Infection Pressure is Necessary, but not Sufficient by Itself, to Explain Toxoplasma gondii Seroprevalence in Intermediate Host Species

Patrick L. Taggart; Bronwyn A. Fancourt; Wayne S. J. Boardman; David E. Peacock; Charles G. B. Caraguel

doi:10.1645/21-28

How to translate text using browser tools

16 July 2021 Infection Pressure is Necessary, but not Sufficient by Itself, to Explain Toxoplasma gondii Seroprevalence in Intermediate Host Species

Patrick L. Taggart, Bronwyn A. Fancourt, Wayne S. J. Boardman, David E. Peacock, Charles G. B. Caraguel

Author Affiliations +

J. of Parasitology, 107(4):554-561 (2021). https://doi.org/10.1645/21-28

Abstract

Parasite infection pressure is suggested to be a strong driver of transmission within ecosystems. We tested if infection pressure drives seroprevalence in intermediate host species for Toxoplasma gondii. We defined Toxoplasma infection pressure to intermediate host species as the combined influence of cat abundance, environmental conditions, and its prevalence in the cat population. We sampled and tested 2 species of rodent and collated information on Toxoplasma seroprevalence in koalas, wallabies, kangaroos, and sheep. All species were sampled using equivalent methods, within a 2-yr period, and from adjacent regions of low and high Toxoplasma infection pressure. The seroprevalence of Toxoplasma in kangaroos scaled with infection pressure, but we observed no statistical difference in seroprevalence for any other species between these 2 regions. Within the region of low infection pressure, Toxoplasma seroprevalence did not differ between species. However, within the region of high Toxoplasma infection pressure, we observed large variation in seroprevalence between species. Our results demonstrate that infection pressure is not sufficient by itself, but merely necessary, to drive Toxoplasma seroprevalence in intermediate host species. Where Toxoplasma seroprevalence in an intermediate host species is already low, further reducing infection pressure will not necessarily further decrease seroprevalence in those species. This has important ramifications for the mitigation of parasite infections and suggests that reductions in Toxoplasma infection pressure, intended to reduce infections, may be most effective and applicable to species that are known to experience high rates of infection.

Toxoplasmosis is a disease of significant health concern for humans, livestock, and wildlife (Canfield et al., 1990; Epiphanio et al., 2001; Dubey, 2009a, 2016). The disease is caused by the cat-borne protozoal parasite Toxoplasma gondii. Felids are the definitive host of the parasite and shed the oocyst stage in their feces, predominately following their first infection (Zulpo et al., 2018). Oocysts are particularly resistant to environmental conditions and can remain infective for at least 18 mo under favorable conditions, but they can be killed rapidly via desiccation (Yilmaz and Hopkins, 1972; Frenkel et al., 1975; Dubey, 1998). Intermediate hosts of T. gondii can be any endotherm, which become infected via two major routes of transmission, oocyst or bradyzoite consumption (Aramini et al., 1999; Hill and Dubey, 2002; Dubey, 2016; Zulpo et al., 2018). Accordingly, based on the major routes of T. gondii transmission to intermediate hosts, we would expect the parasite's infection pressure to be largely dependent on oocyst contamination in the environment. Similarly, oocyst contamination in the environment should be dependent on cat density, environmental conditions, and the prevalence of T. gondii infection in the cat population (Frenkel and Dubey, 1973; Dubey, 1998, 2009b; Zulpo et al., 2018).

Many studies have shown that ecological or physiological characteristics of an intermediate host species, such as age or body mass, can influence T. gondii seroprevalence (Afonso et al., 2007; Tagel et al., 2019). However, the relative contribution of T. gondii infection pressure to explaining seroprevalence in intermediate host species is not well known. This has important ramifications for the mitigation of T. gondii infection via reductions in infection pressure.

We investigated if T. gondii infection pressure is sufficient, by itself, to explain the observed seroprevalence in intermediate host species. We defined T. gondii infection pressure to intermediate hosts as the combined influence of cat density, environmental conditions, and the seroprevalence of the parasite in the cat population. If T. gondii infection pressure is sufficient to drive seroprevalence in intermediate host species, then we would expect that seroprevalence will scale with infection pressure for all species tested. If the relationship between T. gondii seroprevalence and infection pressure is linear, whereby an increase in infection pressure results in a proportional increase in seroprevalence, then the proportional differences in seroprevalence among species will remain constant across regions of differing infection pressure.

To address this question, we sampled and tested house mice (Mus musculus) and bush rats (Rattus fuscipes), and we collated recently published information on T. gondii seroprevalence in koalas (Phascolarctos cinereus), tammar wallabies (Macropus eugenii), western grey kangaroos (Macropus fuliginosus), and sheep (Ovis aries) from a region of low infection pressure and an adjacent region of high infection pressure (Taggart et al., 2019b, 2019c, 2020b). We obtained T. gondii seroprevalence estimates for all species and tested for effects of infection pressure, species, and their interaction on T. gondii seroprevalence. Here, we discuss the role of T. gondii infection pressure in driving seroprevalence in intermediate host species and the implication of this result for mitigating T. gondii infection via reductions in infection pressure, and we hypothesize other factors that may contribute to the observed results.

MATERIALS AND METHODS

Study sites

Study regions included the Fleurieu Peninsula (35°35′18.96″S, 138°11′54.96″E) on mainland South Australia and the adjacent Dudley Peninsula on Kangaroo Island (35°48′5.4″S, 137°58′30.72″E). Both regions experience similar Mediterranean climates (Jenkins, 1985; Schwerdtfeger, 2002) and comprise similar land uses and vegetation types (cropping and pasture land interspersed with patches of native vegetation, largely low Eucalyptus spp. woodlands). These 2 regions are located only 13.5 km apart. This assisted in controlling for any potentially confounding climatic conditions that may contribute to the differential survival of T. gondii oocysts in the environment, and consequently differences in T. gondii seroprevalence in our study species. Cat (Felis catus) abundance on the Fleurieu Peninsula, South Australia, is reported to be approximately 10 times lower than that on the adjacent Kangaroo Island (Bengsen et al., 2011; Taggart et al., 2019a; Hohnen et al., 2020). Similarly, the seroprevalence of T. gondii in cats on the Fleurieu Peninsula would be expected to be lower than that in insular cats, based on its lower seroprevalence in cats from the wider Australian mainland and the known high seroprevalence in insular cats (89.4% seropositive) (O'Callaghan et al., 2005; Fancourt and Jackson, 2014). We, therefore, assumed the Fleurieu Peninsula to be a region of low T. gondii infection pressure and Kangaroo Island to be a region of high T. gondii infection pressure. This assumption is supported by previous work, which has shown a lower seroprevalence of T. gondii in sheep (10%) on the South Australian mainland relative to that on Kangaroo Island (sheep 23%) and a low seroprevalence of T. gondii in rabbits from this region as well (O'Donoghue et al., 1987; McKenny et al., 2020; Taggart et al., 2020b). Hereafter, we refer to the Fleurieu Peninsula on the South Australian mainland as a region of low T. gondii infection pressure (low cat abundance, expected low seroprevalence in cats) and Kangaroo Island as a region of high T. gondii infection pressure (high cat abundance, high seroprevalence in cats).

We sampled house mice and bush rats at 4 sites in the region of low T. gondii infection pressure and 4 sites in the region of high T. gondii infection pressure. Study sites within each region were a subset of the same study sites used to assess cat abundance in each region in Taggart et al. (2019a). These sites were chosen to be representative of the remnant vegetation types in these regions and were all surrounded by agricultural grazing land.

Animal capture

House mice and bush rats were trapped in cages or Elliot traps baited with peanut butter and rolled oats, or in unbaited pitfall traps. Traps were deployed along linear transects within native vegetation patches at intervals of 20 m. Trapping occurred between January 2017 and April 2018.

Blood sampling and processing

We collected blood from conscious house mice via venipuncture of the facial vein (Francisco et al., 2015) and from anesthetized bush rats via jugular venipuncture (Parasuraman et al., 2010). All captured rodents were marked to facilitate the identification of recaptures and to avoid individuals being sampled multiple times.

Blood samples were centrifuged, and sera samples were collected and stored at –20 C as described by Taggart et al. (2019c). Sera samples experienced 2 freeze/thaw cycles before testing. Long-term sera storage does not significantly modify the interpretation of T. gondii serology (Dard et al., 2017).

Toxoplasma gondii antibody test

Sera samples were tested for T. gondii immunoglobulin G (IgG) antibodies using equivalent methods for all individuals and species (Taggart et al., 2019b, 2019c, 2020b). We used a commercially available modified agglutination test (MAT) (Toxo-Screen DA, bioMérieux, Marcy-l'Étoile, France) as described in detail by Taggart et al. (2019c). The MAT is based on the direct agglutination of fixed T. gondii tachyzoites of the RH strain, with sera pre-treated with 2-mercaptoethanol to neutralize IgM antibodies (Desmonts and Remington, 1980; Dubey and Desmonts, 1987). IgG antibodies typically take greater than 1 wk to develop, but once developed, they persist for the remainder of the animal's life. Consequently, this test may give false-negative results within the first week of infection (Dubey and Crutchley, 2008). Sera were screened at 1:40 and 1:4,000 dilutions and classified as positive if agglutination occurred at either dilution. This minimized possible type 2 error due to the prozone effect. With each assay, we included positive and negative control sera from known infected (intra-peritoneal inoculation with T. gondii tachyzoites) and uninfected mice and a negative phosphate-buffered saline (PBS, pH 7.2) control. A serum sample was classified as positive when agglutination of T. gondii formed a mat covering about half or more of the well base.

The MAT has not been evaluated in the study species, but we assumed its diagnostic sensitivity and specificity to be satisfactory based on appropriate quality controls and the high sensitivity and specificity of the assay reported in other species (Mainar-Jaime and Barberan, 2007). To our knowledge cross-reactivity with the MAT is low (Dubey, 2016; Gondim et al., 2017).

Data analysis

Collated information: We combined our data on T. gondii seroprevalence in house mice and bush rats with previously published data on T. gondii seroprevalence in koalas, tammar wallabies, western grey kangaroos, and sheep (Taggart et al., 2019b, 2019c, 2020b). All of these species were sampled within a 2-yr period and tested using equivalent methods from the described regions of low and high infection pressure (Taggart et al., 2019b, 2019c, 2020b). House mice, bush rats, koalas, and western grey kangaroos were sampled in the same regions of low and high T. gondii infection pressure. Tammar wallabies and sheep were only sampled from the region of high T. gondii infection pressure.

Statistics: We used generalized linear models (GLMs) to investigate the association between T. gondii seroprevalence and the predictor variables infection pressure (low vs. high) and species, and their interaction. In each GLM, T. gondii seroprevalence in an animal was treated as a binary response, and the default logit link was used. Statistical significance was determined using a score test (Lagrange multiplier) and model parsimony assessed using the Akaike information criterion (AICc). We considered a model to have substantial support if P values for predictor variables were <0.05 and ΔAICc was <2 (Burnham and Anderson, 2002). Due to zero infections within the region of low infection pressure, the GLM exhibited quasi-complete separation, and so the conventional Wald's test was not useful for posthoc comparisons between species within locations (Mansournia et al., 2018).

Given this separation issue and the finding that there were highly significant species effects in our GLM (see Results), we compared T. gondii seroprevalence between species within the region of high infection pressure only. For each 2 × 2 cross-tabulation of counts of 2 species by T. gondii seropositivity, we used either a Fisher's exact test or chi-squared test with the (n – 1) adjustment (Campbell, 2007), depending on the count of positive animals in the groups being tested. To correct for multiple comparisons, we determined statistical significance according to a Bonferroni adjusted alpha value of 0.003. However, we acknowledge that this correction will be conservative due to known dependence between tests (Abdi, 2007). We present T. gondii seroprevalence and binomial exact 95% confidence intervals. All statistical analyses were performed in base R version R 3.5.1 (R Core Team, 2020).

RESULTS

We sampled 19 mice and 169 rats in the region of low infection pressure and 36 mice and 46 rats in the region of high infection pressure, totaling 270 individuals (Table I). We additionally compiled T. gondii seroprevalence information on another 124 animals across another 2 species from the region of low infection pressure, and another 886 animals across another 4 species from the region of high infection pressure (Table I). The apparent seroprevalence of T. gondii for both mice and rats from the region of low infection pressure, and for mice from the region of high infection pressure was 0% (Fig. 1; Table I). From the region of high T. gondii infection pressure, a single rat was positive, giving an apparent seroprevalence of 2.2% (Fig. 1; Table I).

Table I

Toxoplasma gondii seroprevalence (with 95% confidence intervals [CIs]) by species from a region of low infection pressure and a region of high infection pressure.

Figure 1.

Toxoplasma gondii seroprevalence estimates (with binomial 95% confidence intervals) by species from a region of low infection pressure (blue circles) and a region of high infection pressure (red diamonds). Color version is available online.

Our most parsimonious GLM supported the inclusion of infection pressure and species as fixed effects (infection pressure: Rao score = 16.84, df = 1, P ≤ 0.001; species: Rao score = 228.01, df = 5, P ≤ 0.001; Suppl. Data, Table S1 (para-107-04-02_s01.docx)). The seroprevalence of T. gondii was substantially higher within the region of high infection pressure relative to that within the region of low infection pressure, and large variation in seroprevalence existed between species generally. The interaction infection pressure*species was not supported in GLMs due to the absence of T. gondii infection in all species within the region of low infection pressure. However, we found large variation in T. gondii seroprevalence among species within the region of high infection pressure using chi-squared and Fisher's exact tests (Table II). Within the region of high infection pressure, the seroprevalence of T. gondii in sheep was greater than the seroprevalence of T. gondii in all other species; similarly, the seroprevalence in kangaroos was greater than that in mice, rats, and koalas, and the seroprevalence in wallabies was greater than that in koalas. For all other pair-wise comparisons we found no difference in T. gondii seroprevalence according to our Bonferroni adjusted alpha value of 0.003. We did not test for differences in T. gondii seroprevalence between species within the region of low infection pressure because we observed no infection in any species and hence no variation in seroprevalence between species.

Table II

P values for the comparison of Toxoplasma gondii seroprevalence across species within the region of high infection pressure. Statistically significant comparisons are listed in bold format and were determined based on a Bonferroni adjusted alpha level of 0.003. Numbers in parentheses indicate χ² values where a chi-squared test was used for comparison instead of a Fisher's exact test.

DISCUSSION

If T. gondii infection pressure is sufficient, by itself, to drive seroprevalence in intermediate host species, then seroprevalence must scale with infection pressure for all species. If this relationship is also linear, then the proportional differences in seroprevalence among species will remain constant across regions of differing infection pressure. If intermediate host species seroprevalence scales with infection pressure, but proportional differences in seroprevalence among species are not constant across regions of differing infection pressure, then a sufficient, but non-linear, relationship between T. gondii seroprevalence and infection pressure will exist. However, if intermediate host species seroprevalence does not scale with infection pressure, then T. gondii infection pressure alone cannot be sufficient to drive seroprevalence, and seroprevalence must be strongly driven by other factors in addition to infection pressure. It is not possible for proportional differences in T. gondii seroprevalence among species to remain constant across regions of differing infection pressure if seroprevalence does not scale with infection pressure.

We found no evidence of T. gondii presence within our region of low infection pressure. Consequently, we cannot be certain that our specific study sites on the Fleurieu Peninsula represented a region of low infection pressure and did not represent a region of no/zero infection pressure. This has implications for the testing and interpretation of the conditions necessary to demonstrate a sufficient, or sufficient and linear, relationship between T. gondii infection pressure and intermediate host seroprevalence.

When testing if infection pressure scales with seroprevalence, it is irrelevant if T. gondii actively circulates in our region of low infection pressure or not. For mice, rats, and koalas, we found no evidence of a difference in T. gondii seroprevalence between our regions of low and high infection pressure. Thus, for these 3 species, our data provide evidence that T. gondii seroprevalence does not scale with infection pressure and is not sufficient, by itself, to drive seroprevalence.

When testing if proportional differences in seroprevalence among species remain constant across regions of differing infection pressure, it is important that T. gondii actively circulates to some extent within our region of low infection pressure. If it does not, then our test of the presence of a linear relationship between T. gondii infection pressure and intermediate host seroprevalence is invalid. Although we cannot conclusively demonstrate that T. gondii does circulate at our specific study sites within our region of low infection pressure, we suggest it is unlikely that T. gondii is completely absent from these study sites for the following reasons: (1) T. gondii antibodies have previously been detected in sheep, rabbits, and people on the broader Fleurieu Peninsula region, which encompasses our region of low infection pressure (Johnson et al., 1980; Berger and Gideon Informatics, 2010; Lanyon and O'Handley, 2020; McKenny et al., 2020); (2) our specific study sites within the region of low infection pressure are known to support a wild/feral cat population (Taggart et al., 2019a); (3) a recent systematic review and meta-analysis of T. gondii seroprevalence in felids worldwide and a regional review of T. gondii seroprevalence in cats in Australia both suggest that its seroprevalence in cats in Australia is among the highest worldwide (Fancourt and Jackson, 2014; Montazeri et al., 2020); (4) it is not uncommon for T. gondii seroprevalence values to be low, <1%, but nonetheless T. gondii is still present and actively circulating (Dubey et al., 2006; Murata et al., 2018); (5) T. gondii is considered to be a ubiquitous parasite worldwide (Shwab et al., 2018); and (6) we are unaware of any studies that have demonstrated that T. gondii was absent from locations with a known cat population, climatic conditions conducive to the survival of oocysts in the environment, and known infections in multiple species within close proximity. If T. gondii does truly circulate at our specific study sites on the Fleurieu Peninsula, and this region can truly be considered to be a region of low infection pressure, then our data would also suggest that proportional differences in seroprevalence among species are not constant across regions of differing infection pressure, and infection pressure is not linearly related to seroprevalence in intermediate host species. This would be supported by the large difference in T. gondii seroprevalence between kangaroos and that in mice, rats, and koalas within the region of high infection pressure but no difference in the seroprevalence experienced by these species within the region of low infection pressure.

As we did not observe a consistently lower seroprevalence of T. gondii in intermediate host species within the region of low infection pressure relative to the same species within the region of high infection pressure, our data suggest that T. gondii infection pressure, while necessary, is just one of many factors that influences seroprevalence in an intermediate host species. We cannot be 100% confident if this relationship between T. gondii infection pressure and intermediate host species seroprevalence is linear or not.

Our results have direct relevance to the mitigation of T. gondii infection via reductions in infection pressure, for example, via the removal of cats from an environment. Where T. gondii seroprevalence in an intermediate host species is already low, our results suggest that further reduction in the infection pressure will not necessarily decrease seroprevalence in those species. Instead, our results suggest that reductions in T. gondii infection pressure, intended to reduce infections, may be most effective and applicable to species that are known to experience high rates of infection.

Our data raise 2 additional questions. (1) In addition to T. gondii infection pressure, what drives seroprevalence in intermediate host species within our sampled regions? (2) Are the sampled species important to the epidemiology of T. gondii within the sampled regions? For kangaroos, wallabies, and koalas, T. gondii seroprevalence values and the importance of these species to the epidemiology of T. gondii within our sampled regions were discussed in detail by Taggart et al. (2019b) and Taggart et al. (2019c). However, rodent seroprevalence values are yet to be discussed.

Both mice and rats in our study experienced a low seroprevalence of T. gondii, even within our region of known high infection pressure. As seroprevalence, in general, is known to be driven by both the incidence of infection and duration of seroconversion in a species (Dohoo et al., 2009), it is likely that both ecological and physical traits of the mice and rats sampled contributed to the low T. gondii seroprevalence observed. Both of these species would be expected to spend a large proportion of their time foraging at or below ground level and could therefore ingest T. gondii oocysts in contaminated soil (Gleeson and Van Rensburg, 1982). However, both species are small, have small total energy requirements, and consume small total volumes of food. This would be expected to reduce the incidence of infection that these species would experience (Afonso et al., 2007). Both species are also short-lived (≤1 yr), may suffer mortality or morbidity from toxoplasmosis, or may have an increased risk of predation due to a reduction in their fear response from latent toxoplasmosis, all of which would be expected to reduce the duration of seroconversion that they experience (Matthewson et al., 1994; Dubey, 1996, 2006; White et al., 1996; Berdoy et al., 2000; Vyas et al., 2007; Boillat et al., 2020).

While there are several factors that make it logical for rodents to experience low T. gondii seroprevalence, large variability in seroprevalence in rodents is known to occur (Galeh et al., 2020). Our results are additionally consistent with others on islands where T. gondii infection pressure is known to be high but low seroprevalence values have been recorded in local rodent populations (Dubey et al., 2006; Murata et al., 2018). This may suggest that high infection pressure combined with short species generation times may facilitate rapid evolution and drive such species towards increased resistance to T. gondii infection and consequently a lower observed seroprevalence. While we are not aware of evidence to this effect for T. gondii, we suggest it would be worthy of further investigation in light of rapid evolutionary changes suggested in other species following intense selection pressures (Jolly et al., 2018; Jolly and Phillips, 2020).

Even in the instance that rodents experience a low T. gondii seroprevalence, recent simulations suggest that rodents are still highly important to the epidemiology of T. gondii due largely to the frequency with which they are consumed by felids (Taggart et al., 2020a). For example, the authors suggest that if felids consume an average of 1 rodent per day, then a T. gondii seroprevalence of only 0.2% (1/500 positive) in rodents will cause 51.9% of felids to be exposed to T. gondii annually.

Our study highlights the fact that T. gondii infection pressure is necessary, but not sufficient by itself, to explain seroprevalence in intermediate host species. This suggests that seroprevalence is strongly driven by factors other than infection pressure. When seroprevalence is already low, reductions in infection pressure may not achieve any further noticeable reduction in seroprevalence. Rather, reductions in T. gondii infection pressure intended to reduce infections may be most effective and applicable to species that are known to experience high rates of infection.

ACKNOWLEDGMENTS

The authors assert all applicable international, national, and/or institutional guidelines for the care and use of animals were followed. This work was supported by The Schultz Foundation; Australian Wildlife Society; Nature Foundation of South Australia; Sir Mark Mitchell Foundation; the Holsworth Wildlife Research Endowment; and the Ecological Society of Australia. Thanks go to Randall Neale from Randall Neale Concrete for providing accommodation while staying on Kangaroo Island. Thanks also go to staff from Natural Resources Mt. Lofty Ranges, Natural Resources Kangaroo Island, and Biosecurity South Australia for helping to initiate contact with landholders, loaning field equipment, and assisting with fieldwork. Thanks are extended to volunteers and landholders who helped with fieldwork or provided access to their properties. We thank Dr. Damian Collins for statistical support and discussions. Research ethics for the sampling of all mammals was granted through the University of Adelaide Office of Research Ethics, Compliance and Integrity (permit number S-2016-149).

LITERATURE CITED

1.

Abdi, H. 2007. Bonferroni and Šidák corrections for multiple comparisons. In Encyclopedia of Measurement and Statistics, Vol. 3, N. Salkind (ed.). Sage, Thousand Oaks, California, p. 103–107. Google Scholar

2.

Afonso, E., P. Thulliez, D. Pontier, and E. Gilot-Fromont. 2007. Toxoplasmosis in prey species and consequences for prevalence in feral cats: Not all prey species are equal. Parasitology 134: 1963–1971. Google Scholar

3.

Aramini, J. J., C. Stephen, J. Dubey, C. Engelstoft, H. Schwantje, and C. Ribble. 1999. Potential contamination of drinking water with Toxoplasma gondii oocysts. Epidemiology and Infection 122: 305–315. Google Scholar

4.

Bengsen, A., J. Butler, and P. Masters. 2011. Estimating and indexing feral cat population abundances using camera traps. Wildlife Research 38: 732–739. Google Scholar

5.

Berdoy, M., J. P. Webster, and D. Macdonald. 2000. Fatal attraction in rats infected with Toxoplasma gondii. Proceedings of the Royal Society of London B: Biological Sciences 267: 1591–1594. Google Scholar

6.

Berger, S., and GIDEON INFORMATICS. 2010. Toxoplasmosis: Global Status 2010 edition. Gideon Informatics, Inc., Los Angeles, California, 92 p. Google Scholar

7.

Boillat, M., P.-M. Hammoudi, S. K. Dogga, S. Pagès, M. Goubran, I. Rodriguez, and D. Soldati-Favre. 2020. Neuroinflammation-associated aspecific manipulation of mouse predator fear by Toxoplasma gondii. Cell Reports 30: 320–334e6. https://doi.org/10.1016/j.celrep.2019.12.2019. Google Scholar

8.

Burnham, K. P., and D. R. Anderson. 2002. Model Selection and Multimodel Inference: A Practical Information-Theoretic Approach. Springer Science & Business Media, New York, New York, 512 p. Google Scholar

9.

Campbell, I. 2007. Chi-squared and Fisher–Irwin tests of two-by-two tables with small sample recommendations. Statistics in Medicine 26: 3661–3675. Google Scholar

10.

Canfield, P., W. Hartley, and J. Dubey. 1990. Lesions of toxoplasmosis in Australian marsupials. Journal of Comparative Pathology 103: 159–167. Google Scholar

11.

Dard, C., S. Bailly, T. Drouet, H. Fricker-Hidalgo, M. Brenier-Pinchart, and H. Pelloux. 2017. Long-term sera storage does not significantly modify the interpretation of toxoplasmosis serologies. Journal of Microbiological Methods 134: 38–45. Google Scholar

12.

Desmonts, G., and J. S. Remington. 1980. Direct agglutination test for diagnosis of Toxoplasma infection: Method for increasing sensitivity and specificity. Journal of Clinical Microbiology 11: 562–568. Google Scholar

13.

Dohoo, I. R., W. Martin, and H. Stryhn. 2009. Measures of disease frequency. In Veterinary Epidemiologic Research, 2nd edition, S. M. Mcpike (ed.). VER Inc., Charlottetown, Prince Edward Island, Canada, p. 74–91. Google Scholar

14.

Dubey, J. P. 1996. Pathogenicity and infectivity of Toxoplasma gondii oocysts for rats. Journal of Parasitology 82: 951–956. Google Scholar

15.

Dubey, J. P. 1998. Toxoplasma gondii oocyst survival under defined temperatures. Journal of Parasitology 84: 862–865. Google Scholar

16.

Dubey, J. P. 2006. Comparative infectivity of oocysts and bradyzoites of Toxoplasma gondii for intermediate (mice) and definitive (cats) hosts. Veterinary Parasitology 140: 69–75. Google Scholar

17.

Dubey, J. P. 2009a. Toxoplasmosis in sheep—The last 20 years. Veterinary Parasitology 163: 1–14. Google Scholar

18.

Dubey, J. P. 2009b. General biology. In Toxoplasmosis of Animals and Humans, 1st ed. CRC Press, London, U.K., p. 1–73. Google Scholar

19.

Dubey, J. P. 2016. Toxoplasmosis of Animals and Humans, 2nd ed. CRC Press, Boca Raton, Florida, 340 p. Google Scholar

20.

Dubey, J. P., M. Bhaiyat, C. N. L. Macpherson, C. De Allie, A. Chikweto, O. C. H. Kwok, and R. Sharma. 2006. Prevalence of Toxoplasma gondii in rats (Rattus norvegicus) in Grenada, West Indies. Journal of Parasitology 92: 1107–1108. Google Scholar

21.

Dubey, J. P., and C. Crutchley. 2008. Toxoplasmosis in wallabies (Macropus rufogriseus and Macropus eugenii): Blindness, treatment with atovaquone, and isolation of Toxoplasma gondii. Journal of Parasitology 94: 929–933. Google Scholar

22.

Dubey, J. P., and G. Desmonts. 1987. Serological responses of equids fed Toxoplasma gondii oocysts. Equine Veterinary Journal 19: 337–339. Google Scholar

23.

Epiphanio, S., L. Sá, J. Catao-Dias, and R. Teixeira. 2001. Toxoplasmosis in a wild-caught black lion tamarin (Leontopithecus chrysopygus). Veterinary Record 149: 627–628. Google Scholar

24.

Fancourt, B. A., and R. B. Jackson. 2014. Regional seroprevalence of Toxoplasma gondii antibodies in feral and stray cats (Felis catus) from Tasmania. Australian Journal of Zoology 62: 272–283. Google Scholar

25.

Francisco, C. C., G. S. Howarth, and A. L. Whittaker. 2015. Effects on animal wellbeing and sample quality of 2 techniques for collecting blood from the facial vein of mice. Journal of the American Association for Laboratory Animal Science 54: 76–80. Google Scholar

26.

Frenkel, J., and J. P. Dubey. 1973. Effects of freezing on the viability of Toxoplasma oocysts. Journal of Parasitology 59: 587–588. Google Scholar

27.

Frenkel, J., A. Ruiz, and M. Chinchilla. 1975. Soil survival of Toxoplasma oocysts in Kansas and Costa Rica. American Journal of Tropical Medicine and Hygiene 24: 439–443. Google Scholar

28.

Galeh, T. M., S. Sarvi, M. Montazeri, M. Moosazadeh, M. Nakhaei, S. A. Shariatzadeh, and A. Daryani. 2020. Global status of Toxoplasma gondii seroprevalence in rodents: A systematic review and meta-analysis. Frontiers in Veterinary Science 7: 461. https://doi.org/10.3389/fvets.2020.00461. Google Scholar

29.

Gleeson, J., and P. Van Rensburg. 1982. Feeding ecology of the house mouse Mus musculus on Marion Island. South African Journal of Antarctic Research 12: 34–39. Google Scholar

30.

Gondim, L. F., J. R. Mineo, and G. Schares. 2017. Importance of serological cross-reactivity among Toxoplasma gondii, Hammondia spp., Neospora spp., Sarcocystis spp. and Besnoitia besnoiti. Parasitology 144: 851–868. Google Scholar

31.

Hill, D., and J. P. Dubey. 2002. Toxoplasma gondii: Transmission, diagnosis and prevention. Clinical Microbiology and Infection 8: 634–640. Google Scholar

32.

Hohnen, R., K. Berris, P. Hodgens, J. Mulvaney, B. Florence, B. P. Murphy, S. M. Legge, C. R. Dickman, and J. C. Woinarski. 2020. Pre-eradication assessment of feral cat density and population size across Kangaroo Island, South Australia. Wildlife Research 47: 669–676. Google Scholar

33.

Jenkins, R. B. 1985. Fleurieu Peninsula—The region. In Parks of the Fleurieu Peninsula: Draft Management Plan. National Parks and Wildlife Service, Department of Environment and Planning South Australia, Government of South Australia, Adelaide, Australia, p. 1–20. Google Scholar

34.

Johnson, A. M., H. Roberts, and P. Mcdonald. 1980. Age–sex distribution of Toxoplasma antibody in the South Australian population. Epidemiology & Infection 84: 315–320. Google Scholar

35.

Jolly, C. J., and B. L. Phillips. 2020. Rapid evolution in predator-free conservation havens and its effects on endangered species recovery. Conservation Biology 35: 383–385. Google Scholar

36.

Jolly, C. J., J. K. Webb, and B. L. Phillips. 2018. The perils of paradise: An endangered species conserved on an island loses antipredator behaviours within 13 generations. Biology Letters 14: 20180222. Google Scholar

37.

Lanyon, S., and R. O'handley. 2020. Relationship between Toxoplasma gondii seroprevalence and lamb marking in South Australian sheep flocks. Australian Veterinary Journal 98: 525–528. Google Scholar

38.

Mainar-Jaime, R., and M. Barberan. 2007. Evaluation of the diagnostic accuracy of the modified agglutination test (MAT) and an indirect ELISA for the detection of serum antibodies against Toxoplasma gondii in sheep through Bayesian approaches. Veterinary Parasitology 148: 122–129. Google Scholar

39.

Mansournia, M. A., A. Geroldinger, S. Greenland, and G. Heinze. 2018. Separation in logistic regression: Causes, consequences, and control. American Journal of Epidemiology 187: 864–870. Google Scholar

40.

Matthewson, D., R. Van Aarde, and J. Skinner. 1994. Population biology of house mice (Mus musculus L.) on sub-Antarctic Marion Island. South African Journal of Zoology 29: 99–106. Google Scholar

41.

Mckenny, L., R. O'handley, J. Kovaliski, G. Mutze, D. Peacock, and S. Lanyon. 2020. Evidence of infection with Toxoplasma gondii and Neospora caninum in South Australia: Using wild rabbits as a sentinel species. Australian Veterinary Journal 98: 380–387. Google Scholar

42.

Montazeri, M., T. M. Galeh, M. Moosazadeh, S. Sarvi, S. Dodangeh, J. Javidnia, M. Sharif, and A. Daryani. 2020. The global serological prevalence of Toxoplasma gondii in felids during the last five decades (1967–2017): A systematic review and meta-analysis. Parasites & Vectors 13: 82. https://doi.org/10. 1186/s13071-020-3954-1. Google Scholar

43.

Murata, F. H., C. K. Cerqueira-Cézar, O. C. H. Kwok, K. Tiwari, R. N. Sharma, C. Su, and J. P. Dubey. 2018. Role of rats (Rattus norvegicus) in the epidemiology of Toxoplasma gondii infection in Grenada, West Indies. Journal of Parasitology 104: 571–573. Google Scholar

44.

O'callaghan, M., J. Reddin, and D. Dehmann. 2005. Helminth and protozoan parasites of feral cats from Kangaroo Island. Transactions of the Royal Society of South Australia 129: 81–83. Google Scholar

45.

O'donoghue, P. J., M. J. Riley, and J. F. Clarke. 1987. Serological survey for Toxoplasma infections in sheep. Australian Veterinary Journal 64: 40–45. Google Scholar

46.

Parasuraman, S., R. Raveendran, and R. Kesavan. 2010. Blood sample collection in small laboratory animals. Journal of Pharmacology & Pharmacotherapeutics 1: 87–93. Google Scholar

47.

R CORE TEAM. 2020. R: A Language and Environment for Statistical Computing. R Foundation for Statistical Computing, Vienna, Austria. URL: https://www.R-project.org/ . Google Scholar

48.

Schwerdtfeger, P. 2002. Climate. In Natural History of Kangaroo Island, 2nd ed., M. Davies, C. R. Twidale, and M. J. Tyler (eds.). Royal Society of South Australia, Adelaide, Australia, p. 47–53. Google Scholar

49.

Shwab, E. K., P. Saraf, X.-Q. Zhu, D.-H. Zhou, B. M. Mcferrin, D. Ajzenberg, G. Schares, K. Hammond-Aryee, P. Van Helden, and S. A. Higgins. 2018. Human impact on the diversity and virulence of the ubiquitous zoonotic parasite Toxoplasma gondii. Proceedings of the National Academy of Sciences of the United States of America 115: E6956–E6963. https://doi.org/10.1073/pnas.1722202115. Google Scholar

50.

Tagel, M., B. Lassen, A. Viltrop, and P. Jokelainen. 2019. Large-scale epidemiological study on Toxoplasma gondii seroprevalence and risk factors in sheep in Estonia: Age, farm location, and breed associated with seropositivity. Vector-Borne and Zoonotic Diseases 19: 421–429. Google Scholar

51.

Taggart, P. L., C. G. B. Caraguel, and M. M. Mcallister. 2020a. Fractional seroprevalence rates in common prey species can cause more than half of feral cats to be exposed to Toxoplasma gondii annually. Veterinary Parasitology 288: 109306. https://doi.org/10.1016/j.vetpar.2020.109306. Google Scholar

52.

Taggart, P. L., B. A. Fancourt, A. J. Bengsen, D. E. Peacock, P. Hodgens, J. L. Read, M. M. Mcallister, and C. G. B. Caraguel. 2019a. Evidence of significantly higher island feral cat abundance compared to the adjacent mainland. Wildlife Research 46: 378–385. Google Scholar

53.

Taggart, P. L., B. A. Fancourt, J. Fabijan, D. E. Peacock, K. N. Speight, C. G. B. Caraguel, and M. M. Mcallister. 2019b. No evidence of Toxoplasma gondii exposure in South Australian koalas (Phascolartos cinereus). Journal of Parasitology 105: 638–641. Google Scholar

54.

Taggart, P. L., B. A. Fancourt, D. E. Peacock, C. G. B. Caraguel, and M. M. Mcallister. 2019c. Variation in Toxoplasma gondii seroprevalence: Effects of site, sex, species and behaviour between insular and mainland macropods. Wildlife Research 47: 540–546. Google Scholar

55.

Taggart, P. L., M. M. Mcallister, D. Rutley, and C. G. B. Caraguel. 2020b. Oesophageal sarcocystosis observed at slaughter provides a reliable and efficient proximate measure of Toxoplasma gondii seroprevalence in sheep. Australian Veterinary Journal 98: 305–311. Google Scholar

56.

Vyas, A., S.-K. Kim, N. Giacomini, J. C. Boothroyd, and R. M. Sapolsky. 2007. Behavioral changes induced by Toxoplasma infection of rodents are highly specific to aversion of cat odors. Proceedings of the National Academy of Sciences of the United States of America 104: 6442–6447. Google Scholar

57.

White, R., D. Kennaway, and R. Semark. 1996. Reproductive seasonality of the bush rat (Rattus fuscipes greyi) in South Australia. Wildlife Research 23: 317–331. Google Scholar

58.

Yilmaz, S. M., and S. H. Hopkins. 1972. Effects of different conditions on duration of infectivity of Toxoplasma gondii oocysts. Journal of Parasitology 58: 938–939. Google Scholar

59.

Zulpo, D. L., A. S. Sammi, J. R. Dos Santos, J. P. Sasse, T. A. Martins, A. F. Minutti, S. T. Cardim, L. D. De Barros, I. T. Navarro, and J. L. Garcia. 2018. Toxoplasma gondii: A study of oocyst re-shedding in domestic cats. Veterinary Parasitology 249: 17–20. Google Scholar

Citation Download Citation

Patrick L. Taggart, Bronwyn A. Fancourt, Wayne S. J. Boardman, David E. Peacock, and Charles G. B. Caraguel "Infection Pressure is Necessary, but not Sufficient by Itself, to Explain Toxoplasma gondii Seroprevalence in Intermediate Host Species," Journal of Parasitology 107(4), 554-561, (16 July 2021). https://doi.org/10.1645/21-28

Published: 16 July 2021

Access the abstract

JOURNAL ARTICLE
8 PAGES

DOWNLOAD PAPER + SAVE TO MY LIBRARY