Next Article in Journal
In Vitro Maturation of Cumulus–Oocyte Complexes and In Vitro Sperm Capacitation Significantly Increase the Expression and Enhance the Location of the CXCL12 and CXCR4 Anchoring Attractant Complex in Pigs
Next Article in Special Issue
Toxic Wasting Disorders in Sheep
Previous Article in Journal
Population Structure Assessed Using Microsatellite and SNP Data: An Empirical Comparison in West African Cattle
Previous Article in Special Issue
Haemoparasites—Challenging and Wasting Infections in Small Ruminants: A Review
 
 
Search for Articles:
Title / Keyword
Author / Affiliation / Email
Journal
Article Type
 
 
Advanced Search
 
Section
Special Issue
Volume
Issue
Number
Page
 
Journals
Animals
Volume 11
Issue 1
10.3390/ani11010146
animals-logo
Submit to this Journal Review for this Journal Propose a Special Issue
Article Menu

Article Menu

share Share announcement Help format_quote Cite question_answer Discuss in SciProfiles thumb_up
...
Endorse textsms
...
Comment
first_page
settings
Order Article Reprints
Font Type:
Arial Georgia Verdana
Font Size:
Aa Aa Aa
Line Spacing:
Column Width:
Background:
Article

Growth Performance and Clinicopathological Analyses in Lambs Repetitively Inoculated with Aluminum-Hydroxide Containing Vaccines or Aluminum-Hydroxide Only

by
Ricardo de Miguel
1,†,
Javier Asín
1,†,‡,
Ana Rodríguez-Largo
1,
Irache Echeverría
2,
Delia Lacasta
1,
Pedro Pinczowski
1,§,
Marina Gimeno
1,‖,
Jéssica Molín
1,¶,
Antonio Fernández
1,
Ignacio de Blas
1,3,
Damián de Andrés
2,
Marta Pérez
1,3,
Ramsés Reina
2 and
Lluís Luján
1,3,*
1
Department of Animal Pathology, University of Zaragoza, 50013 Zaragoza, Spain
2
Institute of Agrobiotechnology, CSIC-Government of Navarra, 31192 Mutilva, Spain
3
Instituto Universitario de Investigación Mixto Agroalimentario de Aragón, University of Zaragoza, 50013 Zaragoza, Spain
*
Author to whom correspondence should be addressed.
Both authors contributed equally.
Current affiliation: California Animal Health and Food Safety Laboratory System, University of California, Davis, CA 95616, USA.
§
Current affiliation: New South Wales Department of Primary Industries, Biosecurity and Food Safety, Elizabeth Macarthur Agricultural Institute, Menangle, NSW 2568, Australia.
Current affiliation: University Veterinary Teaching Hospital Camden, The University of Sydney, Brownlow Hill, NSW 2570, Australia.
Current affiliation: Department of Animal Science, University of Lleida, Plaça de Víctor Siurana, 1, 25003 Lleida, Spain.
Animals 2021, 11(1), 146; https://doi.org/10.3390/ani11010146
Submission received: 8 December 2020 / Revised: 4 January 2021 / Accepted: 5 January 2021 / Published: 11 January 2021
(This article belongs to the Special Issue Wasting Diseases Affecting Sheep)
Browse Figures
Versions Notes

Abstract

:

Simple Summary

Aluminum-hydroxide is an effective vaccine adjuvant used in most commercial sheep vaccines. It facilitates the establishment of a robust immune response against the vaccine antigen. During the first decade of the 21st century, repetitive injections with vaccines containing aluminum-based adjuvants were proposed to be linked to a progressive wasting syndrome in sheep. The aim of this work was to analyze several clinicopathological parameters, including growth performance, clinical data, and histopathological observations in lambs intensively injected with aluminum-containing vaccines, aluminum-hydroxide only, or a saline solution as control. Although aluminum-hydroxide was linked to chronic inflammatory reactions at the injection site and the development of behavioral changes in sheep, the results presented here indicate that injected aluminum-hydroxide, either alone or in combination with vaccine antigens, is not enough to induce relevant changes in the parameters studied. Other factors such as sex, breed, age, production system, diet or climate conditions could play a role in the development of the previously described wasting syndrome.

Abstract

Aluminum (Al) hydroxide is an effective adjuvant used in sheep vaccines. However, Al-adjuvants have been implicated as potential contributors to a severe wasting syndrome in sheep—the so-called ovine autoimmune-inflammatory syndrome induced by adjuvants (ASIA syndrome). This work aimed to characterize the effects of the repetitive injection of Al-hydroxide containing products in lambs. Four flocks (Flocks 1–4; n = 21 each) kept under different conditions were studied. Three groups of seven lambs (Vaccine, Adjuvant-only, and Control) were established in each flock. Mild differences in average daily gain and fattening index were observed, indicating a reduced growth performance in Vaccine groups, likely related to short-term episodes of pyrexia and decreased daily intake. Clinical and hematological parameters remained within normal limits. Histology showed no significant differences between groups, although there was a tendency to present a higher frequency of hyperchromatic, shrunken neurons in the lumbar spinal cord in the Adjuvant-only group. Although Al-hydroxide was linked to granulomas at the injection site and behavioral changes in sheep, the results of the present experimental work indicate that injected Al-hydroxide is not enough to fully reproduce the wasting presentation of the ASIA syndrome. Other factors such as sex, breed, age, production system, diet or climate conditions could play a role.

1. Introduction

Vaccines are indispensable tools in animal production to control diseases and increase production rates [1]. In sheep husbandry, vaccination protocols differ depending on a variety of factors such as the production system, geographical location, climate, and/or disease prevalence [2]. Furthermore, health management programs can be modified by compulsory vaccination campaigns to fight against emerging or re-emerging epizootics [3]. A recent example was the compulsory vaccination campaign against bluetongue virus that took place in most European countries during the first decade of the 21st century [4,5]. This immunization campaign effectively controlled virus circulation and stopped disease progression. However, the repetitive vaccination caused diverse side effects of variable intensity that affected productive parameters and animal health in several countries [6,7,8,9,10]. Interestingly, a wasting syndrome associated with neurological signs was described and the aluminum (Al)-based adjuvants—that the used vaccines contained—were incriminated as the potential triggering etiology [11]. The name ovine autoimmune/inflammatory syndrome induced by adjuvants (ASIA syndrome) was proposed for this process [11,12].
In veterinary medicine, Al-hydroxide is a widely employed vaccine adjuvant that efficiently boosts immune responses against the vaccine antigens [13,14]. Therefore, Al is currently present in most ovine commercial vaccines. Previous publications demonstrated that subcutaneous inoculation of Al-hydroxide adjuvants induces the formation of persistent, sterile granulomas composed of abundant Al-laden macrophages in the experimental animals used in the present study [15]. These macrophages can reach regional lymph nodes and potentially disseminate Al throughout the body [15]. Indeed, higher Al levels were demonstrated in the lumbar spinal cord of the Al-hydroxide-inoculated animals [16]. Moreover, Al-hydroxide was linked to the development of an array of behavioral changes in a group of the same lambs [17]. The evaluation of productive and clinical parameters together with a comprehensive pathological analysis in the animals included in the aforementioned publications have never been reported. Moreover, whether repetitive inoculation of Al-hydroxide may induce an ovine wasting syndrome or not is a crucial question that has never been addressed in a large-scale experiment.
The aim of this work was to study the clinical long-term effects and postmortem changes induced by the repetitive injection of Al-hydroxide, either alone or combined into commercial vaccines, in lambs maintained under different environmental conditions and productive systems.

2. Materials and Methods

2.1. Experimental Design

All procedures were carried out under Project License PI15/14 approved by the Ethics Committee for Animal Experiments of the University of Zaragoza. The care and use of animals were performed according to the Spanish Policy for Animal Protection RD53/2013, which meets the European Union Directive 2010/63 on the protection of animals used for scientific purposes.
A total of 84, three-month-old, neutered male lambs were divided into four flocks of 21 animals each. Flock 1 originated from a Rasa Aragonesa breed-accredited commercial farm and was placed in a research facility (Experimental farm, University of Zaragoza) under previously described conditions [15,17]. Animals from flocks 2, 3, and 4 were born, selected, and raised in commercial sheep farms located in different geographical areas [14]. Flocks 2, 3, and 4 remained integrated in their original herd for the entire duration of the experiment. Detailed information of the production systems and climatological parameters is provided in Table 1 and Table A1 (Appendix A), respectively.
Each flock of 21 lambs was split into three treatment groups of 7 animals each: Vaccine group, which was inoculated with commercial vaccines; Adjuvant-only group, which received the equivalent dose of Al-hydroxide (Alhydrogel®, CZ Veterinaria, Porriño, Spain), and Control group, which was injected with phosphate-buffered saline (PBS). Six animals (i–vi) died for reasons unrelated to the treatments: in Flock 3, these included two animals in the Control group (i: urolithiasis and hydronephrosis; ii: aspiration pneumonia), one animal in the Vaccine group (iii: urolithiasis and hydronephrosis), and one animal in the Adjuvant-only group (iv: urolithiasis and hydronephrosis); in Flock 4, dead animals included one animal in the Adjuvant-only group (v: septicemia caused by Pasteurella spp.) and one animal in the Vaccine group (vi: sheep bloat). The final number of animals in each flock was: Flock 1: n = 21; Flock 2: n = 21; Flock 3: n = 17; and Flock 4: n = 19. Therefore, when all flocks were grouped together, each treatment group (Vaccine, Adjuvant-only, Control) consisted of 26 animals at the end of the experiment. Data derived from dead animals were not considered for any of the parameters evaluated.
An accelerated vaccination schedule was applied. The goal was to reproduce, within an acceptable time frame for a 3-year research project, the management field conditions that led to the ovine ASIA syndrome. Animals received a total of 19 subcutaneous inoculations, which mimic the amount of Al that animals can receive during their productive lifespan (a mean of seven years). The last injection was applied 5 days prior to euthanasia in the four flocks. Inoculation schedule is described in Figure 1 and Figure A1 (Appendix B). Details of the vaccines used are described in Table A2 (Appendix C). Vaccine and Adjuvant-only groups received a total of 81.29 mg of Al. The study lasted 15 months, ranging from 432 to 470 days, depending on each flock.

2.2. Productive and Clinical Parameters

In order to analyze animal growth, lamb weights were recorded nine times along the experiment, days between each measurement ranged from 31 to 63 (Figure 1, W1 to W9). Partial and global average daily gain (ADG) were calculated. Partial ADG included all the weighing dates; global ADG was calculated using the first and the last weights and dividing the difference by the number of days between them. General clinical examination was performed periodically (Figure 1), 18 to 41 days after previous inoculation date and just prior to the application of the next inoculation. It included blood sampling, rectal temperature, heart rate, and respiratory rate. Blood samples were obtained by jugular venipuncture with 6 mL EDTA tubes (BD Vacutainer®, Becton Dickinson, Madrid, Spain) and a hematological panel including white blood cell count, red blood cell count, hematocrit, hemoglobin, and platelet count was performed (scil Vet abc Plus™ Animal Blood Counter). Additionally, animals from Flock 1 were subjected to two rounds of behavioral tests (one in summer and another in winter) and these results were previously reported [17]. Urine was analyzed just after euthanasia with a biochemical strip to test pH, glucose, and protein.

2.3. Post-Mortem Studies

Euthanasia was performed by intravenous injection of an overdose of barbiturate solution (Dolethal®, Vetoquinol, Madrid, Spain). Complete post-mortem examinations were performed. Perirenal, mesenteric, pericardial, thoracic, and subcutaneous fat deposits were scored from 0–3 (0: Absence of fat; 1: Scarce fat deposition; 2: Moderate fat deposition; 3: Normal fat deposition), and a fattening index was calculated as the mean value of these five scores. Additionally, thickness of subcutaneous sternal fat was measured.
Systematic sampling of all tissues was performed. Central nervous system (CNS) and peripheral nervous system (PNS) were sampled following a previously-described protocol [18]. Tissues were fixed in 10% neutral-buffered formalin for 48–72 h. Samples were routinely processed for paraffin embedding and production of 4 µm, hematoxylin-eosin (HE)-stained slides. Histopathological analysis of different areas of the CNS (brain: frontal cortex-caudate nucleus, parietal cortex, thalamus-hypothalamus; spinal cord: cervical, thoracic, and lumbar segments), PNS (subcutaneous-thoracic, sciatic, tibial, and radial nerves), liver, kidney, pancreas, spleen, adrenal glands, thyroid, and thymus were performed by a single pathologist (J.A.) who was blinded to the treatment group. The histopathological features evaluated, and the scoring system used in each tissue are described in Table A3, Table A4, Table A5, Table A6, Table A7, Table A8, Table A9, Table A10 and Table A11 (Appendix D).

2.4. Statistical Analysis

All statistical analyses were performed using IBM SPSS 19.0 for Windows (IBM Corp., Armonk, NY, USA). Quantitative variables (i.e., body weight, ADG, fattening index, sternal fat deposits) were analyzed by Shapiro–Wilk test to assess normality of data. Levene’s test was used to test the equality of variances. When data followed a normal distribution and had homogeneous variances, the parametric test ANOVA was used, followed by Duncan’s multiple range test as a post hoc. In normally-distributed quantitative variables with unequal variances, Welch’s t-test was used. In non-normal quantitative variables, the non-parametric Kruskal–Wallis test was used, followed by Dunn’s test as a post hoc. In qualitative variables (i.e., histopathological analyses), assessment of the association between groups was carried out using Pearson’s chi-square test or alternatively Likelihood ratio test and Fisher’s exact test when needed. Statistical significance was considered when p value < 0.05. Statistical tendency was considered when p value ≤ 0.1.

3. Results and Discussion

3.1. Body Weight and Average Daily Gain

Results for body weight and ADG are presented in Table A12 (Appendix E) and Table A13 (Appendix F), respectively. Mild to moderate differences in ADG were observed between treatment groups in each one of the individual flocks. Global ADG of each flock is represented in Figure 2 and indicated a moderate growth rate reduction in Vaccine groups in contrast with Control groups. Adjuvant-only groups showed lower ADG values than Control groups but higher ADG values than Vaccine groups. This data distribution was observed for the ADG values of all flocks, although Flock 2 was the only one where these differences were statistically significant (p = 0.045). Moreover, when all flocks were grouped together, this tendency was maintained although it did not reach significance (p = 0.072).
This lower ADG for the Vaccine and—to a lesser extent—Adjuvant-only groups could be explained by transient, short-term, post-vaccination events, including brief periods (24–48 h) of fever after vaccinations and associated decreased appetite [19,20]. Indeed, it has been observed that booster vaccinations against respiratory pathogens in fattening lambs can cause moderate growth retardation, with animals reaching their optimal sacrifice weight 5 days later than control animals (JM Gonzalez, personal communication). The lambs included in this work likely suffered repetitive episodes of hyperthermia and decreased daily intake, which could have affected ADG and absolute weight at the end of the experiment. In fact, the acute-phase response elicited by vaccination is essential for optimal development of the immune response [21,22]. This response increases nutrient demands so they are redistributed to support the immune system instead of growing, which may lead to reduced growth performance and feed efficiency [23,24]. Moreover, stimulation of immune response can activate the mammalian target of rapamycin (mTOR) signaling pathway and thus affect metabolic routes involved in reduced anabolism [25,26]. The latter is in accordance with energy consumption due to vaccination and may affect the body condition in specific vaccination strategies, especially in negatively energy balanced feedlot animals. In such a scenario, the presence of more severe inflammatory reactions in the injection sites of animals in the Vaccine groups [15] might also help to explain the differences between Vaccine and Adjuvant-only groups. None of the lambs injected with the adjuvant only or with Al-containing vaccines unequivocally developed a wasting syndrome such as the one described after the compulsory vaccination campaigns against bluetongue [11].
Analysis of partial variations in ADG revealed significant differences between weight measurements at dates W4 and W5 (Table A13Appendix F), coinciding with the summer (Figure 1). In Flocks 1 and 2, Vaccine groups showed a significantly lower ADG than Control and Adjuvant-only groups (Flock 1: p = 0.02; Flock 2: p = 0.049). Flock 4 showed similar, although non-significant (p = 0.055) results. No statistically significant variation was observed in Flock 3. When the four flocks were considered altogether, these variations in the Vaccine group also reached statistical significance (p = 0.045). Globally, these variations in ADG are likely associated with the high temperatures reached during this period and detailed in Table A1 (Appendix A). High environmental temperatures induce heat stress and negatively alter lamb growth due to lower feed intake and activation of thermoregulatory mechanisms [27]. Thermoregulatory capacity and productive performance in fattening lambs with heat stress depends on breed, production system, diet, and age [28]. Perhaps these effects were more marked in the Vaccine group because they combined with preexisting stressors in these animals, i.e., persistent injection site reactions [15]. Interestingly, transcriptomic studies performed in Flock 1 of the present work demonstrated that Al adjuvants significantly increased the expression of pro-inflammatory cytokines and genes of the NF-kB and apoptotic pathways [29]. Activation of these pathways may potentially interfere with optimal thermoregulatory mechanisms.

3.2. Clinical and Hematological Examination

Rectal temperatures, heart and respiratory rates, and urine analyses showed no relevant differences between groups in any of the flocks individually or when all flocks were grouped together. Transient pyrexia is a common and expectable post-vaccination effect in feedlot lambs and calves, especially after booster vaccinations [19,20]. In our study, rectal temperature was recorded 18 to 41 days after the previous inoculations (Figure 1), as the main objective was to measure the cumulative, long-term effect of the repetitive injections rather than short-term variations. In this context, it is likely that those transient differences were missed.
Hematological results of the three treatment groups of the four flocks grouped together are detailed in Table A14 (Appendix G). There were point differences between groups both at the individual flock level and when all flocks were considered together, but data were always within normal ranges for sheep. Marked normochromic, non-regenerative anemia was reported as part of the wasting syndrome described after the compulsory bluetongue vaccination campaign [11], but this phenomenon was not observed in this experimental work. This might be due to different factors influencing the development of that particular feature, as experimental conditions in the present study probably could not reproduce the exact scenario that fueled the appearance of the wasting presentation of the ovine ASIA syndrome.

3.3. Post-Mortem Studies

Necropsy findings revealed mild differences in the fattening index and sternal fat deposits (Table 2) when all flocks were considered together. For both parameters, Vaccine group showed lower values than Control group, whereas values in the Adjuvant-only group were higher than the Vaccine group and lower than the Control group. These results parallel the mild differences observed in the ADG of these animals. Therefore, decreased fat deposition at the end of the experiment in the Vaccine group may be also the result of transient periods of anorexia. Sternal fat deposits play an important role in thermogenesis in sheep [30]. There were no other gross abnormalities in any of the treatment groups apart from those previously described [15].
Histopathological results of the four flocks grouped together are detailed in Table 3 and Table A15 (Appendix H). Evaluation of the CNS and PNS showed point differences between treatment groups when each flock was analyzed individually, but they were heterogeneous between flocks and not clearly linked to treatments applied. However, when all flocks where grouped together only a statistical tendency (p = 0.100) to present higher numbers of dark neurons in the lumbar spinal cord (Table 3) was observed in the Adjuvant-only group. The term “dark neuron” defines a hyperchromatic, shrunken neuron [31,32]. This histological finding should be interpreted cautiously as it may be just an artifact [32]. Degenerated necrotic neurons tend to be brightly acidophilic rather than basophilic/dark, although sometimes these two appearances are difficult to differentiate. Furthermore, ischemic neurons in peracute stages of degeneration may be indistinguishable from dark neurons [33,34]. Interestingly, analytical measurements and a lumogallion stain (Al-specific histochemical stain) performed in the CNS of animals from Flock 1 revealed increased levels of Al in the lumbar spinal cord of the Adjuvant-only group [16]. Perhaps this tendency in the number of dark neurons in the spinal cord of the Adjuvant-only group is related to Al accumulation in the same location. Remarkably, this global absence of histological lesions in the encephalon was observed in animals from Flock 1, which showed significant behavioral alterations in a previous study [17]. Furthermore, transcriptomic studies performed in the encephalon of these animals revealed dysregulation of genes related to neurological function and mitochondrial energy metabolism [35]. Most likely, these clinical and molecular differences did not induce structural abnormalities that could be detected with basic histological methods such as HE.
The pancreas showed a significantly (p = 0.012) increased presence of multifocal and/or periductal lymphoplasmacytic inflammatory infiltrates in the Adjuvant-only group when all flocks were considered together (Table 4). Interestingly, pancreatic changes have been reported in guinea pigs inoculated with Al-hydroxide adjuvants either subcutaneously or intraperitoneally [36]. Histopathological results obtained in the rest of organs are presented in Table A16, Table A17, Table A18, Table A19, Table A20 and Table A21 (Appendix I). There was a positive tendency (p = 0.078) in the number of lambs with thyroid follicular cell hypertrophy in the Adjuvant-only and Vaccine groups (Table A20Appendix I), and a significant (p = 0.043) decrease in the number of lambs showing thymic germinal center hyperplasia in the Adjuvant-only and Vaccine groups (Table A21Appendix I). No significant differences were found in any of the parameters analyzed in liver, kidney, spleen, and adrenal gland.

3.4. Study Limitations

The interpretation of these results has some limitations intrinsic to the study design and experimental procedures performed. First, the number of animals used could have limited some of the statistical analyses. Second, most of the descriptions of the wasting syndrome that occurred after the bluetongue vaccination campaigns included adult animals, generally ewes in full production [11]. The animals used in this experiment were growing, male neutered, young lambs, which perhaps limited the capacity of the inoculations to induce severe weight loss. A similar study using adult sheep with stable body weight at the beginning of the experiment could help to clarify this aspect. Lastly, the number of inoculations performed overrates the normal vaccination schedule for sheep in a year. In fact, the wasting syndrome occurred with just four doses in around a month, with an amount of 16 mg of Al inoculated per animal [10,11]. Most likely, in addition to Al, other parameters such as sex, breed, age, productive system, diet, and/or climate conditions (winter cold) are necessary co-factors for the full development of the devastating wasting presentation of the ovine ASIA syndrome.

4. Conclusions

This work summarizes the results obtained on the growth performance and clinicopathological parameters in lambs subjected to repetitive inoculations with saline solution (Control group), Al-hydroxide adjuvants (Adjuvant-only group) or Al-hydroxide-based vaccines (Vaccine group) either under experimental or in field conditions. Mild differences in ADG and fattening index were reported in the Vaccine group and were likely associated with transient post-injection hyperthermia with decreased daily intake and/or intense inflammatory reactions occurring at the injection sites [15]. Clinical, hematological, and histopathological analyses revealed minimal abnormalities, even knowing that previous behavioral and transcriptomic studies performed in one of the flocks studied here revealed significant alterations in the Adjuvant-only and/or Vaccine groups [17,35]. Despite previously-observed results showing the effects of repetitive inoculations of Al-hydroxide containing vaccines and adjuvants in sheep [15,16,17,29,35], the results or this experimental study seem to indicate that injected Al may be necessary, but not sufficient to reproduce all the productive and clinicopathological characteristics of the ovine wasting syndrome (ovine ASIA syndrome) [11].

Author Contributions

Conceptualization, L.L., J.A., D.d.A., R.R., M.P.; data curation J.A., R.d.M., L.L.; formal analysis, R.d.M., J.A., I.d.B., D.L., A.F., I.E., A.R.-L.; funding acquisition, L.L., D.d.A., R.R.; investigation J.A., R.d.M., D.L., J.M., A.F., M.P., L.L., R.R., D.d.A.; methodology J.A., D.L., P.P., M.G., J.M., A.F., M.P.; project administration L.L.; M.P., R.R.; supervision L.L., R.R., D.d.A.; validation I.d.B., D.L., A.F.; writing—original, R.d.M., L.L., M.P.; writing—review and editing, J.A., A.R.-L., I.E., D.L., P.P., M.G., J.M., A.F., I.d.B., D.d.A., R.R. All authors have read and agreed to the published version of the manuscript.

Funding

This work was funded by grants from the Spanish Ministry of Economy, Industry and Competitiveness (AGL2013-49137-C3-1-R and AGL2013-49137-C3-2-R), the Ministry of Science, Innovation and Universities (RTI2018-096172-B-C31 and RTI2018-096172-B-C33) and the Recognized Research Groups of Government of Aragón (A17_17R, Animal Health and Reproduction). RdM was a PhD student funded by the Department of Innovation, Research and University of Aragón. JA and ARL were PhD students funded by the Spanish Ministry of Science, Innovation and Universities (formerly Spanish Ministry of Education). IE was a PhD student funded by the Universidad Pública de Navarra.

Institutional Review Board Statement

The study was conducted according to the guidelines of the Declaration of Helsinki, and approved by the Ethics Committee of the University of Zaragoza (Project License PI15/14, 2nd September 2014).

Informed Consent Statement

Not applicable.

Data Availability Statement

Our study includes all data as Appendix A, Appendix B, Appendix C, Appendix D, Appendix E, Appendix F, Appendix G, Appendix H and Appendix I.

Acknowledgments

J.M. González and A. Auseré are deeply acknowledged for their support in the analysis and interpretation of growth performances. Charo Puyó and Santiago Becerra are sincerely acknowledged for their technical support. Veterinarians of the three commercial herds (M. Vila, L. Figueras and I. Cuartielles) are fully acknowledged. Authors would like to acknowledge the use of Servicio General de Apoyo a la Investigación-SAI, Universidad de Zaragoza. The State Meteorological Agency of the Spanish Government (AEMET) is gratefully acknowledged for climate data [37].

Conflicts of Interest

The authors declare no conflict of interest.

Appendix A

Table
Table A1. Climate conditions along the experiment. Higher and lower temperatures during the experiment are in bold. Higher relative humidity along the experiment is indicated in bold. Data obtained from the State Meteorological Agency (AEMET) of the Spanish Government [37].
Table A1. Climate conditions along the experiment. Higher and lower temperatures during the experiment are in bold. Higher relative humidity along the experiment is indicated in bold. Data obtained from the State Meteorological Agency (AEMET) of the Spanish Government [37].
FLOCK 1 and 4FLOCK 2FLOCK 3
Month–YearT. mean
3		T. min 1T. max 2N0
4		N30
5		RH
6		T. mean
3		T. min 1T. max 2N0
4		N30
5		RH
6		T. mean
3		T. min 1T. max 2N0
4		N30
5		RH
6
MeanAbsMeanAbsMeanAbsMeanAbsMeanAbsMeanAbs
January–20157.12.5−2.011.616.770666.01.15.610.816.9140N/A 75.91−1.810.717.510075
February–20157.12.82.911.318.470616.92.1−4.911.818.4100N/A6.31.25.211.416.78065
March–201511.86.71.316.924.0005611.66.1−1.117.123.730N/A11.45.60.117.123.00061
April–201515.69.44.621.827.9004614.57.61.321.426.8005414.57.92.420.925.50052
May–201520.113.59.426.536.4094319.111.14.62734.0074718.911.25.026.635.10643
June–201525.217.514.032.941.60203823.415.211.731.639.10205023.415.610.631.238.601944
July–201527.920.216.235.543.70273826.718.513.334.742.80284827.319.112.535.542.102939
August–201525.518.814.232.137.20244524.217.311.031.136.80215824.217.211.831.336.502149
September–201520.514.910.726.130.4024819.112.86.825.430.201591912.88.525.130.10259
October–201516.611.54.921.728.3005815.49.62.321.227.4006615.810.32.721.326.30066
November–201512.281.716.424.8007310.97−3.614.822.1308010.97.2−0.914.623.81081
December–20157.63.9−0.211.216.610827.33.4−1.011.116.440878.64.7−0.912.517.93084
January–20169.65.90.213.320.500707.83.4−2.112.218.440787.84.1−1.711.516.52081
February–20169.54.7-0.814.221.2206082.5−4.113.519.690708.23.2−3.913.118.74071
March–201610.35.50.715.124.900589.23.5−1.914.824.220679.33.6−1.315.122.42066
April–2016148.52.619.426.9005112.86.41.019.326.5006012.36.21.518.423.80062
May–201617.912.16.823.731.3024816.49.42.223.329.5005715.89.11.222.530.20157
June–201623.416.411.330.337.00174022.214.28.430.134.90164721.713.97.729.535.901442
1 T. min: Minimum temperature (Mean: Mean of the minimum temperature/Abs: Lowest value for a specific month). 2 T. max: Maximum temperature (Mean: Mean of the maximum temperature/Abs: Highest value for a specific month). 3 T. mean: Mean temperature for a specific month. 4 N0: Number of days with the minimum temperature under 0 °C. 5 N30: Number of days with the maximum temperature over 30 °C. 6 RH: Relative humidity. 7 N/A: Not available.

Appendix B

Animals 11 00146 g0a1 550
Figure A1. Inoculation schedule for each flock individually. All flocks were subjected to the same inoculation schedule and experimental procedures. Differences in the number of days between inoculations in the different flocks and other experimental procedures are shown. Each injection date is indicated by a vertical line and a number. W: Weight measurement. E: Clinical examination. H: Hematological analysis. Information on the injection and vaccines number, season, and month is also provided. Information about the vaccines used is presented in Table A2 (Appendix C).
Figure A1. Inoculation schedule for each flock individually. All flocks were subjected to the same inoculation schedule and experimental procedures. Differences in the number of days between inoculations in the different flocks and other experimental procedures are shown. Each injection date is indicated by a vertical line and a number. W: Weight measurement. E: Clinical examination. H: Hematological analysis. Information on the injection and vaccines number, season, and month is also provided. Information about the vaccines used is presented in Table A2 (Appendix C).
Animals 11 00146 g0a1

Appendix C

Table
Table A2. Vaccines used in the experiment and inoculation date. Aluminum (Al) content was established by inductively coupled mass spectrometry (ICP-MS) and calculated as milligrams (mg) per total dose.
Table A2. Vaccines used in the experiment and inoculation date. Aluminum (Al) content was established by inductively coupled mass spectrometry (ICP-MS) and calculated as milligrams (mg) per total dose.
Vaccine NumberCommercial NameAntigen/sInoculation Date (Figure 1)Al per Dose (mg)
1Heptavac P PlusPasteurella multocida
Mannheimia haemolytica
Clostridium spp.		1, 2, 97.5
2Autogenous vac.Staphylococcus aureus
spp. anaerobius		3, 4, 141.644
3Vanguard RRabies virus51.025
4AgalaxipraMycoplasma agalactiae6, 76.764
5Ovivac CSChlamydia abortus
Salmonella abortus ovis		8, 95.6
6Autogenous vac.Corynebacterium pseudotuberculosis10, 111.32
7Bluevac-1Bluetongue virus Serotype 112, 134.18
8Bluevac-4Bluetongue virus Serotype 412, 134.16
9Bluevac BTV8Bluetongue virus Serotype 815, 164.4

Appendix D

Histopathological features evaluated in the experimental lambs in central and peripheral nervous systems, liver, kidney, pancreas, spleen, adrenal glands, thyroid, and thymus.
Table
Table A3. Histopathological features evaluated in the central nervous system (brain: frontal cortex-caudate nucleus, parietal cortex, thalamus-hypothalamus; spinal cord: cervical spinal cord, thoracic spinal cord, lumbar spinal cord).
Table A3. Histopathological features evaluated in the central nervous system (brain: frontal cortex-caudate nucleus, parietal cortex, thalamus-hypothalamus; spinal cord: cervical spinal cord, thoracic spinal cord, lumbar spinal cord).
FeaturesEvaluationDescription
Perivascular cuffingP/A 1At least one blood vessel surrounded by >2 layers-thick perivascular cuff of lymphocytes, plasma cells, and/or histiocytes.
MeningitisP/AAggregates of lymphocytes, plasma cells, and/or histiocytes in the meninges
Glial nodulesP/AAt least one nodular aggregate of glial cells in the neuropil
Microglial activationP/AAggregates of rod shaped glial cells in the neuropil
Dark neuronsP/ADeeply hyperchromatic, shrunken neurons
1 P/A: Presence/Absence.
Table
Table A4. Histopathological features evaluated in the peripheral nervous system (subcutaneous-thoracic, sciatic, tibial, and radial nerves).
Table A4. Histopathological features evaluated in the peripheral nervous system (subcutaneous-thoracic, sciatic, tibial, and radial nerves).
FeaturesEvaluationDescription
Perineural, perivascular cuffingP/A 1At least one, ≥1 layer thick, perivascular aggregate of lymphocytes, plasma cells, and/or histiocytes in the tissues adjacent to the nerve
Intraneural inflammationP/AAggregates of lymphocytes, plasma cells, and/or histiocytes within the peri- or endoneurium
1 P/A: Presence/Absence.
Table
Table A5. Histopathological features evaluated in the liver.
Table A5. Histopathological features evaluated in the liver.
FeaturesEvaluationDescription
Portal/periportal inflammationP/A 1Inflammatory infiltrates in or around portal spaces
TypeLP: Lymphoplasmacytic
LP + E: Lymphoplasmacytic and eosinophilic
Hepatocellular degenerationP/ASwollen hepatocytes with vacuolated or feathery cytoplasm
Hepatocellular necrosisP/AShrunken eosinophilic hepatocytes with pyknotic nucleus
Hepatocellular atrophyP/AShrunken hepatocyte cords with distended sinusoids
1 P/A: Presence/Absence.
Table
Table A6. Histopathological features evaluated in the kidney.
Table A6. Histopathological features evaluated in the kidney.
FeaturesEvaluationDescription
Glomeruli: ProteinuriaP/A 1Protein globules in the Bowman’s space
Tubules: DegenerationP/ASwollen tubular epithelium with vacuolated or feathery cytoplasm
Tubules: Hyaline dropletsP/ADeeply eosinophilic, 1–3 μm intracytoplasmic droplets
Interstitium: InflammationP/AAggregates of lymphocytes, plasma cells, and/or histiocytes
Medulla: MineralizationP/AFoci of tubulointerstitial mineralization
1 P/A: Presence/Absence.
Table
Table A7. Histopathological features evaluated in the pancreas.
Table A7. Histopathological features evaluated in the pancreas.
FeaturesEvaluationDescription
InflammationP/A 1Interstitial and/or periductal aggregates of lymphocytes, plasma cells, and/or histiocytes
1 P/A: Presence/Absence.
Table
Table A8. Histopathological features evaluated in the spleen.
Table A8. Histopathological features evaluated in the spleen.
FeaturesEvaluationDescription
White pulp hyperplasiaP/A 1Prominent lymphoid follicles with increased numbers of lymphocytes/blasts
Perifollicular PMs 2P/AAggregates of neutrophils and/or eosinophils around the lymphoid follicles
1 P/A: Presence/Absence. 2 PMs: Polymorphonuclear leukocytes.
Table
Table A9. Histopathological features evaluated in the adrenal gland.
Table A9. Histopathological features evaluated in the adrenal gland.
FeaturesEvaluationDescription
Cortical hyperplasiaP/A 1Thickened adrenal cortex
LocalizationFascicular
Reticular
Both
Cortical inflammationP/AAggregates of lymphocytes, plasma cells, histiocytes, and/or neutrophils in the cortex
1 P/A: Presence/absence.
Table
Table A10. Histopathological features evaluated in the thyroid gland.
Table A10. Histopathological features evaluated in the thyroid gland.
FeaturesEvaluationDescription
InflammationP/A 1Aggregates of lymphocytes, plasma cells, and/or histiocytes in the interstitium
Follicular cells hyperplasiaP/AIncreased numbers of follicular cells
Follicular cells hypertrophyP/AIncreased size of follicular cells
C cells hyperplasia/hypertrophyP/AIncreased number and/or size of C cells
1 P/A: Presence/absence.
Table
Table A11. Histopathological features evaluated in the thymus.
Table A11. Histopathological features evaluated in the thymus.
FeaturesEvaluationDescription
Germinal centersP/A 1Presence of conspicuous germinal centers in >80% of the follicles
Degree of involution0No involution: Well-formed follicles.
1Mild involution: Smaller follicles.
2Moderate involution: Smaller follicles with fat-filled areas between them.
3Severe/total involution: Rare thymic remnants
1 P/A: Presence/absence.

Appendix E

Table
Table A12. Body weight (W) along the experiment in Control, Adjuvant-only, and Vaccine groups in each of the four flocks individually (Flock 1–4) and all flocks grouped together (All Flocks). Data represented as mean and standard deviation (SD).
Table A12. Body weight (W) along the experiment in Control, Adjuvant-only, and Vaccine groups in each of the four flocks individually (Flock 1–4) and all flocks grouped together (All Flocks). Data represented as mean and standard deviation (SD).
GroupFlock 1Flock 2Flock 3Flock 4All Flocks
n = 21n = 21n = 17n = 19n = 78
MeanSDpMeanSDpMeanSDpMeanSDpMeanSDp
W1Control31.683.70.942
KW		38.263.40.381
A		38.302.70.956
A		38.612.20.857
A		36.594.20.611
A
Adjuvant31.284.637.714.438.083.438.032.636.144.7
Vaccine31.833.440.744.838.673.938.782.637.415.0
W2Control43.694.60.965
A		45.934.20.433
A		49.802.10.839
A		50.292.70.856
A		47.244.40.709
A
Adjuvant43.164.943.573.249.254.650.084.746.275.2
Vaccine43.662.946.144.648.503.651.173.247.184.4
W3Control49.955.20.524
KW		51.435.70.677
A		48.103.00.535
A		53.293.30.865
A		50.894.60.885
A
Adjuvant49.334.449.794.948.833.654.085.850.434.9
Vaccine49.283.452.436.146.424.452.585.250.235.2
W4Control53.396.10.66
A		55.004.90.408
A		52.502.70.805
A		48.145.50.708
A		52.245.50.499
A
Adjuvant53.654.952.214.953.174.346.255.951.445.6
Vaccine55.694.256.297.051.505.448.915.653.326.1
W5Control54.226.50.622
A		58.004.40.672
A		56.001.70.994
KW		52.364.20.839
A		55.084.90.736
A
Adjuvant54.544.154.935.356.255.751.255.654.285.2
Vaccine52.193.256.508.756.006.350.834.653.926.2
W6Control57.767.20.660
KW		61.434.20.52
A		59.104.60.714
A		54.295.90.833
A		58.076.00.465
KW
Adjuvant58.015.858.644.859.257.452.836.157.276.2
Vaccine57.314.457.868.356.258.052.336.156.066.8
W7Control59.437.60.915
KW		60.934.80.462
A		60.005.60.488
A		56.795.90.744
A		59.236.00.242
KW
Adjuvant57.896.958.144.459.006.155.677.157.75.9
Vaccine58.575.956.938.255.258.454.006.656.317.1
W8Control63.017.00.992
A		66.715.30.416
A		62.403.00.433
A		64.367.90.887
A		64.256.10.355
A
Adjuvant62.577.061.936.661.336.962.671062.137.4
Vaccine62.856.063.368.158.085.962.176.561.736.6
W9Control66.217.40.468
KW		69.866.30.366
A		66.503.80.423
A		67.649.10.705
A		67.636.90.158
A
Adjuvant64.957.064.646.464.678.065.429.264.917.2
Vaccine64.857.665.648.460.927.963.587.563.867.6
KW: Kruskal–Wallis test. A: ANOVA.

Appendix F

Table
Table A13. Average daily gain (ADG) between weighing dates (W) along the experiment in Control, Adjuvant-only, and Vaccine groups in each of the four flocks individually (Flocks 1–4) and all flocks grouped together (All Flocks). Data represented as mean and standard deviation (SD).
Table A13. Average daily gain (ADG) between weighing dates (W) along the experiment in Control, Adjuvant-only, and Vaccine groups in each of the four flocks individually (Flocks 1–4) and all flocks grouped together (All Flocks). Data represented as mean and standard deviation (SD).
GroupFlock 1Flock 2Flock 3Flock 4All Flocks
n = 21n = 21n = 17n = 19n = 78
MeanSDpMeanSDpMeanSDpMeanSDpMeanSDp
ADG1
(W2–W1)		Control273450.982
A		145780.394
A		209640.472
A		216590.898
A		211760.719
A
Adjuvant2704411146203252234320172
Vaccine2693510252179352294819477
ADG2
(W3–W2)		Control116280.763
A		95380.772
KW		−31900.715
A		60220.189
A		67690.227
KW
Adjuvant1142310736−86580597666
Vaccine1044310878−394428545581
ADG3
(W4–W3)		Control72530.164
KW		87460.605
A		88700.865
A		−95 ab570.023
A*		34960.288
KW
Adjuvant904359708739−145 a2227107
Vaccine13488948210248−68 b4269102
ADG4
(W5–W4)		Control13 a570.020
KW*		48 a280.049
KW*		74350.528
KW		84 ab450.055
A#		53 a500.045
KW*
Adjuvant14 a2143 a286643100 a1854 a42
Vaccine−56 b693 b46964338 b5417b76
ADG5
(W6–W5)		Control79920.610
KW		78 a260.011
A*		69870.270
KW		45640.928
A		67680.146
A
Adjuvant774884 a34676237326746
Vaccine1149931 b3566935444876
ADG6
(W7–W6)		Control43530.205
KW		−13270.827
A		23610.451
A		60530.675
A		29540.384
A
Adjuvant−357−1354−65567581061
Vaccine32102−2324−25654056671
ADG7
(W8–W7)		Control64320.608
A		98310.435
KW		38660.962
A		120730.897
A		83580.589
A
Adjuvant845164663742111897465
Vaccine7621109264552130289044
ADG8
(W9–W7)		Control103530.522
KW		92800.838
A		100810.792
KW		94760.662
A		97680.372
A
Adjuvant776080528138791547981
Vaccine65716799695840746174
Global
ADG
(W9–W1)		Control91150.913
A		81 a140.045
A*		71110.229
A		74240.759
KW		80 a180.072
A#
Adjuvant891369 ab116718701974 ab17
Vaccine872364 b115614631668 b20
A: ANOVA. KW: Kruskal–Wallis test. a,b: Statistically significant differences between groups based on post hoc test. *: Statistical significance (p < 0.05). #: Statistical tendency (p ≤ 0.1)

Appendix G

Table
Table A14. Hematological results along the experiment in Control, Adjuvant-only, and Vaccine groups (n = 26 each) of all Flocks grouped together. Data represented as mean and standard deviation (SD). H: Hematology date. A reference threshold is provided at the end of the Table.
Table A14. Hematological results along the experiment in Control, Adjuvant-only, and Vaccine groups (n = 26 each) of all Flocks grouped together. Data represented as mean and standard deviation (SD). H: Hematology date. A reference threshold is provided at the end of the Table.
GroupWBC 1
(×103/mm3)		RBC 2
(×106/mm3)		Hematocrit
(%)		Hemoglobin
(g/dl)		Platelets
(×103/mm3)
MeanSDMeanSDMeanSDMeanSDMeanSD
H1Control7.431.8811.560.9735.523.0111.721.04666145
Adjuvant7.602.3111.650.8735.092.9512.150.99616183
Vaccine7.641.8611.180.7434.532.5711.650.69631157
H2Control7.701.8910.930.9534.292.7611.320.93601223
Adjuvant8.672.5411.140.6434.422.8011.720.83618233
Vaccine7.561.3111.200.8835.212.7711.711.00602215
H3Control7.281.4811.081.1334.963.6011.061.22552197
Adjuvant7.952.8010.960.9534.242.9311.041.02525198
Vaccine7.461.9811.310.7635.682.8011.280.78521139
H4Control8.692.0310.470.9332.493.0110.550.95458156
Adjuvant8.411.8710.610.7132.622.1810.580.73469146
Vaccine8.221.6210.510.7432.512.3810.530.77460118
H5Control7.701.4610.720.9533.503.2710.560.75680338
Adjuvant8.061.9410.800.7733.382.7610.770.82672379
Vaccine7.401.5610.790.9033.593.1510.700.90776385
H6Control6.871.7010.791.7734.645.0710.851.58622290
Adjuvant7.662.3710.971.6234.704.9311.101.60645398
Vaccine6.962.0610.941.3135.114.4211.031.14667316
H7Control7.292.5010.031.7132.585.2610.641.62396128
Adjuvant8.132.1410.401.1733.573.6011.041.21363242
Vaccine6.881.529.941.5532.334.4410.561.35462153
H8Control7.651.9010.361.5734.405.1411.181.29638368
Adjuvant8.111.8010.670.9735.023.3811.700.77524292
Vaccine7.532.1910.191.2733.704.5611.081.11553312
H9Control8.082.3110.401.6134.724.8611.041.68469140
Adjuvant8.422.1810.570.9734.713.7111.081.11477210
Vaccine8.032.3910.571.0135.023.3311.041.01461132
H10Control8.352.7110.411.4234.955.1010.891.36357122
Adjuvant8.101.9110.451.5734.513.9710.781.17437191
Vaccine8.491.9810.891.5836.104.5111.131.22425152
H11Control9.602.519.801.1832.673.9210.581.31370129
Adjuvant8.951.6210.141.2133.203.4310.581.25385134
Vaccine9.563.009.830.9832.492.6410.420.90382151
H12Control7.632.1810.071.7032.975.4910.091.76496171
Adjuvant7.831.6010.481.0333.713.2810.471.03447192
Vaccine7.321.2310.400.9633.692.9810.390.94476171
Reference
Treshold		4–129–1428–408–15250–750
1 WBC: White blood cell count. 2 RBC: Red blood cell count

Appendix H

Table
Table A15. Histopathological findings in the peripheral nervous system in Control, Adjuvant-only and Vaccine groups of all Flocks grouped together. Data provided as animals with the referred histological lesion relative to the total number of animals analyzed. Methodology of histopathological evaluation is detailed in Table A3, Table A4, Table A5, Table A6, Table A7, Table A8, Table A9, Table A10 and Table A11 (Appendix D).
Table A15. Histopathological findings in the peripheral nervous system in Control, Adjuvant-only and Vaccine groups of all Flocks grouped together. Data provided as animals with the referred histological lesion relative to the total number of animals analyzed. Methodology of histopathological evaluation is detailed in Table A3, Table A4, Table A5, Table A6, Table A7, Table A8, Table A9, Table A10 and Table A11 (Appendix D).
LocationGroupPerivascular CuffingInflammation
PresencePresence
Subcutaneous thoracic nerveControl16/241/25
Adjuvant15/261/26
Vaccine17/252/26
p0.706 Xi0.790 LR
Sciatic nerveControl12/251/26
Adjuvant14/260/26
Vaccine16/260/26
p0.622 Xi0.320 LR
Tibial nerveControl11/261/26
Adjuvant15/261/26
Vaccine12/261/26
p0.513 Xi1000 LR
Radial nerveControl15/241/24
Adjuvant13/260/26
Vaccine13/230/23
p0.672 Xi0.324 LR
Xi: Pearson’s chi square test. LR: Likelihood ratio test.

Appendix I

Histopathological results in liver, kidney, spleen, adrenal gland, thyroid gland, and thymus of Control, Adjuvant-only, and Vaccine groups of all Flocks grouped together. Data provided as animals with the referred histological lesion relative to the total number of animals analyzed. Methodology of histopathological evaluation is detailed in Table A3, Table A4, Table A5, Table A6, Table A7, Table A8, Table A9, Table A10 and Table A11 (Appendix D).
Table
Table A16. Histopathological findings in the liver.
Table A16. Histopathological findings in the liver.
LocationGroupPortal/Periportal
Inflammation		Hepatocytes
PresenceTypeDegenerationNecrosisAtrophy
LP 1LP + E 2
LiverControl9/268/91/913/261/2614/26
Adjuvant12/266/126/1215/261/269/26
Vaccine12/269/123/1210/260/2612/26
p0.62 LR0.13 LR0.377 Xi0.439 LR0.374 Xi
1 LP: Lymphoplasmacytic. 2 LP + E: Lymphoplasmacytic and eosinophilic. LR: Likelihood ratio test. Xi: Pearson’s chi square test.
Table
Table A17. Histopathological findings in the kidney.
Table A17. Histopathological findings in the kidney.
LocationGroupGlomeruliTubulesInterstitiumMedulla
ProteinDegenerationHyaline DropletsInflammationMineralization
KidneyControl15/262/2610/268/2610/26
Adjuvant16/262/269/2611/2610/26
Vaccine15/264/2612/2610/269/26
p0.948 Xi0.589 LR0.687 Xi0.681 Xi0.947 Xi
Xi: Pearson’s chi square test. LR: Likelihood ratio test.
Table
Table A18. Histopathological findings in the spleen.
Table A18. Histopathological findings in the spleen.
LocationGroupWhite Pulp HyperplasiaPerifollilular PMs 1
SpleenControl11/2624/26
Adjuvant12/2625/26
Vaccine10/2623/26
p0.854 Xi0.568 LR
1 PMs: Polymorphonuclear leukocytes (i.e., neutrophils, eosinophils). Xi: Pearson’s chi square test. LR: Likelihood ratio test.
Table
Table A19. Histopathological findings in the adrenal gland.
Table A19. Histopathological findings in the adrenal gland.
LocationGroupCortical HyperplasiaInflammation
PresenceLocalizationPresence
FascicularReticularBoth
Adrenal GlandControl13/264/121/127/124/26
Adjuvant15/267/153/155/155/26
Vaccine18/269/181/188/188/26
p0.365 Xi0.558 LR0.376 Xi
Xi: Pearson’s chi square test. LR: Likelihood ratio test.
Table
Table A20. Histopathological findings in the thyroid gland.
Table A20. Histopathological findings in the thyroid gland.
LocationGroupInflammationFollicular Cells
Hyperplasia		Follicular Cells
Hypertrophy		C Cells
Hypertrophy
Thyroid GlandControl8/2616/260/264/26
Adjuvant11/2615/263/264/26
Vaccine4/2613/263/267/26
p0.102 Xi0.694 Xi0.078 LR#0.489 LR
Xi: Pearson’s chi square test. LR: Likelihood ratio test. #: Statistical tendency (p ≤ 0.1).
Table
Table A21. Histopathological findings in the thymus.
Table A21. Histopathological findings in the thymus.
LocationGroupGerminal CentersDegree of Involution
0123
ThymusControl4/2613/2510/250/252/25
Adjuvant1/269/2616/260/261/26
Vaccine0/2611/2611/260/264/26
p0.043 LR*0.364 LR
LR: Likelihood ratio test. *: Statistical significance (p < 0.05).

References

  1. Greenwood, B. The contribution of vaccination to global health: Past, present and future. Philos. Trans. R. Soc. B Biol. Sci. 2014, 369. [Google Scholar] [CrossRef] [Green Version]
  2. Lacasta, D.; Ferrer, L.M.; Ramos, J.J.; González, J.M.; Ortín, A.; Fthenakis, G.C. Vaccination schedules in small ruminant farms. Vet. Microbiol. 2015, 181, 34–46. [Google Scholar] [CrossRef]
  3. Morens, D.M.; Folkers, G.K.; Fauci, A.S. The challenge of emerging and re-emerging infectious diseases. Nature 2004, 430, 242–249. [Google Scholar] [CrossRef]
  4. UE Commission Decision 2008/655/EC, 24 July 2008, Approving the Emergency Vaccination Plans Against Bluetongue of Certain Member States and Fixing the Level of the Community’s Financial Contribution for 2007 and 2008. Available online: https://eur-lex.europa.eu/legal-content/EN/TXT/PDF/?uri=CELEX:32008D0655&from=EN (accessed on 16 November 2020).
  5. Mellor, P.S.; Carpenter, S.; Harrup, L.; Baylis, M.; Mertens, P.P.C. Bluetongue in Europe and the Mediterranean Basin: History of occurrence prior to 2006. Prev. Vet. Med. 2008, 87, 4–20. [Google Scholar] [CrossRef] [PubMed]
  6. Agence Française de Sécurité Sanitaire (AFSS) Review of Adverse Affects Observed after Vaccination Against Bluetongue, Serotype 1 and Serotype 8, as of 31/05/2009. Available online: https://www.anses.fr/en/system/files/ANMV-Fi-VaccinFCOEN.pdf (accessed on 16 November 2020).
  7. Nusinovici, S.; Seegers, H.; Joly, A.; Beaudeau, F.; Fourichon, C. A side effect of decreased fertility associated with vaccination against bluetongue virus serotype 8 in Holstein dairy cows. Prev. Vet. Med. 2011, 101, 42–50. [Google Scholar] [CrossRef]
  8. Dyer, F.; Brown, E.; Cooles, S.; Tait, A. Suspected adverse reactions, 2008. Vet. Rec. 2009, 165, 162–164. [Google Scholar] [CrossRef] [PubMed]
  9. González, J.M.; Figueras, L.; Ortega, M.E.; Lozano, M.; Ruiz De Arcaute, M.; Royo, R.; Cebrián, L.M.; Ferrer, L.M.; Fariñas, F.; De Jalón, J.A.G.; et al. Possible adverse reactions in sheep after vaccination with inactivated BTV vaccines. Vet. Rec. 2010, 166, 757–758. [Google Scholar] [CrossRef]
  10. Asín, J.; Pérez, M.; Pinczowski, P.; Gimeno, M.; Luján, L. From the bluetongue vaccination campaigns in sheep to overimmunization and ovine ASIA syndrome. Immunol. Res. 2018, 66, 777–782. [Google Scholar] [CrossRef] [PubMed]
  11. Luján, L.; Pérez, M.; Salazar, E.; Álvarez, N.; Gimeno, M.; Pinczowski, P.; Irusta, S.; Santamaría, J.; Insausti, N.; Cortés, Y.; et al. Autoimmune/autoinflammatory syndrome induced by adjuvants (ASIA syndrome) in commercial sheep. Immunol. Res. 2013, 56, 317–324. [Google Scholar] [CrossRef]
  12. Shoenfeld, Y.; Agmon-Levin, N. “ASIA”—Autoimmune/inflammatory syndrome induced by adjuvants. J. Autoimmun. 2011, 36, 4–8. [Google Scholar] [CrossRef]
  13. Burakova, Y.; Madera, R.; McVey, S.; Schlup, J.R.; Shi, J. Adjuvants for Animal Vaccines. Viral Immunol. 2017, 31, 11–22. [Google Scholar] [CrossRef] [PubMed]
  14. Shardlow, E.; Mold, M.; Exley, C. Unraveling the enigma: Elucidating the relationship between the physicochemical properties of aluminium-based adjuvants and their immunological mechanisms of action. Allergy Asthma Clin. Immunol. 2018, 14, 80. [Google Scholar] [CrossRef] [PubMed]
  15. Asín, J.; Molín, J.; Pérez, M.; Pinczowski, P.; Gimeno, M.; Navascués, N.; Muniesa, A.; de Blas, I.; Lacasta, D.; Fernández, A.; et al. Granulomas Following Subcutaneous Injection With Aluminum Adjuvant-Containing Products in Sheep. Vet. Pathol. 2019, 56, 418–428. [Google Scholar] [CrossRef] [PubMed] [Green Version]
  16. de Miguel, R.; Asín, J.; Rodríguez-Largo, A.; Molín, J.; Echeverría, I.; de Andrés, D.; Pérez, M.; de Blas, I.; Mold, M.; Reina, R.; et al. Detection of aluminum in lumbar spinal cord of sheep subcutaneously inoculated with aluminum-hydroxide containing products. J. Inorg. Biochem. 2020, 204, 110871. [Google Scholar] [CrossRef] [PubMed]
  17. Asín, J.; Pascual-Alonso, M.; Pinczowski, P.; Gimeno, M.; Pérez, M.; Muniesa, A.; de Pablo-Maiso, L.; de Blas, I.; Lacasta, D.; Fernández, A.; et al. Cognition and behavior in sheep repetitively inoculated with aluminum adjuvant-containing vaccines or aluminum adjuvant only. J. Inorg. Biochem. 2020, 203. [Google Scholar] [CrossRef] [PubMed]
  18. Vandevelde, M.; Higgins, R.J.; Oevermann, A. Veterinary Neuropathology: Essentials of Theory and Practice; John Wiley & Sons, Ltd.: Oxford, UK, 2012. [Google Scholar]
  19. Cerviño, M.; Figueras, L.; Martín, S.; Elvira, L.; Callus, M.; Dowlut, S.; Engelhard, I.; Calvo, E.; Makoschey, B. Specific humoral response and effect on rectal temperature of two clostridial vaccines in lambs. Vet. Rec. 2011, 168. [Google Scholar] [CrossRef]
  20. Troxel, T.R.; Gadberry, M.S.; Wallace, W.T.; Kreider, D.L.; Shockey, J.D.; Colburn, E.A.; Widel, P.; Nicholson, I. Clostridial antibody response from injection-site lesions in beef cattle, long-term response to single or multiple doses, and response in newborn beef calves. J. Anim. Sci. 2001, 79, 2558. [Google Scholar] [CrossRef]
  21. Silva, G.M.; Poore, M.H.; Ranches, J.; Moriel, P. Effects of timing of vaccination relative to weaning and post-weaning frequency of energy supplementation on growth and immunity of beef calves1. J. Anim. Sci. 2018, 96, 318–330. [Google Scholar] [CrossRef] [Green Version]
  22. Arthington, J.D.; Cooke, R.F.; Maddock, T.D.; Araujo, D.B.; Moriel, P.; Dilorenzo, N.; Lamb, G.C. Effects of vaccination on the acute-phase protein response and measures of performance in growing beef calves1. J. Anim. Sci. 2013, 91, 1831–1837. [Google Scholar] [CrossRef]
  23. Moriel, P.; Arthington, J.D. Metabolizable protein supply modulated the acute-phase response following vaccination of beef steers. J. Anim. Sci. 2013, 91, 5838–5847. [Google Scholar] [CrossRef]
  24. Reeds, P.J.; Jahoor, F. The amino acid requirements of disease. Clin. Nutr. 2001, 20, 15–22. [Google Scholar] [CrossRef]
  25. Arts, R.J.W.; Carvalho, A.; La Rocca, C.; Palma, C.; Rodrigues, F.; Silvestre, R.; Kleinnijenhuis, J.; Lachmandas, E.; Gonçalves, L.G.; Belinha, A.; et al. Immunometabolic Pathways in BCG-Induced Trained Immunity. Cell Rep. 2016, 17, 2562–2571. [Google Scholar] [CrossRef] [PubMed] [Green Version]
  26. O’Neill, L.A.J.; Kishton, R.J.; Rathmell, J. A guide to immunometabolism for immunologists. Nat. Rev. Immunol. 2016, 16, 553–565. [Google Scholar] [CrossRef] [PubMed] [Green Version]
  27. Macías-Cruz, U.; Stevens, J.C.; Correa-Calderón, A.; Mellado, M.; Meza-Herrera, C.A.; Avendaño-Reyes, L. Effects of pre-lambing maternal energy supplementation on post-weaning productive performance and thermoregulatory capacity of heat-stressed male lambs. J. Therm. Biol. 2018, 75, 7–12. [Google Scholar] [CrossRef]
  28. Al-Dawood, A. Towards heat stress management in small Ruminants—A review. Ann. Anim. Sci. 2017, 17, 59–88. [Google Scholar] [CrossRef] [Green Version]
  29. Varela-Martínez, E.; Abendaño, N.; Asín, J.; Sistiaga-Poveda, M.; Pérez, M.M.; Reina, R.; de Andrés, D.; Luján, L.; Jugo, B.M. Molecular Signature of Aluminum Hydroxide Adjuvant in Ovine PBMCs by Integrated mRNA and microRNA Transcriptome Sequencing. Front. Immunol. 2018, 9, 2406. [Google Scholar] [CrossRef]
  30. Henry, B.A.; Pope, M.; Birtwistle, M.; Loughnan, R.; Alagal, R.; Fuller-Jackson, J.P.; Perry, V.; Budge, H.; Clarke, I.J.; Symonds, M.E. Ontogeny and thermogenic role for sternal fat in female sheep. Endocrinology 2017, 158, 2212–2225. [Google Scholar] [CrossRef] [Green Version]
  31. Kherani, Z.S.; Auer, R.N. Pharmacologic analysis of the mechanism of dark neuron production in cerebral cortex. Acta Neuropathol. 2008, 116, 447–452. [Google Scholar] [CrossRef] [Green Version]
  32. Zimatkin, S.M.; Bon, E.I. Dark Neurons of the Brain. Neurosci. Behav. Physiol. 2018, 48, 908–912. [Google Scholar] [CrossRef]
  33. Garman, R.H. Histology of the Central Nervous System. Toxicol. Pathol. 2011, 39, 22–35. [Google Scholar] [CrossRef]
  34. Jortner, B.S. The return of the dark neuron. A histological artifact complicating contemporary neurotoxicologic evaluation. Neurotoxicology 2006, 27, 628–634. [Google Scholar] [CrossRef] [PubMed]
  35. Varela-Martínez, E.; Bilbao-Arribas, M.; Abendaño, N.; Asín, J.; Pérez, M.; de Andrés, D.; Luján, L.; Jugo, B.M. Whole transcriptome approach to evaluate the effect of aluminium hydroxide in ovine encephalon. Sci. Rep. 2020, 10, 15240. [Google Scholar] [CrossRef] [PubMed]
  36. Goto, N.; Ueno, G.; Iwasa, S. Swelling Reaction of the Pancreas in Guinea Pigs Caused by Aluminum-Adsorbed Diphtheria-Purified Pertussis-Tetanus Combined Vaccine. Microbiol. Immunol. 1987, 31, 89–93. [Google Scholar] [CrossRef] [PubMed] [Green Version]
  37. AEMET OpenData—State Meteorological Agency—AEMET—Spanish Government. Available online: http://www.aemet.es/en/datos_abiertos/AEMET_OpenData (accessed on 4 December 2020).
Animals 11 00146 g001 550
Figure 1. Global inoculation schedule. Each injection date is indicated by a vertical line and a number (mean value of dpi of the four flocks). W: Weight measurement. E: Clinical examination. H: Hematological analysis. Information on the injection and vaccines number, season, and month is also provided. Inoculation schedule for each individual flock is provided in Figure A1 (Appendix B). Information about the vaccines used is presented in Table A2 (Appendix C).
Figure 1. Global inoculation schedule. Each injection date is indicated by a vertical line and a number (mean value of dpi of the four flocks). W: Weight measurement. E: Clinical examination. H: Hematological analysis. Information on the injection and vaccines number, season, and month is also provided. Inoculation schedule for each individual flock is provided in Figure A1 (Appendix B). Information about the vaccines used is presented in Table A2 (Appendix C).
Animals 11 00146 g001
Animals 11 00146 g002 550
Figure 2. Global average daily gain (ADG) along the experiment in Control (green), Adjuvant-only (yellow), and Vaccine groups (red), both in each individual flock and in all flocks grouped together (All Flocks). Data represented as mean and Standard Error. *: statistical significance (p < 0.05); #: statistical tendency (p ≤ 0.1).
Figure 2. Global average daily gain (ADG) along the experiment in Control (green), Adjuvant-only (yellow), and Vaccine groups (red), both in each individual flock and in all flocks grouped together (All Flocks). Data represented as mean and Standard Error. *: statistical significance (p < 0.05); #: statistical tendency (p ≤ 0.1).
Animals 11 00146 g002
Table
Table 1. Characteristics of the lambs and flocks used in the experiment.
Table 1. Characteristics of the lambs and flocks used in the experiment.
FlockBreedManagementShepherding
1Rasa Aragonesa purebred Experimental farmNo
2Rasa Aragonesa × Romanov crossbredIntensiveNo
3Rasa Aragonesa × Romanov crossbredExtensiveYes
4Rasa Aragonesa purebredExtensiveYes
Table
Table 2. Fattening index and sternal fat deposits in Control, Adjuvant-only, and Vaccine groups (n = 26 each) when all flocks were considered together. Data represented as mean, standard deviation (SD), and interquartile rank (IQR).
Table 2. Fattening index and sternal fat deposits in Control, Adjuvant-only, and Vaccine groups (n = 26 each) when all flocks were considered together. Data represented as mean, standard deviation (SD), and interquartile rank (IQR).
GroupFattening IndexSternal Fat Deposits
MeanSDIQRpMeanSDIQRp
Control2.830.172.80–3.00 a 3.740.383.50–4.00 a
Adjuvant-only2.710.312.60–3.00 a 3.580.703.00–4.27 ab
Vaccine2.520.382.30–2.80 b0.003 KW*3.320.523.00–3.50 b0.008 KW*
a,b: Statistically significant differences between groups based on post hoc test. KW: Kruskal–Wallis test. *: Statistically significant (p < 0.05).
Table
Table 3. Histopathological findings in the central nervous system in Control, Adjuvant-only (Adjuvant), and Vaccine groups (n = 26 each) of all flocks grouped together. Data provided as animals with the referred histological lesion relative to the total number of animals analyzed. Methodology of histopathological evaluation is detailed in Table A3, Table A4, Table A5, Table A6, Table A7, Table A8, Table A9, Table A10 and Table A11 (Appendix D).
Table 3. Histopathological findings in the central nervous system in Control, Adjuvant-only (Adjuvant), and Vaccine groups (n = 26 each) of all flocks grouped together. Data provided as animals with the referred histological lesion relative to the total number of animals analyzed. Methodology of histopathological evaluation is detailed in Table A3, Table A4, Table A5, Table A6, Table A7, Table A8, Table A9, Table A10 and Table A11 (Appendix D).
LocationGroupPerivascular
Cuffing		MeningitisGlial NodulesMicroglial
Activation 		Dark
Neurons
Frontal cortex and Caudate nucleusControl8/260/2619/266/2622/26
Adjuvant10/262/2619/264/2623/25
Vaccine7/262/2614/262/2622/26
p0.662 Xi0.187 LR0.236 Xi0.239 LR0.645 LR
Parietal cortexControl7/261/263/266/2621/26
Adjuvant6/262/262/264/2622/26
Vaccine2/262/262/263/2622/26
p0.177 Xi0.808 Xi0.859 LR0.528 LR0.913 LR
Thalamus and
Hippothalamus 		Control8/260/263/267/2624/26
Adjuvant4/260/261/2612/2625/26
Vaccine7/261/264/2611/2624/26
p0.495 Xi0.329 LR0.335 LR0.311 LR0.793 LR
Cervical spinal cordControl3/262/261/260/269/26
Adjuvant2/261/260/260/2612/26
Vaccine1/260/260/260/2611/26
p0.568 LR0.240 LR0.329 LR-0.690 Xi
Thoracic spinal cordControl0/260/260/260/2617/26
Adjuvant1/260/260/260/2616/26
Vaccine0/260/260/260/2610/26
p0.329 LR---0.108 Xi
Lumbar spinal cordControl1/260/260/2624/2613/26
Adjuvant1/260/261/2625/2620/26
Vaccine0/260/260/2624/2614/26
p0.439 LR-0.329 LR0.793 LR0.100 Xi#
Xi: Pearson’s chi square test. LR: Likelihood ratio test. #: Statistical tendency (p ≤ 0.1).
Table
Table 4. Inflammation (i.e., interstitial and/or periductal aggregates of lymphocytes, plasma cells, and/or histiocytes) in the pancreas in Control, Adjuvant-only (Adjuvant), and Vaccine groups (n = 26 each) of all flocks grouped together. Data provided as animals with the histological lesion relative to the total number of animals analyzed. Methodology of histopathological evaluation detailed in Table A3, Table A4, Table A5, Table A6, Table A7, Table A8, Table A9, Table A10 and Table A11 (Appendix D).
Table 4. Inflammation (i.e., interstitial and/or periductal aggregates of lymphocytes, plasma cells, and/or histiocytes) in the pancreas in Control, Adjuvant-only (Adjuvant), and Vaccine groups (n = 26 each) of all flocks grouped together. Data provided as animals with the histological lesion relative to the total number of animals analyzed. Methodology of histopathological evaluation detailed in Table A3, Table A4, Table A5, Table A6, Table A7, Table A8, Table A9, Table A10 and Table A11 (Appendix D).
ControlAdjuvantVaccinep
Inflammation1/268/262/260.012 LR*
LR: Likelihood ratio test. *: Statistical significance (p < 0.05).
Publisher’s Note: MDPI stays neutral with regard to jurisdictional claims in published maps and institutional affiliations.

Share and Cite

MDPI and ACS Style

de Miguel, R.; Asín, J.; Rodríguez-Largo, A.; Echeverría, I.; Lacasta, D.; Pinczowski, P.; Gimeno, M.; Molín, J.; Fernández, A.; de Blas, I.; et al. Growth Performance and Clinicopathological Analyses in Lambs Repetitively Inoculated with Aluminum-Hydroxide Containing Vaccines or Aluminum-Hydroxide Only. Animals 2021, 11, 146. https://doi.org/10.3390/ani11010146

AMA Style

de Miguel R, Asín J, Rodríguez-Largo A, Echeverría I, Lacasta D, Pinczowski P, Gimeno M, Molín J, Fernández A, de Blas I, et al. Growth Performance and Clinicopathological Analyses in Lambs Repetitively Inoculated with Aluminum-Hydroxide Containing Vaccines or Aluminum-Hydroxide Only. Animals. 2021; 11(1):146. https://doi.org/10.3390/ani11010146

Chicago/Turabian Style

de Miguel, Ricardo, Javier Asín, Ana Rodríguez-Largo, Irache Echeverría, Delia Lacasta, Pedro Pinczowski, Marina Gimeno, Jéssica Molín, Antonio Fernández, Ignacio de Blas, and et al. 2021. "Growth Performance and Clinicopathological Analyses in Lambs Repetitively Inoculated with Aluminum-Hydroxide Containing Vaccines or Aluminum-Hydroxide Only" Animals 11, no. 1: 146. https://doi.org/10.3390/ani11010146

APA Style

de Miguel, R., Asín, J., Rodríguez-Largo, A., Echeverría, I., Lacasta, D., Pinczowski, P., Gimeno, M., Molín, J., Fernández, A., de Blas, I., de Andrés, D., Pérez, M., Reina, R., & Luján, L. (2021). Growth Performance and Clinicopathological Analyses in Lambs Repetitively Inoculated with Aluminum-Hydroxide Containing Vaccines or Aluminum-Hydroxide Only. Animals, 11(1), 146. https://doi.org/10.3390/ani11010146

Note that from the first issue of 2016, this journal uses article numbers instead of page numbers. See further details here.

Article Metrics

Back to TopTop