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Appl Environ Microbiol, June 1998, p. 2278-2280, Vol. 64, No. 6
0099-2240/98/$04.00+0
Copyright © 1998, American Society for Microbiology. All rights reserved.
Detection of Toxoplasma gondii Oocysts
in Drinking Water
Judith
Isaac-Renton,1,*
William R.
Bowie,2
Arlene
King,3
G. Stewart
Irwin,4
Corinne S.
Ong,1
C. P.
Fung,5
M. Omar
Shokeir,1 and
J.
P.
Dubey6
Department of Pathology and Laboratory
Medicine1 and
Division of Infectious
Diseases, Department of Medicine,2
University of British Columbia, and
Epidemiology
Services3 and
Provincial
Laboratory,5 British Columbia Centre for Disease
Control, British Columbia Ministry of Health, Vancouver, and
Water Department, Capital Regional
District,4 Victoria, British Columbia, Canada,
and
Parasite Biology and Epidemiology Laboratory, Livestock and
Poultry Sciences Institute, Agricultural Research Service, U.S.
Department of Agriculture, Beltsville, Maryland6
Received 1 December 1997/Accepted 23 March 1998
 |
ABSTRACT |
The world's largest outbreak of waterborne toxoplasmosis occurred
in a municipality in the western Canadian province of British Columbia.
When drinking water emerged as a possible source of infection during
the outbreak investigation, a laboratory method was needed to attempt
detection of the parasite, Toxoplasma gondii. The method
developed was based on the current U.S. Environmental Protection Agency
method for detection of Cryptosporidium oocysts. Collection
of large-volume drinking water samples and cartridge filter processing
were unchanged, although identification of Toxoplasma oocysts in the filter retentate was carried out by using a previously described rodent model. Validation of the method developed was tested
by using oocysts from a well-characterized Toxoplasma
strain.
| |
TEXT |
A community outbreak of
toxoplasmosis in western Canada prompted extensive epidemiological
investigations. One hundred acute cases and 12 congenital cases of
infection with Toxoplasma gondii were identified during
these investigations. The diagnostic laboratory methods and
epidemiological investigations are described in detail elsewhere
(3). Briefly, a case-control study of symptomatic cases, a
case-control study of women enrolled in the toxoplasmosis screening
program, and geographical mapping of acute cases were carried out. A
clustering of cases was noted in the central area of greater Victoria,
British Columbia. Eighty-eight percent (83 of 94) of the persons
residing in the greater Victoria area with acute infections lived in an
area of the city receiving its water from one of the two treatment
plants (disinfection only). When drinking water emerged as a possible
source of infection, a laboratory method was needed to attempt to
detect T. gondii oocysts in water samples. Based on the
method used to detect Cryptosporidium oocysts (1), the new procedure used to detect the parasite in the
concentrate differed as described below. We propose that this method
could be useful in the investigation of waterborne transmission of
toxoplasmosis parasites, which were not widely recognized as being
spread by this route prior to the Canadian municipal outbreak
(3). The purpose of the present communication is to describe
this method.
The Humpback Reservoir, identified during the investigation as the most
likely source of T. gondii oocysts, supplied one of the two
municipal drinking water treatment plants. A sampling site was set up
at the point where water left this reservoir to enter the Humpback
treatment plant. One or two samples per week (a total of six water
samples) were collected from the Humpback Reservoir over 4 weeks. Water
samples were also collected on the same days as these samples but from
the reservoir supplying the other treatment plant but not implicated in
the outbreak. All samples were raw water collected before the water
entered the chloramination treatment plants.
A method was developed that is similar to the method used for
collection and processing of water samples for
Cryptosporidium sp., a protozoan related to T. gondii. The method is as follows. Large volumes (the target volume
was 1,000 liters; all volumes were greater than 700 liters) were
collected for each sample. Since T. gondii oocysts (10 to 12 µm in diameter) are larger than Cryptosporidium oocysts (3 to 5 µm in diameter), samples were collected by using the recommended
(1) 1-µm nominal porosity, orlon-wound filter cartridge. A
large-volume sample of water was passed through the filter housed in a
portable collection device by keeping the flow rate at 4 to 10 liters/min. Filters were separated from the collection apparatus and
transported in coolers (on ice).
On arrival at the laboratory, filters were cut into four parts and
parasites were eluted by washing in phosphate-buffered saline-0.01%
Tween 80-0.01% sodium dodecyl sulfate. After centrifugation (1,050 × g, 4 min, 4°C), sediments from individual
test tubes were pooled and the pellet was resuspended in distilled
water to a volume of 20 ml. This suspension was layered onto a series of conical test tubes containing 30 ml of a Percoll-sucrose solution (specific gravity, 1.15), and the test tubes were centrifuged (1,050 × g, 10 min, 4°C). The top 25 ml was then
aspirated off into another test tube and diluted fourfold with
phosphate-buffered saline-0.01% Tween 80-0.01% sodium dodecyl
sulfate. Following a final centrifugation step (1,050 × g, 10 min, 4°C), the supernatant was aspirated off and the
sediment was kept for sporulation and inoculation.
An aeration procedure was required to sporulate, and therefore render
infectious, any T. gondii oocysts in this sediment. This
procedure was carried out as follows. One milliliter of sediment was
mixed with 9 ml of 2% sulfuric acid and slowly agitated on a rocking
platform (Red Rocker; Hoefer Scientific, San Francisco, Calif.) at room
temperature for 7 days. The suspension, neutralized by using 3.3%
sodium hydroxide (2% phenol red pH indicator), was centrifuged
(1,050 × g, 10 min, 4°C), the supernatant was
aspirated down to 1 ml per tube, and the pellets were resuspended in
sterile saline. Suspensions were kept at 4°C until inoculation into
mice was carried out.
Female Swiss-Webster mice weighing 25 to 30 g each were ear tagged
and housed separately in sterilized cages with HEPA filters. They were
given irradiated food and sterile water ad libitum. For each water
sample, four test mice were inoculated. For each batch of samples
inoculated, three negative control mice were also inoculated.
One-half milliliter of the aerated, well-mixed, resuspended sample
sediment was inoculated by gavage (with a sterile gavage needle
and plastic tubing) into each of the four test mice (a total of 2 ml
was inoculated per sample). The bedding was discarded and the cages
were sterilized at 24 h postinoculation. Each of the three
negative control mice was inoculated with 0.5 ml of sterile saline on
the day of test sample inoculation.
Mice were observed twice daily for 60 days or until death. If a mouse
died, an autopsy was carried out. Touch preparations and formalin
fixing of appropriate tissues (mesenteric lymph nodes and lung and
cardiac tissues) were performed. Touch preparations fixed with methanol
were stained with Giemsa stain for examination by microscopy. Tissues
fixed in 10% buffered formalin were embedded in paraffin by
using standard histological procedures. After embedding, specimens (sectioned at 5-µm intervals) were stained with
Giemsa. Additional sections were also stained with hematoxylin and
eosin to observe the lesions. Slides were examined microscopically, including a search for parasites by oil immersion (magnification, ×1,000). Toxoplasma tachyzoites were identified when
crescentic, oval, or fusiform nucleated organisms measuring
approximately 2 by 6 µm were seen. If a mouse survived for 60 days,
blood was collected for serological testing (modified agglutination
test [MAT]) for toxoplasmosis (4, 5) in the U.S.
Department of Agriculture Laboratory at Beltsville, Md. Sera were not
collected from rodents that died.
To evaluate this method, oocysts of T. gondii VEG (human
source strain) were used to inoculate Swiss-Webster mice
(5). A series of dilutions ranging from 2.5 × 104 to less than 1 sporulated oocyst were made by using
sterile saline. For each dilution, 0.5 ml of a well-mixed suspension
was given by gavage to each of five test mice. Four negative control
mice were also inoculated with 0.5 ml of sterile saline on the day test
mice were inoculated. Mice were caged separately and observed twice
daily. If a mouse died, tissue specimens were processed as noted above.
Sera were obtained from all surviving mice, diluted 1:25, and tested
for T. gondii by MAT.
Eleven raw water samples were tested, six from the implicated water
source (Humpback Reservoir) and five from the nonimplicated reservoir.
The mean volumes collected were 1,051 liters for Humpback Reservoir
samples and 968 liters for samples from the second reservoir. A total
of 56 mice were inoculated with samples, including 24 mice given
Humpback reservoir samples, 20 mice given second-reservoir samples, and
12 mice used as saline-treated negative controls. At the end of 60 days, none of these mice had died. All were serologically negative for
toxoplasmosis.
A total of 34 mice were inoculated in the experiments using T. gondii VEG. Results are summarized in Table
1. Twenty-three mice showed evidence of
infection. Sixty-five percent (15 of 23) of the infected mice died
between 6 and 11 days postinoculation. Toxoplasmosis was documented
in the animals that died by verifying the presence of the parasite;
parasites were observed in 100% (15 of 15) of lung specimens, 86% (12 of 14) of cardiac specimens, and 73% (11 of 15) of mesenteric lymph
nodes. Necrotizing lymphadenitis was observed in the 11 nodes in which
T. gondii tachyzoites were identified, while significant
histopathology was absent in the 15 lung and 12 cardiac tissue
specimens in which parasite tachyzoites were seen. Infection was
documented in 8 of the 19 surviving mice by positive serology (MAT)
results. As seen in Table 1, none of the saline-treated control mice
showed evidence of infection and none of the mice inoculated with the
lowest dilution (less than 1 oocyst) had evidence of toxoplasmosis.
Inoculation of an estimated 2.5 oocysts resulted in infection in three
of five mice; five of five mice receiving 25 oocysts became infected.
This experiment is consistent with previous descriptions of this rodent
model of toxoplasmosis (5, 6), in which the sensitivity and
specificity are well described.
As noted in the description of this outbreak (3),
investigations implicated the Humpback Reservoir as the source of the T. gondii oocysts. The epidemic curve (7) showed
clusters of persons acutely infected during two periods of time
preceded by peaks in rainfall and turbidity in this unfiltered drinking
water supply. It was hypothesized that parasite contamination of the drinking water occurred during these periods of high runoff. It was
further hypothesized that because the implicated reservoir was
relatively small with a high turnover, sporulated oocysts from an
infected feline(s), the definitive host for T. gondii, were carried into the municipal water distribution system.
In retrospect, since collection of drinking water samples for
laboratory testing was started approximately 12 weeks after the last
human was infected, it was not surprising that attempts to confirm
epidemiological findings by laboratory testing of drinking water
samples were not successful. This large-volume
water sampling method linked to a rodent model does, however, appear to
have the potential to be a sensitive test for detection of
Toxoplasma oocysts.
Clusters or outbreaks of toxoplasmosis have been infrequently
described. Foodborne spread and waterborne spread have been reported
(2, 8), although not previously in a municipal water supply.
Where Toxoplasma contamination of a drinking water supply is suspected, the method described above may be useful in
detecting oocysts of the parasite if samples are collected early in the
outbreak investigation. It is therefore important that water purveyors
and public health workers be aware that T. gondii is yet
another protozoan parasite which may be transmitted through drinking
water.
| |
ACKNOWLEDGMENTS |
We thank P. Lee and R. Yan for their technical assistance. We also
thank the teams in the Parasitology Section, Enhanced Water Laboratory,
Environmental and Non-Viral Serology Sections, Provincial Laboratories,
British Columbia Centre for Disease Control, for their support.
| |
FOOTNOTES |
*
Corresponding author. Mailing address: Division of
Microbiology and Infection Control, Department of Pathology and
Laboratory Medicine, Laurel Street Pavilion, Vancouver General
Hospital, 855 West 12th, Vancouver, British Columbia, Canada V5Z 1M9.
Phone: (604) 875-4631. Fax: (604) 875-4359. E-mail:
isaacren{at}unixg.ubc.ca.
| |
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Appl Environ Microbiol, June 1998, p. 2278-2280, Vol. 64, No. 6
0099-2240/98/$04.00+0
Copyright © 1998, American Society for Microbiology. All rights reserved.
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