O'nyong-nyong virus, Chad.We report the first laboratory-confirmed human infection with O'nyong-nyong virus in Chad. This virus was isolated from peripheral blood mononuclear cells of a patient with evidence of a seroconversion to a virus related to Chikungunya
********** On November 2, 2004, a febrile 19-year-old French soldier staying in Chad and returning from a mission in Sarh, in the southern part of the country, was admitted to the hospital. Clinical examination showed a high body temperature (38[degrees]C), rash, periocular erythema erythema (ĕr'əthē`mə), more or less diffuse redness of the skin due to concentration of an abnormally large amount of blood within the small vessels of the skin (hyperemia), as in burns. , and pharyngitis pharyngitis Inflammation and infection (usually bacterial or viral) of the pharynx. Symptoms include pain (sore throat, worse on swallowing), redness, swollen lymph nodes, and fever. . Abdominal, cardiopulmonary, and neurologic functions were normal. Except for body temperature, biochemical and hematologic hematological, hematologic pertaining to or emanating from blood cells. hematological tests total and differential white cell counts, hematocrit estimation, erythrocyte count. values were normal. Serologic results were negative for Rickettsia rickettsia (rĭkĕt`sēə), any of a group of very small microorganisms, many disease-causing, that live in vertebrates and are transmitted by bloodsucking parasitic arthropods such as fleas, lice (see louse), and ticks. typhi, R. conorii, Legionella pneumophila, Bordetella pertussis, HIV HIV (Human Immunodeficiency Virus), either of two closely related retroviruses that invade T-helper lymphocytes and are responsible for AIDS. There are two types of HIV: HIV-1 and HIV-2. HIV-1 is responsible for the vast majority of AIDS in the United States. , and human herpesviruses Herpesviruses A family of viruses responsible for cold sores, chicken pox, and genital herpes. Mentioned in: Skin Resurfacing 1 and 2. Results of malaria testing were also negative. The patient received intravenous acetaminophen for 2 days, according to the protocol used by the French Armed Forces Medical Service in the event of fever occurring overseas. He recovered after 5 days without sequelae sequelae Clinical medicine The consequences of a particular condition or therapeutic intervention . Serum samples, collected during the acute phase (November 3-5, 2004) and after (November 23 and December 7, 2004; January 10 and February 1, 2005) were transported to our laboratory and tested by ELISA ELISA (e-li´sah) Enzyme-Linked Immuno-Sorbent Assay; any enzyme immunoassay using an enzyme-labeled immunoreactant and an immunosorbent. ELISA n. for immunoglobulin M (IgM) and IgG antibodies to a battery of arboviruses arboviruses (ar´bōvī´r  sz),n. by IgM-antibody capture (MAC-ELISA) and antigen-capture ELISA, respectively (1). Each serum sample was considered positive if the optical density (OD) ratio, OD (viral antigen)/OD (uninfected cells), was >3. The first sample (November 3, 2004) contained no antibodies (OD ratio <2) to dengue viruses, West Nile virus West Nile virus, microorganism and the infection resulting from it, which typically produces no symptoms or a flulike condition. The virus is a flavivirus and is related to a number of viruses that cause encephalitis. , Wesselsbron virus, Rift Valley fever Rift Valley fever An arthropod-borne (primarily mosquito), acute, febrile, viral disease of humans and numerous species of animals. Rift Valley fever is caused by a ribonucleic acid (RNA) virus in the genus Phlebovirus of the family Bunyaviridae. virus, Bunyamwera virus, or Chikungunya virus (CHIKV). Remaining samples contained antibodies to a virus serologically related to CHIKV (OD ratios >3) for both IgM (sample 2 and following samples) and IgG (sample 3 and those following). Antibody titers peaked 20 days (IgM) and 68 days (IgG) after the onset of symptoms (Figure 1). The IgM titer returned to a low level within 2 months after onset of illness. [FIGURE 1 OMITTED] Results of CHIKV-specific real-time reverse transcription--PCRs (2) performed with serum samples as templates were negative. Virus isolation was attempted by incubation of peripheral blood mononuclear cells collected on the day of onset with C6/36 (Aedes albopictus) and Vero (E6 clone) monolayers. After 5 days, supernatants were collected and used to infect fresh cell cultures. After 2 days, cytopathologic effects were observed in Vero monolayers; a high level of cell death was also observed in C6/36 cells. Infected Vero and C6/36 cells were then examined by indirect immunofluorescence assay (IFA Immunofluorescent assay (IFA) A blood test sometimes used to confirm ELISA results instead of using the Western blotting. In an IFA test, HIV antigen is mixed with a fluorescent compound and then with a sample of the patient's blood. ) for 8 different alphaviruses with alphavirus-specific antibodies and in-house mouse hyperimmune hyperimmune /hy·per·im·mune/ (hi?per-i-mun´) possessing very large quantities of specific antibodies in the serum. hyperimmune possessing very large quantities of specific antibodies in the serum. ascitic fluids to CHIKV, Mayaro (MAYV), Tonate (TONV), Semliki Forest (SFV SFV San Fernando Valley (California) SFV Schweizerischer Fussballverband (Swiss Soccer Association) SFV Simple File Verification SFV Semliki Forest Virus SFV Straight-Fixed-Variable ), and Sindbis (SINV) viruses. Results of IFA were positive when alphavirus-specific antibodies and antibodies to CHIKV, MAYV, and TONV were used; no fluorescence was observed when antibodies to SFV and SINV were used at the dilution 1:200. CHIKV-specific real-time RT-PCRs were negative when cell culture supematants were used as samples; this result excluded CHIKV as the etiologic agent. We next used cM3W and M2W2 alphavirus-specific primers (3) to partially amplify viral genome by RT-PCR RT-PCR reverse transcriptase-polymerase chain reaction. See PCR1. . The RT-PCR product was sequenced (GenBank accession no. DQ381540, isolate IMTSSA/5163) and used in a BLAST search that identified O'nyong-nyong virus (ONNV, E value [6e.sup.-130]). Viral RNA RNA: see nucleic acid. RNA in full ribonucleic acid One of the two main types of nucleic acid (the other being DNA), which functions in cellular protein synthesis in all living cells and replaces DNA as the carrier of genetic was amplified for phylogenetic studies by using ONNV-specific primers for nsP3, E2, and E1 sequences (primer sequences are available on request). RTPCR RTPCR Reverse Transcriptase Polymerase Chain Reaction products (614, 728, and 1080-nt long, respectively) were sequenced (GenBank accession nos. DQ383272, DQ383273, and DQ399055, respectively) and compared with ONNV sequences available on GenBank database; alignments were performed with ClustalW 1.7 software. Comparison of partial sequences showed a high degree of homology between the virus we isolated in Chad and strains previously isolated. In all 4 regions sequenced, paired identity at the nucleotide and amino acid level ranged from 92% to 98% and from 95% to 98%, respectively. Compared with ONNV isolate Gulu, the nsP3 sequence of our isolate featured a glycine-encoding codon deletion (nt 5249-5251, according to ONNV strain Gulu numbering). This deletion was also observed in ONNV strains SG650 and IbH 10964, which might indicate a common lineage. Four phylograms were constructed, each based on 1 genomic region we sequenced. Among ONNV sequences, all 4 phylograms exhibited a similar pattern: ONNV isolate IbH 10964 (Nigeria) and ONNV strain SG650 (Uganda) seemed to be closely related, whereas isolates Gulu (Uganda) and IMTSSA/5163 (Chad) were placed in 2 different branches (100% bootstrap value in the 4 phylograms). The phylogenetic tree based on El-encoding sequence (1080-nt long) gave the opportunity to include 2 other ONNV sequences (Figure 2). [FIGURE 2 OMITTED] ONNV (family Togaviridae, genus Alphavirus) was first isolated from human blood and anopheline anopheline pertaining to the anopheles genus of mosquitoes. mosquitoes in Gulu, Uganda, in 1959 (4) and has been responsible for several outbreaks in humans that occurred in East Africa (Kenya, Uganda, Tanzania, Malawi, Mozambique). Fever, headache, joint pains, and rash were the principal signs and symptoms (5,6). Virus isolations from human and animal sera as well as from Anophelesfunestus and A. gambiae have been reported in East Africa (7,8). Human and animal infections based on serologic evidence have also been reported in Nigeria, Ghana, and Sierra Leone (9,10). ONNV was also isolated from sentinel mice in Senegal and caused an outbreak in Cote d'Ivoire in the 1980s (11). To our knowledge, ONNV had never before been isolated in Chad. The Sarh region, where the patient was infected, consists predominantly of plains covered with a mixture of grasses and woodlands. This region receives heavy rainfall during the 6-month rainy season, from May to October. To our knowledge, no recent data are available concerning the presence of Anopheles Anopheles: see mosquito. spp. in this region. Patient infection occurred outside any reported outbreak involving ONNV or another arbovirus arbovirus Any of a large group of viruses that develop in arthropods (chiefly mosquitoes and ticks). The name derives from “arthropod-borne virus.” The spheroidal virus particle is encased in a fatty membrane and contains RNA; it causes no apparent harm to the . Moreover, the mission involved 9 other French soldiers whose serum specimens, collected a few weeks after their return from Sarh and transported to our laboratory, did not show serologic evidence of infection with an alphavirus. SFV antibodies failed to detect ONNV by IFA, although both viruses are members of the same antigenic complex (12). The distribution of ONNV strains observed in the phylograms seemed to be independent of viral isolation locations or years. This finding suggests either a high level of viral genomic sequence stability over time or the circulation of ONNV strains across Africa, which has given rise to a mixing of ONNV strains from different origins in the same areas. However, because of the limited number of sequences available for genetic comparison, this observation on the distribution of ONNV strains needs confirmation. In the absence of virus isolation, the diagnosis of infections with ONNV is difficult because of the close antigenic relationship of this virus with other alphaviruses, especially CHIKV. Development of a specific serologic assay for ONNV within the SFV antigenic complex would be a valuable tool for diagnosis and surveillance studies. Acknowledgments We are indebted to the physicians of 8e regiment d'artillerie de Commercy and 35e regiment d'infanterie de Belfort. We also thank Olivier Merle, Christophe N'Guyen, Yannick Sanson, and Houssem Bouchiba for technical assistance; Jon M. Davis for reviewing the paper; and Nick Karabatsos for providing alphavirus-specific antibodies. References (1.) Peyrefitte CN, Pastorino BA, Bessaud M, Gravier P, Tock F, Couissinier-Paris P, et al. Dengue dengue or breakbone fever or dandy fever Infectious, disabling mosquito-borne fever. Other symptoms include extreme joint pain and stiffness, intense pain behind the eyes, a return of fever after brief pause, and a characteristic rash. type 3 virus, Saint Martin, 2003-2004. Emerg Infect Dis. 2005; 11:757-61. (2.) Pastorino B, Bessaud M, Grandadam M, Murri S, Tolou HJ, Peyrefitte CN. Development of a TaqMan RT-PCR assay without RNA extraction step for the detection and quantification of African Chikungunya viruses. J Virol Methods. 2005; 124:65-71. (3.) Pfeffer M, Proebster B, Kinney RM, Kaaden OR. Genus-specific detection of alphaviruses by a semi-nested reverse transcription-polymerase chain reaction. Am J Trop Med Hyg. 1997;57:709-18. (4.) Haddow AJ, Davies CW, Walker DH. O'nyong-nyong fever: an epidemic virus disease in East Africa. Trans R Soc Trop Med Hyg. 1960;54:517-22. (5.) Marshall TF, Keenlyside R.A, Johnson BK, Chanas AC, Smith DH. The epidemiology of O'nyong-nyong in the Kano Plain, Kenya. Ann Trop Med Parasitol. 1982;76:153-8. (6.) Sanders EJ, Rwaguma EB, Kawamata J, Kiwanuka N, Lutwama JJ, Ssengooba FP, et al. O'nyong-nyong fever in south-central Uganda, 1996-1997: description of the epidemic and results of a household-based seroprevalence seroprevalence Immunology The proportion of a population that is seropositive–ie, has been exposed to a particular pathogen or immunogen; the seropositivity of a population is calculated as the number of individuals who produce a particular antibody divided survey. J Infect Dis. 1999;180:1436-43. (7.) Williams MC, Woodall JP, Corbet PS, Gillett JD. O'nyong-nyong fever: an epidemic virus disease in East Africa. 8. Virus isolations from Anopheles mosquitoes. Trans R Soc Trop Med Hyg. 1965;59:300-6. (8.) Williams MC, Woodall JP, Gillett JD. O'nyong-nyong fever: an epidemic virus disease in East Africa. VII. Virus isolations from man and serological serological pertaining to or emanating from serology. serological test one involving examination of blood serum usually for antibody. studies up to July 1961. Trans R Soc Trop Med Hyg. 1965;59:186-97. (9.) Guyer B. Serological survey for arboviruses in Igbo-Ora, western Nigeria. Ann Trop Med Parasitol. 1972;66:243-50. (10). Woodruff AW, Bowen ET, Platt GS. Viral infections in travellers from tropical Africa. BMJ. 1978; 1:956-8. (11.) Lhuillier M, Cunin P, Mazzariol M J, Monteny N, Cordellier R, Bouchite B. Epidemie rurale a virus "Igbo Ora" (avec transmission inter-humaine) en Coter d' Ivoire en 1984-1985. Bull Soc Pathol Exot. 1988;81:386-95. PMID PMID PubMed-Indexed for MEDLINE PMID Portable Multispectral Imaging Device PMID Process Management Improvement & Deployment PMID Physical Media Id PMID Performance Metric Identifier : 2846194 (12.) Calisher CH, Shope RE, Brandt W, Casals J, Karabatsos N, Murphy FA, et al. Proposed antigenic classification of registered arboviruses I. Togaviridae, Alphavirus. Intervirology. 1980; 14:229-32. Mael Bessaud, * Christophe N. Peyrefitte, * Boris A.M. Pastorino, * Patrick Gravier, * Fabienne Tock, * Fabrice Boete, ([dagger]) Hugues J. Tolou, * and Marc Grandadam * * Institut de medecine tropicale du Service de sante des armees, Marseille, France; and l-Cabinet medical d'unite, Commercy, France Dr Bessaud spent 5 years as a research assistant in the tropical virology unit at the Tropical Medicine Institute of the French Armed Forces Medical Service. He is involved in the diagnosis of outbreaks due to arboviruses; he also researches the flavivirus-encoded protease complex. Address for correspondence: Marc Grandadam, Unite de Virologie Tropicale, IMTSSA, BP 46, 13 998 Marseille armees, France; email: publi.viro@laposte.net |
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