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V Thakur , RC
Guptan, V Arankale*, SK Sarin
Department of Gastroenterology, G.B. Pant Hospital, New Delhi and
National
Institute of Virology, Pune*, India*
Correspondence and reprints requests:
Dr. S.K. Sarin, M.D., D.M.
Professor and Head
Department of Gastroenterology
G. B. Pant Hospital, New Delhi, India
Fax : 91-11-6426896
Email: sksarin@nda.vsnl.net.in
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ABSTRACT
Objective
Third generation anti-HCV ELISA is currently recommended for the
diagnosis of HCV infection. We determined its specificity in
voluntary blood donors (VBDs) and patients with chronic liver
disease (CLD) in relation to confirmatory line immunoassay (LIA)
and reverse transcription polymerase chain reaction
(RT-PCR).
Material and Methods:
1926 serum samples of VBDs and 16 HCV related CLD patients were
screened by ELISA. An optical density/cut-off ratio (OCR) of
>1 was taken as positive for anti-HCV antibodies. Samples
were confirmed by LIA and HCV-RNA detection by RT-PCR.
Interpretation of LIA was done as: indeterminate, reactive or
non-reactive. Every 50th VBD sample, negative for anti-HCV by
LIA was subjected to LIA and RT-PCR to rule out false negativity of
ELISA.
Results:
Anti-HCV was positive in 34 (1.76%) VBDs and all the CLD
patients. Only one (2.9%) VBD was reactive by LIA and 6
(17.6%) were HCV-RNA positive. Serum samples from VBDs
with OCR >3 were significantly more often (p<0.05) PCR
positive than those with an OCR of <3. In the CLD
patients, specimens even with OCR between 1-3 were reactive by PCR.
All ELISA negative samples were non-reactive by LIA and
PCR.
Conclusions:
(i) There is a high false positivity of the third
generation ELISA for the diagnosis of HCV infection in VBDs, (ii)
Higher OCR should be used for improving the specificity of ELISA in
VBDs, (iii) VBDs with an OCR of >3 should be subjected to
HCV-RNA determination.
INTRODUCTION
Serodiagnosis of Hepatitis C Virus (HCV)
infection started about a decade back by employing enzyme
linked immunosorbent assay (ELISA) [1]. There are two
situations where anti-HCV detection is important; blood banks,
where it is routinely used to reduce the risk of post-transfusion
hepatitis C and, in clinical practice, to correlate and confirm the
clinical suspicion of HCV-related chronic liver disease.
First generation assays were less sensitive and specific. To
overcome their drawbacks, confirmatory recombinant immunoblot
assays (RIBA) were developed [2,3]. With further improvement
in the sensitivity and specificity, second and third
generation ELISA and immunoblot assays became available
[4-7].
The presence of anti-HCV antibodies
using these immunological tests does not give any idea about
the viraemic status of a patient or a blood donor.
To overcome these limitations, RIBA tests are often employed which
indicate that most RIBA positive donors have persistent HCV
infection [6]. However, the indeterminate results need to be
ascertained by doing HCV-RNA test.
Prevalence of anti-HCV antibodies in the
blood donor population in India is about 1.7% [8]. The
frequency of anti-HCV false positivity by ELISA and indeterminate
pattern in supplemental tests is not known. This could create
a difficult situation in a low prevalence healthy population
[1,6,9]. We initiated a large prospective study with
the aim of determining the specificity of the third generation
enzyme immunoassay in detecting anti-HCV antibodies in blood donor
population and to compare this with patients with chronic liver
disease due to hepatitis C.
MATERIAL AND
METHODS:
Nineteen hundred and twenty six consecutive healthy voluntary blood
donors (VBDs) attending the blood bank of G. B. Pant Hospital,
New Delhi, India, were included in the study. Blood sample
collection, storage of serum samples and detection of HCV infection
was a simultaneous process. At first, the serum specimen was
subjected to anti-HCV detection using the third-generation, ELISA
(United Biomedical, NY, USA). The test system detects
antibodies directed to core, NS3, NS4 and NS5 regions
of the HCV genome using synthetic peptides. The
assay was carried out according to the manufacturer's
instructions. In each specimen, optical density (OD) to
cut-off ratio (OCR) was calculated. Samples with an OCR
<1 were considered to be positive and those
with OCR <1 were marked as negative for anti-HCV
antibodies. Each positive sample was re-tested to confirm
the positivity using ELISA. On the basis of the OCR, the
samples were divided into 3 groups:
(a) OCR
between 1 � 3,
(b)
OCR between >3 � 6, and
(c) OCR >
6.
To check for false negativity of
anti-HCV ELISA, every 25th serum sample was re-analyzed by
ELISA. Serum transaminase levels were determined for all
the 1926 specimens simultaneously.
A confirmatory third generation Line
Immunoassay (LiaTek, Organon Teknika, The Netherlands), and
HCV RNA detection by RT reverse transcription polymerase chain
reaction (RT-PCR) were performed on all ELISA positive
specimens. The line immunoassay system uses synthetic
peptides, corresponding to HCV envelope (E2 / NS2) in addition to
core, NS3, NS4 and NS5 antigens. The assay and the interpretation
of the results were carried out according to the manufacturer's
instructions. To cross-check the negative ELISA result and to
assess the false negativity of the line immunoassay, every 50th
ELISA negative specimen was reanalyzed by a repeat-line immunoassay
test.
HCV-RNA detection was also carried out
using the RT-PCR in all ELISA positive and every 50th ELISA
negative specimen. RNA was isolated by the
guanidium isothiocynate method [10] and the amplification was
done using oligonucleotide primer sequence from the conserved
region of the HCV genome.
A comparative group of
sixteen biopsy-proven HCV-related patients with chronic liver
disease were also included in the study. Serum of these
subjects were analyzed by all the three assays i.e. ELISA,
line immunoassay and HCV-RNA by RT-PCR.
RESULTS
The results of different assays, namely
ELISA, line immunoassay and RT-PCR in VBD's and chronic liver
disease patients are shown below.
ELISA
Voluntary Blood Donors:
Of the 1926 VBDs screened, 34 (1.76%)
subjects revealed an OCR of >1.00, that is they were
positive for anti-HCV antibodies. On the basis of OCR, the
EIA positive specimens were divided into 3 groups: those
having an OCR between 1-3, between 4-6, and above 6.
Twenty six of the positive specimens had an OCR in the range
of 1-3, seven (21%) revealed a ratio between 4 to 6 and only
one sample had an optical density 10 folds compared to the cut-off
value (Table 1). Every 25th EIA negative sample was found to
be non-reactive on repeat analysis using enzyme
immunoassay.
Chronic Liver Disease Patients:
Samples from all sixteen patients with
chronic liver disease were reactive by enzyme immunoassay, 5
(31%), 6 (38%), and 5 (31%) patients were found to have an OCR
between 1 to 3, 4 to 6 and above 6 respectively. Compared
with the VBD group, a significantly higher number of patients
with chronic liver disease had an OCR of >3.
Line Immuno
Assay Voluntary Blood Donors:
LIA had a very poor correlation with
ELISA in the subjects with OCR between 1 and 3. Twenty-three
of the 26 (86%) ELISA positive specimens were non-reactive by line
immunoassay and three specimens showed indeterminate results.
In the group of subjects with an OCR between 4 and 6, LIA
again showed indeterminate results in six of the seven (86%)
specimens. In the third group, there was only one sample
which had an OCR ~10 by ELISA. This showed a positive
LIA reaction. Every 50th ELISA-negative sample was also
found negative by LIA.
Chronic Liver
Disease Patients:
The LIA results in these specimens were
quite different than that seen in VBDs. Even in the subjects with
an OCR between 1-3, two of the 5 EIA positive samples were
reactive by LIA and the remaining 3 were found to be
indeterminate. In samples with an OCR between 4 to 6, LIA
showed reactive results in four and indeterminate in two. The
sample having an OCR > 6 was found to reactive by
LIA.
HCV-RNA by
Polymerase Chain Reaction Voluntary Blood
Donors:
HCV-RNA detection was undertaken in all
the 34 anti HCV positive VBDS. In the 26 ELISA positive
specimens where the OCR was between 1 and 3, none of
the samples was found positive for HCV RNA. In the groups with
an OCR between 4 to 6 and > 6, five (84%) and one
(100%) subject respectively was found to
be positive. Thus overall, only six of the 34 (6%)
anti-HCV positive samples were found to be HCV-RNA
positive.
Chronic Liver
Disease Patients:
In the group of chronic liver disease
patients, 11 of the 16 (69%) blood samples showed an OCR above 3.
However, irrespective of the OCR, all the 16 anti-HCV positive
patients with chronic liver disease were found to be HCV-RNA
positive (Table 1).
DISCUSSION
The results of our study indicate a poor correlation
between the results of the enzyme immunoassay, the
confirmatory line immunoassay and the HCV-RNA detection by
RT-PCR in the voluntary blood donor population in India. Only
six of the 34 (6%) donors who were found to be
anti-HCV-positive were actually detected to have HCV-RNA in their
blood. Of these however, only one sample was found to
be positive by the confirmatory line immunoassay. This
discrepancy was particularly evident when the OCR was between 1 and
3; 88% of the ELISA positive specimens were found to be negative
by line immunoassay and the remaining 12% were
indeterminate. None of the samples was reactive. Similarly,
at this none of the OCR of 1-3, donors were HCV-RNA
positive. However, if a hyper value of OCR (>3) was
used, the false positivity of ELISA has been well documented
in the healthy population where the prevalence of HCV infection is
low [1,6,9]. Our results of high false positivity of anti-HCV
by 3rd generation ELISA are in conformity with Cordons et al, [11]
who have also recommended the use of the polymerase chain
reaction for improving the specificity of HCV
detection. Few other authors have also concluded that
further refinement of antibody screening and confirmatory assays
and standardization of molecular testing are necessary to optimize
testing and fully characterize the diagnosis of HCV infection [12].
These observations clearly indicate that the addition of
a new antigen in the third generation ELISA kit might have improved
the sensitivity of the assay over the second-generation kits, but
it has not added to the specificity of detection, especially in
serum samples positive for anti-HCV and having a low
OCR.
Our results also bring to attention the
major limitations of the confirmatory immunoblot assays in the
VBD population. These tests were not found helpful as even in
8 of the 9 samples with an OCR of >3, the results of LIA were
indeterminate. In almost every subject who is LIA indeterminate,
HCV RNA testing was required. Hence, there is little rationale for
using immunoblot assay in routine blood bank screening.
This finding reaffirms the observation of Krarup et
al.[13].
On the other hand, the standard third
generation EIA was quite sensitive and specific in the patients
with chronic liver disease. All the sixteen blood samples
that were anti-HCV positive, were also found to be HCV-RNA
positive. RIBA was reactive in only 11 of these patients and
indeterminate in 5. It therefore appears quite clear that the
third generation anti-HCV testing is quite sensitive and specific
for chronic liver disease patients and there is no added advantage
of doing immuno blot assays.
In summary, the third generation ELISA
is quite sensitive and specific for the diagnosis of HCV
infection in patients with chronic liver disease. In the
voluntary blood donor population however, the test is relatively
less specific, specially, at the lower OCR. We recommend that an
assay with a higher OCR should be used for VBDs to reduce the
false positivity. Blood donors with high OCR should be
investigated further by doing RT-PCR testing for
HCV-RNA.
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