Borrelia Diversity and Co-infection with Other Tick Borne Pathogens in Ticks.

Identifying Borrelia burgdorferi as the causative agent of Lyme disease in 1981 was a watershed moment in understanding the major impact that tick-borne zoonoses can have on public health worldwide, particularly in Europe and the USA. The medical importance of tick-borne diseases has long since been acknowledged, yet little is known regarding the occurrence of emerging tick-borne pathogens such as Borrelia spp., Anaplasma phagocytophilum, Rickettsia spp., Bartonella spp., "Candidatus Neoehrlichia mikurensis", and tick-borne encephalitis virus in questing ticks in Romania, a gateway into Europe. The objective of our study was to identify the infection and co-infection rates of different Borrelia genospecies along with other tick-borne pathogens in questing ticks collected from three geographically distinct areas in eastern Romania. We collected 557 questing adult and nymph ticks of three different species (534 Ixodes ricinus, 19 Haemaphysalis punctata, and 4 Dermacentor reticulatus) from three areas in Romania. We analyzed ticks individually for the presence of eight different Borrelia genospecies with high-throughput real-time PCR. Ticks with Borrelia were then tested for possible co-infections with A. phagocytophilum, Rickettsia spp., Bartonella spp., "Candidatus Neoehrlichia mikurensis", and tick-borne encephalitis virus. Borrelia spp. was detected in I. ricinus ticks from all sampling areas, with global prevalence rates of 25.8%. All eight Borrelia genospecies were detected in I. ricinus ticks: Borrelia garinii (14.8%), B. afzelii (8.8%), B. valaisiana (5.1%), B. lusitaniae (4.9%), B. miyamotoi (0.9%), B. burgdorferi s.s (0.4%), and B. bissettii (0.2%). Regarding pathogen co-infection 64.5% of infected I. ricinus were positive for more than one pathogen. Associations between different Borrelia genospecies were detected in 9.7% of ticks, and 6.9% of I. ricinus ticks tested positive for co-infection of Borrelia spp. with other tick-borne pathogens. The most common association was between B. garinii and B. afzelii (4.3%), followed by B. garinii and B. lusitaniae (3.0%). The most frequent dual co-infections were between Borrelia spp. and Rickettsia spp., (1.3%), and between Borrelia spp. and "Candidatus Neoehrlichia mikurensis" (1.3%). The diversity of tick-borne pathogens detected in this study and the frequency of co-infections should influence all infection risk evaluations following a tick bite.

Introduction

In Europe, ticks are the most ecologically important vectors of pathogens that cause both human and animal diseases (de la Fuente et al., 2008). Ixodes ricinus ticks are the most common ticks in Europe, and are broadly distributed across the entire continent. They are capable of transmitting a wide variety of zoonotic pathogens, such as viruses, bacteria, protozoa, and even helminths (Egyed et al., 2012). I. ricinus is also the most common questing tick species in Romania, representing 86.9% of ticks, followed by Dermacentor marginatus (9.5%), Haemaphysalis punctata (2.6%), and D. reticulatus (0.02%) (Mihalca et al., 2012a). Because I. ricinus feeds on a broad range of animals, this particular tick species transmits the widest variety of pathogens, including bacteria, parasites, and viruses. Amongst all I. ricinus-borne diseases reported in Europe, Lyme disease caused by some genospecies of Borrelia burgdorferi sensu lato (s.l.), is by far the most prevalent, with an estimated 85,000 annual cases (Subramanian et al., 2012). B. burgdorferi s.l. group currently comprises over 20 genospecies, nine of which are circulating in Europe (Clark et al., 2014). Among these, five genospecies are human pathogens: B. afzelii, B. garinii, B. burgdorferi sensu stricto (s.s.), B. bavariensis, and B. spielmanii; three are suspected human pathogens: B. lusitaniae, B. valaisiana, and B. finlandensis; and one genospecies, B. bissettii, has no clinical relevance to humans. Another Borrelia genospecies, Borrelia miyamotoi, belongs to the relapsing fever group and is transmitted by the same Ixodes species that also transmits B. burgdorferi s.l.. In 2013 B. miyamotoi was identified as a human pathogen in Europe (Hovius et al., 2013). This bacterium has been also recently identified in Romania (Kalmár et al., 2016).

The same tick may be co-infected with different Borrelia genospecies (Cosson et al., 2014) and various other tick-borne pathogens, with the possibility of co-transmission to either humans or animals (Moutailler et al., 2016). These co-infections might have consequences in terms of pathogen co-transmission (Swanson et al., 2006; Nieto and Foley, 2009; Agoulon et al., 2012; Chowdri et al., 2013; Gugliotta et al., 2013; Horowitz et al., 2013; Hovius et al., 2013; Tijsse-Klasen et al., 2013; Cosson et al., 2014; Knapp and Rice, 2015) that may also have important implications and relevance to public health (Diuk-Wasser et al., 2016). Indeed, co-infection in humans and animals might enhance disease severity as has been reported for concurrent babesiosis and Lyme disease (Grunwaldt et al., 1983; Golightly et al., 1989), or may have consequences in term of treatment and diagnosis (Diuk-Wasser et al., 2016).

The geopolitical location of Romania at the eastern border of the EU is strategically important from an epidemiological point of view. It represents a continual risk for emerging disease, not only in Romania, but also as a gateway into Europe. Only partial data has been collected on the prevalence of the Lyme disease agent or other tick-borne pathogens in eastern Romanian ticks and wildlife. However, it has been shown that Lyme disease is endemic in southern, eastern, and southeastern parts of Romania (Kalmar et al., 2013). From 2010, the Romanian National Centre for Surveillance and Control of Communicable Diseases has issued annual reports detailing the epidemiological situation of Lyme disease in humans. An average of 340 confirmed human Lyme disease cases were recorded annually between 2010 and 2015, with a mean incidence rate of 2.1 per 100,000 population, being situated at the lower level of the European incidence that ranges per country from less than one per 100,000 population to about 350 per 100,000 population (Rizzoli et al., 2011). Several studies have already reported the presence of Borrelia genospecies in questing ticks in Romania. Interestingly, these studies identified B. burgdorferi s.l. in I. ricinus ticks at a lower prevalence compared to the European average of 13.6% (Rauter and Hartung, 2005). A study involving over 12,000 questing ticks collected from 183 localities across all Romanian counties reported an overall B. burgdorferi s.l. prevalence of 1.4% (Kalmar et al., 2013). An alternate study of three southern and central Romanian counties recorded Lyme disease agent prevalence of up to 18.0% in unfed ticks (Coipan and Vladimirescu, 2011). Other studies in Romania have identified B. burgdorferi s.l. in I. ricinus ticks collected from different hosts such as lizards (Majláthová et al., 2008), horses (Ionita et al., 2013), hedgehogs (Dumitrache et al., 2013), and humans (Briciu et al., 2014). There are also reports of B. burgdorferi s.l. in tissues of wild mustelids (Gherman et al., 2012) and red foxes (Dumitrache et al., 2015). In these studies, the most commonly identified genospecies were B. afzelii, B. garinii, and B. burgdorferi s.s.

In Romania, as elsewhere in the world, limited work has been carried out on the occurrence of different Borrelia genospecies co-infections in questing ticks, including Borrelia with other tick-borne pathogens. Indeed, most studies have focused on the identification of single or a specific limited numbers of pathogens (Ionita et al., 2013, 2016; Kalmar et al., 2013; Matei et al., 2015; Kalmár et al., 2016), mainly due to technical constraints. Recently, we have implemented efficient high-throughput methods that enable broad-range co-detection of the most important known or putative tick-borne pathogens (Borrelia spp., Rickettsia spp., A. phagocytophilum, “Candidatus Neoehrlichia mikurensis”, Babesia spp., Bartonella spp. etc.) in individual tick samples (Michelet et al., 2014).

In the present study, our objective was to identify (co-) infection rates for different Borrelia genospecies along with other tick-borne pathogens in questing ticks collected from three sites in eastern Romania: One urban region dedicated to recreational activities and two forested areas.

Materials and methods

Tick sampling

Questing ticks were collected from 19 sampling sites distributed across six counties, covering three geographically distinct areas of eastern Romania (Figure 1). Each area represented a distinct habitat: A forested area in the north-eastern part of the country (sampling area 1), suburban sites intended for recreational activities (sampling area 2), and sites located in the southern part of the country including a forested and an arid region (sampling area 3). Ticks were collected by the dragging method. Dragging was performed over 5 transects of 300 m at each location. Each transect was divided into 10 sub-transects which were separated by 20 m, and the flag was examined after every 10 m of dragging, at the end of each segment. The surface covered at each collection site was ~1.5 hectares. In sampling area 2 (Figure 1), monthly collection was performed at each site, from March until September 2014. Tick collection in areas 1 and 3 was performed only once at each site, between May 2013 and September 2014.

Figure 1

Sampling areas in eastern Romania. Geographical areas were located in eastern Romania, comprising six counties across three distinct zones. Sampling areas 1 and 3 were mainly forested habitats, whereas sampling area 2 included six sites located in the vicinity of Iaşi recreational areas (C.A. Rosetti, Breazu, Ciric, Cetăţuia, Bârnova, and Bucium); Tick sampling took place from May 2013 until September 2014. (1)—Sampling area 1 covering four counties: SV, Suceava; BT, Botoşani; NT, Neamt; BC, Bacău.(2)—Sampling area 2: Iaşi—representing collection sites located in Iaşi recreational areas (Breazu, C.A. Rosseti, Ciric, Cetăţuia, Bârnova, Bucium). (3)—Sampling area 3 located in Tulcea county.

Sampling area 1 included six forested collection sites across four counties that were selected based on their proximity to rural settlements. (46.536747 N, 26.821123 E; 47.23221 N, 26.54634 E; 46.517207 N, 26.187067 E; 47.780000 N, 25.718600 E; 47.550000 N, 25.950000 E; and 47.779500 N, 26.516000 E) (Figure 1).

Sampling area 2 included six collection sites near Iaşi city recreational areas [Breazu (47.212044 N, 27.530304 E), C.A. Rosetti (47.204710 N, 27.556685 E), Ciric (47.178178 N, 27.609791 E), Cetăţuia (47.132564 N, 27.582936 E), Bârnova (47.059598 N, 27.640815 E), and Bucium (47.068330 N, 27.664561 E)] (Figure 1). The main criterion used for selection of collection sites was potential public exposure to vector ticks, and thus we included the major recreational sites around the city of Iaşi. Deciduous trees and meadows are the predominant vegetation at these sites (designated suburban forest) (Pavel et al., 2014).

Sampling area 3 included seven collection sites from Tulcea County (45.269722 N, 28.459722 E; 45.215936 N, 28.415648 E; 45.26293 N, 28.16968 E; 44.891311 N, 28.717223 E; 44.873796 N, 28.735763 E; 44.865767 N, 28.810092 E and 44.86309 N, 28.689242 E) that were located mostly in forested and arid zones (Figure 1). This area has an arid or coastline type climate (Moise and Dumitru, 2012).

Tick species and developmental stages were identified under a stereomicroscope using standard morphological identification keys (Perez-Eid, 2007), then stored individually at −80°C.

DNA and RNA extraction

Individual adult and nymph I. ricinus were lysed using 2.8 mm stainless steel beads in 300 μl of culture cell medium (Dulbecco's Modified Eagle medium, Gibco by Life technologies, UK) complemented with 10% fetal calf serum as previously described (Vayssier-Taussat et al., 2012). Ticks were homogenized using Precellys 24 lyser/homogenizer (Bertin, France) at 5500 rpm for 20 s. After homogenization, each tube was centrifuged at 1,500 rpm for 2 min. DNA and RNA extraction was performed on 100 μL aliquots using the Nucleospin Tissue kit or the Nucleospin RNA II kit (Macherey Nagel, Germany) according to the manufacturer's instructions. Purified DNA and RNA was eluted into 50 μL elution buffer, RNase-free water respectively.

Detection of borrelia genospecies DNA in questing I. ricinus

The BioMark™ real-time PCR system (Fluidigm, USA) was used for high-throughput microfluidic real-time PCR for the detection of the genus Borrelia: Seven genospecies belonging to the Lyme disease spirochete group, B. burgdorferi s.l. (B. burgdorferi s.s., B. afzelii, B. garinii, B. spielmanii, B. valaisiana, B. lusitaniae, and B. bissettii) and one genospecies from the recurrent fever group (B. miyamotoi) (Table 1). A DNA pre-amplification step was performed in a final volume of 5 μL containing 2.5 μL TaqMan PreAmp Master Mix (2X), 1.2 μL of the pooled primer mix (0.2X mix containing specific primer pairs for each of the eight Borrelia genospecies analyzed) and 1.3 μL of tick DNA, with one cycle at 95°C for 10 min, 14 cycles at 95°C for 15 s and 4 min at 60°C. Following pre-amplification, qPCRs were performed using FAM- and black hole quencher (BHQ1)-labeled TaqMan probes (Michelet et al., 2014) with TaqMan Gene Expression Master Mix in accordance with manufacturer's instructions (Applied Biosystems, France). Thermal cycling conditions were as follows: 95°C for 5 min, 45 cycles at 95°C for 10 s, 60°C for 15 s, and 40°C for 10 s. Data were acquired on the BioMark™ real-time PCR system and analyzed using the Fluidigm real-time PCR Analysis software to obtain crossing point (CP) values. Assays were performed in duplicate and two negative water controls were included per analysis and none of them were found positive after amplification. I. ricinus DNA served to confirm the tested tick species and as a DNA extraction control (Michelet et al., 2014). Moreover, to determine if factors present in the samples could inhibit PCR (false negative results), E. coli strain EDC933 DNA was added to each sample as internal inhibition control (Michelet et al., 2014). E. coli and I. ricinus DNA were amplified in all samples confirming the absence of false negative results.

Table 1

Primer sets for pathogen DNA amplification and sequencing in ticks.

Pathogen	Target gene	Primers	Nucleotide sequence (5′–3′)	Amplicon size (bp)	References
Bartonella spp.	gltA	bart781 bart1137	GGGGACCAGCTCATGGTGG AATGCAAAAAGAACAGTAAACA	380–400	Norman et al., 1995
Rickettsia spp.	gltA	Rsfg877 Rsfg1258	GGGGGCCTGCTCACGGCGG ATTGCAAAAAGTACAGTGAACA	381	Regnery et al., 1991
Borrelia spp.	23S rRNA	Bo_bu_sl_23S_F Bo_bu_sl_23S_R Bo_bu_sl_23S_P	GAGTCTTAAAAGGGCGATTTAGT CTTCAGCCTGGCCATAAATAG AGATGTGGTAGACCCGAAGCCGAGT	73	Michelet et al., 2014
Borrelia burgdorferi, sensu stricto	rpoB	Bo_bu_rpoB_F Bo_bu_rpoB_R, Bo_bu_rpoB_P	GCTTACTCACAAAAGGCGTCTT GCACATCTCTTACTTCAAATCCT AATGCTCTTGGACCAGGAGGACTTTCA	83	Michelet et al., 2014
Borrelia garinii	rpoB	Bo_ga_rpoB_F Bo_ga_rpoB_R Bo_ga_rpoB_P	TGGCCGAACTTACCCACAAAA ACATCTCTTACTTCAAATCCTGC TCTATCTCTTGAAAGTCCCCCTGGTCC	88	Michelet et al., 2014
Borrelia afzelii	fla	Bo_af_fla_F Bo_af_fla_R Bo_af_fla_P	GGAGCAAATCAAGATGAAGCAAT TGAGCACCCTCTTGAACAGG TGCAGCCTGAGCAGCTTGAGCTCC	116	Michelet et al., 2014
Borrelia valaisiana	ospA	Bo_va_ospA_F Bo_va_ospA_R Bo_va_ospA_P	ACTCACAAATGACAGATGCTGAA GCTTGCTTAAAGTAACAGTACCT TCCGCCTACAAGATTTCCTGGAAGCTT	135	Michelet et al., 2014
Borrelia lusitaniae	rpoB	Bo_lus_rpoB_F Bo_lus_rpoB_R Bo_lus_rpoB_P	CGAACTTACTCATAAAAGGCGTC TGGACGTCTCTTACTTCAAATCC TTAATGCTCTCGGGCCTGGGGGACT	87	Michelet et al., 2014
Borrelia spielmanii	fla	Bo_spi_fla_F Bo_spi_fla_R Bo_spi_fla_P	ATCTATTTTCTGGTGAGGGAGC TCCTTCTTGTTGAGCACCTTC TTGAACAGGCGCAGTCTGAGCAGCTT	71	Michelet et al., 2014
Borrelia bissettii	rpoB	Bo_bi_rpoB_F Bo_bi_rpoB_R Bo_bi_rpoB_P	GCAACCAGTCAGCTTTCACAG CAAATCCTGCCCTATCCCTTG AAAGTCCTCCCGGCCCAAGAGCATTAA	118	Michelet et al., 2014
Borrelia miyamotoi	glpQ	B_miya_glpQ_F B_miya_glpQ_R B_miya_glpQ_P	CACGACCCAGAAATTGACACA GTGTGAAGTCAGTGGCGTAAT TCGTCCGTTTTCTCTAGCTCGATTGGG	94	Michelet et al., 2014
Anaplasma phagocytophilum	msp2	An_ph_msp2_F An_ph_msp2_R An_ph_msp2_P	GCTATGGAAGGCAGTGTTGG GTCTTGAAGCGCTCGTAACC AATCTCAAGCTCAACCCTGGCACCAC	77	Michelet et al., 2014
Candidatus Neoehrlichia mikurensis	groEL	Neo_mik_groEL_F Neo_mik_groEL_R Neo_mik_groEL_P	AGAGACATCATTCGCATTTTGGA TTCCGGTGTACCATAAGGCTT AGATGCTGTTGGATGTACTGCTGGACC	96	Michelet et al., 2014
TBEV	3′ non-coding region	F-TBE 1 R-TBE 1 TBE-Probe-WT	GGGCGGTTCTTGTTCTCC ACACATCACCTCCTTGTCAGACT TGAGCCACCATCACCCAGACACA	67	Schwaiger and Cassinotti, 2003
	non-structural protein NS5	Outer primers: FSM-1 FSM-2	GAGGCTGAACAACTGCACGA GAACACGTCCATTCCTGATCT	357	Schwaiger and Cassinotti, 2003
	non-structural protein NS5	Inner primers: FSM-li FSM-2i	ACGGAACGTGACAAGGCTAG GCTTGTTACCATCTTTGGAG	251	Schwaiger and Cassinotti, 2003

Detection of co-infections with other tick-borne pathogens

Bartonella spp. and Rickettsia spp.: All DNA samples positive for Borrelia genospecies were screened for the presence of Bartonella spp. and Rickettsia spp. via PCR. Detection was carried out using specific primers targeting the gltA gene of both Bartonella spp. (Norman et al., 1995) and Rickettsia spp. (Table 1) (Regnery et al., 1991). PCR products were amplified using the Thermo Scientific Phusion High-Fidelity PCR Kit (Thermo Scientific, USA). Each reaction was carried out in a 20 μl reaction volume containing 5 μl tick DNA, 4 μl 5 X PCR buffer, 200 μM of each dNTP, 0.5 μM of each primer, and 0.4 U phusion DNA polymerase. Thermal conditions were 98°C for 30 s, followed by 35 cycles at 98°C for 10 s, 52°C (for Bartonella spp.) or 56°C (for Rickettsia spp.) for 30 s, and 72°C for 30 s, with a final elongation at 72°C for 10 min. The 380–400 bp Bartonella-specific fragment and the 381 bp Rickettsia-specific fragment were sequenced by Eurofins MWG Operon (Ebesberg, Germany). Sequences were assembled using BioEdit software (Hall, 1999), and compared to the NCBI database for species identification.

A. phagocytophilum, “C. N. mikurensis”: Real-time PCR assays were performed using primers and probes targeting the msp2 gene for A. phagocytophilum, and the groEL gene for “C. N. mikurensis” (Table 1) (Michelet et al., 2014). All fluorogenic probes were synthesized with a 6-carboxy-fluorescein (FAM) reporter molecule attached to the 5′ end and a Black Hole Quencher 1 (BHQ1) at the 3′ terminus. Real-time Taqman PCR assays were performed in a final volume of 12 μl using the LightCycler® 480 Probe Master mix (Roche Applied Science, Germany) at 1 X final concentration, with primers and probes at 200 nM, and 2 μl DNA. Negative (water) and positive controls were included with each run. Thermal cycling conditions were as follows: 95°C for 5 min, 45 cycles at 95°C for 10 s, then 60°C for 15 s, with a final cooling step at 40°C for 10 s.

TBEV: RNA samples were screened for tick-borne encephalitis virus (TBEV) by rRT-PCR targeting a 3′ non-coding region of the TBEV genome with specific primers and probes (Table 1) (Schwaiger and Cassinotti, 2003). rRT-PCR Taqman assays were performed in a final volume of 20 μl using the LightCycler® 480 RNA Master Hydrolysis Probes master mix (Roche Applied Science, Germany) at 1 X final concentration, with 0.5 μM specific primers and 0.25 μM probes, 3.25 mM manganese acetate [Mn(OAc)2] and 2 μl RNA. Positive and negative (water) controls were included in each run. rRT-PCR thermal cycling conditions were as follows: 63°C for 3 min, 95°C for 30 s, 45 cycles at 95°C for 10 s, then 60°C for 30 s, followed by cooling at 40°C for 10 s. Positive samples were used for one-step RT-PCR and nested PCR targeting the non-structural protein gene NS5 (Puchhammer-Stockl et al., 1995). Positive RNA samples were reverse transcribed using Titan One Tube RT-PCR Systems (Roche Applied Science, Germany) in a 50 μl reaction volume containing 10 μl tick RNA, 10 μl 5 X RT-PCR buffer, 200 μM of each dNTP, 0.4 μM of each primer, 1 μl enzyme mix and 500 μM dithiothreitol (DTT). Thermal cycling conditions were 50°C for 30 min, 95°C for 3 min, followed by 35 cycles at 95°C for 30 s, 40°C for 30 s, and 72°C for 30 s, with a final step at 72°C for 5 min. Nested PCR was performed using the Thermo Scientific Phusion High-Fidelity PCR Kit (Thermo Scientific, USA). PCRs were carried out in a 50 μl reaction volume containing 5 μl tick cDNA, 10 μl 5 X PCR buffer, 200 μM of each dNTP, 0.5 μM of each internal primer, and 1 U Phusion DNA polymerase. Thermal conditions were 98°C for 30 s, followed by 35 cycles at 98°C for 10 s, 53 C for 30 s, and 72°C for 60 s, and a final elongation at 72°C for 10 min.

Statistical analysis

The data were processed using IBM SPSS® Statistics version 21 (IBM® Corporation, Chicago, IL, USA) software. One-way analysis of variance (ANOVA) tests (Bonferroni post-hoc test) were performed on tick infection rates for geographic groups. Prevalence rates were compared between tick developmental stages using independent sample T-tests. In cases of statistical significance, p-values are presented in parentheses. Differences were considered statistically significant when p < 0.05.

Results

Tick collection

Using the dragging protocol, we collected 557 ticks belonging to three different species: I. ricinus (from all sampling areas), Dermacentor reticulatus (only from sampling area 2), and H. punctata (from sampling areas 2 and 3). I. ricinus ticks represented 95.9% (534/557) of the collected ticks, with 77 adult ticks and 457 nymphs, D. reticulatus represented 0.7% (4/557) of collected ticks with four adults, and H. punctata represented 3.4% (19/557) of collected ticks with three adults and 16 nymphs.

Borrelia genospecies detected in ticks

Borrelia spp. DNA was identified in 138/534 (25.8%) of I. ricinus ticks collected from all sampling sites, in none of the four D. reticulatus ticks, and in 1/19 (5.3%) H. punctata collected from area 2. Borrelia genospecies found in H. punctata was identified as B. miyamotoi. The B. miyamotoi-positive H. punctata was not co-infected with other screened tick-borne pathogens.

In I. ricinus ticks, Borrelia spp. infection rates were not significantly different between adults (26.0%; 20/77) and nymphs (25.8%; 118/457) (p > 0.05). Borrelia spp. prevalence was significantly higher in I. ricinus ticks collected from area 3 in the southernmost sector of eastern Romania, than in ticks from areas 1 (p < 0.05) and 2 (p < 0.05) (40.0% vs. 25.0% or 25.0% in adults, and 40.0% vs. 22.0% or 16.7% in nymphs).

Eight genospecies of Borrelia were identified: B. garinii, B. afzelii, B. valaisiana, B. lusitaniae, B. spielmanii, B. burgdorferi s.s., B. bissettii, and B. miyamotoi. The mean infection rate was 14.8% for B. garinii (16.9% of the adults and 14.4% of the nymphs), 8.8% for B. afzelii (7.8% of adults and 9.0% of nymphs), 5.1% for B. valaisiana (5.2% of adults and 5.0% of nymphs), 4.9% for B. lusitaniae (5.2% of adults and 4.8% of nymphs), 1.1% for B. spielmanii (1.3% of adults and 1.1% of nymphs), 0.9% for B. miyamotoi (1.3% of adults and 0.9% of nymphs), 0.4% for B. burgdorferi s.s. (0.4% of nymphs), and 0.2% for B. bissettii (0.2% of nymphs).

The infection rates of different Borrelia genospecies in I. ricinus ticks according to collection site is shown in Table 2. Ticks collected from area 1 were more frequently infected with B. afzelii but did not register statistical significance. Ticks from area 3 were more frequently infected with B. garinii, with a statistically significant difference only when compared to B. garinii infection rates in area 2 (p < 0.05). B. valaisiana also demonstrated a high infection rate in area 3, which was statistically different to the prevalence rate obtained in area 2 (p < 0.05). B. lusitaniae prevalence was significantly higher in area 3 than in areas 1 and 2 (p < 0.05). B. spielmanii was detected in areas 2 and 3 with similar infection rates; B. burgdorferi s.s. was only detected in areas 1 and 2, and B. bissettii was only detected in area 1. Relapsing fever agent B. miyamotoi was only detected in areas 1 and 2 (see Table 2).

Table 2

.

Sampling area	Tick samples (no. of samples)	B. garinii	B. afzelii	B. valaisiana	B. lusitaniae	B. spielmanii	B. burgdorferi s.s.	B. bissettii	B. miyamotoi
Sampling area 1	Adults (8)	2/25.0	1/12.5		1/12.5
	Nymphs (59)	7/11.9	8/13.6				1/1.7	1/1.7	1/1.7
	Total (67)	9/13.4	9/13.4		1/1.5		1/1.5	1/1.5	1/1.5
Sampling area 2	Adults (64)	9/14.1	4/6.3	4/6.3	2/3.1	1/1.6			1/1.6
	Nymphs (233)	19/8.2	18/7.7	6/2.6	4/1.7	2/0.9	1/0.4		3/1.3
	Total (297)	28/9.4	22/7.4	10/3.4	6/2.0	3/1.0	1/0.3		4/1.4
Sampling area 3	Adults (5)	2/40.0	1/20.0		1/20.0
	Nymphs (165)	40/24.2	15/9.1	17/10.3	18/10.9	3/1.8
	Total (170)	42/24.7	16/9.4	17/10.0	19/11.2	3/1.8
Total	Adults (77)	13/16.9	6/7.8	4/5.2	4/5.2	1/1.3			1/1.3
	Nymphs (457)	66/14.4	41/9.0	23/5.0	22/4.8	5/1.1	2/0.4	1/0.2	4/0.9
	Total (534)	79/14.8	47/8.8	27/5.1	26/4.9	6/1.1	2/0.4	1/0.2	5/0.9

.

Co-infections in Ixodes ricinus

Co-infections were identified in 16.7% I. ricinus ticks (89/534), which accounted for 64.5% (89/138) of all infected ticks. Co-infection prevalence was 14.3% (11/77) in adults and 17.1% (78/457) in nymphs. Co-infection rates were significantly higher in area 3 (27.7%; 47/170) than in areas 1 and 2 (14.9%; 10/67 and 10.8%; 32/297, respectively) resulting in a statistically significant difference only when compared to area 2 (p < 0.05).

Co-infection between Borrelia genospecies

The overall prevalence of B. burgdorferi s.l. genospecies co-infection was 9.7% (52/534; 9.1% of adults and 9.8% of nymphs). Forty-five I. ricinus ticks were co-infected with two B. burgdorferi s.l. genospecies. The most frequent Borrelia genospecies association was between B. garinii and B. afzelii (23/534; 4.3%), followed by B. garinii and B. lusitaniae (16/534; 3.0%). Triple B. burgdorferi s.l. genospecies co-infection was identified in seven I. ricinus ticks, four of which were infected with B. garinii, B. afzelii, and B. valaisiana (Table 3). Co-infection rates between Borrelia genospecies were significantly higher in area 3 [15.3% (26/170; 40.0% adults and 14.5% nymphs)] than in areas 1 and 2 [8.9% (6/67; 10.1% nymphs) and 6.7% (20/297; 7.8% adults and 6.4% nymphs)], respectively (p < 0.05).

Table 3

Co-infection between .

Pathogen associations	Area 1			Area 2			Area 3			Total No.
	A	N	Total	A	N	Total	A	N	Total	A	N	Total
B. garinii + B. afzelii		5	5	3	9	12	1	5	6	4	19	23
B. garinii + B. lusitaniae					1	1	1	14	15	1	15	16
B. garinii + B. spielmanii					2	2		1	1		3	3
B. afzelii + B. bissettii		1	1								1	1
B. afzelii + B. lusitaniae					1	1					1	1
B. garinii + B. valaisiana								1	1		1	1
B. garinii + B. afzelii + B. valaisiana					1	1		3	3		4	4
B. garinii + B. afzelii + B. lusitaniae					1	1					1	1
B. garinii + B. afzelii + B. spielmanii				1		1				1		1
B. garinii + B. valaisiana + B. lusitaniae				1		1				1		1
B. garinii + R. monacensis					1	1		1	1		2	2
B. valaisiana + Bartonella spp.				1	1	2				1	1	2
B.afzelii + “C N mikurensis”					2	2					2	2
B. valaisiana + “C N mikurensis”								2	2		2	2
B. valaisiana + R. monacensis				1		1				1		1
B. valaisiana + Rickettsia spp.					1	1					1	1
B. afzelii + Rickettsia spp.		1	1								1	1
B. miyamotoi + “C N mikurensis ”		1	1								1	1
B. miyamotoi + Bartonella spp.					1	1					1	1
B. garinii + Bartonella spp.					1	1					1	1
B. spielmanii + A. phagocytophilum								1	1		1	1
B. garinii + Rickettsia spp.								1	1		1	1
B. garinii + “C N mikurensis”								1	1		1	1
B. afzelii + R. helvetica								1	1		1	1
Borrelia spp. + “C N mikurensis”								1	1		1	1
Borrelia spp. + Bartonella spp.					1	1					1	1
B. garinii + B. afzelii + Rickettsia spp.	1		1		1	1		1	1	1	2	3
B. garinii + B. lusitaniae + Rickettsia spp.	1		1					1	1	1	1	2
B. garinii + B. afzelii + R. monacensis								2	2		2	2
B. valaisiana + B. spielmanii + R. monacensis								1	1		1	1
B. garinii + B. valaisiana + R. helvetica								1	1		1	1
B. garinii + B. afzelii + A. phagocytophilum								1	1		1	1
B. garinii + B. afzelii + “C N mikurensis”								1	1		1	1
B. garinii + B. valaisiana + “C N mikurensis”								1	1		1	1
B. garinii + R. helvetica + Bartonella spp.								1	1		1	1
B. valaisiana + R. monacensis + “C N mikurensis”								1	1		1	1
B. valaisiana + Rickettsia spp. + “C N mikurensis”								1	1		1	1
Borrelia spp. + R. monacensis + “C N mikurensis”								1	1		1	1
B. garinii + B. afzelii + B. lusitaniae + “C N mikurensis”					1	1					1	1
Total	2	8	10	7	25	32	2	45	47	11	78	89

A (Adult ticks), N (Nymphs), “Candidatus Neoehrlichia mikurensis” (“C. N. mikurensis”).

Co-infection between Borrelia genospecies and other tick-borne pathogens

Co-infections of Borrelia genospecies with other tick-borne pathogens occurred in 6.9% of all collected I. ricinus ticks (37/534; 5.2% of adults and 7.2% of nymphs), and were observed in ticks from all three sampling areas as follows: 6.0% of ticks from area 1 (4/67; 25.0% of adults and 3.4% of nymphs), 4.0% of ticks from area 2 (12/297; 3.1% of adults and 4.3% of nymphs), and 12.4% of ticks from area 3 (21/170; 12.7% of nymphs).

Dual co-infection between one Borrelia genospecies and another pathogen occurred in 20 I. ricinus ticks (20/534; 3.7%). The most frequent co-infection was between Borrelia spp. and Rickettsia spp., and between Borrelia spp. and “C. N. mikurensis”, where each association was detected in seven different I. ricinus ticks. Five samples tested positive for Borrelia spp. and Bartonella spp., and one tick was co-infected with Borrelia spp. and A. phagocytophilum.

Association of two Borrelia genospecies with another pathogen genus was detected in 12 ticks (12/534; 2.4%), of which nine ticks tested positive for co-infection with two Borrelia genospecies and one Rickettsia spp. We detected two samples infected with Borrelia genospecies and “C. N. mikurensis”, and one sample co-infected with two Borrelia genospecies and A. phagocytophilum.

We also recorded four (4/534; 0.7%) ticks infected with one Borrelia genospecies and two other pathogen genera: Three ticks positive for the association of Borrelia spp. + Rickettsia spp. + “C. N. mikurensis”, and one tick positive for Borrelia spp., Rickettsia spp., and Bartonella spp. One tick was positive for three different Borrelia genospecies (B. garinii, B. afzelii, B. lusitaniae), and “C. N. mikurensis” (Table 3).

We did not identify co-infections between Borrelia genospecies with tick-borne encephalitis virus.

Discussion

Using a powerful high-throughput tool we performed a comprehensive overview of the epidemiological status of Lyme spirochetes circulating and co-circulating with other important tick-borne pathogens in eastern Romanian ticks. The most important findings were: (1) the identification of seven different genospecies of the Lyme spirochete group—including B. miyamotoi—with an overall high Borrelia prevalence rate (25.8% of ticks infected); (2) the frequency of co-infection: Among Borrelia-infected ticks, 64.5% were co-infected; (3) the unexpected high infection and co-infection rates of ticks collected from the Danube Delta biosphere (area 3). Together, these results may have important implications in terms of public health issues in a country where Lyme disease surveillance has only been implemented since 2009.

In our study, the overall Borrelia prevalence rate across all sampling areas (25.8%), was much higher than compared to previous studies of this Lyme disease agent in questing I. ricinus ticks from Romania that reported prevalences ranging from 3.8 to 18% (Coipan and Vladimirescu, 2011; Kalmar et al., 2013). This result is likely due to high sensitivity of our techniques which combines pathogen DNA pre-amplification steps with specific quantitative amplification of target pathogen DNA.

Different Borrelia genospecies identified

B. garinii and B. afzelii were the most abundant Borrelia genospecies in our study, as has been previously reported in Romanian ticks (Coipan and Vladimirescu, 2010, 2011; Kalmar et al., 2013; Briciu et al., 2014). Several other studies have shown that certain Borrelia genospecies have preferred reservoir hosts; B. garinii is mostly associated with birds, whereas B. afzelii genospecies are predominantly isolated from medium-sized and small mammals, especially rodents (Dubska et al., 2009; Rizzoli et al., 2011; Mannelli et al., 2012). Hence Borrelia genospecies prevalence in specific areas is thus closely related to the abundance of competent reservoir hosts (Rizzoli et al., 2011). The high prevalence of B. garinii might be due to the increased density of bird-based enzootic cycles in eastern Romania, especially in area 3 (Danube Delta region), which represents an important stopover site for over 300 different avian species migrating between northern Eurasia and Africa (Sándor et al., 2014). Northward, near Iaşi, 129 bird species have been identified (Gache, 2016) including song thrushes (Turdus philomelos) and blackbirds (T. merula), reported to be the principle B. garinii reservoir in central Europe (Taragel'ova et al., 2008). B. afzelii was the second most prevalent genospecies, and is predominantly cycled throughout Europe via rodent species (Apodemus sylvaticus, A. agrarius, A. flavicollis, and Myodes glareolus), known common tick hosts (Mihalca et al., 2012b). The 32 species of wild rodents found in Romania (Mihalca et al., 2012b) emphasize the significant biodiversity and availability of putative B. afzelii reservoir hosts.

Borrelia valaisiana and B. lusitaniae had similar infection rates in questing ticks, and B. lusitaniae was detected at all three sampling areas. The pathogenicity of these genospecies is still uncertain, even though there is evidence of their presence in skin biopsies and cerebrospinal fluid of patients with Lyme disease (Diza et al., 2004; Rauter and Hartung, 2005). Similarly to B. garinii, B. valaisiana is more commonly identified in birds, while B. lusitaniae is mainly associated with lizards (Rizzoli et al., 2011; Mannelli et al., 2012). We report higher B. valaisiana and B. lusitaniae infection rates in Romania compared to previous studies (de la Fuente et al., 2008; Kalmar et al., 2013), which may be a result of high reservoir host density. In Romania, lizards are commonly found, the green lizard (Lacerta viridis) and sand lizard (Lacerta agilis) are both widely distributed throughout our study areas (Cogalniceanu et al., 2013). The role of these host species in the transmission cycle of B. lusitaniae has been studied in Slovakia, Poland, and Romania (Majlathova et al., 2006; Majláthová et al., 2008), thus it is likely that their presence induces favorable conditions for B. lusitaniae persistence in eastern Romania.

We also detected three other B. burgdorferi s.l. group genospecies at low levels: B. burgdorferi s.s., B. spielmanii, and B. bissettii. B. burgdorferi s.s. and B. spielmanii are recognized human pathogens in Europe, while B. bissettii's role in human disease remains unclear (Briciu et al., 2014). Small mammals and birds are the preferred reservoir hosts for B. burgdorferi s.s., dormice for B. spielmanii, and rodents for B. bissettii (Eisen et al., 2009).

Borrelia miyamotoi represents the only known relapsing fever group agent transmitted by Ixodes species (Potkonjak et al., 2016) with probable reservoir hosts of field mice, birds, and voles (Krause et al., 2015). B. miyamotoi has sporadic geographic distribution and has been detected in many European countries, in North America, and Asia (Crowder et al., 2014). In 2016, Kalmár et al. first reported the identification of this agent in questing ticks from central Romania (Kalmár et al., 2016). Our study confirms the existence of this pathogen in ixodid ticks from eastern Romania at a low infection rate and with limited geographic expansion.

Prevalence according to collection sites

Borrelia genospecies were detected at all studied areas. Infection rates in ticks from area 1 (deciduous and mixed forest vegetation) was similar to area 2 (urban area, B. burgdorferi s.l. was detected in 18.5% of ticks), thus highlighting a significant Lyme disease risk in area 2 a heavily frequented recreational hotspot. Lyme spirochetes prevalence was surprisingly higher in ticks collected from the forested but arid area 3 in southeastern Romania (40.0%) than in ticks from the other two more northern areas, which both represent a more typical landscape for I. ricinus and Borrelia spirochetes.

Sampling area 3 was located in the Danube Delta Biosphere Reserve known to harbor a wide variety of mammals, migratory and resident bird species all previously described as tick hosts (Sándor et al., 2014). Thus, the combination of abundant bird fauna and the diversity of tick species might explain the high prevalence of bird-associated B. garinii and B. valaisiana.

Interestingly, the second most prevalent genospecies in questing ticks from area 3 was B. lusitaniae (11.2%), which was also more prevalent in area 3 than the other two studied areas. Under natural conditions Borrelia lusitaniae circulates between lizards and ticks (Majláthová et al., 2008), and three lizard species (Podarcis muralis, Lacerta viridis, L. agilis) are designated as B. lusitaniae reservoirs (Majláthová et al., 2008). In area 3, many lizard species have been identified (L. agilis, L. viridis, L. trilineata, P. muralis, P. tauricus) (Cogalniceanu et al., 2013), and likely contribute to the high B. lusitaniae tick infection rate. Under conditions of relatively low humidity, such as in area 3, nymphs seek out their hosts from low growing vegetation, which promotes attachment to small animals during the warmer parts of the day. During these warmer daytime periods, lizards are active and mice become inactive, preferentially favoring tick attachment to lizards and subsequently, B. lusitaniae dominance (Mannelli et al., 2012).

The rodent-associated Borrelia genospecies, Borrelia afzelii, was detected in ticks from all three geographical areas with a relatively high infection rate, which could be due to the high diversity and abundance of rodent species in Romania (Mihalca et al., 2012b). In fact, studies focusing on B. burgdorferi genospecies in Romanian ticks, reported B. afzelii to be the most frequent (Coipan and Vladimirescu, 2010, 2011; Dumitrache et al., 2013; Kalmar et al., 2013; Briciu et al., 2014).

Borrelia spielmanii was only detected in areas 2 and 3, at low infection levels. This genospecies is a pathogenic spirochete transmitted by I. ricinus, and is associated with garden and hazel dormice (Richter et al., 2011). Dormice have a low population density in Romania (Drăgoi and Faur, 2013), which could explain the low prevalence of B. spielmanii in our study.

B. miyamotoi was only identified at areas 1 and 2 in our study, and at a low infection rate (1.5% in area 1, and 1.3% in area 2). No human cases of B. miyamotoi infection have been identified in Romania thus far.

Prevalence in adult ticks and nymph

Usually, adult I. ricinus are more frequently infected with Borrelia spp. than nymphs, and as host-seeking adult ticks require two blood meals during their development, compared to one for nymphs, the likelihood of retrieving the pathogen from infected hosts is increased (Schouls et al., 1999; Geller et al., 2013; Kalmar et al., 2013; Soleng and Kjelland, 2013). Our observed adult and nymph infection rates did not follow this pattern, as I. ricinus adults were only slightly more frequently infected with Borrelia spp. than nymphs. This could be attributed to the high abundance of I. ricinus nymphs in study areas, which is known to positively correlate with a high rate of infected nymphs (Vennestrom et al., 2008). Additionally, adults feed on host species that are not B. burgdorferi s.l.-transmission competent, such as deer, resulting in a similar prevalence in adults compared to nymphs (Gray et al., 1999). Larval stages are more frequently infected with Borrelia genospecies as a result of feeding mostly on rodents, birds, and lizards, and thus acquiring the infection after a blood meal from an infected host, or by co-feeding in the vicinity of an infected nymph (van Duijvendijk et al., 2016).

Tick co-infection and impact on health

In this study, we identified several pathogens co-existing within ticks. Co-infections were detected in 14.3% of adult ticks and in 17.1% of nymphs. Moreover, associations between Borrelia genospecies and between Borrelia and other tick-borne pathogens were detected in 64.5% of infected ticks. Recently, tick co-infections with different tick-borne pathogens have been more frequently reported (Reis et al., 2011; Lommano et al., 2012; Eshoo et al., 2014; Moutailler et al., 2016). This is particularly the case for I. ricinus, due to its capacity to feed on a broad variety of vertebrate species that can host multiple tick-borne pathogens (Reis et al., 2011). In our study, multiple Borrelia genospecies co-existence was identified in 9.7% of ticks, representing 37.7% of Borrelia-positive I. ricinus. Multiple Borrelia infections in individual ticks may occur via several mechanisms, such as: Superinfection of ticks with prior transovarial infection, infection with multiple pathogens via co-feeding, multiple infection after feeding on hosts positive for several Borrelia genospecies, and successive infectious blood meals (Rauter and Hartung, 2005).

In our study, the most common co-infection in individual ticks was between B. afzelii and B. garinii (4.3%), as previously shown (Moutailler et al., 2016). As B. afzelii and B. garinii have different reservoir hosts (rodents and birds respectively) (Mannelli et al., 2012), infection of individual ticks with both genospecies could be the outcome of several possibilities: Immature ticks feeding on both reservoir hosts (as it is the case for positive adult ticks), infection of larvae by co-feeding (Moutailler et al., 2016), or co-infection of reservoir hosts with both B. afzelii and B. garinii.

The second most frequent Borrelia genospecies association was between B. garinii and B. lusitaniae. This mixed infection was predominantly detected in area 3 (Table 3) with many bird varieties existing as common reservoir hosts for both genospecies (Cogalniceanu et al., 2013; Sándor et al., 2014).

We detected 6.9% of ticks positive for the following co-infection associations: (i) dual co-infection with one Borrelia genospecies and another pathogen (20 ticks); (ii) co-infection of two Borrelia genospecies with another pathogen genus (12 ticks); (iii) association of a Borrelia genospecies with two other tick-borne pathogens (4 ticks); and (iv) co-infection with three Borrelia genospecies and one different pathogen genus (1 tick).

The most common tick co-infection was between Borrelia genospecies and Rickettsia monacensis, followed by the association of different Borrelia genospecies and “C. N. mikurensis”. Birds (especially blackbirds—Turdus merula) are reported as competent reservoir hosts for R. monacensis (Marcutan et al., 2016), a role shared with ticks. The association of “C. N. mikurensis” with B. garinii and B. valaisiana is likely due to shared reservoirs, while R. monacensis and B. afzelii co-infection could be the result of co-feeding.

Wild rodents are reservoir hosts for several Borrelia genospecies as well as “C. N. mikurensis” which appears to follow the same distribution pattern as the Lyme disease spirochetes (Burri et al., 2014). As “C. N. mikurensis” transovarial transmission cannot occur, ticks are likely to have been infected with both pathogens from the same host during feeding (Andersson et al., 2013). This type of multiple infection was most frequent in area 3, again likely due to reservoir host abundance. We also detected a small number of associations between Borrelia with A. phagocytophilum and Bartonella spp., adding further evidence to the hypothesis that ticks carry a large number of tick-borne pathogens in eastern Romania.

I. ricinus nymphs represent the most high-risk stage to public health due to their small size, their marked anthropophily, their abundance, and capacity to remain attached to hosts for long durations (Vassallo et al., 2000). In addition to their crucial role as vectors of pathogens, we identified high levels of co-infection which might have important implications for human co-infection. Indeed, the multiple pathogens present in individual ticks could be co-transmitted, either resulting in a co-infection which enhances disease severity—as has been demonstrated for concurrent babesiosis and Lyme disease (Moutailler et al., 2016)—or which might evolve with atypical symptoms, resulting in diagnostic difficulties.

Our findings confirm that ticks are not only important pathogen vectors in forested areas, but also in urban situations. Worth highlighting is the risk that Lyme disease poses in areas with increased recreational activity, as we found high Borrelia genospecies infection rates in questing I. ricinus ticks collected from urban sites. As such, these areas require improved surveillance. We have also identified new risk areas, and have generated detailed data on the occurrence of novel and known zoonotic pathogens, which will act as a solid foundation for further studies examining the risk of human tick-borne disease.

Author contributions

CR collected the samples, performed the experiment, and wrote the MS. IP and DP collected the samples. SM designed the studies. AM and GS discussed the results and wrote the MS. MT designed the studied, analyzed the results and wrote the MS.

Conflict of interest statement

The authors declare that the research was conducted in the absence of any commercial or financial relationships that could be construed as a potential conflict of interest.