Volume 45, Issue 4 pp. 487-491

West Nile virus in Canadian blood donors

Cherie Cameron

Cherie Cameron

From the Canadian Blood Services, Ottawa, Ontario; Saskatchewan Provincial Laboratory Services, Regina, Saskatchewan; the Provincial Laboratory for Public Health, Calgary, Alberta; the Canadian Blood Services, Regina, Saskatchewan; the Canadian Blood Services, Calgary, Alberta, Canada; and the Canadian Blood Services, Winnipeg, Manitoba, Canada.

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Jackie Reeves

Jackie Reeves

From the Canadian Blood Services, Ottawa, Ontario; Saskatchewan Provincial Laboratory Services, Regina, Saskatchewan; the Provincial Laboratory for Public Health, Calgary, Alberta; the Canadian Blood Services, Regina, Saskatchewan; the Canadian Blood Services, Calgary, Alberta, Canada; and the Canadian Blood Services, Winnipeg, Manitoba, Canada.

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Nick Antonishyn

Nick Antonishyn

From the Canadian Blood Services, Ottawa, Ontario; Saskatchewan Provincial Laboratory Services, Regina, Saskatchewan; the Provincial Laboratory for Public Health, Calgary, Alberta; the Canadian Blood Services, Regina, Saskatchewan; the Canadian Blood Services, Calgary, Alberta, Canada; and the Canadian Blood Services, Winnipeg, Manitoba, Canada.

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Peter Tilley

Peter Tilley

From the Canadian Blood Services, Ottawa, Ontario; Saskatchewan Provincial Laboratory Services, Regina, Saskatchewan; the Provincial Laboratory for Public Health, Calgary, Alberta; the Canadian Blood Services, Regina, Saskatchewan; the Canadian Blood Services, Calgary, Alberta, Canada; and the Canadian Blood Services, Winnipeg, Manitoba, Canada.

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Ted Alport

Ted Alport

From the Canadian Blood Services, Ottawa, Ontario; Saskatchewan Provincial Laboratory Services, Regina, Saskatchewan; the Provincial Laboratory for Public Health, Calgary, Alberta; the Canadian Blood Services, Regina, Saskatchewan; the Canadian Blood Services, Calgary, Alberta, Canada; and the Canadian Blood Services, Winnipeg, Manitoba, Canada.

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Bernie Eurich

Bernie Eurich

From the Canadian Blood Services, Ottawa, Ontario; Saskatchewan Provincial Laboratory Services, Regina, Saskatchewan; the Provincial Laboratory for Public Health, Calgary, Alberta; the Canadian Blood Services, Regina, Saskatchewan; the Canadian Blood Services, Calgary, Alberta, Canada; and the Canadian Blood Services, Winnipeg, Manitoba, Canada.

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Dale Towns

Dale Towns

From the Canadian Blood Services, Ottawa, Ontario; Saskatchewan Provincial Laboratory Services, Regina, Saskatchewan; the Provincial Laboratory for Public Health, Calgary, Alberta; the Canadian Blood Services, Regina, Saskatchewan; the Canadian Blood Services, Calgary, Alberta, Canada; and the Canadian Blood Services, Winnipeg, Manitoba, Canada.

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Debra Lane

Debra Lane

From the Canadian Blood Services, Ottawa, Ontario; Saskatchewan Provincial Laboratory Services, Regina, Saskatchewan; the Provincial Laboratory for Public Health, Calgary, Alberta; the Canadian Blood Services, Regina, Saskatchewan; the Canadian Blood Services, Calgary, Alberta, Canada; and the Canadian Blood Services, Winnipeg, Manitoba, Canada.

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John Saldanha

Corresponding Author

John Saldanha

From the Canadian Blood Services, Ottawa, Ontario; Saskatchewan Provincial Laboratory Services, Regina, Saskatchewan; the Provincial Laboratory for Public Health, Calgary, Alberta; the Canadian Blood Services, Regina, Saskatchewan; the Canadian Blood Services, Calgary, Alberta, Canada; and the Canadian Blood Services, Winnipeg, Manitoba, Canada.

John Saldanha, PhD, Roche Molecular Systems Inc., 4300 Hacienda Drive, Pleasanton, CA, 94588, e-mail: [email protected].Search for more papers by this author
First published: 22 March 2005
Citations: 8

Abstract

BACKGROUND: Blood donation screening for West Nile virus (WNV) RNA by nucleic acid testing (NAT) was implemented in Canada in July 2003, and 14 WNV RNA–positive donations were identified. Samples were screened in minipools of six donations with a WNV assay (TaqScreen, Roche). Two of the donors were identified by single-donor screening that was initiated in the province of Saskatchewan, which had the highest prevalence of WNV in the country, in early September 2003.

STUDY DESIGN AND METHODS: The original 14 samples and follow-up samples (2-35 days after donation), available from 13 of the 14 donors were tested with an in-house, real-time, quantitative WNV NAT assay that was specific for WNV. A Health Canada reference reagent was used for calibration. Immunoglobulin M (IgM) and immunoglobulin G (IgG) levels were determined with commercial enzyme-linked immunosorbent assay kits.

RESULTS: All donors tested positive for the presence of WNV with the in-house assay. Two donors, 18 and 19, identified by single-donor testing, had extremely low levels of viremia and that could only be detected in 1:38 or 1:39 replicate tests. The titers of the remaining index samples ranged from below log2.8 (the limit of quantitation) to log4.7 NAT detectable units per mL. Three samples, from Donors 17, 18, and 19, were IgM-positive, whereas samples from Donors 18 and 19 were also IgG-positive. The remaining 10 donors with follow-up samples all seroconverted.

CONCLUSION: The 14 WNV donor samples detected by routine screening were confirmed as WNV RNA–positive by a WNV RNA–specific in-house assay and by demonstration of seroconversion in 13 of the 14 donors.

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