Veterinary Science Collected Works - Theses

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    Laparoscopic & Laparoscopically-Assisted Surgery in Rabbits: Comparison of Isobaric and Insufflated Laparoscopic Techniques to Open Laparotomy
    Mccracken, Blaine David ( 2019)
    The use of laparoscopic surgery for routine procedures such as ovariohysterectomy has been well described for dogs and is common in humans. Rabbits have been previously used as models for human laparoscopic surgery and training models for paediatric surgery, however reported use of clinical laparoscopy in rabbits is rare. There are concerns for use of laparoscopic surgery in rabbits due to the effects of the insufflation on ventilation and the risk of increased morbidity from the insufflation contributing to gastrointestinal stasis, a common and life-threatening complication of any surgery in rabbits. This study is designed to quantify and characterise the changes in the postoperative morbidity between open, insufflated and isobaric laparoscopy in healthy adult rabbits. The hypotheses were that use of isobaric laparoscopy will decrease the morbidity of ovariohysterectomy procedures compared to open and insufflated ovariohysterectomy at the expense of increased surgical time. Various investigations were performed over the research project, including a technical viability cadaveric study, a study describing the effects of isobaric and insufflated pneumoperitoneum on ventilatory capability and abdominal dimensions, a study describing the clinical implementation of a Rabbit Grimace Pain score and Behavioural Pain Score in the detection of postoperative pain, and a clinical trial assessing the effects of both laparoscopy methods and comparing them with open laparotomy for ovariohysterectomy. The overall findings of the study support the implementation of isobaric laparoscopy in the rabbit, and the use of laparoscopy in general as a method of reducing postoperative morbidity compared with equivalent laparotomy approaches.
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    Monitoring Training Load in Thoroughbred Racehorses
    Moodie, Victoria Jane ( 2019)
    Methods of monitoring training load are widely practiced amongst today’s elite, sub-elite and amateur athletes. Monitoring training load can range from simple, cost effective methods to complex, expensive methods. The aim of this research was to investigate different methods of monitoring training loads in young Thoroughbred racehorses in pre-training. Simple, cost effective measurements of proximal hoof circumference and hoof toe angle were investigated as a tool to monitor how the hoof responses to the loads experienced in the first two pre-training preparations in young Thoroughbred racehorses. Left and right proximal hoof circumference (n = 42) and hoof toe angle (n = 39) measurements were obtained weekly. During the first pre-training preparation, a significant reduction was recorded in both proximal hoof circumference and hoof toe angle. In contrast, proximal hoof circumference did not change significantly during the second pre-training preparation, whereas hoof toe angle showed a smaller significant decrease. The advancement of modern technology has allowed for improvements in the simplicity of radiographic measurements. However, the collection of radiographic images is still costly to the Thoroughbred racehorse owner. The response of the third metacarpal bone shape and size to training loads can be easily evaluated through the frequent collection of radiographic images. Firstly, weekly left and right mediolateral and lateromedial (respectively) radiographs of the third metacarpal bone were collected and radiographic measurements of bone shape and size were analysed with proximal hoof circumference. Secondly, measurements of supracondylar modelling were obtained the distal end of these third metacarpal bone radiographs. Fifty-four Thoroughbred racehorses were assessed during the first and second pre-training preparations for both sets of measurements. Forty-four Thoroughbred racehorses were assessed at follow-up supracondylar modelling measurement taken from radiographs at 1.5 or 2.5 years from the original measurements. The results showed a moderately strong positive correlation between supracondylar modelling and the number of days in training. Heart rate recovery (HRR) is a simple and effective method of analysing changing fitness levels in Thoroughbred racehorses. Predominantly, research to observe HRR values has been conducted in the laboratory rather than in the field. In the current study, HRR was assessed in thirty-six Thoroughbred racehorses during the first and last sessions of one pre-training preparation. Heart rate data were collected at peak heart rate, 60- and 120-seconds post peak heart rate, at the end of the training session, and 60- and 120-seconds post training. Heart rate recovery was calculated by subtracting the heart rate value at 60-seconds post peak heart rate from the peak heart rate. A significant difference was found between HRR at the first and last HRR assessments. Heart rate recovery assessments in the field may be more difficult to obtain than HRR assessments in the laboratory due to the separation of the trainer and the Thoroughbred racehorse. Therefore, the use heart rate monitors and GPS devices to collect and store HRR values may be more beneficial as it allows the trainer to analyse the data at the end of a mornings work, when there is sufficient time. After identifying and applying the above objective methods to monitor training load in the young Thoroughbred racehorse, a simple and efficient subjective method of monitoring training load was created. The Equine Perceived Exertion (EPE) scale was established from Borg’s Rate of Perceived Exertion scale and Borg’s CR 1 – 10 scale. Six subjective parameters were used to assess each of seventeen Thoroughbred racehorses immediately following their return from sixty-five separate pre-training session. These parameters were behavioural characteristics, respiratory rate, perspiration, capillary refill time, oral mucous membrane colour, and muscle engorgement. Each parameter was assigned a scale and the sum of all parameters corresponded to an algorithm score. The algorithm scores then corresponded to a specific EPE score. Training load was calculated by multiplying the EPE score by the duration of the training session in minutes. There were weak positive correlations between algorithm score or EPE or training load and heart rate recovery 60-seconds post peak heart rate. It was concluded that monitoring training load in Thoroughbred racehorses in a pre-training program can be accomplished and needs to be multifaceted. The trainer must not rely on one particular method of monitoring training load but use both internal and external methods simultaneously to successfully monitor training load. Overall, this work has identified six methods to monitor the training load of Thoroughbred racehorses in pre-training. Further investigation is required to determine if these methods can be used to monitor the training load of Thoroughbred racehorses in gallop training, undertaking different training programs.
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    Leptospirosis prevalence and vaccination practices in South-West Victorian dairy herds
    Erregger, Elke ( 2019)
    While previous studies of Leptospira Hardjo in Victoria demonstrated a relatively high prevalence of exposure in both cattle (40%; Milner et al. 1980) and humans (22%; Sutherland 1988) these estimates need to be revised since they were made more than 30 years ago and leptospirosis vaccination programmes are now commonplace on Victorian dairy farms. This was a cross-sectional study to estimate the prevalence of Leptospira borgpetersenii sv Hardjo and Leptospira interrogans sv Pomona in dairy herds in South-Western Victoria. Fifty-three herds were enrolled into the study. Herd managers were asked to present 15 late-lactation cows that had fertility issues (cows that had not conceived or had delayed calving to conception intervals). Furosemide 500 mg was injected into the tail vein of eligible cows and a mid-stream urine sample of the second voiding collected to increase the likelihood of sampling leptospira .At the time of each herd visit a questionnaire was administered to herd managers asking them to provide details of methods used for controlling leptospirosis, including vaccination. Urine samples were pooled at the herd level and tested for leptospira spp. using qPCR. Pooled samples were then tested individually and samples that were positive, were tested for Leptospira Hardjo and Leptospira Pomona using qPCR. Three of the 53 pooled urine samples returned a positive result. The leptospira positive pools returned a minimum of three positive individual cow urine samples. Testing of individual cow urine samples identified an additional positive herd (with one weak positive and one inconclusive result), giving an apparent prevalence of approximately 8 (95% CI 1 to 13) leptospira-positive herds per 100 herds at risk. Based on the 53 completed questionnaires, leptospirosis vaccination programs were non-compliant with label directions in 35 out of 52 vaccinated herds: 67 (95% CI 54 to 78) out of 100 herds that routinely vaccinate for leptospirosis were doing so incorrectly. Of the 53 herds that took part in this study, only one herd was completely unvaccinated. Based on the findings from this study, and assuming the herds that took part in this study were an unbiased sample of the dairy herd population at risk, we estimate that close to one out of 10 dairy farms in South-Western Victoria are leptospirosis positive. While most herds are vaccinating for leptospirosis, most are doing so incorrectly. We conclude that herd managers need to be better educated regarding leptospirosis vaccination programs.
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    Luxation following press-fit cementless total hip replacement in dogs: Novel techniques for predicting and treating post-operative luxation
    Monotti, Isobel Catherine ( 2019)
    The objective of this thesis is to investigate the relationship between coxofemoral geometry and luxation of total hip replacements (THR) in dogs. This research question was explored in two parts. Examination of the relevant literature demonstrates that increased pre-operative soft tissue laxity is a risk factor for prosthesis luxation in dogs. However, there is little information pertaining to changes in this soft tissue tension in dogs after surgery and the impact this change may have on prosthesis stability. The first part of the thesis explores the association between radiographic measures of pre-operative soft tissue laxity, or offset, and the occurrence of luxation following total hip replacement. The offset measurements were validated in a pilot study, where ventrodorsal pelvic radiographs were assessed in a dog placed in varying degrees of pelvic rotation. Pre-operative and post-operative offset measurements, as well as measures of prosthesis orientation were made for dogs with confirmed dorsal luxation and compared with those of randomly assigned dogs with uneventful post-operative recovery using a case control study. Univariate generalised linear models were used to identify variables of interest and these were assessed in multivariate logistic models. Global offset of the hip was reduced after surgery in both groups, however, reduction was greater in the luxation group (17.7%) compared to the control group (7.4%) and was associated with an increasing odds of luxation. An open orientation of the acetabular cup was also positively associated with luxation. These results indicate that large changes in soft tissue tension after surgery may be a risk factor for luxation. In the second part of the study, a novel technique for surgical revision of luxated total hip replacements was explored. A triple pelvic osteotomy (TPO) was performed in 17 dogs with dorsal hip luxation and the efficacy of this procedure in preventing luxation recurrence, by altering the geometry of the acetabulum, was reported in a retrospective case series. Measurements of acetabular cup orientation were made from pre- and post-operative radiographs and compared using a parried t-test. The revision TPO was successful in preventing reluxation in fourteen cases and an excellent or good clinical outcome was reported in 12 cases. Ventral luxation occurred in three dogs due to over-rotation of the hemi-pelvis. The TPO significantly reduced the angle of lateral opening by 23.0o and increased the version angle of the acetabular cup by 9.0o. The results of this study show that the TPO is an effective procedure for managing THR luxation with retention of implants, however, careful patient selection is recommended to avoid subsequent ventral luxation. In the closing chapter, the challenges of managing surgical cases with significant pre-operative hip laxity are discussed and potential solutions are explored. Limitations of the studies presented in this thesis are also explored and future directions for research are proposed.
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    Pathogenesis of Bluetongue Disease
    Lean, Fabian Zhi Xiang ( 2019)
    Bluetongue virus (BTV) is an important arthropod-borne virus that causes viral haemorrhagic disease in European adapted sheep. Scientific investigation of the pathogenic processes involved in bluetongue (BT) disease manifestation has been compromised by limitations in two key areas: (i) the detection of BTV antigens by immunohistochemistry (IHC) in formalin-fixed tissues has frequently proved to be problematic; and (ii) the choice between animal-derived virus or cell culture-passaged virus for use in experimental infection of animals remains contentious. In this study, BTV-specific antibodies NS1, NS2 and NS3/3a and VP7 were evaluated for use in IHC on formalin-fixed paraffin-embedded (FFPE) tissue specimens. It was shown that there was cross-reactivity between some of these antibodies with a range of BTV serotypes and other orbivirus species. BTV IHC methods developed as part of this evaluation were then employed to study BTV pathogenesis and pathogenicity using the embryonated chicken egg (ECE) as an alternative animal model. Using a pathogenic isolate of a reference BTV serotype 3 (BTV-3; isolated during the Cyprus 1943 outbreak) contained in the blood collected from an infected sheep, BTV-infected ECE demonstrated both endothelio- and neurotropic properties. Furthermore, the pathogenicity of BTV-3 derived from infectious sheep blood and cell-culture-passaged virus were compared in the ECE. BTV propagated in cell culture showed attenuated pathogenicity that was associated with a reduction in genetic diversity in BTV RNA genome Segment 7, encoding the viral structural protein VP7. A representative BT disease model in Australian Merino sheep was established through infection with the pathogenic BTV-3 derived from infectious sheep blood that was used in the ECE. In the sheep model, peak viraemia was observed at day 4 post-infection and this was associated with transient lymphopenia and onset of pyrexia. In addition, thrombocytopenia and prolongation of prothrombin time were detected during BTV infection, as well as the development of typical BT lesions at clinical end-point between 6 to 10 days post-infection. Immunohistochemical analysis demonstrated microvascular endotheliotropism of BTV in various organs, such as lung, tongue, lips, pulmonary artery and the coronary band; immunolabelling of mononuclear inflammatory cells were observed in lymphoid organs. Based on histopathological assessment, the findings of this study suggested that the development of vascular injury-related lesions, such as in the lung and tongue, could be associated with the recruitment of monocytes into alveolar septum and the submucosa of the tongue. To further understand the pathogenesis of BT disease in sheep, RNA-Sequencing was performed on peripheral blood mononuclear cells (PBMCs) and lungs derived from infected sheep collected at various time-points. Transient host responses were detected from the PBMCs and were associated with lymphopenia and peak viraemia. Upregulated differentially expressed genes in the PBMCs were involved in encoding chemokines and antiviral gene products. In the lungs, the host response increased progressively over the course of infection, which involved upregulation of genes associated with the monocyte-macrophage system, antiviral responses and vascular homeostasis. Importantly, upregulation of macrophage gene encoding CD163 in lung from BTV-infected sheep was confirmed by immunohistochemical analysis whereby the increased CD163+ pulmonary intravascular macrophages correlated with the development of pulmonary lesions. Similarly, activation of macrophages was associated with the pathological changes in the tongue. Based on the mechanistic analysis of BTV infection in sheep, BT disease is hypothesised to be a consequence of overt macrophage activation.
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    Towards unravelling the immunomodulatory mechanisms of S. mansoni & L. major parasites in a mouse model using transgenesis
    Tedla, Mebrahtu Gebreyohannes ( 2019)
    Schistosoma mansoni and Leishmania major parasites use immunomodulatory strategies to evade the host’s immune response and little is known about the mechanisms by which these two parasites modulate host immune responses. As a result, these parasites develop different subversion mechanisms to escape host immunity and controlling such immunomodulatory pathogens is still not successful. In this project we hypothesized that an understanding of the ability of memory T cells to withstand pathogen manipulation is crucial for the development of effective vaccine strategies to control these pathogens. Therefore, in this study, OVA transgenic S. mansoni and OVA transgenic L. major were generated to use as a tool to measure the degree of immune memory resilience (defined as an ability of the immune memory to withstand pathogen manipulation) of T helper cells on the face of pathogen-mediated immune manipulation in vivo. The specific aims of this thesis are: i) Express recombinant OVA in both S. mansoni and L. major, ii) Demonstrate that OT-II TCR transgenic T cells are able to recognise the OVA expressed by the parasites, iii) Differentiate the OT-II cells into Th1, Th2 and Th17 cells in vitro and demonstrate their functional phenotype, and iv) Investigate whether the parasites expressing OVA are able to influence the cytokine expression profile of the Th1, Th2 and Th17 OT-II memory T cells. To achieve this, first OVA expression by S. mansoni and L. major was confirmed using RT-PCR and western blot. Subsequently, in vitro and in vivo analysis for proliferative responses of OT-II T cells revealed OVA was recognized by OT-II T cells. The proliferated cells also produced cytokine signatures following stimulation with the OVA expressing parasites both in vitro and in vivo. To measure the immune memory resilience of memory T cells against such pathogens, an OT-II mouse model was used as a source of naive OT-II T cells. Hence, Th1, Th2, and Th17 polarised memory cells were generated in vitro and these cells were adoptively transferred to recipient mice to investigate the immune memory resilience in the face of pathogen-mediated manipulation. After transferring memory cells, mice were challenged with OVA-transduced S. mansoni eggs and OVA transfected L. major parasites as well as wild-type controls. After recovery of Th memory cells, their proliferation rate and cytokine signature was analysed using flow cytometry. The in vitro differentiated Th1, Th2 and Th17 memory cells produced cytokines when challenged by OVA-expressing S. mansoni eggs and OVA expressing L. major. Indeed, Th1 memory cells produced significant level of IFN-g and TNF, while, Th2 memory cells produced high level of IL-2, IL-6 and IL-10, similarly, Th17 memory cells produced IL-17 when stimulated with OVA-expressing parasite eggs and OVA expressing L. major. However, Th1, Th2, and Th17 memory T cells didn’t proliferate in response to wild type S. mansoni eggs, and wild type L. major, and when they were left unstimulated. Therefore, the Th phenotypes of the memory T cells remains unaltered in the face of stimulation by two immune manipulative pathogens (S. mansoni and L. major). The ability of memory T cells to remain resilient to manipulation by these two pathogens has important implications for the prospect of developing vaccines against these parasites.
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    Genomics and pathogenesis of Australian avian coronaviruses
    Quinteros Ugarte, Jose Antonio ( 2019)
    Studies of the molecular pathogenesis of coronaviruses are important as these viruses are major pathogens of animals and humans. The emergence during the 2000s of severe acute respiratory syndrome (SARS), Middle East respiratory syndrome (MERS) and more recently of SARS-2 as a result of interspecies transmission of coronaviruses from animals to humans has demonstrated the importance of understanding how these viruses evolve and what determines their virulence and tissue tropism. Chickens can be used as an animal model to study coronaviruses, as they are the natural host of the avian coronavirus infectious bronchitis virus (IBV). In the studies described in this thesis, different aspects of the molecular biology of infectious bronchitis virus were examined, including the patterns of recombination in the field and the relationship this may have with pathogenicity. IBVs have been constantly recombining and vaccines have played an important role in these recombination events. An attempt was made to generate a cloned genome of the VicS strain of IBV using Gibson Assembly, but was not successful, suggesting that an alternative approach is needed to generate this tool for further studies of the molecular pathogenesis of this virus. Finally, an \textit{in vivo} infection experiment was performed to study the pathogenicity of Australian strains of IBV. These studies demonstrated a tropism for a broader range of tissues than had previously been recognised for all but the most virulent viruses. Analysis of genomic and pathogenicity data suggested that nsp14 may be playing a significant role in the virulence of IBVs, and that further studies should be performed to examine the role of this protein in the replication of IBV.
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    Tissue tropism and latency of infectious laryngotracheitis virus: A study in the natural host
    Thilakarathne, Dulari Samanthika ( 2019)
    Herpesviruses are evolutionarily successful pathogens that infect a large number of animal species. This success is partly attributed to their capacity to establish latency in the host. The avian alphaherpesvirus infectious laryngotracheitis virus (ILTV) causes an acute upper respiratory tract infection in chickens that has considerable impacts on world poultry economy and welfare. The disease caused by ILTV, infectious laryngotracheitis (ILT), is currently controlled by vaccination principally with live attenuated vaccines. Limitations associated with live attenuated vaccines, including the ability to establish latency, may provide avenues for the emergence of novel, more virulent, recombinant strains of ILTV, further complicating the epidemiology of ILTV. In this project, a sensitive nested polymerase chain reaction (NPCR) protocol was developed and the sensitivity of this assay was compared with that of other commonly used PCRs in ILTV research. A trigeminal ganglia (TG) co-culture system was established and optimised and a tracheal co-culture system was reproduced to study in vitro reactivation of latent ILTV. A genotyping system based on allelic variations in multiple genomic regions of ILTV to discriminate ILTV strains prevalent in Victoria, Australia, is also described. These methodologies revealed that a large proportion of the ILTV-vaccinated birds in a commercial layer flock, close to the end of their productive laying period, were shedding multiple vaccine strains of ILTV in the upper respiratory tract, presumably due to reactivation of latent infection. Further, co-culture systems showed in vitro reactivation of latent ILTV in TG and trachea of these birds. The capacity of four vaccine strains of ILTV (SA2, A20, Serva and a glycoprotein G deleted mutant vaccine candidate) to establish latency in specific pathogen free chicken (SPF) following eye-drop vaccination was investigated in vivo. This study revealed ILTV vaccines differed in their capacities to establish latency in TG, and also showed that nearly half of the population had detectable ILTV in their upper respiratory tract (URT), 21 days post vaccination, possibly due to reactivation of infection. A second in vivo experiment was performed to study latency characteristics and late systemic lymphocyte responses in SPF chickens following intratracheal inoculation with a vaccine ILTV (SA2) or a virulent field ILTV (class 9; CL9) strain. Results from this study indicated that latency characteristics did not significantly differ between these strains at 21 days post inoculation (dpi) or at 35 dpi, and suggested that the trachea may be a more significant site of latency and reactivation than the TG. Moreover, regardless of the ILTV strain inoculated, SPF birds showed lymphocytosis during the latent stage of infection. Additionally, tissue tropism of two newly emerged recombinant strains of ILTV (CL9 and class 10; CL10) was investigated using commercial broiler and SPF chickens. The possibility of using feathers as a diagnostic sample was explored. This study revealed that both CL9 and CL10 ILTV strains caused severe disease in both types of birds, distributed to visceral organs and persisted for up to 14 dpi in URT. The NPCR developed in this project detected ILTV DNA in feathers of infected broiler and SPF birds at 14 dpi. Taken together, these studies have shown that tissue tropism and latency is a complex area of research and to a large extent these properties are strain dependent. The studies reported in this thesis have enriched the literature on tissue tropism and latency of ILTV. The results will be valuable for future latency studies and for selection of vaccines to control ILTV.
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    Chicken immune responses to infectious laryngotracheitis virus (ILTV) glycoproteins
    Sabir, Ahmad Jawad ( 2019)
    Infectious laryngotracheitis virus (ILTV), an alphaherpesvirus, causes acute respiratory disease, primarily infecting the upper respiratory tract and conjunctiva. The disease results in significant economic losses to the poultry industry worldwide. Currently, the immune status of the vaccinated flocks or individuals is assessed by the presence of systemic antibodies using commercially available whole virus ELISAs. These ELISAs are good indicators of exposure to either field or vaccine virus, however, the assays are poor in predictors of the level of protective immunity. In this study, individual ILTV glycoproteins (gC, gD, gE, gG, gI and gJ) were assessed for their potential to predict the levels of protective antibody and/or cell-mediated immunity as well as for their capacity to induce neutralising antibodies. To examine whether antibody responses to individual ILTV glycoproteins are correlated with disease and protection, individual glycoproteins expressed in mammalian cells were used in indirect ELISAs to measure post-vaccination and/or post-challenge chicken serum antibodies. Serum optical density (OD) values detected by the whole virus, gC, gI and gJ were significantly higher in birds vaccinated with the Serva vaccine strain compared to the SA2 vaccine strain. However, the mean ODs detected by gD, gE and gG were not significantly different between the vaccine strains. Examination of post-vaccination pre-challenge antibodies to individual glycoproteins did not find a strong correlation between systemic antibodies to individual glycoproteins and protection. The possibility that the protective epitopes of glycoproteins may not be readily detectable in ELISA was investigated by evaluation of the antibodies to each glycoprotein in an in-vitro virus neutralisation assay. Monospecific polyclonal antibodies to individual ILTV glycoproteins gC, gD, gE, gI and gJ were generated in rats and examined for their capacity to neutralise the virus. Neutralising antibodies were detected to gC, gD and gJ individually or in combination. Polyclonal antibodies to gE and gI failed to neutralise the virus when tested individually or combined. In-vitro splenocyte stimulation assays using individual glycoprotein stimulating antigen were conducted to examine the transcription profiles of selected cytokines from nonvaccinated-nonchallenged (NVXNCh), vaccinated-challenged (VXCh) and nonvaccinated-challenged (NVXCh) groups of chickens. The transcription profiles of cytokines referencing Th1, Th2 and Th17 responses were then examined against tracheal pathology results to identify correlation between responses against viral glycoprotein(s) and protective immune response. Expression of IFN-gamma was significantly upregulated in VXCh and NVXCh groups of birds in response to stimulation with gD, with expression levels moderately correlated with protection. Stimulation with gE and gI resulted in significantly higher levels of IL-6 in VXCh birds and response to gE was moderately correlated with protection. Expression of IL-17a was significantly elevated in response to stimulation with gD in NVXCh birds and results were moderately linked to disease severity. The results of this study suggest that IFN-gamma and IL-6 cytokine responses to gD and gE, respectively, may be correlated with protective cell-mediated immunity, whereas IL-17a cytokine responses to gD may be linked to disease. Finally, whole-genome analysis of an unusually virulent “vaccine-like” isolate revealed a new class of ILTV, identified here as class 7b, emerged as a result of recombination probably between another recombinant strain and a vaccine strain. Further analysis of the genome detected recombination hotspots within the unique long (UL) region comprising of genes encoding gB, gC and gM and assembly proteins UL28 and ICP18.5. Boot-scanning analysis of concatenated glycoprotein sequence alignments detected recombination breakpoints within glycoproteins C and H, but not within glycoproteins located in the unique short (US) region. Further studies would be needed to explore the possible role of these glycoproteins in virulence. Thus, the studies reported in this thesis have contributed to understanding (1) the relationship between antibodies to ILTV glycoproteins and protective immunity, (2) virus neutralisation potential of specific antibodies to ILTV glycoproteins, (3) the potential role of ILTV glycoproteins to induce cell-mediated protective immunity, (4) and laid foundation to explore inter-strain genetic diversity within ILTV glycoproteins.
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    Molecular analysis of pathogenicity of Mycoplasma synoviae
    Kordafshari, Somayeh ( 2019)
    Mycoplasma synoviae is a major pathogen of poultry globally, causing chronic respiratory disease and arthritis. Vaccination is an effective means for the control of the disease. The MS-H vaccine is a live attenuated temperature sensitive strain developed through chemical mutagenesis of an Australian field strain, 86079/7NS. Rarely, the temperature-sensitive MS-H strain may revert to a non-temperature-sensitive phenotype. Due to reversion to non-temperature-sensitive phenotype, vaccine isolates may be difficult to distinguish from field strains. Therefore, there is an urgent need for a reliable and rapid assay that can differentiate the MS-H vaccine from field isolates to evaluate the efficacy of the vaccination programs. However, developing such assays depends on a better understanding of molecular basis behind attenuation of MS-H. Comparison of the whole genome of MS-H with that of its parent strain 86079/7NS in previous studies has shown 32 mutations in the MS-H genome, one of which was a frameshift mutation early in an oligopeptide permease transporter gene oppF. In this study polyclonal antibodies raised against peptides upstream and downstream of the mutation in OppF revealed that only N-terminus of the OppF was expressed in MS-H while the full version was expressed in 86079/7NS. The potential of the recombinant full-length OppF, N- (OppF-N) and C termini (OppF-C) of OppF, upstream and downstream of the mutation site, was evaluated for the discrimination of antibody responses to MS-H versus field strains in indirect ELISA. Comparison of optical densities obtained from the ELISAs based on OppF, OppF-N and OppF-C revealed that the indirect ELISA based on OppF-C had the potential to differentiate between MS-H and field strain antibody responses. The impact of the oppF mutation on the MS-H phenotype was investigated in vitro using a mutant of MS-H complemented with a wild-type copy of oppF gene in the MS-H genome. The results revealed that truncation of oppF impacts on growth characteristics of the MS-Hand provide insight into the molecular pathogenesis of M. synoviae and perhaps of broader mycoplasma species. In addition, to characterise the function of OppF protein in MS-H, the metabolite profile of MS-H was compared with that of its field reisolate which only differed in its oppF gene. The liquid chromatography–mass spectrometry analysis revealed a significant decrease in the abundances of amino acids in MS-H compared to that in its field reisolate. This result was consistent with the role of OppF as a peptide transporter. Also, differences found in the level of other metabolites in MS-H reflected some compensation of the OppF function by pathways involving other metabolites. Moreover, in this study genomes of five M. synoviae isolates from MS-H vaccinated chicken flocks were determined and analysed to confirm their relationship with MS-H and also examine the stability of oppF mutation and other genetic markers of the MS-H vaccine. A total of 25 single nucleotide substitution/insertion/deletion including that of oppF existed among the isolates examined. Four of these mutations were those that had been reported between MS-H and its parent strain 86079/7NS, while the other 21 were found only in the MS-H reisolates tested in this study. Therefore, 28 out of 32 mutations previously detected between MS-H and 86079/7NS remained consistent in 5 MS-H reisolates. These results confirmed that M. synoviae isolates in this study were true MS-H reisolates and that majority of the mutations found in the MS-H vaccine are stable after passage in vivo under field condition. The studies described in this thesis have contributed to expansion of our understanding of putative virulence determinants in M. synoviae and laid foundations for the development of a DIVA (Differentiation of Infected and Vaccinated Animals) test to examine variants of the MS-H vaccine. Also, this thesis provided some information on the dynamics of MS-H population after passage in vivo.