard & Perry Laboratories, Gaithersburg,Md.) was used as the secondary antibody. All serum samples weretested in duplicate. Preimmune and hyperimmune (anti-HEV antibody-positive)swine sera were used as negative and positive controls,respectively.

Statistical analysis. The presence or absence of hepatic lesions was analyzed by Fisher's exact test. Lymphoplasmacytic hepatitis lesion scoreswere analyzed by logistic regression. The lesion score was thedependent variable and, for the analysis, was considered to bean ordinal variable. Explanatory variables included infectiongroup (nominal variable) and the DPI (ordinal variable). A P valueof less than 0.05 was considered significant in allanalyses.

	RESULTS

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Clinical evaluation. Evidence of clinical disease or elevation of liver enzymes or bilirubin was not found in pigs from any of the groups (datanotshown).

Gross and microscopic lesions. The only gross lesions observed were mildly to moderately enlarged hepatic and mesenteric lymph nodes from 7 to 55 DPI inthe groups inoculated with swine or human HEV. Data on microscopicliver lesions are summarized in Tables 1 to 2 and Figures 1to 4. Multifocal lymphoplasmacytic hepatitis was observed in 9of 17 control pigs, 15 of 18 swine-HEV-inoculated pigs, and 16of 19 human-HEV-inoculated pigs. The difference in the numbersof pigs with lymphoplasmacytic hepatitis was significant betweenthe control and human-HEV-inoculated group (P = 0.047) but notbetween the control and swine-HEV-inoculated group (P = 0.057).Compared to those in controls, lymphoplasmacytic hepatic lesionswere significantly more severe in pigs inoculated with human HEV(P = 0.005) or with swine HEV (P = 0.023) than in the controls.Although overall mean hepatitis scores were higher in the human-HEV-inoculatedgroup (1.7) than in the swine-HEV-inoculated group (1.2), thedifferences were not significant. Focal hepatocellular necrosiswas observed in 5 of 17, 10 of 18, and 13 of 19 of the pigs ingroups 1 to 3, respectively. Hepatocellular necrosis was significantly(P = 0.022) more frequent in the human-HEV-inoculated group thanin the controls. Although there were more pigs with hepatocellularnecrosis in the swine-HEV-inoculated group (10 of 18 pigs) thanin the control group (5 of 17 pigs), the differences were notsignificant (P = 0.111). In general, hepatic lesions were verymild in group 1 pigs (controls), mild to moderate in group 2 pigs(swine HEV), and moderate to severe in group 3 pigs (human HEV).Hepatic inflammation and hepatocellular necrosis peaked in severityat 20 DPI and were still moderately severe at 55 DPI in the groupinoculated with human HEV (data not shown). Hepatocellular swellingand vacuolation (Fig. 3) were observed in both HEV-inoculatedgroups from 7 to 27 DPI. Hepatic lesions were absent or nearlyresolved in the swine-HEV-inoculated pigs by 55 DPI. At each datapoint in time (3, 7, 14, 20, 27, and 55 DPI), the types and levelsof severity of liver lesions within each infected group were similarwhether the tissue sample was positive or negative for HEV nucleicacids by RT-PCR. For example, 3 of 3 pigs in the swine-HEV-inoculatedgroup necropsied at 14 DPI had mild lymphoplasmacytic hepatitis,mild vacuolar swelling of hepatocytes, and low numbers of necrotichepatocytes yet only 1 of 3 pigs was positive by RT-PCR for HEVin liver and 3 of 3 pigs were positive for HEV in bile. Lesionsin other tissues were unremarkable.

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TABLE 1. Hepatitis lesions in control and HEV-inoculated pigs

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TABLE 2. HEV RNA in the feces, serum, liver, and bile of control and HEV-inoculated pigs

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FIG. 1. Liver of a sham-inoculated control pig (14 DPI) with rare lymphoplasmacytic infiltrates in hepatic sinusoids. Hematoxylin and eosin staining was performed.

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FIG. 2. Liver of a pig i.v. inoculated with HEV recovered from a U.S. pig. There is mild focal infiltration of lymphocytes, plasma cells, and macrophages and mild diffuse inflammation in hepatic sinusoids at 14 DPI. Hepatocytes are mildly swollen and vacuolated. Hematoxylin and eosin staining was performed.

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FIG. 3. Liver of a pig i.v. inoculated with HEV recovered from a human hepatitis patient in the U.S. There is severe lymphoplasmacytic and histiocytic hepatitis and severe vacuolar degeneration and swelling of hepatocytes at 14 DPI. Hematoxylin and eosin staining was performed.

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FIG. 4. Liver of the same pig as that shown in Fig. 3. Note the individual necrotic hepatocytes (arrow). Hematoxylin and eosin staining was performed.

Detection of HEV RNA. Results of RT-PCR examination of feces, serum, bile, and liver specimens are summarized in Table 2. All pigs were negativefor HEV RNA at 0 DPI, and control pigs remained negative throughoutthe experiment. HEV RNA was detected in the bile, liver, serum,and feces specimens of both swine-HEV- and human-HEV-inoculatedpigs but not in those of control pigs (Table 2). HEV nucleicacids were detected by RT-PCR in the feces at 7 DPI in 100% (31of 31 pigs) of the pigs inoculated with HEV (swine or human HEV).HEV RNA was detected in the bile of 100% (18 of 18 pigs) of theHEV-inoculated pigs (swine and human HEV) necropsied between 3and 14 DPI. Similarly, HEV was detected in the livers of 100%(9 of 9 pigs) of the pigs inoculated with human HEV and necropsiedbetween 3 and 14 DPI. Detection of HEV by RT-PCR in the liversof the swine-HEV-inoculated pigs was less successful. Swine HEVwas detected in 67% (6 of 9) of the livers from the swine-HEV-inoculatedpigs that were necropsied between 3 and 14 DPI; however, 100%of these pigs were positive for HEV nucleic acids in bile andfeces. PCR products amplified from a selected bile sample of aswine-HEV-inoculated pig and from a selected bile sample froma human-HEV-inoculated pig were sequenced. Sequence analysis confirmedthat the virus recovered from the inoculated pigs was the samevirus as the virus in theinocula.

Serology. All pigs were negative for anti-HEV antibodies prior to inoculation, and control pigs remained negative throughout the study.All pigs remained negative through 7 DPI. Anti-HEV antibody wasdetected in the sera of 1 of 14 pigs at 14 DPI, 5 of 11 pigs at20 DPI, 5 of 8 pigs at 27 DPI, 4 of 5 pigs at 42 DPI, and 5 of5 pigs at 55 DPI in the swine-HEV-inoculated group. Anti-HEV antibodywas detected in the sera of 3 of 15 pigs at 14 DPI, 12 of 12 pigsat 20 DPI, 9 of 9 pigs at 27 DPI, 6 of 6 pigs at 42 DPI, and 6of 6 pigs at 55 DPI in the human-HEV-inoculatedgroup.

	DISCUSSION

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HEV infection in pigs appears to be widespread throughout the world. Antibodies to HEV are present in pigs in many industrializedcountries, including the United States (23), Canada (26),Korea (26), Taiwan (12, 40), and Australia (5), and inpigs from countries where HEV is endemic such as Nepal (6),China (26), and Thailand (26). The high degree of geneticsimilarity between swine and human strains of HEV identified inthe same geographic regions suggests that cross-species transmissionmay occur (8, 12, 25, 31, 41). Balayan et al. reportedthat Russian domestic swine could be experimentally infected witha central Asian strain of HEV isolated from a naturally infectedpatient (3). In that study, the infected swine developed jaundice(3). In the present study, we confirmed that SPF pigs are readilysusceptible to infection with two strains of HEV recovered froma human and a pig, respectively. The US-2 strain of human HEVis known to be pathogenic in humans (7, 8, 31). However,in our study, experimental infection of pigs with either the U.S.human or U.S. swine strain of HEV failed to induce clinical diseasein naïve growing pigs. Both strains of HEV replicated in growingpigs since the inoculated pigs seroconverted to anti-HEV antibodyand HEV RNA was detected in the feces, bile, sera, and liver tissuesof inoculated pigs. Therefore, pigs should be considered a reservoirfor HEV and exposure to feces from infected pigs represents arisk for transmission of HEV to other pigs and possibly to otherspecies, includinghumans.

In some control pigs, lymphoplasmacytic inflammation and rare focal necrotic hepatocytes were observed. Lesions characteristicof porcine circovirus infection (lymphoid depletion and granulomatousinflammation) were lacking in the lymphoid tissues and other organs.Porcine circovirus antigen was not detected by immunohistochemistryin liver sections of any of the control or HEV-inoculated pigs(data not shown). All control and HEV-inoculated pigs remainedseronegative for porcine reproductive and respiratory syndromevirus and pseudorabies virus throughout the study (data not shown).The liver sections were blindly examined by a pathologist (P.G. Halbur) in the Iowa State University Veterinary DiagnosticLaboratory. Each year, thousands of pig livers from cases submittedfor diagnosis of a variety of diseases (respiratory, enteric,central nervous system, etc.) are examined by pathologists atthe Iowa State University Veterinary Diagnostic Laboratory. Basedon this experience, mild lymphoplasmacytic infiltrates in hepaticsinusoids and the presence of rare necrotic or apoptotic hepatocytesare considered normal background changes for pig livers. The amountof inflammation and the number of necrotic hepatocytes in theHEV-inoculated pigs, especially those inoculated with human HEV,were above the normal threshold and considered to be evidenceof mild viral hepatitis. Evaluation of microscopic lesions suggestedthat the US-2 strain of human HEV induced more severe and persistenthepatic lesions in pigs than did the swineHEV.

Overall, the liver lesions observed in the HEV-infected pigs were relatively mild. The exact sites of HEV replication arenot known, but it is possible that HEV might replicate in tissuesand organs other than the liver. Studies are under way to identifyhepatic and possible extrahepatic sites of HEV replication byusing immunohistochemistry, negative-strand RT-PCR, and in situhybridization. The inoculation route used in this study was intravenous.However, fecal-oral exposure is thought to be the primary routeof natural infection (28, 30). The infectious dose necessaryfor infection by the oral route is believed to be higher thanthat for infection by the intravenous route, based on a studyof human HEV in nonhuman primates (35). The infectious titersof the standard swine and human HEV pools available may not behigh enough to infect animals by the oral route. Nevertheless,additional research needs to be done to establish the oral routeas the natural route of exposure and to study the pathogenesisof HEV infection in pigs following naturalinfection.

Since anti-HEV antibody is also detected in individuals from large U.S. cities (19, 33), where contact with pigs is uncommon,other sources or reservoirs of HEV are suspected. Recently, Karetnyiet al. (16) found that the anti-HEV antibody prevalence in Iowapatients with non-A, non-B, and non-C hepatitis (4.9%) and infield workers from the Iowa Department of Natural Resources (5.7%)was significantly higher than that in normal blood donors (2%;P < 0.05). This suggests that human populations with occupationalexposure to wild animals may have increased risks of HEV infection.Anti-HEV antibody has been detected in many animal species, includingmonkeys, pigs, rodents, chickens, dogs, cows, sheep, and goats(6, 9, 12, 15, 21, 26, 34, 36, 37). In theUnited States, Kabrane-Lazizi et al. (15) found that about 44to 90% of wild-caught rats from three U.S. states (Maryland, Hawaii,and Louisiana) were positive for anti-HEV antibody. Similarly,Favorov et al. (9) reported the detection of anti-HEV antibodyamong rodents trapped at multiple sites in the United States.The significance of HEV seropositivity in these animal speciesneeds to be determined. The recent identification of numerousgenetically distinct strains of HEV in several countries wherehepatitis E is endemic (4, 13, 38, 39, 40) and nonendemic(8, 11, 12, 31, 32, 41, 42) has led to a hypothesisthat these novel strains of human HEV may be of animal origin(22). The present study confirmed that one human-HEV strain(US-2 strain) was transmissible to pigs (25), although the clinicalmanifestations and course of disease were different from thoseobserved in the single human reported to be infected with thisstrain (8, 18, 31).

There is increasing public health concern over the risk of inadvertent transmission of swine HEV from pig organs to humanrecipients during xenotransplantation (21). The data presentedhere indicated that pigs infected with HEV had microscopic evidenceof liver damage. Therefore, pig livers or cells from the liversof HEV-infected pigs used in xenotransplantation may representa risk for transmission of HEV from pigs to human xenograft recipients.Adequate screening of xenograft donor pigs for HEV infection istherefore recommended for xenotransplantation with pigorgans.

In summary, the results from this study confirm that feces from HEV-infected pigs contain viable HEV, so swine feces may representa risk for transmission of HEV. Our results suggest that swinemay not be a perfect animal model for human HEV since there isa lack of clinical disease in infected pigs, at least with thestrains of HEV we studied. However, the swine model will likelybe useful to better understand some aspects of HEV pathogenesisand epidemiology. HEV should be considered along with porcinereproductive and respiratory syndrome virus, circovirus, and pseudorabiesvirus in the differential diagnosis of viral hepatitis inpigs.

	ACKNOWLEDGMENTS

This study was supported by grants (to P.G.H.) from the National Pork Producers Council and the Iowa Livestock Health AdvisoryCouncil and by grants (to X.J.M.) from the National Institutesof Health (AI01653-01 and AI46505-01).

We thank Isa Mushahwar (Abbott Laboratories) for generously providing us with the US-2 strain of human HEV. We thank DorisWong and Ron Engle for technical assistance with serological testing,Ryan Royer and Jeremy Bruna for animal care, and Prem Paul fortechnical advice and use of laboratory equipment. We also thankBrad Thacker for statistical analysis, G. Haqshenas for reviewof the manuscript, and Carles Rosell for review and consultationon liverhistopathology.

	FOOTNOTES

^* Corresponding author. Mailing address: Department of Veterinary Diagnostic and Production Animal Medicine, College of VeterinaryMedicine, Iowa State University, Ames, IA 50011. Phone: (515)294-1950. Fax: (515) 294-6961. E-mail: pghalbur{at}iastate.edu.

REFERENCES

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Abstract
Introduction
Materials and Methods
Results
Discussion
References

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13. Huang, R., N. Nakazono, K. Ishii, O. Kawamata, R. Kawaguchi, and Y. Tsukada. 1995. Existing variations on the gene structure of hepatitis E virus strains from some regions of China. J. Med. Virol. 47:303-308[Medline].

14. Kabrane-Lazizi, Y., X. J. Meng, R. H. Purcell, and S. U. Emerson. 1999. Evidence that the genomic RNA of hepatitis E virus is capped. J. Virol. 73:8848-8850[Abstract/Free Full Text].

15. Kabrane-Lazizi, Y., J. B. Fine, J. Elm, G. E. Glass, H. Higa, A. Diwan, C. J. Gibbs, Jr., X. J. Meng, S. U. Emerson, and R. H. Purcell. 1999. Evidence for wide-spread infection of wild rats with hepatitis E virus in the United States. Am. J. Trop. Med. Hyg. 61:331-335[Abstract].

16. Karetnyi, Y. V., M. J. Gilchrist, and S. J. Naides. 1999. Hepatitis E virus infection prevalence among selected populations in Iowa. J. Clin. Virol. 14:51-55[CrossRef][Medline].

17. Koonin, E. V., A. E. Gorbalenya, M. A. Purdy, M. N. Rozanov, G. R. Reyes, and D. W. Bradley. 1992. Computer-assisted assignment of functional domains in the nonstructural polyprotein of hepatitis E virus: delineation of an additional group of positive-strand RNA plant and animal viruses. Proc. Natl. Acad. Sci. USA 89:8259-8263[Abstract/Free Full Text].

18. Kwo, P. Y., G. G. Schlauder, H. A. Carpenter, P. J. Murphy, J. E. Rosenblatt, G. J. Dawson, E. E. Mast, 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].

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

20. McCrudden, R., S. O'Connell, T. Farrant, S. Beaton, J. P. Iredale, and D. Fine. 2000. Sporadic acute hepatitis E in the United Kingdom: an underdiagnosed phenomenon? Gut 46:732-733[Abstract/Free Full Text].

21. Meng, X. J. 2000. Zoonotic and xenozoonotic risks of hepatitis E virus. Infect. Dis. Rev. 2:35-41.

22. Meng, X. J. 2000. Novel strains of hepatitis E virus identified from humans and other animal species: is hepatitis E a zoonosis? J. Hepatol. 33:842-845[CrossRef][Medline].

23. 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 is closely related to the human hepatitis E virus. Proc. Natl. Acad. Sci. USA 94:9860-9865[Abstract/Free Full Text].

24. Meng, X. J., P. G. Halbur, J. S. Haynes, T. S. Tsareva, J. D. Bruna, R. 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[CrossRef][Medline].

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

26. Meng, X. J., S. Dea, R. E. Engle, R. Friendship, Y. S. Lyoo, T. Sirinarumitr, K. Urairong, D. Wang, D. Wong, D. Yoo, Y. Zhang, R. H. Purcell, and S. U. Emerson. 1999. Prevalence of antibodies to the hepatitis E virus in pigs from countries where hepatitis E is common or is rare in the human population. J. Med. Virol. 58:297-302.

27. Pringle, C. 1998. Minutes of the 27th International Committee on Taxonomy of Viruses Meeting. Arch. Virol. 143:1449-1459[CrossRef][Medline].

28. Purcell, R. H. 1996. Hepatitis E virus, p. 2831-2843. In B. N. Fields, D. M. Knipe, P. M. Howley, et al. (ed.), Fields virology, 3rd ed., vol. 2. Lippincott-Raven Publishers, Philadelphia, Pa.

29. 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[CrossRef][Medline].

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

31. 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].

32. 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[CrossRef][Medline].

33. 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].

34. Tien, N. T., H. T. Clayson, H. B. Khiem, P. K. Sac, A. L. Corwin, K. S. Myint, and D. W. Vaughn. 1997. Detection of immunoglobulin G to the hepatitis E virus among several animal species in Vietnam. Am. J. Trop. Med. Hyg. 57:211.

35. Tsarev, S. A., T. S. Tsareva, S. U. Emerson, P. O. Yarbough, L. J. Legters, T. Moskal, and R. H. Purcell. 1994. Infectivity titration of a prototype strain of hepatitis E virus in cynomolgus monkeys. J. Med. Virol. 43:135-142[Medline].

36. Tsarev, S. A., T. S. Tsareva, S. U. Emerson, M. K. Rippy, P. Zack, M. Shapiro, and R. H. Purcell. 1995. Experimental hepatitis E in pregnant rhesus monkeys: failure to transmit hepatitis E virus (HEV) to offspring and evidence of naturally acquired antibodies to HEV. J. Infect. Dis. 172:31-37[Medline].

37. Tsarev, S. A., M. P. Shrestha, J. He, R. M. Scott, D. W. Vaughn, E. T. Clayson, S. Gigliotti, C. F. Longer, and B. L. Innis. 1998. Naturally acquired hepatitis E virus (HEV) infection in Nepalese rodents. Am. J. Trop. Med. Hyg. 59:242.

38. Van Cuyck-Gandre, H., H. Y. Zhang, S. A. Tsarev, R. L. Warren, J. D. Caudill, N. J. Snellings, L. Begot, B. L. Innis, and C. F. Longer. 2000. Short report: phylogenetically distinct hepatitis E viruses in Pakistan. Am. J. Trop. Med. Hyg. 62:187-189[Abstract].

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

40. Wang, Y., H. Zhang, R. Ling, H. Li, and T. J. Harrison. 2000. The complete sequence of hepatitis E virus genotype 4 reveals an alternative strategy for translation of open reading frames 2 and 3. J. Gen. Virol. 81:1675-1686[Abstract/Free Full Text].

41. Wu, J. C., C. M. Chen, T. Y. Chiang, I. J. Sheen, J. Y. Chen, W. H. Tsai, Y. H. Huang, and S. D. Lee. 2000. Clinical and epidemiological implications of swine hepatitis E virus infection. J. Med. Virol. 60:166-171[CrossRef][Medline].

42. 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[CrossRef][Medline].

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Antimicrob. Agents Chemother.	Clin. Microbiol. Rev.

Clin. Vaccine Immunol.	ALL ASM JOURNALS

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13.	Huang, R., N. Nakazono, K. Ishii, O. Kawamata, R. Kawaguchi, and Y. Tsukada. 1995. Existing variations on the gene structure of hepatitis E virus strains from some regions of China. J. Med. Virol. 47:303-308[Medline].
14.	Kabrane-Lazizi, Y., X. J. Meng, R. H. Purcell, and S. U. Emerson. 1999. Evidence that the genomic RNA of hepatitis E virus is capped. J. Virol. 73:8848-8850[Abstract/Free Full Text].
15.	Kabrane-Lazizi, Y., J. B. Fine, J. Elm, G. E. Glass, H. Higa, A. Diwan, C. J. Gibbs, Jr., X. J. Meng, S. U. Emerson, and R. H. Purcell. 1999. Evidence for wide-spread infection of wild rats with hepatitis E virus in the United States. Am. J. Trop. Med. Hyg. 61:331-335[Abstract].
16.	Karetnyi, Y. V., M. J. Gilchrist, and S. J. Naides. 1999. Hepatitis E virus infection prevalence among selected populations in Iowa. J. Clin. Virol. 14:51-55[CrossRef][Medline].
17.	Koonin, E. V., A. E. Gorbalenya, M. A. Purdy, M. N. Rozanov, G. R. Reyes, and D. W. Bradley. 1992. Computer-assisted assignment of functional domains in the nonstructural polyprotein of hepatitis E virus: delineation of an additional group of positive-strand RNA plant and animal viruses. Proc. Natl. Acad. Sci. USA 89:8259-8263[Abstract/Free Full Text].
18.	Kwo, P. Y., G. G. Schlauder, H. A. Carpenter, P. J. Murphy, J. E. Rosenblatt, G. J. Dawson, E. E. Mast, 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].
19.	Mast, E. E., I. K. Kuramoto, M. O. Favorov, V. R. Schoening, B. T. Burkholder, C. N. Shapiro, and P. V. Holland. 1997. Prevalence of and risk factors for antibody to hepatitis E virus seroreactivity among blood donors in Northern California. J. Infect. Dis. 176:34-40[Medline].
20.	McCrudden, R., S. O'Connell, T. Farrant, S. Beaton, J. P. Iredale, and D. Fine. 2000. Sporadic acute hepatitis E in the United Kingdom: an underdiagnosed phenomenon? Gut 46:732-733[Abstract/Free Full Text].
21.	Meng, X. J. 2000. Zoonotic and xenozoonotic risks of hepatitis E virus. Infect. Dis. Rev. 2:35-41.
22.	Meng, X. J. 2000. Novel strains of hepatitis E virus identified from humans and other animal species: is hepatitis E a zoonosis? J. Hepatol. 33:842-845[CrossRef][Medline].
23.	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 is closely related to the human hepatitis E virus. Proc. Natl. Acad. Sci. USA 94:9860-9865[Abstract/Free Full Text].
24.	Meng, X. J., P. G. Halbur, J. S. Haynes, T. S. Tsareva, J. D. Bruna, R. 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[CrossRef][Medline].
25.	Meng, X. J., P. G. Halbur, M. S. Shapiro, S. Govindarajan, J. D. Bruna, I. K. Mushahwar, R. H. Purcell, and S. U. Emerson. 1998. Genetic and experimental evidence for cross-species infection by the swine hepatitis E virus. J. Virol. 72:9714-9721[Abstract/Free Full Text].
26.	Meng, X. J., S. Dea, R. E. Engle, R. Friendship, Y. S. Lyoo, T. Sirinarumitr, K. Urairong, D. Wang, D. Wong, D. Yoo, Y. Zhang, R. H. Purcell, and S. U. Emerson. 1999. Prevalence of antibodies to the hepatitis E virus in pigs from countries where hepatitis E is common or is rare in the human population. J. Med. Virol. 58:297-302.
27.	Pringle, C. 1998. Minutes of the 27th International Committee on Taxonomy of Viruses Meeting. Arch. Virol. 143:1449-1459[CrossRef][Medline].
28.	Purcell, R. H. 1996. Hepatitis E virus, p. 2831-2843. In B. N. Fields, D. M. Knipe, P. M. Howley, et al. (ed.), Fields virology, 3rd ed., vol. 2. Lippincott-Raven Publishers, Philadelphia, Pa.
29.	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[CrossRef][Medline].
30.	Reyes, G. R. 1997. Overview of the epidemiology and biology of the hepatitis E virus, p. 239-258. In R. A. Willson (ed.), Viral hepatitis. Marcel Dekker, Inc, New York, N.Y.
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