West Nile Virus antibodies in Colombian horses.To the Editor: 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. (WNV) is rapidly spreading in the Western Hemisphere (1). We report the first evidence for WNV transmission in South America. WNV is serologically related to the Japanese encephalitis complex of flaviviruses (Flaviviridae), which includes Saint Louis encephalitis virus Saint Louis encephalitis virus n. An arbovirus that causes Saint Louis encephalitis and is transmitted by a mosquito. (SLEV SLEV Saint Louis Encephalitis Virus SLEV Surround Level ) (in North and South America), Japanese encephalitis virus (Asia), and Murray Valley encephalitis virus Murray Valley encephalitis virus (MVEV) is a zoonotic flavivirus endemic to northern Australia and Papua New Guinea. It is the causal agent of Murray Valley encephalitis (previously known as Australian encephalitis) and in humans can cause permanent neurological disease or death. (Australia) (2). Because of antigenic cross-reactivity within this complex, WNV serologic diagnosis requires highly specific assays, such as the plaque-reduction neutralization test (PRNT) (3). We used PRNT to evaluate serum collected from 130 healthy equines (horses and donkeys) in Colombia, where WNV had not been previously reported. These equines were sampled between September 15 and October 29, 2004, in the northern departments of C6rdoba and Sucre Sucre, city (1992 pop. 131,769), S central Bolivia, constitutional capital of Bolivia and capital of Chuquisaca dept. Since 1898, La Paz has been the administrative capital of Bolivia. in the Caribbean region of Colombia. Samples were heat-inactivated and titrated ti·trate tr. & intr.v. ti·trat·ed, ti·trat·ing, ti·trates To determine the concentration of (a solution) by titration or perform the operation of titration. by PRNT for antibodies to WNV, SLEV, and 3 other South American flaviviruses: Rocio, Ilheus, and Bussuquara. Twelve specimens (9%) from 10 different premises tested positive for WNV (Table). None of these animals had been vaccinated against WNV or had traveled outside of the region. An equine immunoglobulin (Ig) M-capture enzyme-linked immunosorbent assay enzyme-linked immunosorbent assay n. ELISA. Enzyme-linked immunosorbent assay (ELISA) A diagnostic blood test used to screen patients for AIDS or other viruses. (ELISA ELISA (e-li´sah) Enzyme-Linked Immuno-Sorbent Assay; any enzyme immunoassay using an enzyme-labeled immunoreactant and an immunosorbent. ELISA n. ) that used WNV antigen detected anti-WNV IgM in 2 of the 12 specimens, which indicated that some of these infections were relatively recent (probably within 3 months of sampling). The positive findings in both Cordoba and Sucre were corroborated by a WNV-specific blocking ELISA (4). Numerous other samples exhibited flavivirus reactivity ***** in the neutralization and blocking ELISA assays, mostly because of SLEV. Complete test results from these horses, as well as from Colombian cattle and chickens, will be presented elsewhere. These serologic data should be considered indirect evidence of WNV activity in Colombia. We encourage Colombian human and animal health authorities to enhance surveillance for human, equine, and avian disease attributable to WNV. Efforts are needed to isolate the virus or detect specific 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 to confirm this finding and to identify vectors and vertebrate hosts involved in WNV transmission in Colombia. Acknowledgments We thank Robert Lanciotti, Janeen Laven, Jason Velez, and Vanesa Otero for technical assistance. Salim Mattar, * Eric Edwards, ([dagger]) Jose Laguado, * Marco Gonzalez, * Jaime Alvarez, * and Nicholas Koma ([dagger]) * University of Cordoba, Monteria, Cordoba, Colombia; and ([dagger]) Centers for Disease Control and Prevention Centers for Disease Control and Prevention (CDC), agency of the U.S. Public Health Service since 1973, with headquarters in Atlanta; it was established in 1946 as the Communicable Disease Center. , Fort Collins, Colorado The City of Fort Collins, a home rule municipality situated on the Cache la Poudre River along the Colorado Front Range, is the county seat and most populous city in Larimer County, Colorado. , USA References (1.) Komar N. West Nile virus: epidemiology and ecology in North America. Adv Virus Res. 2003;61:185-234. (2.) Calisher CH, Karabatsos N, Dalrymple JM, Shope RE, Porterfield JS, Westaway EG, et al. Antigenic relationships between flaviviruses as determined by cross-neutralization tests with polyclonal antisera. J Gen Virol. 1989;70:37-43. (3.) Beaty BJ, Calisher CH, Shope RE. Arboviruses arboviruses (ar´bōvī´r  sz),n. . In: Lennette EH, Lennette DA, Lennette ET, editors. Diagnostic procedures for viral, rickettsial rickettsial /rick·ett·si·al/ (ri-ket´se-al) pertaining to or caused by rickettsiae. rick·ett·si·al adj. Relating to, or caused by a member of the genus Rickettsia. , and chlamydial infections. 7th ed. Washington: American Public Health Association The American Public Health Association (APHA) is Washington, D.C.-based professional organization for public health professionals in the United States. Founded in 1872 by Dr. Stephen Smith, APHA has more than 30,000 members worldwide. ; 1995. p. 189-212. (4.) Blitvich BJ, Marlenee NL, Hall RA, Calisher CH, Bowen RA, Roehrig JT, et al. Epitope-blocking enzyme-linked immunosorbent assays for the detection of serum antibodies to West Nile virus in multiple avian species. J Clin Microbiol. 2003;41: 1041-7. Address for correspondence: Nicholas Komar, Centers for Disease Control and Prevention, PO Box 2087, Fort Collins, CO 80522, USA; fax: 970-221-6476; email: nck6@cdc.gov The opinions expressed by authors contributing to this journal do not necessarily reflect the opinions of the Centers for Disease Control and Prevention or the institutions with which the authors are affiliated. Table. PRN[T.sub.90] antibody titers to WNV and other South American flaviviruses for Colombian equine sera *([dagger]) Equine ID ([double Depart- Age dagger]) ment (y) WNV SLEV ILHV ROCV BSQV 3 Cordoba 4 1:40 <1:10 <1:10 <1:10 <1:10 35 Cordoba 5 1:160 <1:10 <1:10 <1:10 <1:10 39 ([section]) Cordoba 4 1:40 <1:10 <1:10 <1:10 <1:10 41 Cordoba 6 1:40 <1:10 <1:10 <1:10 <1:10 48 Cordoba 4 1:640 <1:10 <1:10 <1:10 <1:10 76 Sucre 5 1:80 <1:10 <1:10 <1:10 <1:10 85 Sucre 9 1:80 <1:10 <1:10 <1:10 <1:10 94 Sucre 3 1:40 <1:10 <1:10 <1:10 <1:10 101 Sucre 4 1:40 <1:10 <1:10 <1:10 <1:10 109 Sucre 7 1:160 1:40 1:40 1:10 <1:10 ([section]) 123 Cordoba 6 1:40 <1:10 <1:10 <1:10 <1:10 125 Cordoba 4 1:160 <1:10 <1:10 <1:10 <1:10 * These 12 specimens were considered positive for WNV infection; a 4-fold WNV PRN[T.sub.90] titer compared to that of other flaviviruses was required for a positive determination of previous WNV infection. ([dagger]) PRN[T.sub.90], 90% plaque reduction neutralization test; WNV, West Nile virus; SLEV, Saint Louis encephalitis virus (South American strain); ILHV, Ilheus virus; ROCV, Rocio virus; BSQV, Bussuquara virus. ([double dagger]) All equines were horses except for 76 and 85, which were donkeys. ([section]) Also positive for anti-WNV immunoglobulin M by antibody-capture enzyme-linked immunosorbent assay. |
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