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Introduction
Bartonella are small, pleomorphic, Gram-negative, intracellular bacilli belonging to the order Rickettsiales. Currently the genus Bartonella includes 24 species (9). Bartonella microorganisms can infect dogs, cats, and humans, causing cat-scratch disease. These pathogens are very common in the population of cats (bacteraemia is present in 8%–56% of clinically healthy cats) (4, 22).
The main aetiological factors of feline bartonellosis are B. henselae, B. clarridgeiae, and B. koehlerae. At least two genotypes can be distinguished in B. henselae: Houston-1 and Marseille. The Houston-1 genotype is prevalent in Asia, while the Marseille genotype has a larger presence in the USA, Europe, and Australia (3).
The infections they cause are mainly observed in cats which are less than one year old and live in large groups (e.g. in shelters). The disease is observed in areas where the climate is hot and humid.
The main vectors of feline bartonellosis are ectoparasites (fleas and ticks). In an infected organism the bacteria colonise the vascular endothelium cells, erythrocytes, and bone marrow progenitor cells (19). In the course of the disease, the bacteraemia may persist for weeks or even years (9). The factors that determine the development of the disease include the virulence of the Bartonella strain, living and feeding conditions, concurrent diseases, congenital defects, use of immunosuppressive drugs, etc. The course of bartonellosis may be asymptomatic or the infection may involve non-specific clinical signs, such as gingivitis, arthritis, reproduction disorders, neurological symptoms, uveitis etc.
To date, no epidemiological studies focused on feline bartonellosis have been conducted in Poland. The presence of Bartonella has only been demonstrated in Poland in ticks (25, 29). The aim of this study is to estimate the epizootic situation of feline bartonellosis in eastern Poland.
Material and Methods
Animals and sampling. In the period from January 2017 to July 2018, a total of 672 cats were randomly selected from the nine largest veterinary clinics in eastern Poland for blood sampling for molecular tests concerning Bartonella spp. None of the cats had ever left Polish territory. Of these, 288 were referred to the clinics for prophylactic reasons (vaccination as prophylaxis against ecto- and endoparasites). The remaining 384 cats were referred to veterinary practices with various clinical problems (infectious disease, kidney disease, diarrhoea, diabetes, and allergy). The samples were collected by veterinary practitioners upon request. The owners of all the cats agreed that the cats could participate in the study.
Epidemiological data from all the cats were recorded by means of a questionnaire, completed for each animal and containing the following information:
Region: cats were examined from four provinces (the highest administrative subdivision level of Poland). The study comprised cats from eastern Poland (the Lublin, Podlasie, Masovian, and Subcarpathian provinces). The characteristics of the regions are described by Gorzelak et al. (13).
Breed and sex: the sample included cats from many breeds (504 European Shorthaired cats, 28 Persian, 28 Cornish Rex, 28 Maine Coon, 20 Sphinx, 20 Siamese, 16 Norwegian, 12 Siberian, 12 British, and 4 Japanese), including both males (208) and females (464). As a consequence, it was decided to classify as purebred or mixed breed.
Living conditions: the cats were classified by whether they were kept indoors (336) or could roam freely outdoors (336).
Use of tick- or vector-borne disease control measures (prophylaxis against ectoparasites in the form of a spray, collar, or spot) (272).
Age: the cats were classified as young (under one year old) (112) or adult (one year old or older) (560).
The questionnaires for the cats were completed by the authors.
DNA extraction and PCR amplification. DNA extractions for molecular tests were performed using the DNA Blood kit (A&A Biotechnology, Gdynia, Poland). The extracted DNA was subjected to PCR.
The reaction was performed according to the method described by Staggemeier et al. (28) with minor modifications of the primer targeting fragments of the citrate synthase gene: one generic forward primer (BART-LC-GEN-F: 5′ – ATGGGTTTTGGTCATCGA GT – 3′), one species-specific reverse B. henselae primer (BART-LC-HEN-R: 5′–AA ATCGACATTAGGGTAA AGTTTTT – 3′), and one species-specific reverse B. clarridgeiae primer (BART-LC-CLA-R: 5′- CAAGAAGTGGATCA TCTTGG – 3′).
The products of the PCR were analysed using the electrophoresis method in 1.5% agarose gel, in TBE buffer, at a voltage of 10 V/cm. The gel was stained with ethidium bromide (1 μg/mL) for 15 min. The size of the products was determined according to the weight standard DNA ladder 100 bp (Fermentas, Vilnius, Lithuania).
Statistical analysis. The chi-squared test was used to determine the risk factors associated with the presence of Bartonella DNA in the blood. Explanatory variables associated with Bartonella spp. infection with P < 0.15 were initially selected. Spearman’s Rho (Rho) was used in the second step to determine the collinearity among the selected explanatory variables. If Rho was > 0.4, only the variable more logically associated with Bartonella infection was retained (P associated with Rho was < 0.001 in all cases).
The association between the explanatory variables previously selected and the dependent variable (presence of Bartonella DNA) was investigated using a logistic regression model. Changes in the odds ratio (OR) value greater than 25% were considered indicative of a confounding factor. A forward introduction of the variables was used. The model was re-run until all remaining variables presented statistically significant values (likelihood ratio, Wald’s test, P < 0.05). The statistical analysis was performed using SPSS v22.0 software (IBM SPSS Inc., Armonk, NY, USA).
Results
Among the four regions located in eastern Poland, the Subcarpathian province revealed the highest PCR-determined prevalence of Bartonella infection in cats (53.3%), and this was nearly double the lowest prevalence from the Masovian province (28.5%). The other two regions returned prevalence rates of 47.8% for Podlasie province and 38.0% for Lublin province (Fig. 1).
Fig.1
PCR amplification of a partial sequence of B. henselae citrate synthase gene (product size: 250 bp). M – molecular weight marker (100 bp); 1 – positive control; 2 – negative control; 3–8 – positive samples
The chi-squared test results are presented in Table 1. Five variables were selected for collinearity analysis, at an 85% confidence level (living conditions, breed, region, disease and tick control).
Variables associated (P < 0.15) with Bartonella infection in cats from eastern Poland
Variable
Category
Total (percentage of PCR positive cats)
Total (percentage of PCR negative cats)
P
Sex
Male
79 (38.0)
129 (62.0)
Female
193 (41.6)
271 (58.4)
0.378
Age
Young (<1 year old, (≥1 year old)
42 (37.5)
70 (62.5)
230 (41.1)
330 (58.9)
0.482
Living conditions
Indoors only
84 (25.0)
252 (75.0)
Outdoors and indoors
188 (56.0)
148 (44.0)
<0.001
Breed
Mixed breed
241 (47.8)
263 (52.2)
Purebred
31 (18.5)
137 (81.5)
<0.001
Region
Lublin
84 (38.0)
137 (62.0)
Masovian
53 (28.5)
133 (71.5)
Subcarpathian
81 (53.3)
71 (46.7)
<0.001
Podlasie
54 (47.8)
59 (52.2)
Disease
Yes
169 (43.2)
222 (56.8)
No
103 (36.7)
178 (63.3)
0.087
Tick control
Yes
76 (27.9)
196 (72.1)
No
196 (49.0)
204 (51.0)
<0.001
Collinearity, evaluated by Spearman’s Rho, was not detected among the selected variables (all values were under 0.4). The variables included in the logistic regression model, at a 95% confidence level, are shown in Table 2. It can be observed that the living conditions of the animals (freely roaming outdoors), mixed breed, Subcarpathian region, and absence of tick control were significant risk factors associated with Bartonella infection.
Logistic regression model showing variables significantly associated with Bartonella spp. in eastern Poland (at a 95% confidence level)
Variable
Category
P (Wald’s Statistic)
OR
95% CI
Living conditions
Outdoors and indoors Indoors only
Reference category. Its OR value was 1 in all cases
<0.001
3.36
2.46–4.95
Breed
Mixed breed Pure
Reference category. Its OR value was 1 in all cases
0.001
2.81
1.75–4.51
Region
Lublin
0.684
0.9
0.55–1.48
Masovian
0.471
0.82
0.48–1.4
Subcarpathian
0.013
2.01
1.16–3.47
Podlasie
Reference category. Its OR value was 1 in all cases
Tick control
No Yes
Reference category. Its OR value was 1 in all cases
<0.001
2.02
1.41–2.92
Yes
Reference category. Its OR value was 1 in all cases
Constant
0.001
0.33
Bartonella DNA was demonstrated in the blood of 56% of the free-roaming cats and only in 25% of the cats kept exclusively indoors. It was observed in 47.8% of the mixed-breed cats and only in 18% of the purebred cats, in 49% of the cats that did not receive ectoparasite prevention treatment, and in 27.9% of the cats that received such treatment.
Overall, the presence of B. henselae DNA was detected in the blood of 272 out of the 672 tested animals (40.48%). The size of the amplified citrate synthase gene fragment was 250 bp (Fig. 1). When the PCR product obtained from the cats was sequenced and the nucleotide sequence compared with the one deposited in GenBank under accession number L38987.1, the two showed a level of similarity of 99%–100%. The DNA of B. clarridgeiae was not found in the blood of any animal.
Discussion
In this article we studied a population of domestic cats from eastern Poland to determine the prevalence and associated risk factors for Bartonella infection and to identify endemic Bartonella species.
In our study, the only Bartonella species found in cats was B. henselae. This is the most common Bartonella species type found in cats in Europe (2, 7, 16, 18, 26). We found no presence of B. clarridgeiae in any of the study cats, unlike in studied cat populations in France and the Netherlands (2, 16)
Bartonella henselae has worldwide distribution; high seropositivity to B. henselae in cat populations (18%, 50%, and 58.8%) was recorded in Italy, Spain, and Greece, respectively (8, 14, 24)
The results of our study indicated that eastern Poland is a territory at risk of a feline bartonellosis epizootic. The DNA of this bacterium was found in the blood of 40.48% of animals, and this proportion appears to be high compared to other countries in Europe. For example, in France the bacteraemia caused by Bartonella was found in 11% of pet cats (6), in Germany in 13% of pet cats (26), and in the Netherlands in 22% of shelter cats (2).
Despite some reports suggesting that the sex of a cat may be a factor that predisposes the animal to the development of the disease (22, 25), most studies on the subject, including ours, do not confirm such a relationship (11, 12, 15, 16). Similarly, in our studies we did not observe a relationship between frequency of infection and age of the cat; however, previous studies have indicated that young cats are more often infected with Bartonella (5, 18, 26).
Our study also failed to reveal any statistically significant differences between the frequency of Bartonella DNA detection in the blood of healthy cats and this frequency in those with various health issues. However, it is possible that the immunosuppression associated with some diseases like FeLV or FIV increases the pathogenicity of B. henselae infection in cats, and may be a predisposing factor for disease development (30). It is interesting that the Bartonella infection itself is often asymptomatic in cats, and in the haematological results no statistically significant differences were found between Bartonella spp.-positive and -negative cats (27).
The statistical analysis of the results from our study enabled us to demonstrate that such factors as breed (mixed-breed cats), area of origin (the Subcarpathian province), living conditions (free-roaming), and lack of ectoparasite-prevention treatments are factors conducive to Bartonella-related bacteraemia in cats.
Warm, humid environments, density of the cat population, and unbeneficial aspects of the habitat including state of hygiene and flea infestation, may correlate with a higher prevalence of B. henselae infection (20). A positive correlation between the origin of the cats used in this study (the Subcarpathian province) and the presence of Bartonella infections confirm these observations. Among the four provinces of Poland covered by the study, the Subcarpathian province had the highest annual mean air temperature and mean air humidity.
The fact that bacteraemia is more frequently observed in mixed-breed cats than purebreds is more likely a result of the greater popularity of these animals in Poland than of any breed predisposition. On the other hand, the higher prevalence of Bartonella infection in mixed-breed cats may be connected with the cats’ living conditions, as they are more likely to be kept outdoors. Outdoor or free-ranging animals are more prone to being infected by ectoparasites and transmitted pathogens (24).
The positive association of bacteraemia with the lack of anti-ectoparasite prophylaxis and the living conditions of the cats (free-roaming) is confirmatory of previous studies demonstrating that cat fleas (C. felis) and ticks (Ixodes spp.) may serve as the vectors of B. henselae between cats (5, 10, 17, 21, 30). This association may be connected with a greater exposure to Bartonella vectors in this group of animals and confirms the previous observation of Chomel et al (5), who identified an association between bacteraemia and flea infestation.
Similar investigations were performed by Barradas et al. (1), who did not find significant differences regarding B. henselae infection between age groups, sexes, breeds, living conditions, extents of contact with other animals including rodents, or seasons of sample collection. A statistically significant association was observed only between B. henselae infection and the lack of access to prophylaxis against ectoparasites.
The increased frequency of bartonellosis in cats may be the result of climate change. However, the use of new diagnostic techniques, including molecular methods, in the disease recognition process and better understanding of bartonellosis among veterinarians and cat owners may result in more frequent recognition of the disease in these animals (21, 22).
As more cases of Bartonella infections have been observed recently in cats, there is a continued need to conduct studies on bartonellosis epidemiology, diagnosis, and prevention, and broaden its scope to areas previously not considered endemic for the disease. To successfully prevent bartonellosis, an understanding of the ways the disease spreads, its geographical scope, and the factors that favour its development is necessary.
