Volume 30, Number 3—March 2024
Dispatch
Potentially Zoonotic Enteric Infections in Gorillas and Chimpanzees, Cameroon and Tanzania
Abstract
Despite zoonotic potential, data are lacking on enteric infection diversity in wild apes. We employed a novel molecular diagnostic platform to detect enteric infections in wild chimpanzees and gorillas. Prevalent Cryptosporidium parvum, adenovirus, and diarrheagenic Escherichia coli across divergent sites and species demonstrates potential widespread circulation among apes in Africa.
The close phylogenetic relationship between humans and great apes results in similarities in infection susceptibility and a high potential for pathogen exchange (1,2). Despite this zoonotic potential, previous studies of wild great apes have targeted specific infections (3,4), failing to establish baselines of the diversity of potentially zoonotic infections in these species. To improve our understanding of which enteric infections great apes are exposed to, we examined biobanked fecal samples from 2 biogeographically and phylogenetically divergent wild great ape species in Africa for an array of viral, parasitic, and bacterial enteric targets using a novel real-time PCR diagnostic platform.
During December 2011–January 2012, a total of 58 fecal samples from critically endangered Cross River gorillas (Gorilla gorilla diehli) were noninvasively collected from nest sites and along trails from 2 sites in Cameroon, as detailed in Arandjelovic et al. (5). Sampled gorillas experienced infrequent overlap with humans engaged in research or extraction of nontimber forest products (5). Fecal DNA extract and microsatellite genotyping identified individual gorilla sample donors, confirming repeated sampling of 18 gorillas: 10 from Kagwene Gorilla Sanctuary (≈50% of population) and 8 from Mone River Forest Reserve (≈35%–40% of population) (5). Given that serial sampling can increase chances that an individual tests positive for a target (6), only the first sample collected from each gorilla was screened.
During September 2016–February 2018, fecal samples were noninvasively collected from each of 56 individually recognized endangered eastern chimpanzees (Pan troglodytes schweinfurthii) (≈50% of population) from Gombe National Park, Tanzania, as detailed in Wroblewski et al. (7). Sampled chimpanzees experienced daily overlap with humans engaged in research and tourism following best practices to reduce the risk for pathogen exchange (2) and experienced infrequent overlap with humans when consuming crops at the boundary of the protected area (8). Fecal DNA extract and microsatellite genotyping were used to identify individual chimpanzee sample donors (7).
For all apes sampled, fresh fecal samples were preserved upon collection in Ambion RNAlater (MilliporeSigma, https://www.sigmaaldrich.com) and stored at −20°C until shipping to the United States, where they were stored at −80°C until thawed for extraction. In December 2019, we used the TaqMan Array Card (ThermoFisher Scientific, https://www.thermofisher.com), a novel real-time PCR testing platform, to screen ape fecal samples for 39 unique enteric pathogen targets (Appendix). Targets were pathogen-specific genes associated with either virulence or biology (i.e., specific outer membrane protein genes or housekeeping genes). As detailed in Diaz et al. (8), we extracted DNA and RNA from each fecal specimen using a Roche MagNA Pure Compact magnetic bead Total Nucleic Acid Kit (Roche, https://www.roche.com). For preprocessing, we incubated sample, lysis buffer, and proteinase (56°C, 15 minutes) before 2 cycles on Precellys bead-beater (Bertin Technologies, https://www.bertin-technologies.com) at 5,000 rpm for 60 seconds. We assayed extracts using the Applied Biosystems ViiA7 Real-Time PCR system (ThermoFisher Scientific) with the following cycling conditions: 45°C for 10 minutes, 94°C for 10 minutes, 45 cycles of 94°C for 30 seconds, and 60°C for 60 seconds (8). For validation, we spiked fecal samples with known DNA/RNA concentrations. We evaluated sensitivity with spiked dilution series and specificity through BLAST (https://blast.ncbi.nlm.nih.gov/Blast.cgi) then isolate panel representing targeted organisms. We evaluated exclusivity using nucleic acid from closely related species.
Analyses confirmed presence of nucleic acids of >1 enteric pathogen target in 15 (83%) of the 18 gorillas and 39 (70%) of the 56 chimpanzees. We detected 7 pathogen targets among gorillas (Table 1) and 13 among chimpanzees (Table 2). Adenovirus and Cryptosporidium parvum were the most common pathogen targets detected in both gorillas and chimpanzees, occurring in 33% (95% CI 10%–57%) (adenovirus) and 39% (95% CI 15%–62%) (C. parvum) of gorillas and 52% (95% CI 39%–65%) (adenovirus) and 13% (95% CI 4%–21%) (C. parvum) of chimpanzees. Both adenovirus and C. parvum had previously been detected in wild great ape populations and have received attention, given their zoonotic potential (9,10).
Real-time PCR testing of noninvasively collected wild gorilla and chimpanzee fecal samples from Cameroon and Tanzania provided evidence of widespread enteric infections and demonstrates their potential circulation in ape populations in Africa before 2018. Several pathogen targets detected in the ape species are highly relevant to humans, including those commonly associated with diarrheal disease, such as diarrheagenic E. coli, adenovirus, Shigella spp., Giardia spp., and enterovirus. As human–nonhuman primate contact increases in tropical forest communities, opportunities will continue to arise for both anthroponotic and zoonotic exchange and exposure (11).
Adenoviruses and Cryptosporidium species infect a broad range of hosts (including humans and nonhuman primates), can cause mild to severe disease, and are also associated with high rates of illness and death in children and immunocompromised persons, especially in developing countries (12). Although the pathogenesis of those organisms is less understood in nonhuman primate populations, they are of major zoonotic importance, given the increasing overlap between humans and wild primates and high HIV/AIDS prevalence in humans in regions inhabited by primate populations. Furthermore, because C. parvum and adenoviruses can spread through the fecal–oral route and persist in the environment for extended periods, diverse opportunities exist for direct and indirect transmission between humans and great apes (e.g., tourism and research activities, crop-raiding by apes, and events related to humans living in close proximity to parks).
Of note, many of the observed simian adenoviruses show high degrees of sequence relatedness to human strains, suggesting evidence of past cross-species transmission events and potential risk for such events in the future (10). Differentiating between strains was beyond the scope of this study, but the high detection rate of this viral target and its zoonotic potential warrants further characterization of this viral group and continued surveillance of great ape populations.
The first limitation of our study is that, because of logistical challenges and budgetary constraints, we were only able to focus our surveillance on 2 populations of great apes at specific points in time. In addition, sex and age classes sampled were representative of each ape population apart from infants, which are nearly impossible to sample noninvasively.
Despite those challenges, our data provide insight into the diversity of enteric infections circulating in wild gorilla and chimpanzee populations before 2018. Detection of gene targets of zoonotic potential in 83% of gorillas and 70% of chimpanzees suggests potential health and disease transmission risks. These results are especially pertinent for monitoring these ape species given the previously documented cases of disease and epizootics (e.g., respiratory infections, polio, mange) in Gombe (13), and the lack of such in Cross River gorilla populations. As research, ecotourism, and forest encroachment in wild ape habitat increases, the risk for novel pathogen exposure is heightened, which could have catastrophic impacts on populations. Continued epidemiologic research among wild primate populations has the potential to predict which pathogens might enter both human and great ape populations as contact between species intensifies. Because pathogen exchange occurs across species boundaries, the potential for changes in pathogenicity and host specificity exists, which could have substantial adverse effects on human and wildlife health (14,15).
Ms. Strahan is a recent graduate of the department of environmental sciences at Emory University in Atlanta, Georgia. Her primary research interests relate to wildlife diseases and their implications for public health.
Acknowledgments
We thank the Government of Cameroon and the Ministry of Forests and Wildlife for granting permission to conduct research at Kagwene Gorilla Sanctuary and Mone River Forest Reserve. We thank the Government of Tanzania, TANAPA, TAWIRI, and COSTECH for permission to conduct research in Gombe National Park. We thank the Wildlife Conservation Society and Working Dogs for Conservation for logistical assistance in Cameroon and the Jane Goodall Institute and the staff of the Gombe Stream Research Center for logistical support in Tanzania. We thank A. Hurt and N. Richards for technical assistance, B. Hahn for providing samples, and J. Clennon, M. Diaz, M. Parsons, and J. Winchell for helpful discussion and feedback on an earlier draft of this manuscript.
This work was funded by the National Institutes of Health (grants R01 AI58715, R00 HD057992), the National Institutes of Health National Institute on Aging (grant R37-AG049395), the US Fish and Wildlife Great Ape Conservation Fund, the Arcus Foundation, the North Carolina Zoo, the Wildlife Conservation Society, a Robert W. Woodruff Foundation Synergy II Award, and the James G. Lester Fund of Emory University.
References
- Calvignac-Spencer S, Leendertz SAJ, Gillespie TR, Leendertz FH. Wild great apes as sentinels and sources of infectious disease. Clin Microbiol Infect. 2012;18:521–7. DOIPubMedGoogle Scholar
- Gilardi KV, Gillespie TR, Leendertz FH, Macfie EJ, Travis DA, Whittier CA, et al. Best practice guidelines for health monitoring and disease control in great ape populations. Gland, Switzerland: IUCN SSC Primate Specialist Group; 2015.
- Mubemba B, Chanove E, Mätz-Rensing K, Gogarten JF, Düx A, Merkel K, et al. Yaws disease caused by Treponema pallidum subspecies pertenue in wild chimpanzee, Guinea, 2019. Emerg Infect Dis. 2020;26:1283–6. DOIPubMedGoogle Scholar
- Scully EJ, Basnet S, Wrangham RW, Muller MN, Otali E, Hyeroba D, et al. Lethal respiratory disease associated with human rhinovirus C in wild chimpanzees, Uganda, 2013. Emerg Infect Dis. 2018;24:267–74. DOIPubMedGoogle Scholar
- Arandjelovic M, Bergl RA, Ikfuingei R, Jameson C, Parker M, Vigilant L. Detection dog efficacy for collecting faecal samples from the critically endangered Cross River gorilla (Gorilla gorilla diehli) for genetic censusing. R Soc Open Sci. 2015;2:
140423 . DOIPubMedGoogle Scholar - Miller IF, Schneider-Crease I, Nunn CL, Muehlenbein MP. Estimating infection prevalence: Best practices and their theoretical underpinnings. Ecol Evol. 2018;8:6738–47. DOIPubMedGoogle Scholar
- Wroblewski EE, Norman PJ, Guethlein LA, Rudicell RS, Ramirez MA, Li Y, et al. Signature patterns of MHC diversity in three Gombe communities of wild chimpanzees reflect fitness in reproduction and immune defense against SIVcpz. PLoS Biol. 2015;13:
e1002144 . DOIPubMedGoogle Scholar - Diaz MH, Waller JL, Theodore MJ, Patel N, Wolff BJ, Benitez AJ, et al. Development and implementation of multiplex TaqMan Array Cards for specimen testing at Child Health and Mortality Prevention Surveillance site laboratories. Clin Infect Dis. 2019;69(Suppl 4):S311–21. DOIPubMedGoogle Scholar
- Parsons MB, Travis D, Lonsdorf EV, Lipende I, Roellig DMA, Collins A, et al. Epidemiology and molecular characterization of Cryptosporidium spp. in humans, wild primates, and domesticated animals in the Greater Gombe Ecosystem, Tanzania. PLoS Negl Trop Dis. 2015;9:
e0003529 . DOIPubMedGoogle Scholar - Wevers D, Metzger S, Babweteera F, Bieberbach M, Boesch C, Cameron K, et al. Novel adenoviruses in wild primates: a high level of genetic diversity and evidence of zoonotic transmissions. J Virol. 2011;85:10774–84. DOIPubMedGoogle Scholar
- Estrada A, Garber PA, Rylands AB, Roos C, Fernandez-Duque E, Di Fiore A, et al. Impending extinction crisis of the world’s primates: Why primates matter. Sci Adv. 2017;3:
e1600946 . DOIPubMedGoogle Scholar - Kotloff KL, Nataro JP, Blackwelder WC, Nasrin D, Farag TH, Panchalingam S, et al. Burden and aetiology of diarrhoeal disease in infants and young children in developing countries (the Global Enteric Multicenter Study, GEMS): a prospective, case-control study. Lancet. 2013;382:209–22. DOIPubMedGoogle Scholar
- Lonsdorf EV, Travis DA, Raphael J, Kamenya S, Lipende I, Mwacha D, et al. The Gombe Ecosystem Health Project: 16 years of program evolution and lessons learned. Am J Primatol. 2022;84:
e23300 . DOIPubMedGoogle Scholar - Baker RE, Mahmud AS, Miller IF, Rajeev M, Rasambainarivo F, Rice BL, et al. Infectious disease in an era of global change. Nat Rev Microbiol. 2022;20:193–205. DOIPubMedGoogle Scholar
- Brook CE, Boots M, Chandran K, Dobson AP, Drosten C, Graham AL, et al. Accelerated viral dynamics in bat cell lines, with implications for zoonotic emergence. eLife. 2020;9:
e48401 . DOIPubMedGoogle Scholar
Tables
Cite This ArticleOriginal Publication Date: February 13, 2024
Table of Contents – Volume 30, Number 3—March 2024
| EID Search Options |
|---|
Advanced Article Search – Search articles by author and/or keyword.
|
Articles by Country Search – Search articles by the topic country.
|
Article Type Search – Search articles by article type and issue.
|
Please use the form below to submit correspondence to the authors or contact them at the following address:
Thomas R. Gillespie, Departments of Environmental Sciences and Environmental Health, Emory University and Rollins School of Public Health, 400 Dowman Dr, Ste E510, Atlanta, GA 30322, USA
Top