Hostname: page-component-586b7cd67f-tf8b9 Total loading time: 0 Render date: 2024-11-23T08:55:26.412Z Has data issue: false hasContentIssue false
  • English
  • Français

Rabies outbreak in black-backed jackals (Canis mesomelas), South Africa, 2016

Published online by Cambridge University Press:  07 January 2022

E. Ngoepe ,
J. G. Chirima ,
D. Mohale ,
K. Mogano ,
T. Suzuki ,
K. Makita Open the ORCID record for K. Makita [Opens in a new window]  and
C. T. Sabeta Open the ORCID record for C. T. Sabeta [Opens in a new window]
E. Ngoepe
Affiliation:
Agricultural Research Council, Onderstepoort Veterinary Institute, Onderstepoort, 0110, Pretoria, Gauteng, South Africa
J. G. Chirima
Affiliation:
GeoInformation Science Division, Agricultural Research Council, Institute for Soil, Climate and Water 600, Belvedere St, Arcadia, Pretoria, Gauteng, South Africa Department of Geography, Geoinformatics and Meteorology, Centre for Geoinformation Science, University of Pretoria, Pretoria, Gauteng, South Africa
D. Mohale
Affiliation:
Agricultural Research Council, Onderstepoort Veterinary Institute, Onderstepoort, 0110, Pretoria, Gauteng, South Africa
K. Mogano
Affiliation:
GeoInformation Science Division, Agricultural Research Council, Institute for Soil, Climate and Water 600, Belvedere St, Arcadia, Pretoria, Gauteng, South Africa Department of Geography, Geoinformatics and Meteorology, Centre for Geoinformation Science, University of Pretoria, Pretoria, Gauteng, South Africa
T. Suzuki
Affiliation:
Department of Veterinary Medicine, School of Veterinary Medicine, Rakuno Gakuen University, 582 Bunkyodai Midorimachi, Ebetsu, Hokkaido, 069-8501, Japan
K. Makita
Affiliation:
Department of Veterinary Medicine, School of Veterinary Medicine, Rakuno Gakuen University, 582 Bunkyodai Midorimachi, Ebetsu, Hokkaido, 069-8501, Japan
C. T. Sabeta*
Affiliation:
Agricultural Research Council, Onderstepoort Veterinary Institute, Onderstepoort, 0110, Pretoria, Gauteng, South Africa Veterinary Tropical Diseases, University of Pretoria, Onderstepoort, 0110, Pretoria, Gauteng, South Africa
*
Author for correspondence: C. T. Sabeta, E-mail: [email protected]
Rights & Permissions [Opens in a new window]

Abstract

Rabies, a fatal and vaccine-preventable disease, is endemic throughout Africa. In 2016, a rabies outbreak occurred in black-backed jackals (Canis mesomelas) along the western boundary of Gauteng Province, South Africa. We investigated the possible drivers of the 2016 outbreak and established its origin. Using spatio-temporal locations of cases, we applied logistic regression and Geographic Information System techniques to investigate environmental covariates driving occurrences of emerging rabies cases in Gauteng Province. About 53.8% of laboratory-confirmed lyssaviruses in Gauteng Province in 2016 originated from jackals. Phylogenetic trees reconstructed from a partial region of the glycoprotein gene of these and historical rabies viruses (RABVs) demonstrated the lyssaviruses to be of canid origin with 97.7% nucleotide sequence similarity. The major cluster comprised jackal RABVs from the 2012 KwaZulu/Natal outbreak and the 2016 outbreak in Gauteng Province. The second cluster was composed of both jackal and dog RABVs. Both clusters correlated with independent RABV introductions into Gauteng by dogs and jackals, respectively. This study demonstrated an expansion of a jackal rabies cycle from north-west Province into Gauteng Province during the 2016 dry period, as jackals ranged widely in search for food resources leading to increased jackal-dog interactions, reminiscent of the intricate links of domestic and wildlife rabies cycles in South Africa.

Keywords

Black-backed jackalC. mesomelascross-species transmissionLyssavirusesrabiesSouth Africa
Type
Original Paper
Information
Epidemiology & Infection , Volume 150 , 2022 , e137
Check for updates
Creative Commons
Creative Common License - CCCreative Common License - BY
This is an Open Access article, distributed under the terms of the Creative Commons Attribution licence (http://creativecommons.org/licenses/by/4.0/), which permits unrestricted re-use, distribution and reproduction, provided the original article is properly cited.
Copyright
Copyright © Agricultural Research Council of South Africa 2022. Published by Cambridge University Press

Introduction

Rabies virus (RABV), is a prototype species of the Lyssavirus genus (Rhabdoviridae family, order Mononegavirales), and currently consists of 17 viral species [1]. In addition, Kotalahti bat lyssavirus (KBLV), a putative species discovered in a Brandt's bat (Myotis brandtii) in Finland, is still awaiting formal classification [Reference Kokkonen2]. All lyssaviruses are capable of causing an encephalitic disease in all warm-blooded vertebrates. The domestic dog (Canis familiaris) is the primary vector species for rabies and is responsible for at least 59 000 human deaths annually [Reference Hampson3], with the majority (⩾95%) of these deaths occurring in the low endemic countries of Africa and Asia [4, Reference Knobel5]. Rabies is a neglected and re-emerging zoonosis in specific regions of Africa and Asia, and poses a significant public health problem in these geographical areas [Reference Fooks6, Reference Rupprecht7]. In the rabies endemic regions of Africa and Asia, the disease is highly under-reported primarily due to inadequate diagnostic facilities and the long distances specimens have to be transported to reach the diagnostic facilities [Reference Knobel5, Reference Fooks6]. Unlike in Africa, in Europe and North America, rabies was eliminated through parenteral dog vaccination [Reference Tolson8, Reference Mähl9]. However, the disease is still endemic in some wildlife species [such as red foxes (Vulpes vulpes) and raccoon dogs (Nyctereutes procyonoides)] in some European countries [Reference Tolson8, Reference Mähl9].

In South Africa, rabies cycles are maintained by both domestic and wildlife host species in specific geographical regions of the country. Cross-species transmission events (CSTEs), between domestic dogs and two wildlife host species, the black-backed jackals and the bat-eared fox Otocyon megalotis, facilitate the ease of exchange of canid RABVs in the northern and western regions of South Africa [Reference Bingham10Reference Sabeta16]. On the Highveld plateau of the Free State province of South Africa, mongoose rabies, believed to be indigenous to the sub-region, and introduced over 200 years ago, is maintained by a diverse group of members of the Herpestidae family [Reference Nel17]. The presence of two independent rabies cycles of the canid and mongoose rabies biotypes is unique and complicates rabies epidemiology in the country [Reference Sabeta16]. However, mongoose rabies does not appear to pose much of a public health threat compared to canid rabies [Reference Nel17]. Recent trends analyses from the Onderstepoort Records seem to suggest that the aardwolf (Proteles cristata), a small insectivorous mammalian carnivore native to East and Southern Africa, could potentially maintain canid rabies (Onderstepoort rabies records).

RABVs originating from dogs and jackals are very closely related and highlight CSTEs of RABV variants between domestic (dogs) and wildlife host species black-backed jackals in commercial farming areas in central and north-western Limpopo [Reference Zulu15, Reference Sabeta16]. Rabies cycles are evidently maintained by both domestic dogs and black-backed jackals in specific geographical areas. The cycles are more pronounced in Zimbabwe, in communal areas adjacent to nature reserves and commercial farming areas [Reference Bingham13, Reference Bingham14, Reference Cumming18Reference Cleaveland20]. Jackal rabies (canid rabies) which originated from dogs [Reference Zulu15, Reference Sabeta16, Reference Brückner21] has been maintained in jackal species consistently for at least 50 years in northern South Africa. Similarly, in Zimbabwe, rabies epidemics in jackal species are thought to have been initiated through similar spillover events and once they were established, the epidemics were maintained by black-backed jackals [Reference Bingham14]. Incidentally, black-backed jackals were believed incapable of maintaining continuous rabies cycles because of their low population densities when compared to domestic dogs [Reference Bingham14, Reference Rhodes22, Reference Haydon23].

In South Africa, there are two testing laboratories for animal rabies, one the OIE Rabies Reference Laboratory at Onderstepoort, in Gauteng Province, and the Allerton Provincial Laboratory in Pietermaritzburg KwaZulu/Natal (KZN). Firstly, we wanted to establish rabies trends in this wildlife carnivore species in Gauteng Province and secondly, to antigenically and genetically characterise RABVs originating from the 2016 jackal rabies outbreak. Thirdly, we wanted to assess the relations between spatial and temporal rabies cases with environmental explanatory variables as a way to identify risk factors in historically unrecorded areas, and finally, we wanted to reconstruct phylogenetic relationships of the RABVs from the 2016 outbreak together with previously characterised viruses from other wildlife and domestic host species.

Materials and methods

Specimens

Specimens from a variety of central nervous system tissues, mostly in the form of intact brain tissues obtained in 2016 through the national rabies surveillance programme, were submitted to the Agricultural Research Council-Onderstepoort Veterinary Institute (ARC-OVI) for lyssavirus diagnosis (Fig. 1, Table 1). In terms of the Animal Disease Act of the Republic of South Africa (Act 35 of 1984), rabies is a controlled disease. By law, a controlled animal disease is a disease that must be reported to the nearest state veterinarian and control measures must be prescribed for its control. Hence, any procedures for collecting specimens including euthanising animals to enable laboratory diagnosis of the specimens, are vested in the state veterinarian through the Act.

Fig. 1. Jackal cases for the periods 2013–2014, 2015–2016 and 2017.

Table 1. Epidemiological information of RABVs genetically characterised in this study

A total of 190 brain specimens originating from both domestic and wildlife host species were received. These included specimens from domestic dogs (Canis familiaris) (n = 71, 37.4%), bovines (Bos taurus) (n = 11; 5.8%), domestic cats (Felis catus) (n = 31; 16.3%), mongooses and other Herpestidae species (n = 17; 8.9%), black-backed jackal species (n = 39; 20.5%), unidentified bat species (Chiroptera) (n = 2; 1.1%), ovines (Ovis aries) (n = 2; 1.1%), equines (Equus caballus) (3; 1.6%) and baboons (Papio ursinus) (n = 2; 1.1%). The remainder (n = 12) were from honey badgers (Mellivora capensis) (n = 2), mice (Mus musculus) (n = 3), one each from a porcine (Suidae), rabbit (Oryctolagus cuniculus), rat (Rattus rattus), kudu (Tragelaphus strepsiceros), warthog (Phacochoerus africanus), impala (Aepyceros melampus) and sable antelope (Hippotragus niger).

Primary rabies diagnosis

All the specimens including a positive and negative control, were tested using the direct fluorescent antibody (DFA) test described previously [Reference Dean, Meslin, Kaplan and Koprowski24]. After staining, the slides were examined under ultra-violet fluorescence (Zeiss, Germany). The results of the DFA were recorded as positive [on a scale from + 1 (lyssavirus antigen present in 25% of the fields of the examined smear) to + 4 (lyssavirus antigen present in 100% of fields of the examined smear)] or negative (–).

Antigenic typing

Antigenic typing of the lyssaviruses was performed using a panel of 16 murine anti-lyssavirus nucleocapsid monoclonal antibodies (anti-N Mabs), a donation kindly provided by Dr Christine-Fehlner Gardiner (Centre of Expertise for Rabies, Canadian Food Inspection Agency, Canada). The 16 anti-N Mab panel, included 14 anti-RABV nucleoprotein mAbs, an anti-human adenovirus type-5 mAb (1C5) as a negative control and positive control (38HF2). The reactivity patterns generated from this Mab panel are capable of discriminating the different southern African Lyssavirus species and antigenic variants [Reference Ngoepe25] (Table 2). Brain smears were prepared on Teflon-coated 5 mm well slides (Thermo Fisher Scientific, USA) and were acetone-fixed as per the DFA, described under primary rabies diagnosis. After staining with FITC-conjugated goat anti-mouse IgG antibody (Sigma-Aldrich, USA), the slides were blot-dried, an aqueous mounting medium added and then examined under ultra-violet microscopy (Carl Zeiss, Germany). The reactivity for each mAb was recorded as positive (on a scale from 1–3) or negative (−) for each lyssavirus to generate the overall staining pattern.

Table 2. The reactivity patterns of the rabies viruses analysed

Key: Var, Some isolates within the species react with the Mab and others do not; +++, Reactivity observed; –, No reactivity observed.

Total RNA extractions, reverse transcription PCR (RT-PCR), nucleotide sequencing and phylogenetic reconstruction

Total RNAs were extracted from approximately 100 ng of brain-infected tissues using TriReagent® (Sigma Aldrich, USA). Complementary DNA (cDNA) was synthesised using standard guidelines [Reference Sabeta26, Reference Sacramento27] and the highly variable glycoprotein and G-L intergenic region of each virus was sequenced (Table 1). The nucleotide sequences for the forward and reverse primers used in the RT-PCR, G(+) and L(−), are 46655GAC TTG GGT CTC CCG AAC TGG GG34687 & 55205CAA AGG AGA GTT GAG ATT GTA GTC35543, respectively. The annealing positions and polarity are designated according to the Pasteur Virus genome [Reference Sabeta26, Reference Sacramento27]. The primers were synthesised by Inqaba Biotechnical Industries (Pty) Ltd (Pretoria, South Africa).

In brief, approximately 1 μg of total viral RNA and G(+) primer were annealed at 70 °C. Thereafter, the RNAs were reverse-transcribed in a 20-μl reaction mixture, that consisted of 200 U of Superscript III Reverse Transcriptase (Invitrogen, USA), 5× SS III reaction buffer, 20 mm dNTP mix (Takara, Japan), 40 U RNasin RNase inhibitor of murine origin (New England Biolabs, USA), and ultrapure diethyl-pyrocarbonate (DEPC)-treated water (Invitrogen, USA). The reaction mixture was incubated at 50 °C for 50 min and then the cDNA mixture inactivated at 85 °C for 10 min.

Two microliters of cDNA were used as template in a 50 μl-PCR reaction comprising 20 pmoles each of the G(+) and L(−) primers [Reference Sabeta26, Reference Sacramento27], 20 mm dNTP mixture, 1.5 mm MgCl2, 5 ×  Taq DNA polymerase reaction buffer and 1.25 U of Takara Taq DNA polymerase (Takara, Japan). The reaction mixture was thermal-cycled starting with an initial denaturation at 94 °C for 2 min, then followed by 30 cycles of denaturation, 94 °C for 50 s, annealing 42 °C for 90s, extension 72 °C for 2 min and a final extension for 10 min. The PCR amplicons (5-μl volumes) were separated on 1% ethidium bromide-stained gels. Amplicons (45-μl volumes) were then purified using spin-columns.

The purified amplicons were sequenced bidirectionally using the reverse and forward primers and the edited nucleotide sequences aligned in ClustalW [Reference Thompson28]. Thereafter, phylogenetic trees were reconstructed using both the Neighbour-Joining (NJ) method and Maximum Likelihood, ML [Reference Kumar29] algorithms. Duplicate nucleotide sequences were removed from the analysis. The topology of the trees was validated with 1000 bootstrap replicates [Reference Hills30].

Spatio-temporal variation of rabies cases in Gauteng

To assess for spatial heterogeneity and temporal dependence of cases in Gauteng, we extracted spatially explicit environmental covariates as predictor variables: Normalised Difference Vegetation Index (NDVI) (surrogate for forage productivity and forage retention), rainfall and temperature. Then, we applied logistic regression [Reference Burnham and Anderson31] to relate these candidate predictors to rabies cases for the period 2009–2018.

Rainfall and temperature data

ArcMap 10.6 (Esri, Redlands, CA, USA) was used for all the spatial techniques described. First, a shapefile of all South African provinces was imported into, projected into Universal Transverse Mercator 1984, and then clipped to select only the area of interest, the Gauteng Province. Second, an Excel sheet of geo-locations of confirmed rabies positive cases obtained from the ARC-OVI was converted to a shapefile and overlaid on the Gauteng province shapefile to identify specific areas in the province with rabies cases (Fig. 1). Then, environmental covariates were derived for the Gauteng Province for specific locations of confirmed rabies cases and non-rabies cases.

Temperature surface maps were created for the following periods: pre-dry conditions (2009 up to 2013/2014), during dry conditions (2015–2016), and post-dry conditions (post 2017–2018). Weather station data available from the Agricultural Research Council (ARC) of South Africa and the South African Weather Services (SAWS) were obtained. Thin plate splines and regression interpolation of the weather station data as a function of latitude, longitude and elevation, was used to create climate surfaces. The mean annual temperature surface and dry season mean temperatures surface were indicative of possible heat stress and quick drying of forage.

An inverse distance weight method was applied to create a smooth surface trend on monthly rainfall using data available from the ARC and additional records from SAWS. The above rainfall surface was used to extract values of annual mean rainfall, dry season mean at a 1 km resolution. A long-term mean rainfall figure for each calendar month was extracted per weather station and a trend surface created from these monthly data using the inverse distance weight interpolation method. A spatial filter was applied to the interpolated surface to create a smooth trend surface. Then, regression analysis was applied to relate the differences between the rainfall values at a specific station and the value given by the trend surface to topographic indices such as terrain ruggedness, rain shadow, aspect, etc. The relationship and trend surface for each month were used to model a mean rainfall surface from spatial topographic indices. To obtain an annual total mean rainfall surface, the individual monthly surfaces were summed. Long-term average rainfall and temperature (monthly surfaces) for the period prior to dry conditions (2009 up to 2013/2014), during dry conditions (2015–2016), and post-dry period (post 2017–2018) were developed as predictors (Table 3).

Table 3. Comparative fit of alternative models relating to rabies cases during the period pre-dry conditions, dry conditions and post dry conditions

Models with good fit/low AIC values have an asterisk symbol (*). Models on top per each period are the most parsimonious.

Vegetation index data

The normalised vegetation index difference for the selected periods, pre-dry conditions (2009 to 2013/2014), during dry conditions (2015–2016), and post-dry period (post 2017–2018) were retrieved from PROBA V data. PROBA-V is a small satellite assuring the succession of the Vegetation instruments on board the French SPOT-4 and SPOT-5 Earth observation missions. The data were downloaded, missing data pixels removed, georeferenced and area of interest clipped using the Gauteng Province shapefile. The annual maximum, minimum and mean NDVI values were calculated for selected periods. Furthermore, monthly dry season values (May–October) were also derived.

Model fitting

We modelled the presence/absence of rabies cases as a function of environmental predictors using logistic regression [Reference Burnham and Anderson31]. For fitting all models, backward stepwise procedures in R software and the Akaike Information Criterion (AIC) were applied to assess the relative fit (R version 4.0.2 (2020-06-22) – ‘Spring Dance’ Copyright (C) 2020. The R Foundation for Statistical Computing). AIC model selection procedures provided the relative support for each individual model via comparing AIC values between the various models [Reference Hosmer and Lemeshow32]. Burnham and Anderson [Reference Burnham and Anderson31] proposed that models with delta AIC values <2 have equally good fit and in the event of several models presenting delta AIC values of <2, the model with the fewest parameters (i.e. the most parsimonious) is the best [Reference Hosmer and Lemeshow32]. Models with substantial support that could be considered candidates for the best model should be within 4–7 AIC units of the best model, and models with delta AIC values >10 are not supported.

Results

Primary rabies diagnosis

The majority of the specimens, 72.1% (n = 137) were submitted as intact brain tissues in glycerol-saline preservative, and 27.9% (n = 53) were submitted as carcasses. Two jackal specimens (695/16 & 848/16) were deemed unfit for testing. Of the 190 specimens received, 27.9% were positive for lyssavirus antigen (n = 52) and 71.6% (n = 136) were negative. More than half of the 52 positive samples (n = 28, 53.8%) were recovered from black-backed jackals. This is the highest incidence observed in this wildlife carnivore from Gauteng Province between 2010 and 2020. With the exception of two bovine samples (592/16 & 988/16), both with a + 3 grading, apple-green fluorescing viral particles typical of lyssavirus infection against a reddish background were observed in 100% of the microscopic fields of all the smears examined under UV-fluorescence. Trend analyses showed that lyssavirus antigen was laboratory-confirmed consistently in domestic dogs throughout the 10 years with up to 40 infected dogs observed during the 2010 & 2011 outbreak, and fewer than 10 infected dogs observed for each of the years from 2015 to 2018 (Fig. 2). However, many RABV positive cases were laboratory-confirmed in black-backed jackals in 2016, coinciding with the 2016 rabies outbreak in this wildlife species on the periphery of the province.

Fig. 2. Rabies trends in Gauteng, 2009–2019.

Antigenic typing

The canid RABV biotype isolates gave two different reactivity patterns, with differences in reactivity observed only with a single mAb, 32GD12 (Table 2). The majority of the jackal viruses (n = 24, 85.7%) were stained by this mAb (referred to as reactivity pattern I). Although viruses that conformed to canid biotype reactivity pattern II were less common (usually seen to react with viruses from canids from Brits and Thabazimbi located in the north-west region of South Africa, unpublished data), they exhibited a similar geographic distribution to viruses that conformed to canid biotype reactivity pattern I (Fig. 1). Spillover of infection from jackals to dogs as well as jackals to cattle was evident.

Total RNA extractions, RT-PCR, nucleotide sequencing and phylogenetic reconstruction

Phylogenetic reconstruction using nucleotide sequences of a 592-nucleotide region encompassing the cytoplasmic domain of the glycoprotein and the G-L intergenic regions of the RABVs from the 2016 outbreak and other historically sequenced RABVs demonstrated two very distinct clusters, and the nodes supporting these clusters had significantly high bootstrap values of 84% and 83% respectively. One cluster was composed exclusively of jackal RABVs (canid rabies biotype) from the 2016 outbreak as well as other viruses from the wildlife host carnivores from the North-West province. Interestingly RABVs recovered from the 2012 jackal rabies outbreak in KZN, were 97.7% nucleotide sequence identical to those from the 2016 Gauteng outbreak probably demonstrating a common progenitor. The second cluster consisted of viruses originating from wildlife (jackals, honey-badgers and a wild-cat) (sub-cluster 1 of the recent RABVs) and the other sub-cluster consisted of dog and jackal viruses (mean sequence identity of 99.6%) (Fig. 3). The topology of both the NJ and ML trees were similar (only the NJ tree is shown).

Fig. 3. Phylogenetic analysis of RABVs included in this investigation. A 592-nucleotide portion encompassing the cytoplasmic domain of the glycoprotein and the G-L intergenic regions of the virus isolates included in this study. A neighbour-joining tree of the G-L intergenic region sequences illustrating the genetic relationships of canid RABVs from Gauteng, Limpopo, North West and KwaZulu-Natal provinces respectively. The viral sequences obtained from both black-backed jackal and domestic dogs from KwaZulu-Natal are in black, Gauteng viral isolates are in red, North West province in green and Limpopo province in dark blue. The horizontal lines are proportional to the evolutionary distances between sequences and the scale bar represents nucleotide substitutions per site. Key: bbj, black-backed jackal; dog, domestic dog; bov, bovine; cat, wild cat

Rabies cases and environmental covariates

Table 3 presents models per period: pre-dry conditions, during dry conditions and post-dry conditions. Models with low AIC have an asterisk symbol (*) (i.e. AIC values <2 of best model) demonstrating evidence of good fit. Models on top per each period are the most parsimonious.

Evidence suggests that prior to the dry period of 2015–2016, although forage production was relatively high across the Gauteng Province, RABV cases were not associated with vegetation indices. Prior to the dry period (2015/2016), all models of RABV cases as a function of vegetation indices, temperature or total rainfall exhibited a poor fit (i.e. not significant) implicating other factors influencing rabies incidences. Further evidence suggests that the onset of the dry period was progressive from around 2013 onwards. After 2013, a weak but significant association of rabies cases with vegetation was becoming evident (Table 3). This relationship continued to strengthen during the drought and became even stronger after the drought (Table 3). Only models for the dry season during the drought period and post-drought period somewhat received substantial support and were closer to the best model.

Discussion

We undertook this study to establish the origin of the 2016 rabies outbreak that occurred in jackal species in Gauteng Province and to identify the possible drivers resulting in the expansion of the range of this wildlife host species. It had always been thought that Gauteng Province was a rabies-free province. However, the dog rabies outbreak in 2010 [Reference Sabeta33], representing a major outbreak arising from an imported RABV-infected dog from KZN, and more recently, the jackal rabies outbreak on the periphery of the province in 2016 (this study), dispute the notion of a rabies-free Gauteng Province. Furthermore, these outbreaks (2010, 2012 and 2016) highlight that rabies can emerge and re-emerge should environmental conditions become conducive or in areas where it has been previously under control.

Investigations of the two rabies outbreaks in Gauteng show that from the beginning of 2010 to the end of 2011, 16.5% of the specimens tested at ARC-OVI were lyssavirus positive, with the majority of the RABVs being of dog origin. One human fatality to rabies infection was reported during the 2010 outbreak and the source was traced to a dog rabies cycle from KZN [Reference Sabeta33]. Jackal rabies has historically been associated with the northern Limpopo Province and the North-West Province (Fig. 1). In 2016, jackals were observed on the periphery of Gauteng Province and characteristically displayed loss of fear for humans, a typical symptom displayed by rabid wildlife species. Jackal rabies cases were laboratory-confirmed in 53.8% of the samples tested from Gauteng in 2016. The large proportion of rabies positive cases in jackals coupled to an unprecedented dry period in the country led us to explore the exact drivers for the movement of this wildlife host species from its historical niche areas into Gauteng Province [Reference Tswai34, Reference Winkler35].

The nucleoprotein (N) is the most abundant protein produced during lyssavirus replication, making it a useful target for the diagnosis of lyssaviruses and for the differentiation of lyssavirus variants. For instance, monoclonal antibody typing detects nucleocapsid epitopes that are characteristic of particular lyssavirus species/variants (Table 2). Hence, a specific reactivity pattern defines the biotype. These antigenic types demonstrate specific events or situations including spill-over of infection and reservoir host species of a specific biotype.

In South Africa, dogs, bat-eared foxes and black-backed jackals maintain the canid rabies biotype within specific geographical zones, and consistently give homogeneous reactivity patterns different to those of the mongoose rabies biotype on antigenic typing. Previously, it was observed that canid RABVs produced two reactivity patterns and these differed by a single mAb (32GD12) [Reference Sacramento27] (Table 2). The epitope recognised by mAb 32GD12 is now believed to be unstable given that after the passage of some RABVs in neuroblastoma cells (C-1300), reactivity with mAb 32GD12 was restored suggesting that the epitope recognised by this mAb is indeed unstable.

Reverse-transcription polymerase chain reaction (RT-PCR), sequencing of specific gene products and reconstruction of phylogenetic trees that demonstrate genetic relationships between taxa, are now more widely accepted for the diagnosis of rabies particularly in laboratories adequately equipped for applying molecular technologies. These technologies underpin lyssavirus surveillance further contribute to risk analysis and improve knowledge and understanding of disease epidemiology. Three regions of the rabies viral genome, the N, the P and the G-L intergenic gene regions, are generally sequenced for inferring molecular relationships amongst lyssaviruses. The N gene is highly conserved, a feature that makes it useful for long-term evolutionary studies. For studies more focused towards a better understanding of the spread of a specific lyssavirus variant in a much smaller geographical unit, less conserved and highly variable genomic regions such as P or the cytoplasmic domain of the glycoprotein and the G-L intergenic regions, are more appropriate as targets for short-term genetic evolutionary events [Reference Sacramento27].

Genetic typing by nucleotide sequence analysis is more precise than Mab typing as it facilitates the determination of the origin of an outbreak/case. Phylogenetic analysis using sequences from our existing RABV nucleotide sequence database discriminated the viruses involved in the two rabies outbreaks of 2007 and 2016. It is evident that RABV infection was introduced into Gauteng Province via two independent albeit unrelated introductions, one in 2007 (in the north of the province bordering the Limpopo Province) and the most recent in 2016 in the western part of the province. The rabies outbreak in 2007 was probably initiated by a dog-RABV variant, whereas the 2016 rabies outbreak involved an expansion of a jackal rabies cycle from the North-West Province with spillover into dogs and cattle. Interestingly, the jackal viruses involved in the recent Gauteng Province outbreak (in 2016) were closely linked (genetically) to those from the 2012 jackal outbreak in KZN, a province that has been associated with dog rabies for over four decades [Reference Gummow36]. The domestic dog is the principal vector species maintaining rabies transmission cycles in KZN [Reference Winkler35, Reference Koeppel37, Reference Skinner38]. However, in 2012 a rabies outbreak in the black-backed jackal population in the uThukela area of KZN is believed to have resulted from CSTEs. This is the first time that a wildlife host species has sustained a rabies outbreak independent of domestic dogs in this part of the country. Confirmed rabies cases in South Africa suggest that jackals have either increased in numbers or have expanded home ranges and this may partly explain the emergence of jackal rabies outbreaks in KZN and Gauteng Province, in 2012 and 2016. Coetzer et al., 2017 [Reference Coetzer39] linked the 2012 jackal rabies outbreak in KZN to an endemic sylvatic cycle. However, an independent research group attributed jackals to be the progenitor of the 2012 rabies outbreak [Reference Shwiff40]. Our data analyses confirm a close genetic link between the 2012 KZN rabies outbreak and the jackal rabies cycle from the North West Province in 2016. It was observed during the 2012 jackal rabies outbreak in KZN that 62% of the positive rabies cases originated from this wildlife host species, and that overall dog rabies cases had been reduced by 93% through parenteral dog vaccination (Department of Agriculture, Land Reform and Rural Development, KZN). Rabies outbreaks in black-backed jackals generally followed outbreaks in domestic dog populations in Zimbabwe, highlighting dogs as the potential source of the disease in wildlife [Reference Cumming18], contrary to events leading to the KZN 2012 jackal outbreak. Contact between wild carnivore species such as jackals with domestic dogs is a common observation in Zimbabwe and this physical contact provides an ideal opportunity for rabies transmission [Reference Bingham14, Reference Cumming18, Reference Sabeta41], given the highly opportunistic nature of the canid rabies variant [Reference Bingham11, Reference Sabeta26].

Spatio-temporal analyses can detect clusters of infectious disease spread and are pivotal in enhancing our understanding of the dynamics of disease dispersion including dispersion of rabies. Analysis of spatial and temporal variations facilitate the identification of high-risk localities and periods of higher transmission risks, and are key attributes in surveillance and control of infectious diseases. In the case of South Africa, spatial and temporal analyses can inform policy makers on appropriate strategies for disease control and management [Reference Raghavan42]. In the past, methods were developed to model some of the aspects of infectious diseases in human populations and to some degree in companion and food animals [Reference Kumar29, Reference Hills30, Reference Raghavan42], but is difficult to quantify the space-time epidemic processes for those diseases vectored by wildlife carnivore species [Reference Raghavan42].

In many parts of the world, wildlife diseases such as rabies are not regularly monitored. Often times when they are studied, the infection rates can be heterogeneous over different landscapes in addition to confounding by host factors such as age, sex and genotype [Reference Sabeta41, Reference Archer43]. This requires the infection data to be analysed using statistical methods that can account for spatial, temporal and host-level heterogeneities. One limitation with reference to rabies in C. mesomelas is the general lack of active surveillance data for wildlife. Sampling efforts to accurately quantify rabies in jackal species in South Africa are not available despite adequate evidence for the presence of rabies in this host species in Limpopo and the North West provinces [Reference Knobel5, Reference Nel12]. A different source for disease prevalence data is veterinary diagnostic laboratories (Onderstepoort Veterinary Institute and the Allerton Provincial Laboratories), where routine rabies testing is performed. The data collected from national surveillance systems for rabies come with inherent limitations including underreporting due to inadequate surveillance. Passive surveillance has two main drawbacks as it makes the findings reported here only directly applicable to a sub-population of jackal species. The majority of jackal specimens submitted for testing likely had a history of human/domestic animal contact or loss of fear for humans, thereby introducing both a population and spatial bias. To circumvent this problem, carefully designed prospective studies to eliminate all population and spatial biases are warranted. The present study therefore underscores a need for such an effort since any and all of the information currently available on the space-time dynamics or eco-epidemiological drivers of jackal rabies exists only in the form of passive surveillance data.

The threat of rabies to communities in South Africa has led to several studies on jackal and mongoose populations [Reference Koeppel37]. Rabies transmission in mongooses, jackals and foxes are density-dependent. In addition to population density, wide-ranging movements in search of food could facilitate re-infection of terrestrial animals in rabies-free areas and equally reduce the efficiency of rabies control programmes. Black-backed jackals forage in pairs and are found throughout southern Africa where they have a wide habitat tolerance in different ecosystems including the Nama-Karoo, open savannas, arid grasslands, woodlands and deserts [Reference Skinner38]. The species can also live in peri-urban areas, and open terrain such as farms and even suburbs, making Gauteng Province a potential habitat. Immature jackals (<3 years of age) move over significantly large areas, up to 30 km during a single night, although home ranges of 244 km2 during the winter months have been recorded [Reference Ferguson44].

Winkler et al. [Reference Winkler35], using both drought severity and indicators of relative drought duration, suggested that the 2015/16 summer rainfall season in the terrestrial Southern African Development Community (SADC) region was the most severe since the droughts of the early 1980s and 1990s. In the 2015/16 rainy season, above-normal maximum temperatures, especially during early- and mid-summer, exacerbated the longer-term effect of below-normal rainfall that continued from the 2014/15 season [Reference Archer43]. The positive association of rabies incidences with NDVI values during the prolonged dry period (2015–2016) implies the availability of forage resources of prey species for jackals. This in turn suggests an indirect mechanism for food availability for rabies hosts, the yellow mongoose (Cynictis penicillata) and jackal species, as predominant factors influencing this relationship. High temperatures and low rainfall can be directly associated with accelerated drying or non-retention of greenness in forage species [Reference Ogutu and Owen-Smith45, Reference Seydack46], thus presenting a weak but still positive association with rabies incidences. The preliminary spatial analysis data indicated that an increase in jackal rabies cases in Gauteng Province resulted from a secondary mechanism of prey availability for the rabies hosts. When food became scarce during dry periods, jackals and mongooses tended to move widely in search of prey [Reference Seydack46, Reference Klein and Roehrig47]. These wide movements bring them closer to human communities where virus exchanges with domestic dogs and humans can potentially occur. Territorial jackals are generally more spatially confined than dispersing jackals, and travel in straight lines and distances in excess of 8 km from core areas to seek food and water resources. In contrast, dispersal and floater jackals wander over long distances seeking those areas with the least competition from dominant jackals for space and food resources. In addition, the wandering facilitates breeding opportunities. Therefore, worsening drought conditions and associated food deprivations are pivotal factors in the poor performance of jackals during this period. The increased availability of food from the extraordinarily large amount of ungulate drought-related mortalities that were present in the field during the latter half of 2015 likely favoured jackal pup survival. The findings of this study are important in the context of rabies management in relation to wildlife (such as jackals and mongooses) in South Africa and the sub-region. It elucidates the contributions and relevance of extreme climatological factors as risk factors facilitating wildlife to human rabies transmissions.

The rabies outbreak in Gauteng Province in 2016 primarily involved black-backed jackals [Reference Tswai34], a wildlife carnivore host found in peri-urban environments. The ecological conditions tended to promote an increase in jackal population numbers. Previous studies reported the highest incidence of rabies in this wildlife species during the winter months [Reference Gummow36, Reference Koeppel37]. During the 2016 jackal rabies outbreak, common risk contacts for potential rabies transmission included bite contact and handling of infected carcasses. Thirty-four people received post-exposure prophylaxis as they were directly exposed to the jackals and/or infected livestock, further highlighting the public health significance of rabies to farm and field workers.

The emergence of rabies outbreaks in geographical areas where rabies was previously under control, including heightened incidences in provinces where rabies is endemic, has raised concerns about possible problems associated with an increase in jackal populations or their movements. Provincial control efforts in response to these outbreaks and aimed at eliminating rabies in Gauteng were immediately implemented. These measures were effective in eliminating these outbreaks and are convincing as dog rabies cases in Gauteng Province decreased from 2017 onwards. Parenteral dog vaccination campaigns have led to an overall decrease in the number of dog and human rabies cases. Vaccination of domestic dogs should therefore be a priority but ideally complemented with baited vaccines to reach stray dogs and other wildlife hosts in order to eliminate dog-mediated human rabies in South Africa and the region. As demonstrated in Europe, oral rabies vaccination has been a proven and effective tool to eliminate rabies in domestic dogs. Practically, the whole of Europe is rabies-free but the risk of re-introduction of the disease always exists, through either the transboundary routes, and/or animal and human trafficking. In South Africa and probably in other regions of the continent, vaccination of domestic dogs should ideally be performed in synergy with the other wildlife carnivore species that maintain sylvatic rabies cycles.

Conclusion

In conclusion, this study has demonstrated an expansion of a jackal rabies cycle from North West Province into the Gauteng Province during the dry period of 2016, as the black-backed jackals ranged widely in search for food resources. This resulted in jackal-dog interactions, reminiscent of the links between domestic and wildlife rabies cycles in South Africa. Clearly, the transmission of the RABV is neither restricted by administrative/provincial boundaries nor the history of occurrence of the disease, but is modulated by the surrounding environmental variables, such as climate and/or human habitats which in turn exhibit spatial heterogeneity. Thus, to control rabies, it is necessary to analyse risks associated with rabies at the case level in order to identify the influence of the geographic determinants on case distributions. The latter is crucial because the spatial pattern of human rabies cases has strong relations with the distribution and movement of rabies in animal hosts and likely the movement of stray and roaming dogs.

Acknowledgements

We are grateful to the Dr Christine Fehlner-Gardiner of the Canadian Food Inspection Agency for providing us with the panel of anti-N Mabs for antigenic typing of southern African lyssaviruses.

Financial support

The study was partly funded by the EVAglobal, a project that received funding from the European Union's Horizon 2020 Research and Innovation under grant agreement no. 871029, and through a Japan/South Africa Joint Science and Technology Research Collaboration 2018 project on ‘Spatial temporal analysis of animal and human rabies cases in South Africa: 1998–2017’, (NRF grant unique #114679, ARC grant# P10000130).

Conflict of interest

None.

Data availability statement

The data used to reach conclusions in this publication are publicly available as nucleotide sequences of RABVs can be retrieved from Genbank using the specific accession numbers for the taxa included in the publication. The raw data that was used to generate rabies trends for Gauteng Province can be requested from the Agricultural Research Council (South Africa) and can be provided through either, a materials transfer agreement (MTA) or project agreement.

References

International Committee on the Taxonomy of Viruses (2017) The ICTV Online (10th) Report on Virus Taxonomy. Available at https://talk.ictvonline.org/taxonomy (Accessed 7 December 2020).Google Scholar
Kokkonen, NTU et al. (2018) Tentative novel lyssavirus in a bat in Finland. Transboundary and Emerging Diseases 65, 593596.Google Scholar
Hampson, K et al. (2015) Estimating the global burden of endemic canine rabies. Plos Neglected Tropical Diseases 9, e0003709.CrossRefGoogle ScholarPubMed
WHO (2016) Human rabies transmitted by dogs: current status of global data 2015. Weekly Epidemiological Record 2, 1322.Google Scholar
Knobel, DL et al. (2005) Re-evaluating the burden of rabies in Africa and Asia. Bulletin of the World Health Organisation 83, 360368.Google ScholarPubMed
Fooks, AR et al. (2014) Current status of rabies and prospects for elimination. Lancet (London, England) 384, 13891399.CrossRefGoogle ScholarPubMed
Rupprecht, CE et al. (2002) Rabies re-examined. Lancet Infectious Diseases 2, 327343.CrossRefGoogle ScholarPubMed
Tolson, ND et al. (1998) Immunization of foxes against rabies with a vaccinia recombinant virus expressing the rabies glycoprotein. Archives of Virology 102, 297301.CrossRefGoogle Scholar
Mähl, P et al. (2014) Twenty-year experience of the oral rabies vaccine SAG2 in wildlife: a global review. Veterinary Research 45, 77.CrossRefGoogle ScholarPubMed
Bingham, J et al. (1993) Jackal rabies in Zimbabwe. Onderstepoort Journal of Veterinary Research 60, 365366.Google ScholarPubMed
Bingham, J (2005) Canine rabies ecology in Southern Africa. Emerging Infectious Diseases 11, 13371342.CrossRefGoogle ScholarPubMed
Nel, L et al. (1997) Natural spillover of a distinctly Canidae-associated biotype of rabies virus into the expanded wildlife host range in Southern Africa. Virus Genes 15, 7982.CrossRefGoogle ScholarPubMed
Bingham, J et al. (1999a) The epidemiology of rabies in Zimbabwe. 1. Rabies in dogs (Canis familiaris). Onderstepoort Journal of Veterinary Research 66, 110.Google Scholar
Bingham, J et al. (1999b) The epidemiology of rabies in Zimbabwe. 2. Rabies in jackals (Canis adustus and Canis mesomelas). Onderstepoort Journal of Veterinary Research 66, 1123.Google Scholar
Zulu, GC et al. (2009) Molecular epidemiology of rabies: focus on domestic dogs (Canis familiaris) and black-backed jackals (Canis mesomelas) from northern South Africa. Virus Research 140, 7178.CrossRefGoogle ScholarPubMed
Sabeta, C et al. (2007) Molecular epidemiology of rabies in bat-eared foxes (Otocyon megalotis) in South Africa. Virus Research 129, 110.CrossRefGoogle ScholarPubMed
Nel, LH et al. (2005) Mongoose rabies in Southern Africa: a re-evaluation based on molecular epidemiology. Virus Research 109, 165173.CrossRefGoogle ScholarPubMed
Cumming, DHM (1982) A case history of the spread of rabies in an African country. South African Journal of Science 78, 443447.Google Scholar
Wandeler, AI. (1993) Wildlife rabies in perspective. Onderstepoort Journal of Veterinary Research 60, 347350.Google Scholar
Cleaveland, S et al. (1995) Maintenance of a microparasite infecting several host species: rabies in the Serengeti. Parasitology 111, S33S47.CrossRefGoogle ScholarPubMed
Brückner, GK et al. (1978) Field observations on the occurrence of rabies in cattle in the magisterial districts of Soutpansberg and Messina. Journal of the South African Veterinary Association 49, 3336.Google ScholarPubMed
Rhodes, CJ et al. (1998) Rabies in Zimbabwe: reservoir dogs and the implications for disease control. Philosophical Transactions of the Royal Society of London Bulletin of Biological Science 353, 9991010.CrossRefGoogle ScholarPubMed
Haydon, DT et al. (2002) Identifying reservoirs of infection: a conceptual and practical challenge. Emerging Infectious Diseases 8, 14681473.Google ScholarPubMed
Dean, D et al. (1996) The fluorescent antibody test. In Meslin, FX, Kaplan, MM and Koprowski, H (eds), Chapter 7 in Laboratory Techniques in Rabies, 4th Edn. Geneva: World Health Organisation, pp. 8895.Google Scholar
Ngoepe, E et al. (2014) Antigenic characterisation of lyssaviruses in South Africa. Onderstepoort Journal of Veterinary Research 81, 19. doi: 10.4102/ojvr.v81i1.711.CrossRefGoogle ScholarPubMed
Sabeta, CT et al. (2003) Molecular epidemiology of canid rabies in Zimbabwe and South Africa. Virus Research 91, 203211.CrossRefGoogle ScholarPubMed
Sacramento, D et al. (1992) Molecular epidemiology of rabies virus in France: comparison with vaccine strains. Journal of General Virology 73, 11491158.CrossRefGoogle ScholarPubMed
Thompson, JD et al. (1994) CLUSTALW: improving the sensitivity of progressive multiple sequence alignment through sequence weighting, position-specific gap penalties and weight matrix choice. Nucleic Acids Research 22, 46734680.CrossRefGoogle Scholar
Kumar, S et al. (2004) MEGA3: integrated software for molecular evolutionary genetics analysis and sequence alignment. Briefings in Bioinformatics 5, 150163.CrossRefGoogle ScholarPubMed
Hills, DM et al. (1993) An empirical test of bootstrapping as a method for assessing confidence in phylogenetic analysis. Systematic Biology 42, 182192.CrossRefGoogle Scholar
Burnham, KP and Anderson, DR (2002) Model Selection and Multimodel Inference: A Practical Information-Theoretic Approach, 2nd Edn. New York: Springer Publishers.Google Scholar
Hosmer, DW and Lemeshow, S (2000) Applied Logistic Regression. New York: John Wiley & Sons Publishers.CrossRefGoogle Scholar
Sabeta, C et al. (2013) Emergence of rabies in the Gauteng Province, South Africa: 2010–2011. Journal of the South African Veterinary Association 84, 15. doi: 10.4102/jsava.v84i1.923.CrossRefGoogle ScholarPubMed
Tswai, DR (2016) Phase 1 of Desertification, Land Degradation and Drought (DLDD) land cover mapping impact indicator of the United Nations Convention to Combat Desertification (UNCCD). ISCW report number GW/A/2016/29, Unpublished, ARC-ISCW, Pretoria.Google Scholar
Winkler, K et al. (2017) Identifying droughts affecting agriculture in Africa based on remote sensing time series between 2000–2016: rainfall anomalies and vegetation condition in the context of ENSO. Remote Sensing 9, 831.CrossRefGoogle Scholar
Gummow, B et al. (2010) Rabies in South Africa between 1993 and 2005 – what has been achieved? Journal of the South African Veterinary Association 81, 1621.CrossRefGoogle ScholarPubMed
Koeppel, KN et al. (2020) Oral bait preferences for rabies vaccination in free-ranging black-backed jackal (Canis mesomelas) and non-target species in a multi-site field study in a peri-urban protected area in South Africa. Preventive Veterinary Medicine 175, 104867.CrossRefGoogle Scholar
Skinner, JD et al. (2005) Black Backed Jackal. The Mammals of Southern African Sub-Region. Cape Town: cambridge University Press, pp. 486490.CrossRefGoogle Scholar
Coetzer, A et al. (2017) Epidemiology of rabies in Lesotho: the importance of routine surveillance and virus characterisation. Tropical Medicine and Infectious Diseases 2, 30.CrossRefGoogle Scholar
Shwiff, SA et al. (2016) Towards canine rabies elimination in KwaZulu-Natal, South Africa: assessment of health economics data. Transboundary and Emerging Diseases 63, 4084015.CrossRefGoogle Scholar
Sabeta, CT et al. (2018) Rabies of canid biotype in wild dog (Lycaon pictus) and spotted hyaena (Crocuta crocuta) in Madikwe Game Reserve, South Africa in 2014–2015: diagnosis, possible origins and implications for control. Journal of the South African Veterinary Association 89, e1e13.CrossRefGoogle ScholarPubMed
Raghavan, RK et al. (2016) Bayesian spatiotemporal pattern and eco-climatological drivers of striped skunk rabies in the north-central plains. Plos Neglected Tropical Diseases 10, 116. doi: 10.1371/journal.pntd.0004632.CrossRefGoogle ScholarPubMed
Archer, ERM et al. (2017) Understanding the evolution of the 2014–2016 summer rainfall seasons in Southern Africa: key lessons. Climate Risk Management 16, 2228.CrossRefGoogle Scholar
Ferguson, JWH et al. (1983) Social organization and movement patterns of black-backed jackals. Journal of Zoology 199, 487502.CrossRefGoogle Scholar
Ogutu, JO and Owen-Smith, N (2003) ENSO, rainfall and temperature influences on extreme population declines among African savanna ungulates, Ecology Letters 6, 412419.CrossRefGoogle Scholar
Seydack, AH et al. (2012) Large herbivore population performance and climate in a South African semi-arid savanna. Koedoe 54, 120. doi: 10.4102/koedoe.v54i1.1047.CrossRefGoogle Scholar
Klein, D and Roehrig, J (2006) How does vegetation respond to rainfall variability in a semi-humid West African in comparison to a semi-arid East African environment? Proceedings of the 2nd Workshop of the EARSeL SIG on Land Use and Land Cover Bonn, Germany, pp. 149156.Google Scholar
Figure 0

Fig. 1. Jackal cases for the periods 2013–2014, 2015–2016 and 2017.

Figure 1

Table 1. Epidemiological information of RABVs genetically characterised in this study

Figure 2

Table 2. The reactivity patterns of the rabies viruses analysed

Figure 3

Table 3. Comparative fit of alternative models relating to rabies cases during the period pre-dry conditions, dry conditions and post dry conditions

Figure 4

Fig. 2. Rabies trends in Gauteng, 2009–2019.

Figure 5

Fig. 3. Phylogenetic analysis of RABVs included in this investigation. A 592-nucleotide portion encompassing the cytoplasmic domain of the glycoprotein and the G-L intergenic regions of the virus isolates included in this study. A neighbour-joining tree of the G-L intergenic region sequences illustrating the genetic relationships of canid RABVs from Gauteng, Limpopo, North West and KwaZulu-Natal provinces respectively. The viral sequences obtained from both black-backed jackal and domestic dogs from KwaZulu-Natal are in black, Gauteng viral isolates are in red, North West province in green and Limpopo province in dark blue. The horizontal lines are proportional to the evolutionary distances between sequences and the scale bar represents nucleotide substitutions per site. Key: bbj, black-backed jackal; dog, domestic dog; bov, bovine; cat, wild cat