Investigation of suspected viral hepatitis outbreaks in North West India

Mini P Singh; Manasi Majumdar; Kapil Goyal; P V M Lakshmi; Deepak Bhatia; R K Ratho

doi:10.1016/j.diagmicrobio.2015.12.002

Investigation of suspected viral hepatitis outbreaks in North West India

Diagn Microbiol Infect Dis. 2016 Apr;84(4):309-14. doi: 10.1016/j.diagmicrobio.2015.12.002. Epub 2015 Dec 12.

Authors

Mini P Singh¹, Manasi Majumdar², Kapil Goyal³, P V M Lakshmi⁴, Deepak Bhatia⁵, R K Ratho⁶

Affiliations

¹ Department of Virology, Postgraduate Institute of Medical Education & Research, Chandigarh, India 160012. Electronic address: minipsingh@gmail.com.
² Department of Virology, Postgraduate Institute of Medical Education & Research, Chandigarh, India 160012. Electronic address: manasivirol@gmail.com.
³ Department of Virology, Postgraduate Institute of Medical Education & Research, Chandigarh, India 160012. Electronic address: kapilgoyalpgi@gmail.com.
⁴ School of Public Health, Postgraduate Institute of Medical Education & Research, Chandigarh, India 160012. Electronic address: lakshmi.pvm@pgimer.edu.in.
⁵ Integrated Disease Surveillance Project, Directorate of Health & Family Welfare, Punjab, Chandigarh, India. Electronic address: idspb@gmail.com.
⁶ Department of Virology, Postgraduate Institute of Medical Education & Research, Chandigarh, India 160012. Electronic address: rathopgi@yahoo.com.

PMID: 26853491
DOI: 10.1016/j.diagmicrobio.2015.12.002

Abstract

Hepatitis E (HEV) infection is diagnosed on the basis of serum anti-HEV IgM detection. In outbreaks, early diagnostic method is important for prompt control measures. This study compared 3 diagnostic methods in 60 serum samples collected in suspected HEV outbreaks. The suitability of saliva samples for antibody detection was also evaluated in 21 paired serum saliva samples. The anti-HEV IgM, HEV-Ag, and HEV-RNA were detected in serum samples of 52 (86.66%), 16 (26.66%), and 18 (30%) patients, respectively. The concordance between serum and saliva IgM was found to be 76.91%. The positivity of PCR and HEV-Ag detection was 100% within 1 week of illness which declined to 5-10% thereafter. The outbreak was attributed to HEV genotype 1, subtype 1a, and the clinical and environmental strains clustered together. HEV-antigen and RNA were an early diagnostic marker with 96.66% concordance. Saliva samples can be used as an alternative in outbreak setting.

Keywords: HEV-antigen; Hepatitis E virus; Outbreak; Phylogenetic analysis; Saliva.

Publication types

Evaluation Study

MeSH terms

Adolescent
Adult
Antigens, Viral / blood
Clinical Laboratory Techniques / methods*
Diagnostic Tests, Routine / methods*
Disease Outbreaks*
Female
Genotype
Hepatitis Antibodies / analysis*
Hepatitis E / diagnosis*
Hepatitis E / epidemiology
Hepatitis E virus / classification
Hepatitis E virus / genetics
Hepatitis E virus / immunology*
Humans
Immunoglobulin M / analysis*
Immunoglobulin M / blood
India / epidemiology
Male
Middle Aged
RNA, Viral / blood
RNA, Viral / genetics
Retrospective Studies
Saliva / chemistry
Sensitivity and Specificity
Young Adult

Substances

Antigens, Viral
Hepatitis Antibodies
Immunoglobulin M
RNA, Viral