Comparative performances of an HTLV-I/II EIA and other serologic and PCR assays on samples from persons at risk for HTLV-II infection

B J Poiesz; S Dube; D Choi; E Esteban; J Ferrer; M Leon-Ponte; G E de Perez; J Glaser; S G Devare; A S Vallari; G Schochetman

doi:10.1046/j.1537-2995.2000.40080924.x

Comparative performances of an HTLV-I/II EIA and other serologic and PCR assays on samples from persons at risk for HTLV-II infection

Transfusion. 2000 Aug;40(8):924-30. doi: 10.1046/j.1537-2995.2000.40080924.x.

Authors

B J Poiesz¹, S Dube, D Choi, E Esteban, J Ferrer, M Leon-Ponte, G E de Perez, J Glaser, S G Devare, A S Vallari, G Schochetman

Affiliation

¹ Department of Medicine, State University of New York, Health Science Center, Syracuse, New York 13210, USA. poieszb@mailbox.hscsyr.edu

PMID: 10960518
DOI: 10.1046/j.1537-2995.2000.40080924.x

Abstract

Background: HTLV-I and HTLV-II are related exogenous pathogenic human retroviruses. Until recently, ELISAs based on HTLV-I antigens have been used to screen for the presence of HTLV-I or -II antibodies. The HTLV-I-based assays have not been as sensitive in detecting antibodies to HTLV-II as in detecting antibodies to HTLV-I. The Abbott HTLV-I/HTLV-II ELISA uses a combination of HTLV-I and HTLV-II antigens to detect antibodies to the whole HTLV group. The performance of this ELISA was compared to that of several HTLV-I-based serologic assays and an HTLV-II PCR assay in cohorts of South American Indians and New York City IV drug users (IVDUs) in whom HTLV-II is endemic.

Study design and methods: Sera from 429 South American Indians and New York City IVDUs were evaluated for HTLV antibodies by the use of three ELISAs (rgp21-enhanced HTLV-I/II, Cambridge Biotech; Vironostika HTLV-I/II, Organon Teknika; and HTLV-I/HTLV-II, Abbott), and a Western blot (WB) assay. Peripheral blood leukocyte DNA from each person was analyzed for HTLV-I and HTLV-II pol DNA via PCR. The HTLV-II PCR-positive samples were further subtyped via cloning and sequencing and/or oligomer restriction.

Results: Two hundred four samples (48%) were positive for HTLV-II by serologic and/or PCR assays. All of the positive samples from the Indians and approximately one-third of the positive samples from the IVDUs were of the HTLV-IIB subtype. Comparative analyses indicate that the sensitivity and specificity of the various assays were: PCR, 98 and 100 percent; Abbott HTLV-I/HTLV-II, 78 and 95 percent; Cambridge Biotech HTLV-I/II, 76 and 96 percent; Vironostika HTLV-I/II, 71 and 98 percent; and WB, 73 and 100 percent, respectively.

Conclusion: There were no significant differences among the sensitivities and specificities of the HTLV-I/II ELISAs (p values, 0.056-0.438). The WB and PCR assays were much more specific than the other serologic assays (p</=0.03). However, the PCR assay is significantly (p<0.001) more sensitive than any of the serologic assays in the detection of HTLV-II infection. Thus, optimal detection of HTLV-II infection would seem to require both serologic and DNA PCR assays.

Publication types

Comparative Study
Research Support, Non-U.S. Gov't
Research Support, U.S. Gov't, P.H.S.

MeSH terms

Enzyme-Linked Immunosorbent Assay
HTLV-I Antibodies / immunology*
HTLV-II Antibodies / immunology*
HTLV-II Infections / genetics*
Humans
Polymerase Chain Reaction
Statistics as Topic

Substances

HTLV-I Antibodies
HTLV-II Antibodies

Grants and funding

N01-HB-67021/HB/NHLBI NIH HHS/United States