Emerging Infectious Diseases
[Volume 5 No.2 / March - April 1999]

Dispatches

Acute Hemorrhagic Conjunctivitis Due to Enterovirus 70 in India

R.S. Maitreyi, L. Dar, A. Muthukumar, M. Vajpayee, I. Xess, R.B. Vajpayee,
P. Seth, and S. Broor
All India Institute of Medical Sciences, New Delhi, India

---------------------------------------------------------------------------
      An outbreak of acute hemorrhagic conjunctivitis occurred in
      Delhi, India, during August and September 1996. The etiologic
      agent was confirmed as enterovirus type 70 by a modified
      centrifugation-enhanced culture method followed by
      immunofluorescence and neutralization tests. After nearly a
      decade, this virus is reemerging as a cause of acute
      hemorrhagic conjunctivitis in India.

Acute conjunctivitis can be caused by viruses including enterovirus 70
(EV-70), coxsackievirus A24, and epidemic adenoviruses. These viruses may
also lead to acute hemorrhagic conjunctivitis (AHC), characterized by
photophobia, watering, and foreign body sensation, eyelid edema,
conjunctival hemorrhages, and superficial punctate keratitis. The disease
is self-limiting.

In 1996, an outbreak of AHC occurred in Delhi, north India, during the
rainy season (August and September). We conducted a study to identify the
etiologic agent by viral culture, immunofluorescence and neutralization
tests, and polymerase chain reaction (PCR).

The Study

We enrolled 13 patients with clinically diagnosed bilateral AHC who
attended the outpatient clinic of Rajendra Prasad Centre for Ophthalmic
Sciences during the outbreak. At the initial visit, all patients had a
complete ophthalmic examination, including slit-lamp biomicroscopy.
Conjunctival swabs were taken from the right eye of each patient. These
swabs were collected in 2 ml of Hanks balanced salt solution with
antibiotics and were transported on wet ice to the virology laboratory for
processing.

All samples were vortexed thoroughly and treated with antibiotics (1,000
IU/ml penicillin and 1,000 µg/ml streptomycin). Specimens were clarified by
centrifugation at 700 x g for 10 minutes at 4°C. Supernatant fluid was
separated and used for inoculation in cell culture. The samples were stored
at -70°C until they were processed.

For virus culture, Hep-2cell monolayers were grown in 24-well plates,
containing 12-mm cover slips (Bellco Glass Inc., New Jersey, USA). Each
plate was seeded with 1 ml of Hep-2cell suspension, incubated at 37°C in a
5% CO(sub 2) atmosphere, and used for a modification of the
centrifugation-enhanced viral culture technique (1).

Cover-slip monolayers were washed twice with phosphate-buffered saline
(PBS) before specimen inoculation. Two hundred microliters of each specimen
was inoculated in parallel in two 24-well plates containing Hep-2cell
monolayers grown onto 12-mm cover slips. Plates were centrifuged at 700 x g
for 60 minutes at room temperature. Inoculum was discarded and washed once
with PBS; infected cells were re-fed with 1.0 ml of Eagle's minimum
essential medium containing 2% fetal calf serum. The plates were reincubated 
at 37°C in a 5% CO(sub 2) atmosphere. Cover slips from one plate were
removed, washed twice with PBS, and fixed with chilled acetone at 48 hours
postinoculation for immunofluorescence. The parallel 24-well plate cultures
were observed for viral cytopathic effect, which included rounding and
refractility of cells and destruction of the monolayer at 2 to 4 days; the
resulting effect suggested enteroviral infection. Because a standardized
reverse transcriptase-PCR test for enteroviral RNA was available at the All
India Institute of Medical Sciences, New Delhi, India, we screened the
samples with this test.

Ten of the 13 clinical samples and the positive control showed the amplicon
band, while the negative control did not (Figure). The PCR results
suggested enteroviral infection, helped narrow the search for the etiologic
agent, and provided a rapid preliminary diagnosis.

Viral antigen was detected by indirect immunofluorescence staining (on the
fixed cover slips stored earlier) using specific antibodies to EV70,
coxsackievirus A24, and adenoviruses (Chemicon International Inc., CA,
USA). Infected cover-slip monolayers were stained with 25 µl of monoclonal
antibodies, incubated in a moist chamber at 37°C for 45 minutes, and washed
twice with PBS for 10 minutes each. Fluorescein-labeled anti-mouse
conjugate was added, and the cover slips were reincubated at 37°C for 45
minutes, followed by a PBS washing step, as described above. The cover
slips were air-dried, mounted with glycerol buffer, and examined under
fluorescence microscopy.

		  [fig]    		 Figure: Reverse transcriptase-polymerase
                               chain reaction (RT-PCR) for enteroviral RNA
 from acute hemorrhagic conjunctivitis cases. Lane 1: pX174 DNA/Hae III
 marker; lane 2: negative control; lane 3: positive control (enteroviral
 RNA); lanes 4-6: clinical samples.

 For PCR, viral RNA was extracted by the guanidinium thiocyanate method
 (2) from 200 µl of clinical specimen. The RNA pellet was resuspended in
 10 µl of diethyl pyrocarbonate treated water. A 5-µl volume was used for
 cDNA synthesis. The primers used for PCR amplification were selected from
 the highly conserved 5' noncoding region of enterovirus described by
 Rotbart et al. (3) and, using the same protocol, cDNA for PCR was
 synthesized by reverse transcription. Briefly, cDNA (10µ Cl) was
 amplified in a PCR mix volume of 50 µl, containing 100 ng of each primer,
 250 µl of each dNTP, 1.5 mM MgCl(sub 2), 2.5 units Taq polymerase, and 
 5 µl of 10X PCR buffer. The tubes were subjected to 30 cycles at 94°C for 1
 minute, 58°C for 1 minute, and 72°C for 2 minutes, respectively, followed
 by a final extension for 7 minutes at 72°C. A 154-bp sized band of the
 PCR-amplified product was visualized under UV illumination on a 2%
 agarose gel after ethidium bromide staining.

The samples showing a viral cytopathic effect were given a second passage,
and if the effect was seen again, the 50% tissue infective dose of the
virus isolate was calculated. A virus neutralization test was performed
using 100 50% tissue infective doses of the isolate and virus-specific
antiserum.

Findings

All 13 patients enrolled in the study (9 male and 4 female, ages 14 to 37
years) had bilateral ocular involvement and described redness and watering
of the eyes, mild photophobia, and severe foreign body sensation. Ocular
examination showed severe conjunctival congestion, interspersed
subconjunctival hemorrhages, and superficial punctate epithelial keratitis.
No neurologic manifestations (as reported in an earlier epidemic) were
observed (4).

Cover-slip monolayers infected with a known EV-70 prototype (Kono)–like
strain from a previous outbreak (5) and 10 of the 13 clinical specimens
showed specific cytoplasmic fluorescence with monoclonal antibodies to
EV-70. Infected monolayers tested with monoclonal antibodies to adenovirus
and coxsackievirus A24 yielded negative results. Neutralization test
results confirmed the identification, as all 10 clinical isolates were
neutralized by EV-70–specific antisera. Also, the known EV-70 prototype
(Kono)–like strain was neutralized by pooled convalescent-phase sera from
the patients in this outbreak. PCR was positive for EV-70 in 11 of the 13
cases, including the 10 culture-confirmed cases.

Conclusions

An outbreak of AHC was first reported from Ghana in 1969 and was referred
to as Apollo conjunctivitis (6). A new enterovirus (EV-70) was identified
as the etiologic agent of AHC (7); subsequently it spread to other parts of
Africa and Asia including India.

The first serologic evidence of EV-70 infection in India came from Bombay
(western India) in 1971-72 (4), and the first isolation was reported from a
single case during a small epidemic in southern India in 1975 (8). During
an epidemic in north India in 1981 (also during the rainy season), two
isolates of EV-70 prototype (Kono)–like strain were reported from Delhi
(5), and antigen-positive cases were found by immunofluorescence in the
city of Chandigarh (9). The last reported outbreak of EV-70 from this
region (July to September 1986) was also confirmed only by demonstration of
antigen in cell scrapings by immunofluorescence (10). AHC due to EV-70
appears to have reemerged in north India after nearly a decade. During the
intervening period, a coxsackievirus A24 variant was circulating as a cause
of AHC in this region of India (11). However, a prime-type EV-70 isolate
was obtained from a case-patient during an outbreak in Pune, western India,
nearly 1,200 km from Delhi, in 1991 (12).

In this outbreak of AHC, we achieved an unusually high isolation rate of
EV-70 (10 of 13 cases) by using a modification of centrifugation-enhanced
culture. The results of neutralization tests indicate that the strains
circulating in this part of India continue to resemble the prototype strain
(also reported during the 1981 epidemic). PCR was useful because of its
rapidity and help in narrowing the search for an etiologic agent to
enteroviruses. With the availability of PCR based on EV-70 specific primers
(13), this highly sensitive centrifugation-enhanced technique is likely to
be used increasingly in the future.

---------------------------------------------------------------------------

      Dr. Maitreyi is a senior research fellow, Department of Microbiology,
All India Institute of Medical Sciences, New Delhi, India. Her areas of
expertise include tissue culture and molecular biology, and her research
focuses on respiratory viruses and enteroviruses.

      Address for correspondence: Shobha Broor, Department of Microbiology,
All India Institute of Medical Sciences, Ansari Nagar, New Delhi-110029,
India; fax: 91-11-686 2663; e-mail: broor@medinst.ernet.in.

References

  1. Pass RF, Britt WJ, Stagno S. Cytomegalovirus. Diagnostic procedures
     for viral, rickettsial and chlamydial infections, 7th ed. In: Lennette
     EH, Lennette DA, Lennette ET, editors. Washington: American Public
     Health Association; 1995.
  2. Chomczynski P, Sacchi N. Single step method of RNA isolation by acid
     guanidinium thiocyanate phenol chloroform extraction. Ann Clin Biochem
     1987;162:156-9.
  3. Rotbart HA. Enzymatic amplification of the enteroviruses. J Clin
     Microbiol 1990;28:438-42.
  4. Kono R, Miyamura K, Tajiri E, Shiga S, Sasagawa A, Irani PF, et al.
     Neurological complications associated with acute haemorrhagic
     conjunctivitis virus infection and its serological confirmation. J
     Infect Dis 1974;129:590-3.
  5. Manjunath N, Balaya S, Mahajan VM. Isolation of enterovirus 70 during
     conjunctivitis epidemic in Delhi in 1981. Indian J Med Res
     1982;76:653-5.
  6. Chatterjee S, Quarcoopome CO, Apenteng A. Unusual type of
     conjunctivitis in Ghana. Br J Ophthalmol 1970;54:628-30.
  7. Kono R, Sasagawa A, Ishii K, Sugiura S, Ochi M, Matsumiya H, et al.
     Pandemic of new type of conjunctivitis. Lancet 1972;i:1191-4.
  8. Christopher S, John J, Charles V, Ray S. Coxsackie virus A24 variant
     EH 24/70 and enterovirus type 70 in an epidemic of acute haemorrhagic
     conjunctivitis-a preliminary report. Indian J Med Res 1977;65:593-5.
  9. Pal SR, Szucs Gy, Melnick JL, Kaiwar R, Bharadwaj G, Singh R, et al.
     Immunofluorescence test for the epidemiological monitoring of acute
     haemorrhagic conjunctivitis cases. Bull World Health Organ
     1983;61:485-90.
 10. Kishore J, Manjunath N, Bareja U, Verma LK, Broor S, Seth P. Study of
     an outbreak of epidemic conjunctivitis in Delhi in 1986. Indian J
     Pathol Microbiol 1989;32:266-9.
 11. Broor S, Kishore J, Dogra V, Satapathy G, Seth P. An epidemic of acute
     haemorrhagic conjunctivitis caused by Coxsackie A24 variant. Indian J
     Med Res 1992;95:253-5.
 12. Bhide VS, Prasad SR, Gogate SS. Isolation of a variant of enterovirus
     70 from a patient during an epidemic of acute haemorrhagic
     conjunctivitis in Pune in 1991. Acta Virol 1994;38:245-6.
 13. Uchio E, Yamazaki K, Aoki K, Ohno S. Detection of enterovirus 70 by
     polymerase chain reaction in acute haemorrhagic conjunctivitis. Am J
     Ophthalmol 1996;122:273-5.


Emerging Infectious Diseases
National Center for Infectious Diseases
Centers for Disease Control and Prevention
Atlanta, GA

URL: ftp://ftp.cdc.gov/pub/EID/vol5no2/ascii/maitreyi.txt

Please note that figures and equations are not available in ASCII format; 
their placement within the text is noted by [fig] and [eq], respectively. 
Greek symbols are spelled out. The following codes are used: 
(ft) for footnote; (sup) for superscript; (sub) for subscript; 
>/= for greater than or equal to.