Extended characterisation of five archival tick-borne viruses provides insights for virus discovery in Australian ticks

Background A subset of Australians who have been bitten by ticks experience a complex of chronic and debilitating symptoms which cannot be attributed to the known pathogenic species of bacteria present in Australia. As a result, there has been a renewed effort to identify and characterise viruses in Australian terrestrial ticks. Recent transcriptome sequencing of Ixodes and Amblyomma ticks has revealed the presence of multiple virus sequences. However, without virus isolates our ability to understand the host range and pathogenesis of newly identified viruses is limited. We have established a successful method for high-throughput virus discovery and isolation in mosquitoes using antibodies to double-stranded RNA. In this study we sought to characterise five archival tick-borne viruses to adapt our virus discovery protocol for Australian ticks. Methods We performed virus characterisation using a combination of bioinformatic sequence analysis and in vitro techniques including replication kinetics, antigenic profiling, virus purification and mass spectrometry. Results Our sequence analysis of Nugget virus, Catch-me-Cave virus and Finch Creek virus revealed marked genetic stability in isolates collected from the same location approximately 30 years apart. We demonstrate that the Ixodes scapularis-derived ISE6 cell line supports replication of Australian members of the Flaviviridae, Nairoviridae, Phenuiviridae and Reoviridae families, including Saumarez Reef virus (SREV), a flavivirus isolated from the soft tick Ornithodoros capensis. While antibodies against double-stranded RNA could be used to detect replication of a tick-borne reovirus and mosquito-borne flavivirus, the tick-borne flaviviruses Gadgets Gully virus and SREV could not be detected using this method. Finally, four novel virus-like sequences were identified in transcriptome sequencing of the Australian native tick Ixodes holocyclus. Conclusions Genetic and antigenic characterisations of archival viruses in this study confirm that three viruses described in 2002 represent contemporary isolates of virus species first identified 30 years prior. Our findings with antibodies to double-stranded RNA highlight an unusual characteristic shared by two Australian tick-borne flaviviruses. Finally, comparative growth kinetics analyses of Australian tick-borne members of the Flaviviridae, Nairoviridae, Phenuiviridae and Reoviridae families in ISE6 and BSR cells will provide a useful resource for isolation of Australian tick-borne viruses using existing cell lines. Graphical Abstract Supplementary Information The online version contains supplementary material available at 10.1186/s13071-022-05176-z.

is a sub-Antarctic island located halfway between the Australian state of Tasmania and Antarctica. The island is home to large rookeries of penguins and the ticks that infest them, including the hard tick I. uriae. Collections of I. uriae from Macquarie Island between 1972 and 1979 led to the isolation of Gadgets Gully virus (GGYV, Flaviviridae), Precarious Point virus (PPV, Phenuiviridae), Taggert virus (TAGV, Nairoviridae) and Nugget virus (NUGV, Reoviridae) [9,10]. In addition, Saumarez Reef virus (SREV, Flaviviridae) was isolated from seabird-associated ticks collected on Saumarez Reef off the coast of Queensland (QLD; O. capensis) and Tasmania (I. eudyptidis) in 1974 ( Fig. 1) [11]. Serology-based analyses showed each of these viruses shared antigenic relatedness to tick-borne viruses of the Northern Hemisphere, some of which include human pathogens such as Kemerovo virus and tick-borne encephalitis virus [9][10][11]. PPV, TAGV, GGYV and SREV have since been sequenced, further supporting these links with the Northern hemisphere [12][13][14].
A re-survey of I. uriae ticks from Macquarie Island in 2002 resulted in the re-isolation of GGYV [15], approximately 30 years after its initial isolation [10]. Despite the length of time between collections, sequencing of the E and NS1 genes showed minimal genetic variation between these isolates. This study also yielded three additional arbovirus isolates, Sandy Bay virus (SBaV, Reoviridae), Finch Creek virus (FCV, Nairoviridae) and Catch-me-cave virus (CMCV, Phenuiviridae), for which partial genome sequence was obtained ( Fig. 1) [15]. A comparison of the S segment of CMCV and PPV indicated that the two viruses were closely related; however, the L and M segment of CMCV could not be obtained. At the time of this study no genomic information was available for TAGV; however, in 2016 sequencing of this virus showed it to be very similar to the available sequence of FCV, specifically, a 392 nt region of the L segment [14].
To our knowledge the only viruses to be isolated from ticks on the Australian mainland are Lake Clarendon virus, Vinegar Hill virus (VINHV) and a strain of Kao Shuan virus all of which were derived from the soft tick A. robertsi (Fig. 1) [16][17][18]. Little is known about the pathogenicity of these archival viruses, although antibodies to VINHV and GGYV have been identified in human sera with no known reports of illness in the serum donors [17,19]. Mostly, these viruses are not deemed to pose an imminent risk to public health or agriculture, or they are isolated from regions not populated by humans. As a result, for many of these isolates little characterisation has been undertaken since the initial reports.
Recent meta-transcriptomic surveys of ticks from New South Wales (NSW), Australia, have identified a number of novel virus sequences including Shelly Headland virus, which groups with the human pathogens Colorado tick fever virus and Eyach virus [20,21]. While next generation sequencing technologies are an invaluable asset in the field of virus discovery, isolation of viruses of interest is necessary to further our understanding of host range and pathogenesis for potential emerging viruses [22].
We have developed a novel system for broad-spectrum identification of RNA viruses based on the detection of double-stranded RNA (dsRNA) [23]. The MAVRIC (monoclonal antibodies to viral RNA intermediates in cells) system identifies cultures positive for virus replication in a sequence-independent manner. Based on the successful implementation of this system for virus discovery in Australian mosquitoes [24][25][26][27][28][29], we assessed the utility of the MAVRIC system for virus discovery in Australian tick populations. Traditionally, arbovirus isolation has been performed on vertebrate cell lines, with Vero and BHK cells commonly used. However, even these cell lines can show varying levels of permissiveness to different viruses [26,30]. The ISE6 cell line is a well-established cell line derived from I. scapularis, a tick species found in eastern USA and Canada. This cell line has been shown to support replication of a number of tick-borne viruses as well as the mosquito-borne flavivirus West Nile virus New York 99 strain [31][32][33]. However, the permissiveness of this cell line for isolation of viruses from native Australian ticks is unclear [34].
In this study we assessed the potential for the use of the MAVRIC system for discovery and isolation of Australian tick viruses. Using a panel of Australian archival tick viruses, we sought to further characterise the replication of these viruses and the utility of MAVRIC for Australian tick virus discovery.

Methods
Tick cell culture ISE6 (I. scapularis) cells were maintained in complete ISE6 cell medium containing L-15B300 media supplemented with 0.1% LipiMAX bovine lipoprotein solution (Selbourne Biological, Tasmania, Australia), 10% tryptose phosphate broth (Oxoid (Thermo Fisher), Basingstoke, UK) and 5% fetal bovine serum (FBS, Bovogen, Victoria, Australia). L-15B300 medium was made in house using triple-autoclaved ultrapure water, Leibovitz-15 (L-15) media (Lonza, Gibco) and trace minerals as per [35]. The details for each reagent are described in Additional file 1: Table S1. Cells were frozen in complete medium containing 15% FBS and 10% DMSO using the CoolCell LX cell freezing container (Corning). Cells were revived in a T25 non-vented flask and maintained by replacing media every 7-10 days for 1 month before upscaling to a T75 non-vented flask. Upscaled cells were maintained for a minimum of 1 month before seeding for experiments. Cells were maintained at 34 °C without CO 2 .

Vertebrate and mosquito cell culture
Vero (Chlorocebus monkey kidney cells), BHK (baby hamster kidney cells, Mesocricetus auratus) and BSR (clone of baby hamster kidney cell line, Mesocricetus auratus) cells were maintained in Dulbecco's Modified Essential Medium (DMEM) supplemented with 5% FBS. Opossum (Didelphidae) kidney (OK) cells were maintained in Roswell Park Memorial Institute (RPMI) medium supplemented with 5% FBS. All vertebrate cells were maintained at 37 °C in the presence of 5% CO 2 . C6/36 cells (Aedes albopictus, mosquito larvae-derived) were cultured in RPMI supplemented with 5% FBS and grown at 28 °C without CO 2 .

Production of stocks of archival viruses
Virus stocks were prepared by inoculation of vertebrate or C6/36 cells as per Table 1 at approximately 80% confluency. Where titres were known, inoculation was performed at a multiplicity of infection (MOI) of 0.1. Where virus titres in the inoculum were unknown, 100 µl of inoculum was used. After an adsorption period of 1 h at room temperature with agitation, virus inoculum was removed and replaced by DMEM (or RPMI for C6/36 cells) supplemented with 2% FBS. Cells were incubated at 37 °C for 2-7 days. Supernatant was harvested and clarified by centrifugation at 3000g for 15 min at 4 °C. FBS content in culture supernatant was raised to 10% prior to aliquoting and storage at − 80 °C.
All viruses were titrated onto BSR and Vero cells and titres were determined by TCID 50 using the Reed-Muench method [36]. Virus replication was determined by fixed-cell ELISA using the pan-flavivirus mAb 4G2 for SREV and GGYV, MAVRIC for NUGV and anti-FCV mouse immune serum for FCV and TAGV. Replication of CMCV was determined by the presence or absence of cytopathic effect (CPE).

Tick homogenisation and passaging
Adult I. holocyclus ticks collected in Lismore, which had been blood fed on rats for an unrelated experiment, were stored at − 80 °C. Pools of five ticks were thawed on ice and added to 5 ml microcentrifuge tubes with 4 ml of chilled complete ISE6 media. Homogenisation was performed with a 5-mm stainless steel bead for 2 min, followed by centrifugation at 3000 g for 15 min at 4 °C to pellet debris. Clarified supernatant was passed through a 0.2-µm filter. Filter-sterilised supernatant was used immediately to inoculate cells and thereafter stored at − 80 °C. Inoculum was removed from vertebrate cells after 2 h and replaced with appropriate maintenance media before cells were incubated at 37 °C with 5% CO 2 for 5 days post-infection (dpi). Inoculum was left on ISE6 cells for 7-9 dpi at 34 °C without CO 2 .

RNA extraction and RT-PCR
RNA extraction was performed on homogenates and cell culture supernatant using the Machery Nagel Viral RNA isolation kit as per manufacturers' instructions. RT-PCR testing was performed using the SuperScript ™ III One- Step RT-PCR System with Platinum ™ Taq DNA Polymerase (Invitrogen) and primer sets listed in Table 2 Plates were pre-blocked with 150 µl/well TENTC blocking buffer (2% w/v casein, 0.05% v/v Tween-20, 10 mM Tris, 0.2 M NaCl, 1 mM EDTA, pH 8.0) for 1 h at room temperature. A cocktail of monoclonal antibodies (mAbs) 3G1 and 2G4 (MAVRIC) was prepared by diluting hybridoma supernatant in TENTC blocking buffer to previously determined optimal concentrations. Blocked plates were incubated with 50 µl/well MAVRIC for 1 h at 37 °C, followed by four washes with PBS containing 0.05% v/v Tween-20 (PBS-T). A 1:2000 dilution of secondary goat anti-mouse HRP (DAKO) in TENTC blocking buffer (50 µl/well) was then added, followed by another incubation for 1 h at 37 °C. Plates were washed six times with PBS-T and developed using 100 µl/well of substrate buffer (1 mM 2,2*-Azino-bis(3-ethylbenzothiazoline-6-sulfonic acid) (ABTS), 2.5 mM H 2 O 2 , in a solution prepared by mixing 0.1 M citric acid with 0.2 M Na 2 HPO 4 to give a pH of 4.2) for 1 h at room temperature, protected from light. Absorbance was measured at 405 nm and samples with an average OD 405nm equal to or greater than twice that of the average mock reading were considered positive.

Antigenic analyses
Antigenic analysis of SREV and GGYV was performed on BHK cells infected at a MOI of 0.1 for 48 h in 96-well plates and fixed with 20% acetone fixative buffer as described above. Serial two-fold dilutions of mAbs in TENTC blocking buffer were tested. For mAbs in hybridoma supernatant a starting dilution of neat (P3H8) or 1:5 (4G2, 6B6C) was used, while 1D1 (purified mAb) and M2-1E7 (ascitic fluid) were used at a starting dilution of 1:500. Primary antibody was added to plates at 50 µl/ well and incubated at 37 °C for 1 h. Fifty µl of goat antimouse HRP (1:2000) was added to plates and incubated for 30 min at 37 °C.
Anti-FCV ELISA using mouse immune sera was performed on BSR cells infected with FCV or TAGV at MOI of 0.1 for 5 days and fixed with acetone fixative buffer as described above. Serial dilutions of anti-FCV serum of 1:200 to 1:25,600 were prepared in TENTC blocking buffer. Both primary and secondary antibodies (goat antimouse 1:2000, DAKO) were added to plates at a volume of 50 µl/well and incubated for 1 h at 37 °C.
All plates were pre-blocked, washed and developed as described for the MAVRIC ELISA.

Purification of viruses
Partial purification was performed on CMCV and FCV. Five T175 flasks per virus were seeded with BSR cells at 80% confluence 1 day prior to infection. Cells were infected with CMCV or FCV at a MOI of 0.1 for 1 h at room temperature with gentle agitation. Inoculum was removed and replaced with 18 ml 2% FBS/DMEM per flask. Cells were incubated for 5 days at 37 °C before harvesting supernatant and clarifying by centrifugation at 3000 g for 15 min at 4 °C. Two parts clarified supernatant was mixed with one part 40% PEG6000 solution (40% w/v polyethylene glycol 6000 in PBS) overnight at 4 °C. Virus was pelleted by centrifugation at 21,612g for 1 h at 4 °C in a JLA16.250 Beckman-Coulter rotor. Precipitated virus was resuspended in cold PBS. As the pathogenicity of CMCV and FCV in mice is unknown, the virus preparations were inactivated in preparation for their use as antigens for immunisation of mice. To do this a solution of binary ethyleneimine (BEI) was prepared by the addition of 3-10 mM 2-bromoethylamine to DMEM brought to pH 9.0 with 2 N NaOH and warmed to 37 °C. PEGprecipitated virus was resuspended in the BEI-DMEM solution and incubated at 37 °C overnight before BEI was neutralised by the addition of sodium thiosulfate to a final concentration of 0.1 M. The inactivated virus preparation was then layered onto a cushion of 20% sucrose in NTE buffer (10 mM Tris, 1 mM EDTA, 120 mM NaCl, pH 8.0) followed by ultracentrifugation at 133,668g for 2 h at 4 °C in a SW32 Ti rotor (Beckman-Coulter). Pelleted virus was incubated in PBS at 4 °C overnight. After pellets were resuspended, the samples underwent three rounds of buffer exchange in 5 ml PBS using high molecular weight (100 K) MWCO Spin-X UF concentrator

Protein analysis by SDS-PAGE and western blot
Purified virus preparations were diluted in 4 × NuPAGE LDS sample buffer (Invitrogen) without boiling or reducing and analysed by SDS-PAGE using a 4-12% Bis-Tris gel (NuPAGE) at 170 V for 42 min in 1 × Tris-glycine running buffer. Gels were stained using SYPRO Ruby protein stain (Thermo Fisher Scientific) as per manufacturer's instructions and imaged on a UV transilluminator. FCV or uninfected cell lysate was prepared by harvesting BSR cells from a T75 flask in NP-40 lysis buffer (1% NP-40 in 150 mM NaCl, 50 mM Tris-HCl [pH 7.3], 1:100 protease inhibitor cocktail (P8340, Sigma, St Louis, MO, USA)) for 30 min at 4 °C. Lysate was clarified by centrifugation at 10,000 g for 10 min at 4 °C and stored at − 80 °C until use. To test anti-FCV immune sera, electrophoresis of cell lysates was performed as described above and proteins were transferred to a nitrocellulose membrane at 30 V for 60 min. The membrane was pre-blocked with TENTC blocking buffer and probed with anti-FCV serum diluted 1:200 in TENTC blocking buffer. The membrane was washed three times with Tris-buffered saline (20 mM Tris-HCl pH 7.5, NaCl: 150 mM, 0.05% v/v Tween-20 detergent) before addition of goat-anti mouse conjugated with IRDye800 (LI-COR) diluted at 1:8000 in blocking buffer for 1 h at room temperature. The blot was imaged using the Odyssey CLx.

Mass spectrometry
FCV protein bands, which were visible by eye after gel electrophoresis, were excised under UV illumination and stored at − 20 °C. Gel slices were destained overnight at 37 °C in a solution of 50% acetonitrile/50 mM ammonium acetate. Proteins were reduced with 10 mM dithiothreitol for 1 h and cysteine residues were alkylated by addition of 25 mM acrylamide and incubated for 1 h at 23 °C. Gel slices were dried and peptides were digested overnight with 500 ng trypsin in a solution containing 50 mM ammonium acetate solution. Digested peptides were desalted and analysed using liquid chromatography mass spectrometry (LC-MS/MS) as described in [37]. Peptides were identified using ProteinPilot Software 5.0.2.0 (SCIEX) and a custom protein database containing Mesocricetus auratus (BSR cell line) proteins and the amino acid sequences of FCV RdRp, nucleocapsid and glycoprotein precursor. Standard search settings included: sample type, identification; digestion, trypsin; Cys alkylation, acrylamide; search effort, thorough; ID focus, biological modifications. False discovery rate analysis using ProteinPilot was performed on all searches.

Generation of mouse immune serum to Finch Creek virus
All animal procedures had received prior approval from The University of Queensland Animal Ethics Committee (AEC #SCMB/329/15/ARC) and, where necessary, were performed under ketamine:xylazine anaesthesia. BEIinactivated FCV along with inulin-based adjuvant Advax (Vaxine Ltd., Adelaide, Australia) was used to immunise a 6-week-old BALB/c mouse (Animal Resources Centre, Murdoch, Western Australia, Australia) via the subcutaneous route (s.c.). Mice were kept on clean bedding and given food and water ad libitum. The immunized mouse was bled via the tail vein at 2 weeks following immunization and the serum tested for evidence of seroconversion to FCV using a fixed-cell ELISA as described above. A second dose of antigen was delivered 6 weeks after the initial dose. Two weeks after receiving the second dose, the mouse was killed by a ketamine:xylazine overdose and blood for serum-procurement was harvested via cardiac puncture.

Sequencing of viruses
Nugget virus (NUGV, MI14847) RNA was extracted from culture supernatant from an archival virus stock using the QIAamp Viral RNA extraction kit (QIAGEN, Hilden, Germany) with carrier RNA omitted and DNA Wipeout was used to remove residual cell line DNA (Qiagen). First-strand cDNA synthesis was performed with Protoscript II kit using the supplied random primer mix (New England Biolabs; Ipswich, MA, USA). Secondstrand DNA synthesis was performed using the NEBNext mRNA Second-Strand Synthesis Module (New England Biolabs). The Nextera XT library kit (Illumina; San Diego, CA, USA) was used to construct cDNA libraries with individual samples barcoded. All reactions were performed according to the conditions recommended by the respective manufacturers. Library sequencing was performed by the Australian Genome Research Facility (AGRF) on a HiSeq Illumina sequencer (125 nt paired end reads). Sequence assembly was performed using the de novo assembly tool in Geneious v8 at low sensitivity using 125 bp read lengths.
Preparations of FCV EB06 and CMCV I-2 for sequencing were generated by PEG-precipitation of virus from supernatant of 2 × T175 flasks of BSRs as described above. Sequencing for these viruses was performed as described for NUGV with the following modifications; DNAse treatment was performed using Heat&Run DNase (ArcticZymes); second-strand DNA synthesis was performed using Escherichia coli DNA ligase, DNA polymerase I and ribonuclease H (New England Biolabs). The resulting libraries were sequenced on a NextSeq 500 generating 2 × 151 base pair paired reads. The viral genome was assembled using Geneious R8 software as described above.

Growth kinetics
ISE6 and BSR cells were seeded in 24-well plates at a density of 10 5 cells per well, 24 h prior to infection. For NUGV, one replicate from each time point was seeded onto sterile glass coverslips in 24-well plates. On the day of infection, seeding media was removed and virus inoculum prepared in complete ISE6 cell media (10% FBS, 10% tryptose phosphate broth, 0.1% bovine lipoprotein solution, pH 7.5) or 2% FBS/DMEM was added to cells at a MOI of 0.1. Inoculated cells were incubated at room temperature with gentle rocking for 1 h before inoculum was removed and monolayers were washed three times with 1 ml/well sterile PBS. Supernatant from triplicate wells was harvested at 2, 12, 24, 48, 72, 96, 120 and 168 h post-infection (hpi) and stored at − 80 °C. For NUGV, supernatant was also harvested at 144 hpi and coverslips were harvested at each time point and fixed with 1 ml of formaldehyde fixative buffer (4% formaldehyde, 0.5% v/v Triton X-100 in PBS) at 4 °C for 10 min and air dried for at least 48 h before storing at − 20 °C.
Quantification of viral titres in supernatants collected at each time point was determined using a modified TCID 50 method described in [27,38]. Briefly, ten-fold dilutions of supernatant (undiluted to 1:10 8 ) were prepared in 2% FBS/DMEM. Each dilution (50 µl) was added to four replicate wells of a 96-well plate and incubated for 5 days at 37 °C with 5% CO 2 . Flavivirus (GGYV, SREV, WNV KUN NSW2011 strain), NUGV and FCV supernatant titrations were performed on BSR cells, while CMCV titrations were performed on Vero cells. After 5 days, plates containing flaviviruses and FCV were fixed using acetone fixative buffer and virus replication was determined by fixed-cell ELISA using anti-flavivirus E mAb 4G2 or anti-FCV immune serum as described above. NUGV-infected cells were fixed with 150 µl/well formaldehyde fixative buffer for 10 min at 4 °C and virus replication was determined by MAVRIC ELISA as described previously [27]. For CMCV, virus replication was scored by the presence or absence of CPE. Viral titres in each sample were then calculated using the Reed-Muench guidelines [36].

Immunofluorescence assays
ISE6 cells were seeded on glass coverslips in 24-well plates at 10 5 cells per well 1 day prior to infection. Cells were infected at MOI 0.1 for 1 h at room temperature before inoculum was removed and replaced with 1 ml complete ISE6 medium. Cells were incubated at 34 °C without CO 2 . At 7, 14 and 28 dpi supernatants were harvested and stored at − 80 °C and coverslips were fixed by submerging in 100% ice-cold acetone for 5 min before air drying and storing at − 20 °C. Viral titres in supernatants were determined as described in the previous section. The protocol for E and dsRNA dual-labelling is as follows. All antibodies were diluted in TENTC blocking buffer to previously determined optimal concentrations before use. Coverslips were blocked with 900 µl of TENTC blocking buffer for 1 h at room temperature, followed by incubation with 300 µl anti-E mAb 4G2 at 28 °C for 1 h. Coverslips were washed thrice with 1 ml PBS-T (PBS with 0.05% v/v Tween-20) and incubated with 150 µl 1:500 Alexa Fluor 488-conjugated goat anti-mouse in TENTC blocking buffer for 1 h at 28 °C. Another 3 × PBS-T washes were performed followed by addition of 300 µl/well MAVRIC hybridoma supernatant (a cocktail of mAbs 3G1 and 2G4) and incubation at 37 °C for 1 h. Coverslips were again washed three times and Alexa Fluor 594-conjugated goat anti-mouse IgM (µ chain) diluted 1:500 in blocking buffer was added at 150 µl/well at 28 °C for 1 h. Secondary anti-IgM antibody solution was then removed and nuclear staining was performed with 150 µl/well Hoechst 33342 for 5 min at room temperature, protected from light. Three final PBS-T washes were performed, followed by one wash with PBS (without Tween-20), and coverslips were mounted on glass microscope slides using ProLong Gold Antifade mountant (ThermoFisher, Carlsbad, CA, USA). Images were taken on a Zeiss EPI fluorescence microscope.
For comparison of MAVRIC and J2 dsRNA immunolabelling, BSR cells were infected with GGYV, SREV or WNV NSW2011 at MOI 0.1 for 5 days and fixed with 1 ml Table 3 Reactivity of pan-flavivirus mAbs and MAVRIC against SREV and GGYV in fixed-cell ELISA a + + + , OD 405nm ≥ 2 for all tested dilutions; + + , OD 405nm ≥ 1 for all tested dilutions; +, OD 405nm < 1 for all tested dilutions; −, OD 405nm ≤ mock OD for all tested dilutions b mAb prepared by A.K. Falconar, London School of Hygiene and Tropical Medicine, London, UK c Greater than mock OD but beneath the threshold for a positive score (2 × mock OD 405nm ). Negative for MAVRIC in fixed cell ELISA using both 20% acetone and 4% formaldehyde with 0.5% Triton X-100 fixation per well of 4% formaldehyde in PBS at 4 °C for 10 min and air dried for at least 48 h before storing at − 20 °C. Prior to labelling, coverslips were thawed and permeabilised by incubation in 1 ml of 0.5% Triton X-114 v/v or 0.5% w/v digitonin in PBS for 10 min at 4 °C. For the anti-dsRNA time course, coverslips containing BSR cells infected with GGYV at MOI 0.1 were harvested at 12, 24, 48 and 96 hpi and fixed with 100% acetone as described above.
Immunolabelling for dsRNA was performed on preblocked coverslips with 300 µl of MAVRIC hybridoma supernatant or 150 µl of purified IgG mAb J2 diluted 1:200 in blocking buffer for 1 h at 37 °C. Coverslips were washed as described above and incubated with 150 µl of Alexa Fluor 488-conjugated goat anti-mouse (H + L) diluted in 1:500 TENTC blocking buffer for 1 h at 37 °C. Nuclear staining and mounting were performed as described above. Coverslips were imaged using a Zeiss LSM 510 META confocal microscope.

Sequence annotation and phylogenetic analysis
Pairwise alignments of the nucleotide and amino acid sequences of archival viruses were performed in Geneious Prime v2019 using MUSCLE or ClustalW algorithms respectively. Sequence annotation for CMCV and FCV was performed using the following platforms: protein topology, Phobius [39]; N-and O-linked glycosylation site prediction, NetNGlyc 1.0 and NetOGlyc 4.0 servers [40]; domain prediction, HMMER EBI tools web server [41]; cleavage site predictions, ProP 1.0 server [42].
Nucleotide coding sequences for NUGV and orbivirus VP1, VP7 (T13), T2 and VP5 (OC2) proteins were aligned using the MAFFT v7.471 tool via the CIPRES gateway [43,44]. Alignments were trimmed to the length of each NUGV segment and JModelTest2 via the CIPRES gateway was used to determine the best available model for each gene [45]. Trees were constructed in MEGA7 using the maximum likelihood method based on the Jukes-Cantor model with complete deletion of gaps and missing data with the following models for rates among sites used; for VP1 JC + G with four discrete categories, for VP7 (T13), T2 and VP5 (OC2) JC + I. Phylogenetic tests were performed for each node using 1000 bootstrap replicates. Neighbour-Join and BioNJ algorithms were used to generate initial trees based on a matrix of pairwise distances estimated using the maximum composite likelihood (MCL) approach.
Virus-like contigs generated from I. holocyclus transcriptome data [46] were first assessed by a Blastx database search (database: nr, August 2021) and open reading frames were determined using the Translate Tool via the ExPASy website. Amino acid sequences for the nucleocapsid proteins of Phlebovirus-like sequence 1 (PVL1) and 3 (PVL3) were aligned with selected phlebovirus nucleocapsid proteins using the MAFFT alignment algorithm via the EBI-EMBL web interface [39]. Maximum-likelihood analysis was performed on a MAFFT alignment of 27 sequences trimmed to 338 amino acids before non-conserved regions were removed using GBlocks with less stringent settings (smaller final blocks, gap positions in final blocks and less stringent flanking positions allowed). A final alignment of 99 positions was used for phylogenetic analysis in MEGA7 using the LG model with 1000 bootstrap replicates. Gamma distribution was used to model evolutionary rate differences among sites with some sites allowed to be evolutionarily invariable (LG + G + I). Neighbour-Join and BioNJ algorithms were applied to a matrix of pairwise distances estimated using the Jones Taylor Thornton (JTT) method to generate the initial trees and topology with superior log likelihood value was selected automatically.
The protein structures of PVL1 and PVL3 nucleocapsid proteins were predicted using the Phyre2 Protein Fold Recognition Server based on an alignment with Toscana virus N protein with 100% confidence [47]. The 3D protein model figures were produced using Chimera software version 1.13.1 [48] and regions were annotated based on domains identified in [49,50].

Growth and antigenic characterisation of Australian tick-borne flaviviruses
The mosquito-borne flavivirus West Nile virus subtype Kunjin (WNV KUN ) is routinely used as a positive control for double-stranded RNA production in the MAVRIC system [23]. Therefore, for adapting the assay for discovery of tick viruses, we assessed two tick-borne flaviviruses GGYV and SREV for this purpose. Initially we compared the reactivity of a panel of six pan-flavivirus anti-E mAbs against WNV KUN -, GGYV-and SREV-infected BHK cells in fixed-cell ELISA. Five of the six mAbs tested reacted to all three flaviviruses (Table 3). However, we found that the anti-E reactive mAb M2-1E7 bound to GGYV but not SREV (Table 3). Neither GGYV or SREV was detected in infected BHK cells by MAVRIC ELISA after fixation with 20% acetone fixative buffer or 4% formaldehyde with 0.5% Triton X-100, despite detecting WNV KUN under both conditions (Table 3).
To understand the growth dynamics of tick-borne flaviviruses compared to their mosquito-borne relatives, a growth kinetics assay was performed on WNV KUN , GGYV and SREV in vertebrate and tick cells over 7 days. As our preliminary data indicated that prototype WNV KUN strain (MRM61C) did not replicate in ISE6 cells, we tested for replication of the more neuroinvasive WNV KUN strain NSW2011 [51]. This assay revealed a similar growth pattern for all three flaviviruses in BSR cells. However, both tick-borne viruses reached peak titre at 48 hpi, 24 h earlier than the mosquito-borne WNV KUN (Fig. 2). GGYV replicated robustly in ISE6 cells, reaching an average peak titre of 10 7.19 /ml at 72 hpi, which was within 1 log of the titre recovered from vertebrate cells at this time point (average titre 10 7.77 /ml) (Fig. 2a). While the growth curve of SREV in ISE6 cells mirrored that  of the virus in BSRs, viral titres recovered from the tick cells were lower than those recovered from BSR cells at all time points, with > 2 log difference between the peak titres recovered from each cell line (ISE6: 10 4.97 /ml, BSR 10 7.13 /ml) (Fig. 2b). No infectious virus could be detected in supernatant from WNV KUN -infected tick cells from 72 hpi onwards. However, a small amount of virus (average titre 10 1.8 /ml) was detected in supernatant harvested from three replicate wells at both 12 and 24 hpi followed by a decline at 48 hpi, indicating that some viral replication may occur in these cells during the early stages of infection (Fig. 2c).

Detection of double-stranded RNA in tick-borne flavivirus replication
While our growth kinetics data indicated that GGYV and SREV replicated in both tick and vertebrate cell lines, we were unable to detect dsRNA in cells infected with either virus using the MAVRIC ELISA. To investigate this further we performed an immunofluorescence assay (IFA) on ISE6 cells infected with GGYV or SREV. Infectious virus was detected in supernatant from cells infected with SREV at 7, 14 and 28 dpi, but only from GGYV-infected cells at 7 and 14 dpi (Fig. 3). Envelope protein could be detected by IFA for both viruses at all time points; however, no dsRNA was detected in these cells by co-labelling with MAVRIC (Fig. 3). To confirm that the lack of dsRNA immunolabelling was not related to our anti-dsRNA antibodies, we compared detection of dsRNA in SREV-, GGYV-and WNV KUN -infected cells using MAVRIC (mAbs 3G1 and 2G4) and the commercial anti-dsRNA antibody J2 (IgG, Scicons) [52]. While both antibodies detected dsRNA in WNV KUN -infected BSR cells at 5 dpi, neither J2 nor MAVRIC detected significant amounts of dsRNA in SREV-and GGYV-infected cells at this time point following formaldehyde fixation and permeabilisation with 0.5% Triton X-114 (Fig. 4a, b). This result was also observed in cells fixed and permeabilised using 4% formaldehyde with 0.5% digitonin (Additional file 1: Fig.  S1).
As we were unable to detect dsRNA by IFA or ELISA at 5 dpi onwards, we performed anti-dsRNA labelling on GGYV-infected BSRs at earlier time points. This analysis showed that dsRNA was not detected using J2 at 24, 48 and 96 hpi (Fig. 4c). However, a small percentage of cells with perinuclear dsRNA signal were observed at 12 hpi (Fig. 4c).

Growth kinetics and in situ detection of NUGV in vertebrate and tick cells
NUGV is an orbivirus that was isolated from I. uriae ticks collected at Macquarie Island [9]. We first assessed its ability to replicate and produce sufficient levels of accessible viral dsRNA in inoculated BSR and ISE6 cells for detection by MAVRIC.
Growth kinetics analysis showed NUGV replicated to an average peak titre of 10 7.62 /ml by 24 hpi in BSR cells. This was followed by a steady decline in titre over the next 6 days (Fig. 5a), which coincided with overt cytopathic effect in these cells. In ISE6 cells, an average peak titre of 10 6.47 /ml was detected at 96 hpi, with titres staying relatively stable from this point on (Fig. 5a). Infected cells were fixed at each time point and immunolabelled Table 4 Summary of sequence data generated for Nugget virus a Segment predictions are based on GIV segment designations [77] b Viral protein designations (VP) are based on Bluetongue virus nomenclature as per [78]. Pol, RNA-dependent RNA polymerase; T2, conserved major subcore protein with T = 2 symmetry; CaP, capping enzyme; TuP, tubule forming protein; OC1, outer capsid protein 1; OC2, outer capsid protein 2; T13, major core protein with T = 13 symmetry; ViP, viral inclusion body protein; Hel, ssRNA-and dsRNA-binding helicase; NS, non-structural protein c GIV nucleotide sequences (NC_014522 to NC_014531), amino acid sequences (YP_003896058 to YP_003896068) d SBaV nucleotide sequences (EU685329 to EU685333), amino acid sequences (ACD38335 to ACD38337 and ACD38339) for dsRNA using MAVRIC. Significant amounts of dsRNA were first detected in BSR cells at 24 hpi, coinciding with the peak titre of the virus (Fig. 5b). In ISE6 cells, a strong dsRNA signal was detected from 48 hpi onward (Fig. 5c).

Genomic sequence analysis of NUGV
Although NUGV was first isolated in 1972 [9], to date no sequence analysis has been conducted on the viral genome. We performed deep sequencing on an archival stock of the prototype NUGV strain (MI14847) and obtained partial sequence for all ten genome segments (Table 4). Pairwise alignments with available sequence for SBaV, an orbivirus isolated from I. uriae collected on Macquarie Island in 2002 [15], showed high similarity at both the nucleotide (96.4-98.4%) and amino acid (97-100%) levels for VP4 (CaP), VP5 (OC2), NS2 (ViP) and NS3 (Table 4). NUGV also shares approximately 75% nucleotide and 90-91% amino acid identity with the T2 and T13 sequences of Great Island virus (GIV) ( Table 4). Phylogenetic analysis of the nucleotide sequences of VP1 genes shows that NUGV groups with GIV within the tick-borne orbivirus clade (Fig. 6a). This grouping was also supported by phylogenetic trees constructed from the nucleotide sequences of the T2 and VP7 (T13) structural genes (Additional file 1: Fig. S2). Maximum likelihood analysis of the nucleotide sequence of VP5 (OC2) shows that NUGV and SBaV cluster with other members of the GIV species (Fig. 6b).

Characterisation of CMCV
We previously isolated CMCV from I. uriae ticks collected in 2002 from Macquarie Island [15] and reported that it phylogenetically clustered with other phleboviruses and was genetically similar to PPV, a virus previously isolated from the same tick species collected on the island almost 30 years earlier [10]. However, only the S segment of CMCV was originally sequenced. To complete the characterisation of this virus and its genetic relationships to other tick-borne viruses found in the same region, we performed next generation sequencing on a stock of CMCV. This yielded full-length L segment and near full-length sequence for the M segment (excluding the first 10 bases of the 5′ and last 4 bases of 3′ genomic termini). From this, the complete coding sequences (CDS) of the L protein and glycoprotein precursor were identified and annotated (Fig. 7a). The nucleotide sequences of the L and M segment shared 94.7% and 94.4% similarity with PPV, while the L protein and glycoprotein precursor shared > 99% amino acid similarity with this virus (Fig. 7b). The S segment of CMCV that had been generated previously shares 95.7% nucleotide similarity with the S segment of PPV and 100 and 96.2% amino acid similarity with PPV nucleocapsid and non-structural proteins respectively (Fig. 7b) [15]. Protein analyses of purified CMCV showed the Gn and Gc glycoproteins run at apparent molecular weights of 47.2 and 53.2 kDa (Fig. 7c). A third band was identified at 258.3 kDa, which may represent viral ribonucleoprotein complexes (RNP). Growth kinetics analysis showed that CMCV replicated to higher titres in ISE6 cells between 24 and 72 hpi compared to BSR cells (Fig. 7d). Peak titres were detected in both cell lines by 120 hpi (5 dpi) with the titres from BSR cells (10 6.91 /ml) surpassing that of ISE6 cells (10 6.63 /ml) (Fig. 7d).

Genetic characterisation of FCV
We performed similar analyses on FCV, a nairovirus isolated from I. uriae also collected at Macquarie Island in 2002 [9]. Complete open reading frames (ORFs) for all three genome segments were generated by next generation sequencing and the resulting proteins annotated (Fig. 8a). The newly obtained L segment sequence shared 97.7% nucleotide and 99.2% amino acid similarity with the partial L segment sequence previously reported for this virus (Table 5) [15]. All three segments also shared high similarity at both the nucleotide (97.8-99.6%) and amino acid (99.6-100%) levels with the sequence of the prototype isolate of TAGV (MI14850), isolated from the same tick species collected on Macquarie Island in 1972 (Table 5) [9,14]. FCV appears less closely related to a new variant of TAGV identified in I. uriae ticks collected in 2017 from Antarctica [53], with 81.4% nucleotide 94% amino acid sequence shared across the L segment, the most conserved of the three segments (Table 5).

In vitro characterisation of FCV
We observed that after passaging FCV in ISE6 cells, the virus caused inconsistent CPE when inoculated onto mammalian cells and therefore could not be reliably quantified by CPE scoring. To circumvent this, we purified the virus for immunization of mice to generate virus-specific immune serum. As the pathogenicity of FCV in mice and humans is unknown, the virus was inactivated by the addition of binary ethylenimine (BEI) to cell culture supernatant prior to purification. SDS-PAGE analysis of the purified virions revealed two prominent bands at apparent molecular weights of 261.2 and 54.8 kDa (Fig. 8b). Both bands were determined by mass spectrometry to contain the nucleocapsid (N) protein (Fig. 8b, Additional file 2: Dataset S1). Three additional bands were identified at apparent molecular weights of 181.2, 72.2 and 62.2 kDa, which presumably contain the L protein, Gc and Gn glycoproteins respectively (Fig. 8b). Mouse immune serum raised to this virus preparation was assessed in western blot and showed reactivity to the N protein in FCV-infected cell lysate (Fig. 8c). Titration of the immune serum on FCV and TAGV infected BSRs in fixed-cell ELISA showed the serum detected both viruses equally well up until an end point dilution of 1:6400 (Fig. 8d).
Growth kinetics analysis of FCV showed that the virus replicated rapidly in the first 24 h followed by a plateau in both vertebrate and tick cell lines (Fig. 8e). In BSR cells an average peak titre of 10 5.91 /mL was detected at 96 hpi followed by a decline at 120 and 168 hpi. FCV replicated less efficiently in ISE6 cells with recovered titres being 2-3 logs lower than the titres from BSR cells at time points 24-120 hpi (Fig. 8e). However, peak titre in this cell line was only detected at 168 hpi (7 dpi, average titre 10 4.41 / mL), suggesting that productive infection in ISE6 cells may persist past the time points sampled in this study.

Virus-like sequences in transcriptome data of I. holocyclus ticks
We were given access to viral sequence contigs previously assembled from transcriptome sequencing of I. holocyclus ticks collected in South-East Queensland (QLD) and Northern New South Wales (NSW, Table 6) [46,54]. Our analysis focussed primarily on contigs with similarity to RNA viruses and excluded any sequences of the tick-specific IhIV which we have reported previously [34]. While IhIV sequence was detected in five of the 6 data sets [34], only three data sets yielded potential arbovirus-like sequences ( Table 6, Fig. 9).
From the viscera of ticks collected from paralysed cats and dogs, three distinct sequences were identified which resembled the phlebovirus nucleocapsid gene (Fig. 9). These sequences will be referred to from herein as PVL (Phlebovirus-like) 1, 2 and 3. PVL1 and 2 were identified in ticks collected in the Wynnum-Manly region of QLD, while PVL3 was identified in pooled viscera of ticks collected in Northern NSW and South-east QLD (Fig. 9). Only one sequence, PVL1 was identified in datasets from paired viscera and salivary glands (Fig. 9). PVL1 and 3 showed sequence homology to two variants of Ronne virus, a novel phlebovirus identified in I. uriae ticks from Antarctica and Norway (Table 7) [53,55]. These sequences also shared 66.7% nucleotide and 76.9% amino acid identity with one another. PVL2 showed homology to Timbillica virus, a novel virus identified in I. holocyclus ticks from Southern NSW [20] (Table 7). Finally, a small contig with similarity to the rhabdovirus RdRp gene was identified in sequence data from salivary glands, but not paired viscera, of ticks collected in Wynnum-Manly, QLD (Fig. 9, Table 7).

Sequence analysis of two phlebovirus-like sequences from I. holocyclus ticks
PVL1 and 3 both contained a 711 nucleotide-long ORF encoding a 237 amino acid nucleocapsid-like protein (Fig. 10a, b). This protein shares homology at both sequence and structural levels with phlebovirus nucleocapsid (N) proteins (Fig. 10b, Additional file 1: Fig.  S3). However, both proteins lacked alpha helices 1 and 2, which make up the N-terminus arm shown to be responsible for stabilisation of Rift Valley fever and Toscana virus nucleoprotein hexamers [49,56] (Fig. 10b, Additional file 1: Fig. S3). PVL3 contained all conserved structural elements found in the globular domains of phlebovirus nucleocapsid proteins (alpha helices 3-13), while in PVL1 alpha helix 3 (a3) was substituted for a beta strand (Fig. 10b, Additional file 1: Fig. S3). PVL1 and 3 also contained a second short ORF in the reverse orientation (Fig. 10a). The resulting proteins from this ORF share 64% amino acid similarity with one another but do not show any conservation to known proteins by BLAST or HMMER database searches (Fig. 10a, c). Maximum-likelihood analysis performed on the nucleocapsid proteins of PVL1, PVL3 and selected phleboviruses suggested that PVL1 and 3 cluster with other virus sequences identified in I. uriae and I. holocyclus ticks from the Southern hemisphere (Fig. 10d).

Attempts to isolate viruses from I. holocyclus ticks
Primers were designed to test for each of the viral sequences identified above in homogenates of I. holocyclus ticks collected in northern NSW between 2000 and 2001. All four sequences were detected by RT-PCR in ticks of this cohort ( Table 8). The amplified sequences shared high sequence similarity with the original sequences; however, attempts to amplify additional sequence from these samples using degenerate primers and next generation sequencing were unsuccessful.
As no further sequence could be amplified from homogenates, attempts were made to isolate viruses in cell culture. Three serial passages of RT-PCR positive homogenates were performed on cell lines derived from rodent (BHK), marsupial (OK) and tick (ISE6) origins. However, no viral isolates were identified by RT-PCR analysis or CPE scoring.

Discussion
The field of tick-borne virus research in Australia is experiencing a new wave of focus due to advances in metagenomic sequencing technologies [17,20,57]. However, in vitro characterisation of newly identified viruses is currently lacking. A wealth of information is available from archival virus isolates, most of which were first reported between 1975 and 1985. We sought to provide additional characterisation of five tick-borne viruses isolated from seabird-associated ticks around Australia to establish a protocol for virus discovery and isolation based on the MAVRIC system [23].
We performed growth kinetics analysis on five Australian tick-borne viruses in vertebrate and tick cells. This analysis shows that all five viruses replicate rapidly and to high titres in the rodent-derived BSR cell line. The mammalian tick-borne flavivirus GGYV, orbivirus NUGV and phlebovirus CMCV replicated robustly in the I. scapularis-derived ISE6 cells, reaching peak titres within 1-1.5 log of their peak titre in vertebrate cells. In contrast to GGYV, the seabird tick-associated flavivirus SREV replicated to lower titres in ISE6 cells compared to BSR cells at all tested time points. Although SREV has been isolated from the Australian Ixodes species I. eudyptidis, the CSIRO 4 strain used in this study is derived from the soft tick O. capensis [11]. Furthermore, the closest relative of SREV, Meaban virus has been primarily isolated from Onithodoros species ticks possibly indicating a preference of these viruses for an Ornithodoros vector [58,59]. If this is the case, an Ornithodoros-derived cell line may provide a better alternative for growth of these viruses [60]. Interestingly, SREV could still be recovered from ISE6 cells 4 weeks after infection suggesting an ability for this virus to persist in an Ixodes-derived cell line longer than GGYV, an Ixodes tick-borne flavivirus. FCV, a nairovirus isolated from I. uriae, also produced lower titres in ISE6 cells compared to BSR cells between 1 and 5 dpi. However, an increase in titre at 7 dpi may indicate that peak replication of this virus occurs after the time points sampled in this study. In line with this, growth kinetics of  another Ixodes-borne nairovirus, Hazara virus, in ISE6 cells showed the virus reached peak titre at 8 dpi [61]. As the MAVRIC system has been successfully used for detection of mosquito-borne flaviviruses [23,25], we first assessed its use with the tick-borne flaviviruses GGYV and SREV. Despite replication of both tick-borne flaviviruses in BSR and ISE6 cells, dsRNA could not be detected in either cell line by IFA or ELISA. This unexpected finding was confirmed using the commercial anti-dsRNA antibody J2, which has successfully been used to detect dsRNA in Langat virus-infected ISE6 and Vero cells permeabilised with 0.1% Triton X-100 [62], and TBEVinfected vertebrate cells following permeabilization with either 0.1% Triton X-100 or 0.05% saponin [63,64]. We examined multiple methods of cell permeabilisation including 20% acetone and 0.5% Triton X-100 detergent in ELISA and 100% acetone, Triton X-114 and digitonin in IFA. All of the conditions tested in this study allowed for visualisation of dsRNA in cells infected with the mosquito-borne flavivirus WNV KUN , but not those infected with GGYV or SREV. Flavivirus replication requires the production of dsRNA as intermediates for the generation of nascent RNA genomes. This process is sequestered within invaginations of the host cell membranes which house the viral proteins responsible for RNA synthesis [62,65]. Considering that this process has been demonstrated in both mosquito-and tick-borne flavivirus infection [64,66], it seems likely that the lack of dsRNA detected in GGYV and SREV-infected cells is a result of poor exposure of the replicative intermediates during immunolabelling rather than an absence of dsRNA. Furthermore, detection of dsRNA in GGYV-infected cells at 12 hpi but not at later time points could suggest that the virus replication complexes become less permeable as infection progresses. Previously we have demonstrated that 20% acetone fixation does not sufficiently expose dsRNA during dengue virus infection; however, in this instance dsRNA could be detected following fixation with 100% acetone [23]. In lieu of MAVRIC, our antigenic analyses identified five pan-flavivirus mAbs reactive to the E-protein that can be used for detection of both a mammalian-and a seabird-associated tick flavivirus. Furthermore, we found that one mAb, M2-1E7, could be used to distinguish between the two viruses.
In contrast to our findings with SREV and GGYV, the archival tick-borne orbivirus NUGV was detectable using our anti-dsRNA mAbs from 12 hpi in vertebrate cells and 48 hpi in tick cells. In this study we also report the first genomic sequence data for NUGV. Our data shows that NUGV clusters with the GIV species, consistent with previous serological data [9]. Furthermore, NUGV shares high nucleotide (96-98%) and amino acid (97-100%) similarity with the available sequences for Sandy Bay virus (SBaV) encompassing the outer capsid protein VP5, the capping enzyme VP4 and two non-structural proteins NS2 and NS3. As these genes are typically less conserved between orbiviruses [67,68], the high level of sequence similarity indicates that SBaV is likely a contemporary isolate of NUGV. However, sequencing of the additional genome segments of SBaV is required to confirm this.
We generated complete ORF sequences for the L and M segments of the phlebovirus CMCV and all three segments of the nairovirus FCV. Both viruses share high similarity with archival viruses isolated from Macquarie Island 27-30 years earlier [9,10]. These data suggest that these viruses represent conventional isolates of the phlebovirus PPV and nairovirus TAGV. Furthermore, we demonstrated that serum raised to FCV detected both FCV and TAGV equally well in fixed-cell ELISA. The closeness of FCV to the original TAGV isolate is particularly interesting considering recent detections of two TAGV variants in I. uriae ticks from Antarctica in 2017 and 2018 which share 94-99% nucleotide identity to one another but are divergent from the prototype TAGV strain and FCV [53,55]. Access to transcriptome sequencing of I. holocylcus ticks allowed us to identify four virus-like sequences. These sequences were all related to, but distinct from, sequences previously described in meta-transcriptomic surveys of I. holocyclus ticks collected in Sydney and Southern NSW, and I. uriae ticks collected in Norway and Antarctica between 2016 and 2017 [20,53,55]. RT-PCR analysis of I. holocyclus ticks collected in Northern NSW 10-12 years earlier confirmed the presence of all four sequences. However, attempts to generate additional sequence or obtain isolates in cell culture were unsuccessful. Two sequences, Phlebovirus-like (PVL) sequence 1 and 3, encoded proteins with homology to phlebovirus nucleocapsid proteins. Phylogenetic analysis of these proteins indicated that they clustered with other tick-specific phlebovirus sequences identified in the southern hemisphere. However, both proteins contained a truncated N-terminus contrasting with findings for other recently identified tick phleboviruses, which have significantly larger nucleocapsid proteins with elongated N-terminal domains [20,53,69]. At this stage it is unclear whether these sequences represent viruses or viral integrations. However, the presence of PVL1 in the viscera and salivary glands of ticks from Queensland is particularly interesting in the context of IhIV, which was also identified in both the salivary glands and viscera of I. holocyclus ticks but did not replicate in ISE6 cells [34]. Neither the four virus-like sequences described in this study nor their relatives described in [20] were identified in a recent meta-transcriptomic study performed on unfed adult I. holocyclus ticks collected in Northern NSW [21].

Conclusion
In this study we performed extended characterisation on five archival Australian tick viruses in vertebrate and tick cells to discern whether our mosquito-virus discovery method could be adapted for Australian ticks. Our findings indicate that the established I. scapularis ISE6 cell line can support replication of Australian tick-borne arboviruses, including a flavivirus from an Argasid tick. Furthermore, we have demonstrated that a combined approach of anti-dsRNA and pan-flavivirus mAbs should allow for identification of reoviruses and flaviviruses from Australian ticks. However, the ability of a northern hemisphere-derived tick cell line to support replication of Australian tick-specific viruses is still unclear. Cell lines derived from Australian native ticks may be necessary for future characterisation of tick-specific viruses in this region. Finally, next generation sequencing of NUGV, CMCV and FCV further highlights the need for sequencing of archival viruses to prevent isolates of a single virus receiving multiple names.
Additional file 1: Table S1. List of reagents used in complete ISE6 cell media available in Australia. Product codes and company from which each reagent was purchased are described. Figure S1. Double-stranded RNA immunolabelling in flavivirus-infected cells after permeabilization with digitonin. Immunofluorescence images of BSR cells infected with tick-borne flaviviruses Saumarez Reef virus (SREV), Gadgets Gully virus (GGYV) or mosquito-borne West Nile virus subtype Kunjin (WNV KUN ). Cells were fixed with 4% formaldehyde and permeabilised using a solution of 0.5% w/v digitonin prior to labelling with anti-dsRNA monoclonal antibodies (a) MAVRIC or (b) J2. Images were taken on a Zeiss LSM 510 microscope at 20 × magnification. Blue, nuclei; green, dsRNA. Figure S2. Phylogenetic relationship of NUGV and members of the genus Orbivirus. Phylogenetic analysis of the nucleotide coding sequences of (a) T2 and (b) VP7 (T13) genes. Phylogenetic analyses were performed in MEGA7 using the JC + I model. Bold branches denote members of the tick-borne orbivirus group. The percentage of trees in which the associated taxa clustered together is shown next to the branches. Figure S3. Tertiary structure predictions of Phlebovirus-like nucleocapsid sequences. Predicted protein structure of nucleocapsid-like proteins encoded by (a) PVL1 and (b) PVL3. Protein structures were predicted using Phyre2 based on alignment with Toscana virus N protein (100% confidence). Predicted domains are colour coded as follows: green, N-lobe of globular core domain; magenta, C-lobe of globular core domain; grey, c-terminus not involved in RNA binding; Brown, N-terminus of PVL1 contains a predicted beta strand in lieu of alpha helix 3; black, N-terminus arm domain.
Additional file 2: Dataset S1. Mass spectrometry analysis of Finch Creek virus proteins. Excel file containing the results of analysis of mass spectrometry data from two proteins of Finch Creek virus identified in