Avian influenza virus (H5N1) replication in feathers of domestic waterfowl.We examined feathers of domestic ducks and geese inoculated with 2 different avian influenza virus (H5N1) genotypes. Together with virus isolation from the skin, the detection of viral antigens and ultrastructural observation of the virions in the feather epidermis raise the possibility of feathers as sources of infection. ********** Since 1997, an epidemic of avian influenza (AI) virus subtype H5N1 has spread in Asia, causing fatal infections in poultry, wild birds, mammals, and humans (1). Wild waterfowl, including ducks and geese, are natural hosts of AI virus of all 16 hemagglutinin subtypes in nature (2,3). Generally, AI virus is transmitted by the fecal-oral route without causing clinical signs (2-4). Although current AI virus (H5N1) strains have mild to severe pathogenicity in waterfowl (5-7), these birds can still be carriers of the virus (7). Even asymptomatic domestic ducks can shed the virus from the cloaca and oral cavity (7,8) and contribute to viral maintenance and spread (9,10). Therefore, focusing on the epidemiologic role of domestic waterfowl in AI (H5N 1) outbreaks is important. We previously reported that the Japanese AI virus (H5N1) isolated in 2004 causes necrosis of the feather epidermis with viral antigens in domestic ducks, a finding that demonstrates the possibility of viral release from feathers (11). In addition, these affected feathers can cause infection in orally inoculated domestic ducks (12). Except for our previous studies, to our knowledge this feather lesion has not been reported in AI (H5N1)-infected waterfowl. However, if the feather lesion is common to other waterfowl species and AI (H5N 1), affected feathers might involve the spread of the virus. We describe the pathologic, virologic and ultrastructual findings of the feather in domestic waterfowl infected with AI (H5N1). The Study Two species of domestic waterfowl, ducks (n = 4) and geese (n = 4), were used. Domestic ducks (Anasplaty rhynchos var. domestica) called Aigamo in Japanese are a crossbreed of wild mallard and domestic ducks; they are free-ranging ducks in water-soaked rice paddy fields and are used for weed control and meat production. Domestic geese (Anser cygnoides var. domestica) are reared for food production on farms. We selected geese because wild geese (A. indicus) accounted for a large proportion of the deaths in AI (H5N1) outbreaks at Qinghai Lake in People's Republic of China in 2005 (5). These 2 species of birds were obtained from the farm at 1 day of age and raised with commercial food in an isolated facility. Birds were moved into negative-pressure isolators of Biosafety Level 3-approved laboratories (National Institute of Animal Health, Tsukuba, Japan) for acclimation 1 week before inoculation. Two different AI virus (H5N1) genotypes were used. A/chicken/Yamaguchi/7/2004 (Ck/Yama/7/04) is classified as genotype V (13). A/chicken/Miyazaki/K11/2007 (Ck/ Miya/K11/07) belongs to genotype Z and H5 clade 2 subclade 2 (M. Mase, unpub, data), which is now circulating from China to Japan, Europe, and Africa (5,14). The stored virus was propagated for 36-48 hours in the allantoic cavity of 10-day-old embryonated chicken eggs at 37[degrees]C. The infectious allantoic fluid was harvested and stored at -80[degrees]C until use. All experimental procedures were approved by the Ethics Committee of the National Institute of Animal Health in Japan. For each species, two 4-week-old birds were inoculated intranasally with 0.1 mL of the inoculum containing 108 50% egg infectious dose ([EID.sub.50) per mL of each AI virus (H5N 1) genotype. Each inoculated group was kept in a separate isolator. Inoculated birds were euthanized with an overdose injection of sodium pentobarbital (i.v.) on days 3 and 5 postinoculation. For histopathology, the skin, including numerous feathers, was removed from the head, neck, back, shoulder, abdomen, thigh, and tail. Samples were fixed in 10% neutral-buffered formalin, embedded in paraffin, sectioned at 4 gm, and stained with hematoxylin and eosin. Immunohistochemistry was performed to detect the viral antigen with a Histofine Simple Stain PO (M) kit (Nichirei Inc., Tokyo, Japan). A mouse monoclonal antibody specific for the influenza A matrix protein (diluted 1:500; clone GA2B, AbD Serotec, Kidlington, UK) was used as the primary antibody (11). For the virus isolation, clean dry skin was collected from the neck and stored at -80[degrees]C (11). The viral titer of the samples was determined with 10-day-old embryonated chicken eggs and expressed as [EID.sub.50]/g as previously described (13). The viral titer <102 [EID.sub.50]/g was considered negative for virus isolation. For the electron microscopic examination, flesh contour feathers were fixed in 3% glutaraldehyde in 0.1 M phosphate buffer, postfixed in 1% osmium tetroxide, and embedded in epoxy resin. Ultrathin sections were stained with uranyl acetate and lead citrate and examined under a Hitachi H-7500 transmission electron microscope (Hitachi Corp., Tokyo, Japan). Inoculated birds did not exhibit apparent clinical signs, except for unilateral corneal opacity in a goose inoculated with Ck/Yama/7/04 on day 5 postinoculation. Results of histopathologic and virologic examinations are summarized in the Table. Histologically, viral antigens were occasionally detected in the feather epidermal cells with or without epidermal necrosis (Figure 1, panels A and B). Some affected feathers were accompanied by heterophilic and lymphocytic infiltration in the inner feather pulp. Other tissues in the skin were negative for influenza virus by immunohistochemical analysis with the exception of very rare positive reaction in stromal cells in the feather pulp. Virus isolation from the skin was positive in 1 duck and 1 goose inoculated with Ck/Yama/7/04; the viral titers were [10.sup.3.5] and [10.sup.4.5] [EID.sup.50]/g, respectively. All ducks and geese inoculated with Ck/Miya/K11/07 tested positive for the isolation; the viral titers were [10.sup.2.5]-[10.sup.4.5] [EID.sup.50]/g. Ultrastructurally, round, enveloped virions 80 to 100 nm in diameter were observed between feather epidermal cells in both domestic ducks and geese (Figure 2, panels A and B). Spherical virions budding from cell surface were occasionally observed (Figure 2, panel C). Conclusions We found that 2 different AI virus (H5N 1) genotypes that were isolated in 2004 and 2007 can replicate in the feather epidermal cells of domestic ducks and geese. To our knowledge, this is the first report of in vivo ultrastructural observation of AI (H5N 1) replication in waterfowl. The important finding is that the histologic feather finding and virus isolation from the skin were found in inoculated birds that did not exhibit apparent clinical signs. Although 1 goose inoculated with Ck/Yama/7/04 was negative for all examinations, this might have resulted from individual differences in susceptibility or the limited area of the skin used for the examination. Nevertheless, our data indicate that recent AI (H5N 1) strains are likely to replicate in feather epidermal cells of domestic ducks and geese. All birds inoculated with Ck/Miya/K11/07, which belongs to the current lineage spreading to Europe and Africa, tested positive for virus isolation, compared with the results with Ck/Yama/7/04. Feathers can easily drop off, blow away, or be reduced to dust, suggesting that affected feathers of waterfowl infected with influenza (HSN 1) virus can be potential sources of infection, along with their feces and respiratory secretions (7,8). At this time, it is unclear to what extent affected feathers contribute to the epidemiology of AI (H5N1) field outbreaks. However, more attention needs to be paid to persons who handle domestic waterfowl possibly infected with AI virus (H5N1). [FIGURE 1 OMITTED] [FIGURE 2 OMITTED] Acknowledgments We are grateful to Masaru Kobayashi and Megumi Shimada for their technical assistance. This study was supported by a grant-in-aid for scientific research from the Zoonoses Control Project of the Ministry of Agriculture, Forestry and Fisheries of Japan. Dr Yamamoto is a veterinary pathologist at the National Institute of Animal Health in Japan. His research interests are the pathogenesis and diagnosis of animal diseases. References (1.) Webster RG, Peiris M, Chen H, Guan Y. H5N 1 outbreaks and enzootic influenza. Emerg Infect Dis. 2006; 12:3-8. (2.) Olsen B, Munster V J, Wallensten A, Waldenstrom J, Osterhaus AD, Fouchier RA. Global patterns of influenza A virus in wild birds. Science. 2006;312:384-8. (3.) Webster RG, Bean WJ, Gorman OT, Chambers TM, Kawaoka Y. Evolution and ecology of influenza A viruses. Microbiol Rev. 1992;56:152 79. (4.) Webster RG, Yakhno M, Hinshaw VS, Bean WJ, Murti KG. Intestinal Influenza: replication and characterization of influenza viruses in ducks. Virology. 1978;84:268-78. (5.) Chen H, Smith GJD, Zhang SY, Qin K, Wang J, Li KS, et al. Avian flu: H5N1 virus outbreak in migratory waterfowl. Nature. 2005;436:191-2. (6.) Ellis TM, Bousfield RB, Bissett LA, Dyrting KC, Luk GSM, Tsim ST, et al. Investigation of outbreaks of highly pathogenic H5N 1 avian influenza in waterfowl and wild birds in Hong Kong in late 2002. Avian Pathol. 2004;33:492-505. (7.) Sturm-Ramirez KM, Hulse-post D J, Govorkova EA, Humbred J, Seiler P, Puthavathana P, et al. Are ducks contributing to the endemicity of highly pathogenic H5N1 influenza virus in Asia? J Virol. 2005;79:11269 79. (8.) Hulse-post D J, Sturm-Ramirez KM, Humbred J, Seiler P, Govorkova EA, Krauss S, et al. Role of domestic ducks in the propagation and biological evolution of highly pathogenic H5N1 influenza virus in Asia. Proc Natl Acad Sci U S A. 2005; 102:10682 7. (9.) Gilbert M, Chaitaweesub P, Parakamawongsa T, Premashthira S, Tiensin T, Kalpravidh W, et al. Free-grazing ducks and highly pathogenic avian influenza, Thailand. Emerg Infect Dis. 2006;12:227-34. (10.) Martin V, Sims L, Lubroth J, Pfeiffer D, Slingenbergh J, Domenech J. Epidemiology and ecology of highly pathogenic avian influenza with particular emphasis on South East Asia. Dev Biol (Basel). 2006; 124:23-36. (11.) Yamamoto Y, Nakamura K, Kitagawa K, Ikenaga N, Yamada M, Mase M, et al. Severe non-purulent encephalitis with mortality and feather lesions in call ducks (Anas platyrhyncha var. domestica) inoculated intravenously with H5N1 highly pathogenic avian influenza virus. Avian Dis. 2007;51:52 7. (12.) Yamamoto Y, Nakamura K, Kitagawa K, Ikenaga N, Yamada M, Mase M, et al. The pathogenesis in call ducks inoculated intranasally with H5N 1 highly pathogenic avian influenza virus and transmission by oral inoculation of infective feathers from an infected call duck. Avian Dis. 2007;51:744-9. (13.) Mase M, Tsukamoto K, Imada T, Imai K, Tanimura N, Nakamura K, et al. Characterization of H5N1 influenza A viruses isolated during the 2003-2004 influenza outbreaks in Japan. Virology. 2005;332:167-76. (14.) Bragstad K, Jorgensen PH, Handberg K, Hammer AS, Kabell S, Fomsgaard A. First introduction of highly pathogenic H5N1 avian influenza A viruses in wild and domestic birds in Denmark, Northern Europe. Virol J. 2007;4:43. Yu Yamamoto, * Kikuyasu Nakamura, * Masatoshi Okamatsu, * Manabu Yamada, * and Masaji Mase * * National Institute of Anirnal Health, Tsukuba, Ibaraki, Japan Address for correspondence: Yu Yamamoto, National Institute of Animal Health, 3-1-5 Kannondai, Tsukuba, lbaraki, 305-0856 Japan; email: yyu@ affrc.go.jp All material published in Emerging Infectious Diseases is in the public domain and may be used and reprinted without special permission; proper citation, however, is required.
Table. Histopathology of feathers and virus isolation from the skin in
domestic ducks and geese inoculated with 2 different avian influenza
virus (H5N1) genotypes *
A/chicken/Yamaguchi/7/2004
PID Duck Goose
3 +/+ ([dagger]) (3.5) ([double dagger]) -/- (-)
5 +/+ (-) +/+ (4.5)
A/chicken/Miyazaki/K11 /2007
PID Duck Goose
3 +/+( 4.5) +/+ (4.4)
5 -/+ (3.8) +/+ (2.5)
* PID, postinoculation day.
([dagger]) Epidermal necrosis of feathers/detected viral antigens; +,
positive; -, negative.
([double dagger]) Viral titer of the skin expressed as [log.sub.10] 50%
infectious dose ([EID.sub.50])/g; -, negative (<[10.sup.2]
[EID.sub.50]/g).
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