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Article

Molecular Detection of Selected Pathogens with Zoonotic Potential in Deer Keds (Lipoptena fortisetosa)

by
Remigiusz Gałęcki
1,*,
Jerzy Jaroszewski
2,
Tadeusz Bakuła
1,
Eloiza M. Galon
3 and
Xuenan Xuan
3
1
Department of Veterinary Prevention and Feed Hygiene, Faculty of Veterinary Medicine, University of Warmia and Mazury in Olsztyn, 10-719 Olsztyn, Poland
2
Department of Pharmacology and Toxicology, Faculty of Veterinary Medicine, University of Warmia and Mazury in Olsztyn, 10-719 Olsztyn, Poland
3
National Research Center for Protozoan Diseases, Obihiro University of Agriculture and Veterinary Medicine, Obihiro 080-8555, Japan
*
Author to whom correspondence should be addressed.
Pathogens 2021, 10(3), 324; https://doi.org/10.3390/pathogens10030324
Submission received: 31 January 2021 / Revised: 27 February 2021 / Accepted: 7 March 2021 / Published: 10 March 2021
(This article belongs to the Special Issue Current Research on Infectious Diseases of Domestic Animals in a One Health Perspective)
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Abstract

:
Deer keds are obligatory hematophagous ectoparasites of birds and mammals. Cervids serve as specific hosts for these insects. However, ked infestations have been observed in non-specific hosts, including humans, companion animals, and livestock. Lipoptena fortisetosa is a weakly studied ectoparasite, but there is evidence to indicate that it continues to spread across Europe. The existing knowledge on deer keds’ impact on wildlife is superficial, and their veterinary importance is enigmatic. Lipoptena fortisetosa is a species with vectorial capacity, but potential pathogen transmission has not been assessed. The objective of this study was to evaluate the prevalence of selected pathogens in L. fortisetosa collected from cervids and host-seeking individuals in the environment. Out of 500 acquired samples, 307 (61.4%) had genetic material from at least one tested pathogen. Our research suggests that L. fortisetosa may be a potential vector of several pathogens, including A. phagocytophilum, Babesia spp., Bartonella spp., Borellia spp., Coxiella-like endosymbionts, Francisiella tularensis, Mycoplasma spp., Rickettsia spp., and Theileria spp.; however, further, more extensive investigations are required to confirm this. The results of the study indicate that keds can be used as biological markers for investigating the prevalence of vector-borne diseases in the population of free-ranging cervids.

1. Introduction

The role of vectors in the transmission of infectious diseases has been researched extensively in recent years. The main arthropods with vector capacity are ticks, mosquitos, black flies, fleas and lice. Many indigenous insects with vector capacity have not been thoroughly investigated in Europe [1,2,3]. One of the most underestimated ectoparasites is the deer ked.
Deer keds (syn. louse flies) of the genus Lipoptena (family Hippoboscidae) are potential vectors of infectious diseases that have not been thoroughly studied to date [4]. Special attention should be paid to Lipoptena fortisetosa, an invasive species that continues to spread across Europe. Lipoptena fortisetosa is a blood-feeding ectoparasite that specifically targets cervids, including the sika deer (Cervus nippon), Siberian roe deer (Capreolus pygargus), and roe deer (Capreolus capreolus). This parasite also uses the red deer (Cervus elaphus), fallow deer (Dama dama), and moose (Alces alces) [5]. Lipoptena fortisetosa originates from eastern Siberia and the Far East [6]. The species was first described by Maa in Japan [6]. In Poland, L. fortisetosa was first identified in the region of Lower Silesia in the late 1980s, and its presence was confirmed in the Tatra Mountains and in northern Poland in 2007–2012 [5,7,8,9,10,11,12]. This ectoparasite was also isolated in the region of Wielkopolska in 2017 [13]. Deer keds target forest animals during host-seeking flights [14]. The duration of the host-seeking period is determined by the local microclimate and the insect’s phenology [14]. Louse flies shed wings when they find a definitive host. They are highly mobile on the host’s skin [15]. Deer keds reproduce by adenotrophic viviparity. The prevalence of Lipoptena spp. infestations in specific hosts ranges from 64% to 78%, depending on the species [16,17]. These ectoparasites were also identified in non-specific hosts. Lipoptena fortisetosa has been isolated from dogs [13]. Izdebska [18] confirmed the presence of Lipoptena spp. in bison (Bison bonasus). Deer keds were also found to attack cattle and horses [19,20]. Louse fly attacks and bites have also been reported in humans [21,22,23]. A single host can be infested by up to 16,000 insects [24]. Bites of the Lipoptena spp. may cause acute to chronic, eosinophilic to lymphocytic deer ked dermatitis [25]. Other infection symptoms include loss of hair, allergic rhinitis, conjunctivitis, or even anaphylactic shock [25,26,27,28].
Vectors are part of the One Health concept because they are responsible for the transmission of pathogens between wildlife, livestock, companion animals and humans [29,30]. Pathogens carried by arthropods cause vector-borne diseases. Vectors can carry viruses, bacteria, protozoa and helmints. Vector-borne viruses include, among others, the Chikungunya virus, bluetongue disease virus, dengue virus, Crimean-Congo hemorrhagic fever virus, West Nile virus, hantavirus, and Zika virus. The following bacteria are also transmitted by vectors: Anaplasma spp., Bacillus spp., Bartonella spp., Borellia spp., Brucella spp., Clostridium spp., Coxiella spp., Erysipelothrix spp., Francisella spp., Leptospira spp., Listeria spp., Mycoplasma spp., Pasteurella spp., Rickettsia spp., Salmonella spp., and Yersinia spp. Vectors also play a very important role in the life cycle of protozoa, including Babesia spp., Leishmania spp., Plasmodium spp., Theileria spp., and Trypanosoma spp. Similarly to other flies of the family Hippoboscidae [31], L. fortisetosa are potential vectors of infectious diseases [4,32]. DNA of Coxiella spp., Theileria luwenshuni, and T. ovis have been identified in L. fortisetosa in molecular analysis [33]. Lipoptena fortisetosa can also act as a vector for Trypanosoma spp. [34]. Trypanosome DNA was detected in 20% of L. cervi and in 48.64% of L. fortisetosa [35]. Deer keds harbored genetic material of Anaplasma spp. and Rickettsia spp. [36,37]. In isolated cases, DNA of Borrelia spp. was identified in louse flies [38,39]. The prevalence of Bartonella spp., which is transmitted vertically in deer keds, has been widely researched [40,41,42,43]. These pathogens’ DNA was found in up to 98% of louse flies [42,43].
The European population of L. fortisetosa continues to spread, and further research is needed to evaluate this ectoparasite’s role in the spread of infectious diseases. The expansion of the insect’s geographic range was confirmed by Italian and Estonian studies [44,45]. The existing research is largely based on single detections of the pathogen’s genetic material. Most of the research was conducted in small and limited locations. Louse flies’ impact on wildlife populations, livestock, companion animals and humans has not been fully elucidated. The identification of genetic material in these ectoparasites could contribute important information about pathogens.
The aim of this study was to identify pathogens with zoonotic potential (A. ovis, A. phagocytophilum, Babesia spp., Bartonella spp., Borellia spp., Coxiella spp., Francisiella tularensis, Mycoplasma spp., Rickettsia spp., and Theileria spp.) in L. fortisetosa infesting cervids and in host-seeking louse flies in the environment.

2. Results

Overall, 9 of the 10 analyzed pathogens’ DNA was identified, including 5 in group E and 9 in group A. In group A, A. phagocytophilum was identified in 20 (8%) samples, Babesia spp. —in 51 (20.4%) samples, Bartonella spp. —in 158 (63.2%) samples, Borrelia spp. —in 12 (4.8%) samples, Coxiella spp. —in 12 (4.8%) samples, Francisella spp. —in 7 (2.8%) samples, Mycoplasma spp. —in 74 (29.6%) samples, Rickettsia spp. —in 76 (30.4%) samples, and Theileria spp. —in 49 (19.6%) samples. In group E, Bartonella spp. was identified in 89 (35.6%) samples, Coxiella spp. —in 3 (1.2%) samples, Francisella tularensis, —in 2 (0.8%) samples, Mycoplasma spp. —in 17 (6.8%) samples, and Rickettsia spp. —in 30 (12%) samples. Detailed data are presented in Table 1. The representative sequences of selected pathogens were deposited in the GenBank database of the National Center for Biotechnology Information under the following accession numbers: A. phagocytophilum MW531454, MW531455; Babesia spp. MT350573, MW522567; Bartonella spp. MW531456, MW531457; Borrelia spp. MW531458, MW531459; Coxiella spp. MW526947, MW526948; Francisella spp. MW531460; Mycoplasma spp. MW547438, MW547439; Rickettsia spp. MW531461, MW531462; Theileria spp. MW531681, MW531682. The phylogenetic trees for the obtained sequences are presented in Figure 1, Figure 2, Figure 3, Figure 4, Figure 5, Figure 6, Figure 7, Figure 8, Figure 9 and Figure 10.
Anaplasma phagocytophilum sequences (MW531454, MW531455) were characterized by 99.76% similarity with sequences from Hungary (MF974860) and Slovakia (HQ661159). One sequence (MT350573) was identical with Babesia odocoilei from Norway (MK612774). One sequence (MW522567) was identical with Babesia spp. from the Czech Republic (MG344773). Bartonella schoenbuchensis sequences (MW531456, MW531457) were identical with sequences from France (AY116639) and Poland (EF418048, EF418052). Coxiella spp. sequences (MW531458, MW531459) were characterized by 97.63–97.64% similarity with sequences from South Korea (KU356909-KU356913). One sequence (MW531460) was identical with the Francisella tularensis subsp. holarctica sequence from Germany (EF418048, EF418052). The remaining sequences of Francisella spp. have been identified as Arsenophonus spp. One sequence (MW547438) was identical with the Candidatus Mycoplasma erythrocervae sequence from Japan (KF306251, KF306247, AB558897). Another Mycoplasma spp. sequence (MW547439) was identical with Mycoplasma ovis sequences, from Hungary (EU165509) and Turkey (MF377462). Sequences of Rickettsia spp. (MW531461, MW531462) were identical with Rickettsia helvetica sequences from Russia (KU310588) and France (U59723). One sequence (MW531681) was characterized by 99.73% similarity with the Theileria capreoli sequence from Turkey (MN463019). A second Theileria spp. sequence (MW531682) was identical with sequences from Turkey (MN463019) and Spain in red deer imported from Germany (AY421708).
Deer keds sampled from animals were significantly more likely to harbor pathogens than the insects from environmental samples. Detection of pathogens’ genetic material was significantly higher in female than male flies. DNA of A. phagocyphilum was more frequently identified in females than males. Babesia spp. genetic material was significantly more prevalent in L. fortisetosa sampled in the Warmia-Masuria and Lubusz voivodeships. The prevalence of Bartonella spp., Coxiella spp., Mycoplasma spp., and Rickettsia spp. DNA was significantly higher in group A than in group E. Genetic material of Theileria spp. was less frequently detected in insects sampled in the Lubusz voivodeship. Detailed data are presented in Table 2.
Significant relationships between the prevalence of the examined pathogens were observed. The values of Cramer’s V were indicative of the absence of associations or weak associations. The relationships between the prevalence of the analyzed pathogens are presented in detail in Table 3.

3. Discussion

The results of this study indicate that L. fortisetosa is ubiquitous in the analyzed voivodeships. In a previous study, this ectoparasite was identified only in isolated locations [5]. Deer keds could spread to new locations due to low level of host specificity as well as animal migrations. Lipoptena fortisetosa is an invasive species in Poland, but its population has been expanding steadily, which suggests that it has adapted well to the environmental conditions of Central Europe [14]. Louse flies infest hosts directly after pupation, and the emerged insects cover areas with a radius of 50 m [46]. Winged flies are responsible for the majority of non-specific host infestations, including in humans [23], companion animals [13], and livestock [19]. The host-seeking flights of L. fortisetosa may pose a threat for forest workers and hunters [23,47]. Hunters may become infested with Lipoptena spp. during the evisceration of wild animals. Hunting dogs may be attacked by these ectoparasites during tracking [13]. Cattle and horses grazing in the vicinity of forests also may be at risk of L. fortisetosa infestation [19,20]. People wearing dark clothing and animals with a dark fur coat are most susceptible to insect flights [48].
In this study, the prevalence and number of pathogens were lower in winged deer keds than in individuals sampled from cervids. Due to the fact that louse flies drop their wings upon attachment to the host, any subsequent switch in host is made more difficult [49]. However, Lipoptena spp. may switch hosts during the breeding season of cervids [50]. Infested mothers can also transmit these ectoparasites to their offspring [51]. In addition to insect bites, the infectious agent could also be transmitted when an insect is crushed on the skin [52]. Our results showed that Lipoptena fortisetosa carry DNA of pathogens, which might be collected through bloodmeal and transferred during the embryonic development of the larvae. The genetic material of Babesia spp., Borrelia spp., and Theileria spp. was detected only in deer keds that had direct contact with cervids. This is the first study to detect genetic material of Babesia spp. in deer keds. In addition, it is interesting to identify the DNA of Borrelia spp. in these ectoparasites in light of the fact that cervids are incompetent hosts for these bacteria [53]. The genetic material of Bartonella spp., Mycoplasma spp., and Rickettsia spp. was identified additionally in winged insects sampled from the environment. The presence of the wings means that these individuals had no previous contact with the host [54]. Some pathogens may be carried by vectors without direct contact with a host. This is generally the result of acquiring a blood meal by a female. Due to the characteristic development of the new generation, host seekers may still carry remnants of a previous blood meal.
Interestingly, the analyzed insects also harbored Coxiella spp. and Francisella tularensis, and the prevalence of these bacteria in deer keds has been poorly investigated to date. These bacterial species were identified in both insect groups; however, most of the obtained sequences were identified as endosymbionts. In addition, the present findings do not provide sufficient evidence to substantiate the above claim because the isolation kit used in this study is intended to detect trace amounts of DNA. Pupae developing in the forest understory could have been contaminated with environmental bacteria. Coxiella spp. and Francisella spp. colonize soil [55,56], where pupation occurs. Additionally, it is interesting to find the Candidatus Mycoplasma erythrocervae bacterium, which was most closely related to isolates from Japan [57]. Either the variance of this genetic material associated with the DNA fragment under test is low, or the pathogen has been introduced with sika deer (Cervus nippon). It is possible that with the introduction of this species to Poland, the pathogen expanded in the population of native cervids. The possible presence of another pathogen of Japanese origin (Bartonella spp.) was also suggested in other studies [43].
Our description of pathogens ‘genetic material detection with molecular tests might be an important consideration in research on deer keds’ role in the transmission of infectious diseases. This research allows for a preliminary determination of potential pathogens for which L. fortisetosa may serve as vector. However, the transmission of the infectious agents by L. fortisetosa should be evaluated with the use of Koch’s postulates [58,59,60]. For example, the development of Babesia spp. and Theileria spp. in Lipoptena spp. seems doubtful because ticks are the only known definitive hosts for these protozoa [61]. However, further research is needed to confirm this assumption. Despite the above, deer keds may act as mechanic vectors for these pathogens [4,37]. Lipoptena cervi has been suggested to mechanically transmit A. phagocytophilum to cervids [37,62]. Hornok et al. [63] identified Theileria spp. in stable flies (Stomoxys calcitrans) and suggested that this ectoparasite may pose a risk of mechanical transmission of theilerioses. Therefore, the research should assess whether a similar phenomenon may occur in deer keds. Lipoptena fortisetosa may be the potential biological vector for Trypanosoma spp. [35]. Currently, Bartonella spp. is the most comprehensively studied pathogen carried by Lipoptena spp., which appears to pose the greatest risk in infestation with these ectoparasites [40,41,42,43].
In the present study, genetic material of pathogens was more frequently identified in female than male L. fortisetosa, which could be explained by the fact that, in some ectoparasite species, females ingest more food than males [64,65]. Female insects of the genus Lipoptena spp. suck blood to draw nutrients that are needed for embryogenesis and intrauterine feeding of larvae [66]. Moreover, the exposure to microorganisms that are sucked with blood by females might last longer in the next generation. The logistic regression model revealed differences in pathogen prevalence between groups, which could suggest that some pathogen DNA may still be present in host-seeking ectoparasites. This study explored the idea that several of the detected microorganisms’ DNA might have been vertically transmitted. Some pathogens were also more prevalent in selected voivodeships. These differences can probably be attributed to variations in pathogen prevalence across cervid populations [67,68]. The calculated values of Cramer’s V point to the absence of significant associations between the prevalence of the studied pathogens, which could suggest that other vectors play a role in the transmission of these infectious agents.
In the future, deer keds could be used as biological markers of vector-borne diseases in cervid populations, due to the biology and behavior of these ectoparasites as well as specific ectoparasite-host relationships [46]. The acquisition of biological material—in particular, blood—that is suitable for molecular analyses could be problematic if the appropriate transportation and analytical equipment and facilities are not available. Alternatively, Lipoptena spp. can be obtained from hosts that are more accessible during field studies. The present study demonstrated that DNA of the infectious agents might be identified in deer keds. In order to fully assess the potential of these ectoparasites as biological markers, it is necessary to compare the results of molecular analyses examining the blood samples with insects collected from the same animal.
Our studies showed that deer keds may harbor pathogenic microorganisms of significance; however, further investigation is needed to confirm whether intact and viable pathogens are indeed present, and if so, whether they can be transmitted by deer keds. Experiments performed on laboratory animals, which have not been performed to date, would elucidate the role of Lipoptena spp. in the eventual transmission of vector-borne diseases. Future research should focus on methods of controlling these ectoparasites and protecting humans and animals against their attacks. Greater attention should also be paid to L. fortisetosa in Central Europe, because its impact on indigenous cervid populations remains largely unknown.

4. Materials and Methods

4.1. Sample Collection

Deer keds were sampled in 2019 in five Polish voivodeships: Greater Poland, Kuyavia-Pomerania, Lubusz, Pomerania, and Warmia-Masuria. The location of these voivodeships on a map of Poland is presented in Figure 11. The collected specimens of L. fortisetosa were divided into two groups: Animals (A)—insects sampled from cervids, and Environment (E)—host-seeking insects sampled from the environment. A total of 500 L. fortisetosa individuals were sampled for the study. Group A was composed of 250 deer keds. Insects were collected from the bodies of dead or living cervids. One ectoparasite from each animal was randomly selected for analysis. Fifty individuals were acquired from each studied voivodeship. Group E consisted of 250 deer keds. Insects were collected in randomly selected Central European mixed forests. Up to 5 individuals of L. fortisetosa were acquired from each site. The investigator walked through the forest in the vicinity of wild animal habitats, wearing brown cotton clothing. Insects were captured after landing on the clothing and were immediately placed in test tubes. Fifty insects were obtained from each examined voivodeship. Group A and E ectoparasites were immersed in 70% ethanol in test tubes.

4.2. Species Identification

The sampled insects were analyzed in the Biological Hazard Laboratory at the Faculty of Veterinary Medicine of the University of Warmia and Mazury in Olsztyn. The species and sex of L. fortisetosa were identified based on the number of erect hairs on the mesonotum, the length and structure of palpi, wing venation, and body dimensions [3,44]. Images were acquired under the Leica M165C stereoscopic microscope (Leica, Wetzlar, Germany) with the use of Leica Application Suite 4.4 software (Leica, Wetzlar, Germany). Samples containing different insect species were excluded from further analysis.

4.3. DNA Extraction

Lipoptena fortisetosa were removed from test tubes, dried at room temperature for 15 min, and crushed individually with a sterile glass rod in sterile test tubes. Genomic DNA was extracted from each sample with the Sherlock AX universal kit (A&A Biotechnology, Gdynia, Poland) according to the manufacturer’s instructions. DNA was eluted in 40 µl of TE buffer. The concentration of the final product was determined with the Nano Drop 2000 spectrophotometer (Thermo Fisher Scientific, Waltham, USA). The extracted DNA was stored at −20 °C until analysis.

4.4. Selection of Pathogens for Analysis

Based on a review of the literature [67,68,69,70,71,72,73,74,75,76,77,78,79,80], the following pathogens were selected and identified: Anaplasma ovis, A. phagocytophilum, Babesia spp., Bartonella spp., Borellia spp., Coxiella burnetii, Francisiella tularensis, Mycoplasma spp., Rickettsia spp., and Theileria spp.

4.5. Polymerase Chain Reaction

Primer sequences and PCR conditions are presented in Table 4. Every reaction was carried out in a final volume of 25 µL, containing 2.5 µL of 10× Standard Taq Reaction Buffer (Biolabs, Boston, MA, USA, USA), 0.5 μL of 10 mM dNTPs (Biolabs, USA), 0.5 μL of 10 μM solution of each primer, 1 μL of extracted DNA, 0.125 µL of Taq DNA polymerase (Biolabs, USA), and 19.875 µL of double-distilled water. The reaction was carried out in the Veriti Thermal Cycler (Applied Biosystems, Foster City, CA, USA). DNA was replaced with double-distilled water in the negative sample. The positive sample consisted of DNA samples of each analyzed pathogen and L. fortisetosa collected in a previous study. PCR products were electrophoresed on 1.5–2.5% agarose gel using a 100 bp DNA ladder as a molecular-weight size marker, stained with ethidium bromide, and viewed under a UV transilluminator. The two strongest expressed bands in each studied pathogen were sequenced. All PCR products that were DNA positive for Francisella spp. were validated using sequencing.

4.6. Sequencing

DNA samples were purified by ethanol precipitation. Cycle-sequencing reactions were carried out with the use of the described primers, BigDye Terminator Cycle Sequencing Kit (Applied Biosystems, Foster City, CA, USA), and the ABI PRISM 3100 Genetic Analyzer (Applied Biosystems, Foster City, CA, USA). The obtained nucleotide sequences were edited in the BioEdit program [91] and compared with GenBank data in the BLAST-NCBI program. A phylogenetic analysis of the obtained sequences and the corresponding GenBank sequences was conducted by the Neighbor Joining estimation in MEGA 10.1.17 [92]. Bootstrap confidence values for estimating branching reliability were calculated in 10,000 replicates.

4.7. Statistical Analysis

The significance of possible relationships between the presence of pathogens and sample characteristics was determined in a logistic regression model, where the dependent variable was the dichotomous variable (absence (0)/presence (1) of the analyzed pathogen), whereas the insects’ sex (male/female), group (A or E), and site (examined voivodeships) were the independent variables. The associations between the prevalence of the analyzed pathogens were examined by calculating Cramer’s V, where values close to 0 denoted weak associations and values approximating +1/−1 denoted stronger associations. Data were processed statistically in the Statistica 13.3 program (TIBCO Software Inc., Palo Alto, Santa Clara, CA, USA).

5. Conclusions

The analyzed deer ked samples, obtained from animals and the environment, harbored the genetic material of A. phagocytophilum, Babesia spp., Bartonella spp., Borellia spp., Coxiella-like endosymbionts, Francisiella tularensis, Mycoplasma spp., Rickettsia spp., and Theileria spp. Deer keds may be used as biological markers for identifying pathogens in cervid populations, but further research is needed to confirm this assumption. Future research might reveal the competency of the L. fortisetosa as a biological or mechanical vector. The role of L. fortisetosa as a vector of pathogens requires further, more extensive investigations due to their new colonization sites and attacks on humans and animals. These are important considerations that require further attention.

Author Contributions

Conceptualization, R.G.; methodology, R.G.; software, R.G.; validation, R.G.; formal analysis, R.G. and E.M.G.; investigation, R.G.; resources, R.G.; data curation, R.G.; writing—original draft preparation, R.G.; writing—review and editing, R.G.; visualization, R.G.; supervision, J.J., X.X. and T.B.; project administration, R.G.; funding acquisition, R.G., J.J., X.X and T.B. All authors have read and agreed to the published version of the manuscript.

Funding

The project was financially supported by the Minister of Science and Higher Education under the program entitled “Regional initiative of Excellence” for the years 2019–2022, Project No. 010/RID/2018/19, amount of funding PLN 12,000,000. The funders had no role in the study design, data collection and analysis, decision to publish, or preparation of the manuscript.

Institutional Review Board Statement

Not applicable.

Informed Consent Statement

Not applicable.

Data Availability Statement

The original contributions presented in the study are included in the article. Further inquiries can be directed to the corresponding author.

Acknowledgments

The authors would like to thank the “Healthy Animal—Safe Food” Scientific Consortium of the Leading National Research Center (KNOW) (grant No. 05-1/KNOW2/2015) for supporting cooperation between the Faculty of Veterinary Medicine of the University of Warmia and Mazury in Olsztyn and the National Research Center for Protozoan Diseases of the Obihiro University of Agriculture and Veterinary Medicine. The authors are also grateful to hunters and forestry employees for their assistance in collecting research samples.

Conflicts of Interest

The authors declare no conflict of interest.

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Figure 1. Phylogenetic topology for Neighbor Joining analysis of the MSP4 gene sequence of Anaplasma phagocytophilum. The unique haplotypes identified in this study are labeled with the corresponding sequence identification numbers and with dots. The reference sequences from GenBank are indicated in the tree. Bootstrap confidence values for branching reliability were calculated in 10,000 replicates.
Figure 1. Phylogenetic topology for Neighbor Joining analysis of the MSP4 gene sequence of Anaplasma phagocytophilum. The unique haplotypes identified in this study are labeled with the corresponding sequence identification numbers and with dots. The reference sequences from GenBank are indicated in the tree. Bootstrap confidence values for branching reliability were calculated in 10,000 replicates.
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Figure 2. Phylogenetic topology for the Neighbor Joining analysis of the partial 18S rRNA gene sequence of Babesia spp. The unique haplotypes identified in this study are labeled with the corresponding sequence identification numbers and with dots. The reference sequences from GenBank are indicated in the tree. Bootstrap confidence values for branching reliability were calculated in 10,000 replicates.
Figure 2. Phylogenetic topology for the Neighbor Joining analysis of the partial 18S rRNA gene sequence of Babesia spp. The unique haplotypes identified in this study are labeled with the corresponding sequence identification numbers and with dots. The reference sequences from GenBank are indicated in the tree. Bootstrap confidence values for branching reliability were calculated in 10,000 replicates.
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Figure 3. Phylogenetic topology for the Neighbor Joining analysis of the partial 16-23S gene sequence of Bartonella spp. The unique haplotypes identified in this study are labeled with the corresponding sequence identification numbers and with dots. The reference sequences from GenBank are indicated in the tree. Bootstrap confidence values for branching reliability were calculated in 10,000 replicates.
Figure 3. Phylogenetic topology for the Neighbor Joining analysis of the partial 16-23S gene sequence of Bartonella spp. The unique haplotypes identified in this study are labeled with the corresponding sequence identification numbers and with dots. The reference sequences from GenBank are indicated in the tree. Bootstrap confidence values for branching reliability were calculated in 10,000 replicates.
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Figure 4. Phylogenetic topology for the Neighbor Joining analysis of the partial flagellin gene sequence of Borrelia spp. The unique haplotypes identified in this study are labeled with the corresponding sequence identification numbers and with dots. The reference sequences from GenBank are indicated in the tree. Bootstrap confidence values for branching reliability were calculated in 10,000 replicates.
Figure 4. Phylogenetic topology for the Neighbor Joining analysis of the partial flagellin gene sequence of Borrelia spp. The unique haplotypes identified in this study are labeled with the corresponding sequence identification numbers and with dots. The reference sequences from GenBank are indicated in the tree. Bootstrap confidence values for branching reliability were calculated in 10,000 replicates.
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Figure 5. Phylogenetic topology for the Neighbor Joining analysis of the partial 16S rRNA gene sequence of Coxiella spp. The unique haplotypes identified in this study are labeled with the corresponding sequence identification numbers and with dots. The reference sequences from GenBank are indicated in the tree. Bootstrap confidence values for branching reliability were calculated in 10,000 replicates.
Figure 5. Phylogenetic topology for the Neighbor Joining analysis of the partial 16S rRNA gene sequence of Coxiella spp. The unique haplotypes identified in this study are labeled with the corresponding sequence identification numbers and with dots. The reference sequences from GenBank are indicated in the tree. Bootstrap confidence values for branching reliability were calculated in 10,000 replicates.
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Figure 6. Phylogenetic topology for the Neighbor Joining analysis of the partial TUL4 gene sequence of Francisella spp. The unique haplotypes identified in this study are labeled with the corresponding sequence identification numbers and with dots. The reference sequences from GenBank are indicated in the tree. Bootstrap confidence values for branching reliability were calculated in 10,000 replicates.
Figure 6. Phylogenetic topology for the Neighbor Joining analysis of the partial TUL4 gene sequence of Francisella spp. The unique haplotypes identified in this study are labeled with the corresponding sequence identification numbers and with dots. The reference sequences from GenBank are indicated in the tree. Bootstrap confidence values for branching reliability were calculated in 10,000 replicates.
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Figure 7. Phylogenetic topology for the Neighbor Joining analysis of the partial 16S rRNA gene sequence of Arsenophonus spp. The unique haplotypes identified in this study are labeled with the corresponding sequence identification numbers and with dots. The reference sequences from GenBank are indicated in the tree. Bootstrap confidence values for branching reliability were calculated in 10,000 replicates. The obtained sequences were acquired by cross-reaction.
Figure 7. Phylogenetic topology for the Neighbor Joining analysis of the partial 16S rRNA gene sequence of Arsenophonus spp. The unique haplotypes identified in this study are labeled with the corresponding sequence identification numbers and with dots. The reference sequences from GenBank are indicated in the tree. Bootstrap confidence values for branching reliability were calculated in 10,000 replicates. The obtained sequences were acquired by cross-reaction.
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Figure 8. Phylogenetic topology for the Neighbor Joining analysis of the partial 16S rRNA gene sequence of Mycoplasma spp. The unique haplotypes identified in this study are labeled with the corresponding sequence identification numbers and with dots. The reference sequences from GenBank are indicated in the tree. Bootstrap confidence values for branching reliability were calculated in 10,000 replicates.
Figure 8. Phylogenetic topology for the Neighbor Joining analysis of the partial 16S rRNA gene sequence of Mycoplasma spp. The unique haplotypes identified in this study are labeled with the corresponding sequence identification numbers and with dots. The reference sequences from GenBank are indicated in the tree. Bootstrap confidence values for branching reliability were calculated in 10,000 replicates.
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Figure 9. Phylogenetic topology for the Neighbor Joining analysis of the partial gltA gene sequence of Rickettsia spp. The unique haplotypes identified in this study are labeled with the corresponding sequence identification numbers and with dots. The reference sequences from GenBank are indicated in the tree. Bootstrap confidence values for branching reliability were calculated in 10,000 replicates.
Figure 9. Phylogenetic topology for the Neighbor Joining analysis of the partial gltA gene sequence of Rickettsia spp. The unique haplotypes identified in this study are labeled with the corresponding sequence identification numbers and with dots. The reference sequences from GenBank are indicated in the tree. Bootstrap confidence values for branching reliability were calculated in 10,000 replicates.
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Figure 10. Phylogenetic topology for the Neighbor Joining analysis of the partial 18S rRNA gene sequence of Theileria spp. The unique haplotypes identified in this study are labeled with the corresponding sequence identification numbers and with dots. The reference sequences from GenBank are indicated in the tree. Bootstrap confidence values for branching reliability were calculated in 10,000 replicates.
Figure 10. Phylogenetic topology for the Neighbor Joining analysis of the partial 18S rRNA gene sequence of Theileria spp. The unique haplotypes identified in this study are labeled with the corresponding sequence identification numbers and with dots. The reference sequences from GenBank are indicated in the tree. Bootstrap confidence values for branching reliability were calculated in 10,000 replicates.
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Pathogens 10 00324 g011 550
Figure 11. Map of Poland highlighting voivodships where Lipoptena fortisetosa samples were collected. Legend: GP—Greater Poland voivodeship; KP—Kuyavia-Pomerania voivodeship; L—Lubusz voivodeship; P—Pomerania voivodeship; WM—Warmia-Masuria voivodeship.
Figure 11. Map of Poland highlighting voivodships where Lipoptena fortisetosa samples were collected. Legend: GP—Greater Poland voivodeship; KP—Kuyavia-Pomerania voivodeship; L—Lubusz voivodeship; P—Pomerania voivodeship; WM—Warmia-Masuria voivodeship.
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Table
Table 1. Prevalence of selected pathogens in Lipoptena fortisetosa with a division into voivodeships, groups, and sexes.
Table 1. Prevalence of selected pathogens in Lipoptena fortisetosa with a division into voivodeships, groups, and sexes.
SpeciesGroup AGroup ETotal n-500
n-250n-250
MFMF
n-99n-151n-115n-135
Anaplasma ovis0
(0%)		0
(0%)		0
(0%)		0
(0%)		0
(0%)
Anaplasma phagocytophilum6
(6.0%)		14
(9.3%)		0
(0%)		0
(0%)		20
(4%)
Babesia spp.21
(21.21%)		30
(19.86%)		0
(0%)		0
(0%)		51
(10.2%)
Bartonella spp.64
(64.65%)		94
(62.25%)		37
(32.17)		52
(38.52%)		247
(49.4%)
Borrelia spp.3
(3.03%)		9
(6.6%)		0
(0%)		0
(0%)		12
(24.30%)
Coxiella spp.3
(3.03%)		9
(6.6%)		1
(2.87%)		2
(1.48%)		15
(3%)
Francisella spp.2
(2.02%)		5
(3.31%)		0
(0%)		2
(1.48%)		9
(1.8%)
Mycoplasma spp.22
(22.22%)		52
(34.44%)		9
(7.82%)		8
(5.93%)		91
(18.2%)
Rickettsia spp.30
(30.30%)		46
(30.46%)		14
(12.17%)		16
(3.2%)		106
(21.2%)
Theileria spp.22
(22.22%)		27
(17.88%)		0
(0%)		0
(0%)		49
(9.8%)
Legend: A—Animals group; E—Environment group; M—male; F—female.
Table
Table 2. Logistic regression model presenting statistically significant relationships between the analyzed pathogens vs. the sex, group, and sampling site of deer keds.
Table 2. Logistic regression model presenting statistically significant relationships between the analyzed pathogens vs. the sex, group, and sampling site of deer keds.
Parasite Species
(Dependent Variables)		p-Value
(for the Model)		Independent VariablesSEWp-Value *OR
Total number<0.001sexM0.324.060.0440.584
F1.476
groupA0.2292.32<0.0018.04
E0.12
Anaplasma phagocytophilumsexM0.562.850.031.24
F0.88
Babesia spp.siteWM0.544.330.0373.09
L0.553.670.0452.85
Bartonella spp.groupA0.2026.04<0.0012.803
E0.36
Coxiella spp.groupA0.5824.4450.0353.410
E0.293
Mycoplasma spp.groupA0.28335.53<0.0015.40
E0.19
Rickettsia spp.groupA0.22616.559<0.0012.51
E0.40
Theileria spp.siteL0.6536.4830.0110.19
Legend: *—p-value < 0.05; SE—standard error; W—Wald coefficient; OR—odds ratio; M—male; F—female; A—animals group; E—environment group; WM—Warmia-Masuria; L—Lubusz.
Table
Table 3. Associations between the prevalence of the analyzed pathogens in Lipoptena fortisetosa, based on the calculated values of Cramer’s V.
Table 3. Associations between the prevalence of the analyzed pathogens in Lipoptena fortisetosa, based on the calculated values of Cramer’s V.
SpeciesAnaplasma phagocytophilumBabesia spp.Bartonella spp.Borrelia spp.Coxiella spp.Francisella tularensisMycoplasma spp.Rickettsia spp.Theileria spp.
Anaplasma phagocytophilum-0.033 b0.013 b0.21 *,a0.20 *,a0.057 b0.062 b0.035 b0.040 b
Babesia spp.0.079 a-0.024 b0.026 b0.029 b0.11 b0.041 b0.011 b0.050 b
Bartonella spp.0.026 a0.094 *,a-0.005 b0.016 b0.037 b0.029 b0.009 b0.04 b
Borrelia spp.0.21 *,a0.077 a0.032 a-0.032 b0.043 b0.1 b0.027 b0.078 b
Coxiella spp.0.16 *,a0.010 a0.037 a0.043 a-0.045 b0.073 b0.080 b0.025 b
Francisella spp.0.035 a0.12 *,a0.024 a0.025 a0.30 a-0.063 b0.059 b0.041 b
Mycoplasma spp.0.01 a0.13 *,a0.028 a0.128 *,a0.032 a0.13 a-0.028 b0.055 b
Rickettsia spp.0.01 a0.069 a0.077 a0.0080 a0.11 *,a0.039 a0.050 a-0.046 b
Theileria spp.0.08 *,a0.16 *,a0.11 a0.12 *,a0.012 a0.008 a0.052 a0.090 a-
Legend: *—χ2 p-value < 0.05; a—Cramer’s V for all samples; b—Cramer’s V for animals group samples.
Table
Table 4. Primers and PCR conditions.
Table 4. Primers and PCR conditions.
SpeciesTarget GeneName of PrimerPrimer Sequence (5′–3′)Expected Size (bp)PCR Cycle ConditionsReference
Anaplasma ovisMSP4MSP43RCCG GAT CCT TAG CTG AAC AGG AAT CTT GC34794 °C/5 min; 40 cycles: 94 °C/30 s, 60 °C/30 s, 72 °C/1 min; 72 °C/7 min Ochirkhuu et al. [81]
MSP45FGGG AGC TCC TAT GAA TTA CAG AGA ATT GTT TAC
Anaplasma phagocytophilumMSP4Aphamsp4FATGAATTACAGAGAATTGCTTGTAGG84994 °C/5 min; 40 cycles: 94 °C/10 s, 58 °C/10 s, 72 °C/50 s; 72 °C/5 minBown et al. [82]
Aphamsp4RTTAATTGAAAGCAAATCTTGCTCCTATG
Bovine * Babesia spp.18S rRNABabsppF1GTTTCTGMCCCATCAGCTTGAC44045 cycles: 94 °C/30 s, 61 °C/30 s, 72 °C/45 s; 72 °C/10 minHilpertshauser et al. [83]
BabsppRCAAGACAAAAGTCTGCTTGAAAC
Bartonella spp.16–23S geneBartonella spp. F(C/T)CTTCGTTTCTCTTTCTTCA154-26095 °C/2min; 45 cycles: 95 °C/1 min, 60 °C/1 min, 72 °C/30 s; 72 °C/5 min Jensen et al. [84]
Bartonella spp. RAACCAACTGAGCTACAAGCC
Borrelia spp.flagellinBorrelia spp. flaFACATATTCAGATGCAGACAGAGGT35095 °C/5 min; 40 cycles: 95 °C/1 min, 55 °C/1 min, 72 °C/30 s; 72 °C/5 min Barbour et al. [85]
Borrelia spp. flaRAACAGCTGAAGAGCTTGGAATG
Coxiella burnetii16S rRNACoxiella 16SrRNA FATTGAAGAGTTTGATTCTGG145795 °C/3 m; (2 cycles: 95 °C/30 s, 58 °C/30 s, 72 °C/2 min; 10 cycles: 95 °C/30 s, 58–50 °C/30 s (–2 every 2 cycles), 72 °C/2 min; 30 cycles: 95 °C/30 s, 48 °C/30 s, 72 °C/2 min); 72 °C/5 min Zheng et al. [86]
Coxiella 16SrRNA R CGGCTTCCCGAAGGTTAG
Francisella tularensisTUL4Ff393ATGGCGAGTGATACTGCTTG24898 °C/30 s; 35 cycles: 98 °C/10 s, 53.4 °C/ 30 s, 72 °C/1 min; 72 °C/10 minLong et al. [87]
Ff642GCATCATCAGAGCCACCTAA
Mycoplasma spp.16S rRNAHBT-FATA CGG CCC ATA TTC CTA CG59594 °C/10 min; 40 cycles: 95 °C/30 s, 60 °C/30 s, 72 °C/30 s; 72 °C/10 minLiu et al. [88]
HBT-RTGC TCC ACC ACT TGT TCA
Rickettsia spp.gltARickettsia gltA FGCAAGTATCGGTGAGGATGTAAT40195 °C/3 min; 40 cycles: 95 °C/15 s, 48 °C/30 s, 72 °C/30 s; 72 °C/7 min Labruna et al. [89]
Rickettsia gltA RGCTTCCTTAAAATTCAATAAATCAGGAT
Theileria spp.18S rRNA989AGT TTC TGA CCT ATC AG109894 °C/5 min; 35 cycles: 94 °C/30 s, 53 °C/30 s, 72 °C/1 min; 72 °C/7 min Li et al. [90]
990TTG CCT TAA ACT TCC TTG
Legend: *—B. divergens, B. bigemina, B. major.
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Gałęcki, R.; Jaroszewski, J.; Bakuła, T.; Galon, E.M.; Xuan, X. Molecular Detection of Selected Pathogens with Zoonotic Potential in Deer Keds (Lipoptena fortisetosa). Pathogens 2021, 10, 324. https://doi.org/10.3390/pathogens10030324

AMA Style

Gałęcki R, Jaroszewski J, Bakuła T, Galon EM, Xuan X. Molecular Detection of Selected Pathogens with Zoonotic Potential in Deer Keds (Lipoptena fortisetosa). Pathogens. 2021; 10(3):324. https://doi.org/10.3390/pathogens10030324

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Gałęcki, Remigiusz, Jerzy Jaroszewski, Tadeusz Bakuła, Eloiza M. Galon, and Xuenan Xuan. 2021. "Molecular Detection of Selected Pathogens with Zoonotic Potential in Deer Keds (Lipoptena fortisetosa)" Pathogens 10, no. 3: 324. https://doi.org/10.3390/pathogens10030324

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