Performance of ORTHO HCV core antigen and trak-C assays for detection of viraemia in pre-seroconversion plasma and whole blood donors

L H Tobler; S L Stramer; S R Lee; D Baggett; D Wright; D Hirschkorn; I Walsh; M P Busch

doi:10.1111/j.1423-0410.2005.00687.x

Performance of ORTHO HCV core antigen and trak-C assays for detection of viraemia in pre-seroconversion plasma and whole blood donors

Vox Sang. 2005 Nov;89(4):201-7. doi: 10.1111/j.1423-0410.2005.00687.x.

Authors

L H Tobler¹, S L Stramer, S R Lee, D Baggett, D Wright, D Hirschkorn, I Walsh, M P Busch

Affiliation

¹ Blood Systems Research Institute, San Francisco, CA, USA. ltobler@bloodsystems.org

PMID: 16262752
DOI: 10.1111/j.1423-0410.2005.00687.x

Abstract

Objective: Logistics and cost of nucleic acid amplification testing (NAT) screening preclude its current use in many developing countries. Development of hepatitis C virus (HCV) core antigen assays offer an alternative to NAT. We evaluated two specimen populations to assess the sensitivity, relative to NAT, of the HCV core antigen (HCVcAg) ELISA (enzyme-linked immunosorbent assay) test system and the trak-C assay: (1) plasma donor HCV NAT-conversion panels and (2) cross-sectional whole blood donor NAT yield specimens.

Methods: Differential sensitivities among NAT (NGI; Chiron/Gen-Probe) and both HCVcAg assays (Ortho-Clinical Diagnostics, Rochester, NY) were evaluated using: (1) 102 serial ramp-up phase specimens from 37 plasma donor NAT-conversion panels (Alpha Therapeutic/BioClinical Partners); and (2) 42 cross-sectional whole blood donor NAT yield specimens (confirmed RNA positive, antibody negative) plus 54 NAT false-positive specimens (American Red Cross).

Results: Viral load among the plasma donor NAT-conversion panels at the cutoffs for HCVcAg and trak-C assays were 32 000 copies/ml (95% confidence interval [CI] 8000-120 000) and 8000 copies/ml (95% CI: 2200-28 000), respectively. The mean (95% CI) difference in window period reduction compared to routine mini-pool NAT screening (estimated sensitivity 100 copies/ml) was delayed 5.2 days (2.2-7.6 days) for HCVcAg assay and 3.8 days (2.1-5.5 days) for the trak-C assay. Among the 42 NAT yield specimens, the HCVcAg assay detected 31 (74%) as core antigen-positive while the trak-C assay detected 37 (88%) as core antigen-positive. Viral loads for the five specimens not detected by the trak-C HCVcAg assay ranged from 100 to 7770 copies/ml. All 54 NAT false-positive specimens were non-reactive on both HCV core antigen assays.

Conclusion: These data indicate that the trak-C assay has sensitivity approaching routine mini-pool NAT screening for the detection of seronegative HCV infection. In the absence of routine NAT screening for early HCV infection, the use of an HCV core antigen assay should be considered.

Publication types

Evaluation Study
Research Support, N.I.H., Extramural

MeSH terms

Blood Donors*
Enzyme-Linked Immunosorbent Assay / methods
Hepatitis C Antibodies / chemistry
Hepatitis C Antibodies / immunology
Hepatitis C Antigens / blood*
Hepatitis C Antigens / immunology
Humans
Sensitivity and Specificity
Viral Core Proteins / blood*
Viral Load / methods
Viremia / blood*
Viremia / diagnosis
Viremia / immunology

Substances

Hepatitis C Antibodies
Hepatitis C Antigens
Viral Core Proteins

Grants and funding

1R01 HL076902-01/HL/NHLBI NIH HHS/United States