Comparison of serological assays to titrate Hantaan and Seoul hantavirus-specific antibodies

Weihong Li; Shouchun Cao; Quanfu Zhang; Jiandong Li; Shuo Zhang; Wei Wu; Jing Qu; Chuan Li; Mifang Liang; Dexin Li

doi:10.1186/s12985-017-0799-0

Comparison of serological assays to titrate Hantaan and Seoul hantavirus-specific antibodies

Virol J. 2017 Jul 18;14(1):133. doi: 10.1186/s12985-017-0799-0.

Authors

Weihong Li^{1

2}, Shouchun Cao³, Quanfu Zhang¹, Jiandong Li¹, Shuo Zhang¹, Wei Wu¹, Jing Qu¹, Chuan Li¹, Mifang Liang¹, Dexin Li⁴

Affiliations

¹ Key Laboratory for Medical Virology, National Health and Family Planning Commission of the People's Republic of China; Laboratory for Viral Hemorrhagic Fever, National Institute for Viral Disease Control and Prevention, China CDC, Beijing, 102206, People's Republic of China.
² Institute for Infectious Disease and Endemic Disease Control, Beijing CDC, Beijing, 100013, People's Republic of China.
³ National Institutes for Food and Drug Control, Beijing, 100050, People's Republic of China.
⁴ Key Laboratory for Medical Virology, National Health and Family Planning Commission of the People's Republic of China; Laboratory for Viral Hemorrhagic Fever, National Institute for Viral Disease Control and Prevention, China CDC, Beijing, 102206, People's Republic of China. lidx@chinacdc.cn.

Abstract

Background: Hantaan and Seoul viruses, in the Hantavirus genus, are known to cause hemorrhagic fever with renal syndrome (HFRS). The plaque reduction neutralization test (PRNT), as conventional neutralization test for hantaviruses, is laborious and time-consuming. Alternatives to PRNT for hantaviruses are required.

Methods: In this study, the methods for Hantaan and Seoul viruses serological typing including microneutralization test (MNT), pseudoparticle neutralization test (PPNT) and immunofluorescence assay based on viral glycoproteins (IFA-GP) were developed and compared with PRNT using a panel of 74 sera including 44 convalescent sera of laboratory confirmed HFRS patients and 30 patients sera of non-hantavirus infection. Antibody titres and serotyping obtained with different methods above were analyzed by paired-t, linear correlation, McNemar χ² and Kappa agreement tests.

Results: Antibody titres obtained with MNT₅₀, PPNT₅₀ and IFA-GP were significantly correlated with that obtained with PRNT₅₀ (p < 0.001). GMT determined by PPNT₅₀ was statistically higher than that determined by PRNT₅₀ (p < 0.001), while GMT determined by MNT₅₀ and IFA-GP were equal with (p > 0.05) and less than (p < 0.001) that obtained with PRNT₅₀ respectively. Serotyping obtained with MNT₅₀ and PRNT₅₀, PPNT₅₀ and PRNT₅₀ were highly consistent (p < 0.001), whereas that obtained with IFA-GP and PRNT₅₀ were moderately consistent (p < 0.001). There were no significant differences for serotyping between PRNT₅₀ and MNT₅₀, as well as PRNT₅₀ and PPNT₅₀ (p > 0.05). IFA-GP was less sensitive than PRNT₅₀ and MNT₅₀ for serotyping of hantaviruses infection (p < 0.05). However, for 79.5% (35/44) samples, serotyping determined by IFA-GP and PRNT₅₀ were consistent.

Conclusions: MNT₅₀ and PPNT₅₀ both can be used as simple and rapid alternatives to PRNT₅₀, and MNT₅₀ is more specific while PPNT₅₀ is more sensitive than other assays for neutralizing antibody determination. So far, this work has been the most comprehensive comparison of alternatives to PRNT.

Keywords: Glycoproteins; Hantaan; Immunofluorescence assay; Microneutralization test; Plaque reduction neutralization test; Pseudoparticle neutralization test; Seoul; Serotyping.

Publication types

Comparative Study
Evaluation Study

MeSH terms

Antibodies, Viral / blood*
Hantaan virus / immunology*
Humans
Sensitivity and Specificity
Seoul virus / immunology*
Serotyping / methods*

Substances

Antibodies, Viral