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The effect of intermittent hypoxia under different temperature on the immunomodulation in Streptococcus agalactiae vaccinated Nile tilapia (Oreochromis niloticus)
Accepted Manuscript The effect of intermittent hypoxia under different temperature on the immunomodulation in Streptococcus agalactiae vaccinated Nile tilapia (Oreochromis niloticus) Jing Wang, Dan-Qi Lu, Biao Jiang, Heng-Li Luo, Ge-Ling Lu, An-Xing Li PII:
S1050-4648(18)30225-0
DOI:
10.1016/j.fsi.2018.04.040
Reference:
YFSIM 5256
To appear in:
Fish and Shellfish Immunology
Received Date: 22 November 2017 Revised Date:
16 March 2018
Accepted Date: 19 April 2018
Please cite this article as: Wang J, Lu D-Q, Jiang B, Luo H-L, Lu G-L, Li A-X, The effect of intermittent hypoxia under different temperature on the immunomodulation in Streptococcus agalactiae vaccinated Nile tilapia (Oreochromis niloticus), Fish and Shellfish Immunology (2018), doi: 10.1016/ j.fsi.2018.04.040. This is a PDF file of an unedited manuscript that has been accepted for publication. As a service to our customers we are providing this early version of the manuscript. The manuscript will undergo copyediting, typesetting, and review of the resulting proof before it is published in its final form. Please note that during the production process errors may be discovered which could affect the content, and all legal disclaimers that apply to the journal pertain.
ACCEPTED MANUSCRIPT
The effect of intermittent hypoxia under different temperature on the
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immunomodulation in Streptococcus agalactiae vaccinated Nile tilapia
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(Oreochromis niloticus)
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Jing Wang a, Dan-Qi Lu a, Biao Jiang a, Heng-Li Luo a, Ge-Ling Lu a, An-Xing Li a, b,
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*
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a
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Aquatic Economic Animals, School of Life Sciences, Sun Yat-Sen University,
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Guangzhou 510275, Guangdong Province, PR China;
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b
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State Key Laboratory of Biocontrol/Guangdong Provincial Key Laboratory for
Laboratory for Marine Fisheries Science and Food Production Processes, Qingdao
National Laboratory for Marine Science and Technology, Qingdao 266235, Shandong
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Province, PR China.
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*Corresponding author: An-Xing Li, State Key Laboratory of Biocontrol/Guangdong
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Provincial Key Laboratory for Aquatic Economic Animals, School of Life Sciences,
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Sun Yat-Sen University, 135 Xingang West Street, Haizhu District, Guangzhou
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510275, Guangdong Province, PR China.
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E–mail address: [email protected] (A.-X. Li)
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ABSTRACT Dissolved oxygen (DO) and temperature are the potential immunomodulators in
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fish and play the important roles in regulating immunity. We studied the effect of
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intermittent hypoxia under different temperature on the immunomodulation in
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vaccinated Nile tilapia (Oreochromis niloticus). The expression of immune-related
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genes, enzymatic activities, histology, cumulative mortality, and S. agalactiae
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clearance were assessed. Study conditions were intermittently hypoxic (4.0 ± 1.0
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mg/L DO) at 30 ± 0.5°C or 35 ± 0.5°C. Interleukin-1beta (IL-1β), tumor necrosis
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factor alpha (TNF-α) and gamma interferon (IFN-γ) mRNA expression in spleen and
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head kidney were significantly lower in vaccinated hypoxic fish compared to the
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vaccinated normoxic fish. Levels of heat shock protein 70 (HSP70) in tissues showed
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an opposite tendency. Superoxide dismutase (SOD), catalase (CAT) and glutathione
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peroxidase (GSH-Px) activities were significantly lower in vaccinated hypoxic fish.
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Malondialdehyde levels were significantly greater under hypoxic conditions. In vitro
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studies evaluated the effects of intermittent hypoxia at different temperatures on cells
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of vaccinated O. niloticus. Phagocytic activity of peripheral blood leucocytes (PBLs)
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and intracellular reactive oxygen species (ROS) production in head kidney cells were
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significantly decreased by intermittent hypoxia at either 30°C or 35°C, while nitric
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oxide levels in tissues cells increased significantly under hypoxic conditions. These
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changes were well reflected by the further suppression modulation on S. agalactiae
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clearance in vaccinated O. niloticus and higher cumulative mortality by intermittent
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hypoxia. Taken together, intermittent hypoxia at either 30°C or 35°C could suppress
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immunomodulation in vaccinated Nile tilapia.
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Keywords: Streptococcus; Intermittent hypoxia; Temperature; Vaccination; Challenge;
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Nile tilapia
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1. Introduction Streptococcus agalactiae is a common pathogen that causes septicemia,
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meningoencephalitis, exophthalmia, anorexia and ascites in many fish species [1, 2].
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High mortality rates caused by S. agalactiae have caused significant economic losses,
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and it has become a major problem in the aquaculture industry, especially in Nile
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tilapia (Oreochromis niloticus) [3–5]. Though S. agalactiae strains isolated from fish
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in China have been found that are resistant to penicillin, ceftriaxone and clindamycin,
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the misuse of antibiotics could provoke the selection of antibiotic resistant bacteria,
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and increased the risk to the environment and human health [6, 7]. Therefore,
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vaccines are considered a promising approach to prevent bacterial diseases, including
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streptococcosis, in fish [8, 9]. Over these years, attempts were made to control
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diseases by immunization, and it has been demonstrated that vaccination can
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effectively prevent S. agalactiae infection [10–12].
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The immune response in fish is regulated by several factors, including
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administration route, endogenous factors and exogenous factors, such as stocking
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densities, pH, salinities, temperature, dissolved oxygen and water quality [13–16].
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Among these factors, dissolved oxygen (DO) level and temperature are especially
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important because they are closely related to disease outbreaks [17–21]. Previous
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studies have found that the innate immunity and specific antibody titer decreased as
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DO level decreased when fish exposed to pathogenic Edwardsiella ictaluri,
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Aeromonas hydrophila or S. agalactiae [22–24]. In addition, the immune response
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and tolerance to various pathogens can also be lowered by temperatures [25]. Most
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outbreaks of streptococcosis in tilapia farms occur during warm months when water
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temperatures were above 26°C [26]. Though S. Gallage et al. (2017) [24] had reported
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that cumulative mortality of vaccinated fish under moderate hypoxia was significantly
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higher than vaccinated fish under normoxic conditions, the water temperature was
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designed at 25 ± 0.5 °C during the study, which is lower than the sensitive
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temperature of S. agalactiae. In fact, high water temperature and/or intermittent
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hypoxia usually occur during the hot months in tilapia farms, and these conditions
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ACCEPTED MANUSCRIPT have some effect on growth performance and innate immunity in fish [20,23].
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However, recent studies were mainly focused on investigating the impact of high
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temperature stress on Nile tilapia infected by S. agalactiae [18, 27] or the impact of
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moderate hypoxia on immunomodulation in vaccinated tilapia at normal temperature
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(~25 °C) [24]. There is little information about the influence of temperature and DO
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on the immunomodulation in S. agalactiae vaccinated Nile tilapia, including high
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temperature with normal oxygen, high temperature with intermittent hypoxia, or
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intermittent hypoxia under different temperature conditions.
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This study is focused on assessing the immunomodulation of S. agalactiae
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vaccinated Nile tilapia under intermittent hypoxia at different temperature conditions
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by testing the expression profile of immune-related genes, enzymatic activities, cell
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abilities, histology, cumulative mortality and S. agalactiae clearance. By discussing
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the possible impact of intermittent hypoxia under different temperature on vaccinated
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tilapia, reminding people the water environment should be attention in vaccinated fish
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and making the vaccine efficacy optimize against S. agalactiae.
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2. Materials and methods
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2.1. The fish and bacterial strain
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Tilapia (Oreochromis niloticus) juveniles were obtained from the Panyu Tilapia
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Breeding Farm of Guangdong Province (China) and transported to the laboratory,
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where they were reared in 1,000 L circulating tanks with constant aeration and a 29 ±
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1°C water temperature. They were acclimatized for 30 d and fed twice daily with
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commercial feed (Guangdong Evergreen Feed Industry Co., Ltd, China). Before
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experiment initiation, all tested fish were confirmed to be S. agalactiae-free following
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bacteriological examination. Approval was obtained from the Animal Ethics
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Committee of the Life Science Institute prior to using the animals for research.
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S. agalactiae strain THN0901 (serotype Ia) was preserved in our lab. THN0901
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was isolated from an intensive tilapia farm with a typical streptococcosis outbreak in
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the Hainan province of China in 2009. Strain THN0901 has been demonstrated to be a
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fatal pathogen of tilapia [28].
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2.2. Vaccine preparation This work was performed by Yongshun Biological Pharmaceutical Co., Ltd
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(Guangzhou China). Briefly, S. agalactiae (THN0901) strains were cultured on
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brain-heart infusion (BHI) agar culture-medium and incubated at 37 °C for 24 h.
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Propagation of bacteria was then done by inoculating into brain-heart infusion broth
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(BHIB) and incubated in shaker bath at 180 rpm at 28 °C for 12 h, and then overnight
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cultured cell were diluted into 1:100 in BHIB medium. The cultured cells were grown
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until the early stationary phase (10h) and harvested centrifugation at 10,000×g for 10
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min at 4 °C. The cell pellet was washed repeatedly with phosphate buffered saline
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(PBS) and then re-suspended with 0.4% buffered formalin overnight at 4°C for
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inactivation. The formalin-killed bacteria were washed and then re-suspended in
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sterile PBS. The suspension was streaked on BHI agar and incubated for 24 h at 30°C
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to ensure that all S. agalactiae cells were killed and there was no contamination.
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Finally, 70 % white oil adjuvant (Yongshun, Guangdong, China) was added to
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improve the immune response and the final inactivated bacterial concentration was
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3×109 CFU/ml. The prepared inactivation vaccine was stored at -4°C until use.
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2.3. Experimental design and sample collection
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The experiment was conducted during August to September in 2017. Intermittent
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hypoxia with flow-through fresh water was delivered at either 30 ± 0.5°C or 35 ±
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0.5°C. A total of 720 Nile tilapia juveniles (mean weight = 20.0 ± 3.0 g) were selected
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for this study. They were acclimatized 14 d to intermittent hypoxic (4.0 ± 1.0 mg/L
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DO) or normoxic (8.0 ± 0.5 mg/L DO) conditions. The rearing water temperature was
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adjusted concurrently. The intermittent hypoxic groups were treated from 7:00-11:00
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am and 18:00-22:00 pm daily. During the other times of the day, oxygen was
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administrated like the normoxic groups. Dissolved oxygen in tanks was adjusted by
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manipulating aeration and injecting N2 into the tanks through aerators connected with
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and temperature in each tank were measured three times per day using an oxygen
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meter (JPB-70A, China). The pH was 6.8 ± 0.3 and nitrite was less than 0.5 mg/L.
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The selected fish were divided evenly into twenty-four floating glass tanks (30
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fish/tank), and there were eight treatments in triplicate. The four control groups were
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administrated intraperitoneally with 100 µl PBS, and the other four treatment groups
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were administrated intraperitoneally with 100 µl of prepared vaccine at 0 d (the day
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when we immunized the fish was defined as day 0). The eight groups were
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administrated as follows, 30°C + normoxic (No.) + PBS, 30°C + No. + vaccination
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(Vac.), 30°C + intermittent hypoxic (In. Hy.) + PBS, 30°C + In. Hy. + Vac., 35°C +
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No. + PBS, 35°C + No. + Vac., 35°C + In. Hy. + PBS, 35°C + In. Hy. + Vac.. The
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fish were fed with commercial dry feed (Evergreen, Guangdong, China) twice daily
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and feeding was discontinued 24 h before vaccination, challenge or sampling.
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Fish (n = 3) were sampled randomly from each experiment group at different
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sampling points for different purpose. After anesthetization with MS-222, spleen and
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head kidney samples were collected at 48 h post-vaccination from each group for the
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determination of immune-related gene expression. Organ samples were separated
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immediately under sterile operation and stored in a Sample Protector for RNA/DNA
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(Takara, Dalian, China) at -80°C until RNA extraction. Peripheral blood, spleens,
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head kidneys and distal intestine were collected at 28 d post-vaccination. The serum
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of peripheral blood without heparin was isolated by centrifugation (4000 rpm, 10 min)
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for use in determining serum superoxide dismutase (SOD), catalase (CAT),
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glutathione peroxidase (GSH-Px) activities and malondialdehyde (MDA) levels.
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Peripheral blood mixed with precooled heparin for use leukocytes isolation. The
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peripheral blood leukocytes (PBLs) were isolated immediately for measuring
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phagocytic activity. The primary spleen cells and primary head kidney cells were
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isolated immediately from spleens and head kidneys at 28 d post-vaccination for
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measuring respiratory burst response and nitric oxide response. Distal intestine and
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head kidneys were obtained at 28 d post-vaccination and were fixed in 4%
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paraformaldehyde at least 24 h for use histology observation.
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2.4. Expression of immune-related genes Total RNA from collected organs was extracted using TRIzol reagent (Takara)
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and the nucleic acid quality was measured by agarose gel electrophoresis, and the
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concentration was determined by the absorbance at 260 nm using a Nanodrop
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ND-2000 spectrophotometer (Quawell Technology Inc., San Jose, CA, USA). cDNA
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was then synthesized from 1 µg total RNA using a PrimeScript RT reagent Kit with
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gDNA Eraser (Takara). All cDNA samples were preserved at -20°C until quantitative
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PCR was processed.
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Real-time Quantitative PCR (RT-qPCR) for analysis of gene expression was
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conducted in a LightCycler 480 Real Time System (Roche, Switzerland) with SYBR
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Green Real-time PCR MasterMix (Takara). The relative expression levels of four
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immune-related genes including interleukin-1beta (IL-1β), tumor necrosis factor alpha
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(TNF-α), gamma interferon (IFN-γ) and heat shock protein 70 (HSP70) in spleen and
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head kidney were examined with RT-qPCR, while β-actin, a housekeeping gene, was
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chosen as an internal standard. All qPCR primers were designed using the software of
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Beacon Designer 17.0 software based on the gene sequences in GenBank and are
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listed in Table 1. The PCR cycles was conducted at 95°C for 30 s, followed by 40
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cycles, each consisting of at 95°C for 5 s, and 60°C for 30 s. Each sample was run in
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triplicate. Additionally, dissociation-curve analysis was performed and showed a
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single peak in all cases. The relative expression was analyzed using the 2
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method according to Livak and Schmittgen [29].
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2.5. Non–specific immune parameters assay
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SOD, CAT, GSH-Px activities and MDA content in serum were measured using
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assay kits (Nanjing Jiancheng Ins., China) according to the manufacturer’s
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instructions. Details of the procedures were described by the previous methods [30–
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32].
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2.6. Phagocytosis activity, respiratory burst and nitric oxide assay
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2.6.1. Isolation of PBLs, spleen and head kidney cells Peripheral blood was collected and PBLs were isolated immediately as described
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by Ding et al. (2012) [33]. Briefly, the blood was diluted with an equal volume of
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RPMI 1640 (GE, USA) medium. The suspension was transferred to the surface of
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Ficoll-Paque PLUS (GE, USA) with a pipette, then isolated by centrifugation at 1600
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rpm for 45 min at 19°C. PBLs collected at the interphase between the first and second
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gradient interfaces. Then cells were removed and washed by resuspension five times
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with equal volumes of RPMI 1640. The leucocytes were then resuspended with tissue
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culture medium (TCM), which was prepared from RPMI 1640 medium supplemented
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with 10% fetal bovine serum (FBS) (Sigma, St. Louis, MO, USA) and 1%
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streptomycin/penicillin (Sigma). The quality and quantity of isolated leucocytes were
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tested using a cell counter (Cellometer AUTO 1000, USA) and then adjusted to 1 ×
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10 6 cells/ml for using to phagocytosis activity analysis.
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Primary spleen cells and primary head kidney cells were obtained from tilapia as
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previously described by Peng et al. (2016) [34]. The spleens and head kidneys of
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individual fish were aseptically removed and immediately placed in TCM. The
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spleens and head kidneys were then ground into pieces with 180 °C-treated frosted
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glass slides in TCM and were filtered through a 100-µm cell strainer. The obtained
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cells were washed with RPMI 1640 twice, and resuspended in TCM. The quality and
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quantity of cells were tested as above for use in respiratory burst response and nitric
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oxide response.
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2.6.2. Phagocytosis activity
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S. agalactiae strain (THN0901) was killed as described in 2.2. Inactivated bacteria
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(1 × 109 CFU/ml) were resuspended with TCM. The bacteria were incubated 1 h with
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1 mg/ml fluorescein isothiocyanate (FITC) at 30°C. After washing five times with
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RPMI 1640, 200 µl FITC-bacteria were added into the prepared PBLs (800 µl, 1 × 10
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min and washed three time with RPMI 1640. The precipitate was incubated 5 min
cells/ml) and cultured 1 h at 28°C. Then they were centrifuged at 500 rpm for 10
ACCEPTED MANUSCRIPT with 1 ml 0.125% trypan blue to quench extracellular fluorescence. After washing
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three times with PBS, the precipitate resuspended with 0.9% NaCl. The phagocytosis
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activity of resuspended PBLs was analyzed by flow cytometry (FCM) (FC500, USA).
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Side-scatter (SSC) and forward-scatter (FSC) parameters were used to determine cell
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granularity and cell size, respectively.
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2.6.3. Respiratory burst assay
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Intracellular superoxide production was measured using a nitro blue tetrazolium
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assay (NBT assay) as described by Peng et al. (2016) [34]. Briefly, primary spleen
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cells and primary head kidney cells were isolated from three fish of each group
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respectively. A 100 µl amount of cells suspension was immediately seeded into
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96-well transparent plates at a density of 1 × 106 cells/ml. The plate was incubated for
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5 min and then centrifuged at 1500 rpm for 5 min at room temperature. The
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supernatant was replaced immediately with 100 µl PBS + 100 µl NBT (2 mg/ml,
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Sigma), 100 µl inactive S. agalactiae (1 × 109 CFU/ml) + 100 µl NBT, and 100 µl
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phorbol ester (PMA) (100 ng/ml, Sigma) + 100 µl NBT, respectively. The production
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in NBT caused by cells alone was used as a base line. The ROS production caused by
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PMA was used as the positive control. At the end of the 1 h incubation at room
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temperature, the non-reduced NBT was removed using 70% methanol. The cell button
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was air dried and the reduced NBT was dissolved using 120 µl KOH (2 M). A total of
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140 µl DMSO (Sigma) was added to dissolve the blue crystals that had formed in the
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cytoplasm. Then the OD values were read at 630 nm using a microplate reader
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(TECAN infinite M200 Pro Nanoquant, Swizerland).
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2.6.4. Nitric oxide assay
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Primary spleen cells and primary head kidney cells were isolated immediately
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from three fish of each group respectively as described in 2.6.1. Nitrite concentration
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in tissue cells was measured as an indicator of NO production according to the Griess
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reaction using a NO determination kit (Beyotime, Jiangsu, China) as described by Bai
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96-well transparent plates at a density of 1 × 106 cells/ml. Then they were mixed with
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50 µl Griess reagent Ι and 50 µl Griess reagent ΙΙ, and then the absorbance was read at
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550 nm using a microplate reader (TECAN, Swizerland).
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2.7. Distal intestine and head kidney histology
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The sections of tissues were made according to standard histological techniques as
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described by Su et al. (2017) [36]. Fixed samples of the distal intestine and head
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kidney were routinely dehydrated in ethanol, equilibrated in xylene and embedded in
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paraffin, and cut into 4 µm thick sections on a rotary microtome RM2135 (Leica,
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Wetzlar, Germany). The sections were stained with hematoxylin and eosin (HE) for
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histology observation. Blinded evaluation of the histological samples was performed
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using an optical microscope DFC495.
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2.8. Experimental challenge
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S. agalactiae (THN0901) strain was cultured as described in 2.2. The median
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lethal dose (LD50) in a challenge test was determined from a preliminary experiment
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(data not shown). The final bacterial concentrations were confirmed by plating
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ten-fold serial dilutions onto BHI agar medium.
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Fish (n=16) from each tank were infected by intraperitoneal injection with live S.
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agalactiae (THN0901, 2×107 CFU/fish) and returned to their original treatment tanks
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at 29 d following vaccination. 384 fish were used with 48 per group (triplicate tanks).
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Mortality was recorded for 14 d after challenge and cumulative mortality was
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statistically calculated. Additionally, the re-isolation of the S. agalactiae strain from
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all dead fish was confirmed. The relative percentage survival (RPS) was calculated
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using the following formula:
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RPS = [1 − (%Mortality in vaccinated group/%mortality in control group)] × 100
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2.9. Clearance of S. agalactiae
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Gallage et al. (2017) [24]. Briefly, fish (n=3) were randomly sampled to collect blood,
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spleen, head kidney and brain samples from each experimental group at 1 d and 3 d
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post-challenge. After anesthetization with MS-222, blood was collected from the
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caudal vein using a 1 ml sterile syringe, mixed with precooled heparin to prevent
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clotting and kept on ice. Spleen, head kidney and brain were aseptically removed and
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immediately placed in 5 ml RPMI 1640 medium RPMI 1640 without antibiotic
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supplement. Samples were kept on ice until use for bacteria re-isolation.
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A 500 µl sample of heparinized blood was added to 500 µl of distilled water to
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disrupt the cells and release any surviving bacteria within the cells. The suspension
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was serially diluted in PBS. A 100 µl sample of each dilution was plated on BHI and
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incubated at 37°C for 24 h prior to CFU determination. CFU was expressed as mean
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CFU (n=3 from each group at each sampling point) and the bacteria count was given
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as CFU/ml of blood. Spleen, head kidneys and brains (100 mg from each) were
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ground into pieces and serially diluted in PBS, separately. A 100 µl sample of each
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dilution was plated on BHI and incubated at 37°C for 24 h, CFU were calculated as
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above.
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The CFU /ml of blood = No. of CFU counted on plate × dilution factor
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The CFU /g of tissue = No. of CFU counted on plate × dilution factor
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2.10.
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Statistical analysis
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Each group in the present experiment was performed in triplicate. Data were
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expressed as means ± SD. The significant values were calculated using ANOVA and
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Ducan’s test by SPSS 19.0 (IBM, USA). The results were considered as significant at
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p < 0.05.
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3. Results
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3.1. Expression of immune-related genes
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In both tissues, the expression levels of IL-1β, TNF-α, IFN-γ, and HSP70 were all
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significantly up-regulated (p < 0.05) in vaccinated fish compared to non-vaccinated
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fish at 48 h post-vaccination at either 30°C or 35°C. In the spleen (Fig. 1), IL-1β (Fig. 1 A), TNF-α (Fig. 1 B) and IFN-γ (Fig. 1 C)
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mRNA levels were all significantly down-regulated (p < 0.05) in vaccinated hypoxic
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fish compared to vaccinated normoxic fish at either 30°C or 35°C. However, HSP70
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(Fig. 1 D) mRNA levels in vaccinated hypoxic groups were significantly up-regulated
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(p < 0.05) compared to vaccinated normoxic fish at both temperatures. In the head
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kidney (Fig. 2), the expression levels of IL-1β (Fig. 2 A), TNF-α (Fig. 2 B), IFN-γ
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(Fig. 2 C) and HSP70 (Fig. 2 D) were similar to the expression levels in spleen.
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3.2. Non–specific immune parameters assay
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The SOD, CAT, GSH-Px activities and MDA content in the serum of each group
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at 28 d post-vaccination were studied. Fig. 3 shows that SOD (Fig. 3 A), CAT (Fig. 3
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B), GSH-Px (Fig. 3 C) activities were significantly higher (p < 0.05) in the
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vaccination groups than the non-vaccination groups. At 30°C or 35°C, SOD (Fig 3 A),
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CAT (Fig 3 B) and GSH-Px (Fig. 3 C) activities in vaccinated fish maintained under
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hypoxic conditions decreased significantly (p < 0.05) compared to vaccinated fish
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under normoxic conditions. MDA (Fig. 3 D) content increased significantly (p < 0.05)
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in hypoxic fish, and no significant differences (p < 0.05) were found between
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vaccinated hypoxic group and non-vaccinated hypoxic group at either 30°C or 35°C.
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3.3. Phagocytosis activity
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To elucidate the possible impact of intermittent hypoxia at different temperatures
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on cells of the vaccinated fish, phagocytic activity was subsequently determined by
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flow cytometry at 28 d post-vaccination. Fig. 4 A showed that PBLs with
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FITC-bacteria were gated (P) on forward and side scatter (FS-SS) do plot, Q
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demonstrated the bacteria distribution (no showed). Phagocytic percentages from
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histograms (Fig. 4 A30 – D35) were statistically calculated and showed by bar graph
ACCEPTED MANUSCRIPT (Fig. 4 B). Fig. 4 B shows that the phagocytic percentage of PBLs towards S.
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agalactiae increased significantly (p < 0.05) in the vaccination groups compared to
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the PBS groups. The phagocytic capacity of PBLs decreased significantly (p < 0.05)
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in the intermittent hypoxic and vaccinated groups compared to normoxic and
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vaccinated groups at 30°C or 35°C.
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3.4. Respiratory burst assay
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The effects of S. agalactiae on ROS production in tilapia primary spleen cells and
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head kidney cells are shown in Fig. 5. In primary spleen cells, a significantly lower (p
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< 0.05) ROS production was observed in vaccinated hypoxic fish compared to
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vaccinated normoxic fish caused by S. agalactiae at 35°C (Fig. 5 B), but significant
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differences were not found between these two groups at 30°C (Fig. 5 A). In primary
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head kidney cells, a significant decrease (p < 0.05) was found in vaccinated hypoxic
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fish compared to vaccinated normoxic fish caused by S. agalactiae at either 30°C (Fig.
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5 C) or 35°C (Fig. 5 D).
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3.5. Nitric oxide assay
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The possibility that intermittent hypoxia under different temperature induced the
334
changes of nitric oxide levels was investigated in primary spleen cells and head
335
kidney cells. Tilapia spleen and head kidney cells were stimulated with S. agalactiae.
336
Nitric oxide levels in spleen cells and head kidney cells are shown in Fig, 6 A and Fig.
337
6 B, respectively. In both tissue cells, nitric oxide levels increased significantly (p <
338
0.05) in vaccinated hypoxic fish compared to vaccinated normoxic fish at either 30°C
339
or 35°C.
340
3.6. Distal intestine and head kidney histology
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341
The results of HE staining in distal intestine and head kidney of vaccinated fish
342
under different DO and temperature conditions at 28 d post-vaccination show in Fig.7
343
(the tissue sections of non-vaccinated fish under different conditions do not showed
ACCEPTED MANUSCRIPT here because no significant differences were found between vaccinated fish and
345
non-vaccinated fish under the same treatment). In distal intestine, villus showed some
346
degree of shedding in vaccinated hypoxic fish at 30°C (Fig. 7 In-B) and 35°C (Fig. 7
347
In-D) compared to vaccinated normoxic fish at 30°C (Fig. 7 In-A) and 35°C (Fig. 7
348
In-C). In head kidney, intercellular hyperplasia and healthy red cells decreasing were
349
found in vaccinated hypoxic fish at 30°C (Fig. 7 HK-B) and 35°C (Fig. 7 HK-D)
350
compared to vaccinated normoxic fish at 30°C (Fig. 7 HK-A) and 35°C (Fig. 7 HK-C).
351
Furthermore, substantial hemosiderin was found in vaccinated normoxic fish and
352
vaccinated hypoxic fish in head kidney at 35°C.
353
3.7. Cumulative mortality following challenge
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To assess the protective efficacy of vaccine in vaccinated fish under different
355
temperature and dissolved oxygen conditions, tilapias were separately immunized
356
with PBS and inactivation S. agalactiae vaccine on day 0, and then challenged with S.
357
agalactiae on day 29. Fig. 8 shows the percentage cumulative mortality of tilapia.
358
Tilapia mortalities occurred in large quantities from 1 to 7 d post-challenge, and
359
vaccinated fish had a significantly lower (p < 0.05) cumulative mortality compared to
360
non-vaccinated fish. The final mortality of each group was 54.17 ± 2.95 % (30°C
361
normoxic control), 10.42 ± 2.95 % (30°C normoxic vaccinated), 58.33 ± 5.89 %
362
(30 °C intermittent hypoxic control), 14.58 ± 2.95 % (30 °C intermittent hypoxic
363
vaccinated), 68.75 ± 5.10 % (35°C normoxic control), 18.75 ± 5.10 % (35°C
364
normoxic vaccinated), 72.92 ± 5.89 % (35°C intermittent hypoxic control) and 27.08
365
± 2.95 % (35°C intermittent hypoxic vaccinated), respectively. The RPSs of normoxic
366
vaccinated fish at 30°C, intermittent hypoxic vaccinated fish at 30°C, normoxic
367
vaccinated fish at 35°C and intermittent hypoxic vaccinated fish at 35°C compared to
368
the PBS groups were 81.02 ± 4.58%, 75 ± 4.08%, 72.32 ± 8.20% and 62.47 ± 6.05%,
369
respectively.
370
3.8. Clearance of S. agalactiae in blood, spleen, head kidney and brain
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ACCEPTED MANUSCRIPT During the challenge period, the overall bacterial burden was significantly higher
372
(p < 0.05) in the PBS groups compared to the vaccination groups (Table 2). In blood,
373
culturable S. agalactiae cells were not detected in vaccinated fish at 3 d
374
post-challenge. At 1 d post-challenge, the bacterial burdens in vaccinated fish spleen
375
and head kidney were significantly higher (p < 0.05) in hypoxic groups compared to
376
normoxic groups either at 30°C or 35°C. Furthermore, spleen in non-vaccinated fish
377
kept under 35°C and hypoxic condition contained the highest bacterial burden at 1 d
378
post-challenge.
379
4. Discussion
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Both temperature and DO at the time of vaccination are recognized as important
381
factors in the development of protective immunity in ectothermic vertebrates [18, 22,
382
24]. To address the potential role of intermittent hypoxia at different temperatures on
383
immune adjustment in vaccinated Nile tilapia, in vivo and in vitro experiments were
384
studied. The present study showed that IL-1β, TNF-α and IFN-γ mRNA levels were
385
all strongly down-regulated in vaccinated hypoxic fish at either 30°C or 35°C. This
386
suggests that intermittent hypoxia at either 30°C or 35°C may have an inhibitory
387
effect on the expression of important pro-inflammatory genes (IL-1β, TNF-α and
388
IFN-γ). These results are also supported by recent studies, demonstrating that IL-1β
389
transcription decreases in response to acute hypoxia in Nile tilapia [37] and long-term
390
hypoxia either reduces or delays the expression of IL-1β, TNF-α and IFN-γ genes in
391
Atlantic salmon (Salmo salar L.) [38].The modulated effects by inhibitory
392
immune-related genes were further detected in primary cells from tilapia peripheral
393
blood, spleen and head kidney, including restraining phagocytosis, respiratory burst
394
activities and enhancement of nitric oxide production in vaccinated hypoxic fish at
395
both temperatures in the present study. These changes in vitro are closely related to
396
the functions of pro-inflammatory cytokines because IL-1β can increase yeast
397
phagocytosis by recruiting and proliferating head kidney leukocytes [39], TNF-α can
398
result in priming of the respiratory burst of the peritoneal exudate and head kidney
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ACCEPTED MANUSCRIPT leukocytes [40], and stimulation of peripheral blood leukocytes with IFN-γ-related
400
protein resulted in the activation of IFN-γ receptor and marked induction of inducible
401
nitric oxide synthase gene expression [41], so these three immune-related genes could
402
lead to changes in phagocytosis, respiratory burst and nitric oxide production by
403
above ways. Additionally, HSP70, a member of the HSP protein family, has powerful
404
immune regulatory effects [42, 43]. Under stress such as hypoxia, the anti-apoptosis
405
and synergetic immunity of HSP70 can be strengthened in order to protect cells from
406
environmental stressors [44, 45], this may be the reason why HSP70 mRNA levels
407
were strongly up-regulated in vaccinated hypoxic fish at both temperatures in present
408
study.
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In non-specific immune system, oxygen consumption is necessary to maintain the
410
NADPH oxidase level in phagocytes in order to activate biochemical reactions that
411
generate ROS [46]. SOD, CAT and GSH-Px, as important antioxidants, play vital
412
roles on transferring ROS for protecting membranes and DNA from damage [47,48].
413
However, teleost fish have a low capacity for regulation of internal levels of dissolved
414
oxygen or temperature by adjusting their physiological, biological mechanisms or
415
behavior [49]. When fish are under hypoxic conditions, the immune system may
416
experience a similar phenomenon because their functions may be affected by the level
417
of hypoxia [24]. Furthermore, substantial hemosiderosis were found in head kidney of
418
vaccinated fish at 35°C in present study. Hemosiderin often forms after hemorrhage.
419
When blood leaves a ruptured blood vessel, the red blood cell dies and the
420
hemoglobin of the cell is released into the extracellular space [50]. In this study,
421
excessive hemosiderin to accumulate may be for red blood cell destruction under
422
hypoxic and high temperature condition. This suggests that the ability of transporting
423
oxygen by red blood cells could be weakened in vaccinated fish under these
424
conditions. Therefore, the activities of SOD, CAT and GSH-Px may be weak driven
425
by lower dissolved oxygen level and/or high temperature. Meanwhile, as the
426
breakdown product of lipid peroxides, increasing MDA content due to hypoxia may
427
have strong cytotoxicity [51]. These negative effects could further suppress the
428
phagocytic activity in cells of the immune system.
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ACCEPTED MANUSCRIPT The pathogen clearance study demonstrated that a higher blood and tissue
430
bacterial burden was present in vaccinated fish under hypoxic conditions. This may
431
relate to the lower phagocytic capacity and ineffective vaccine absorption. The villus
432
showed shedding in vaccinated hypoxic fish in the present study and this can directly
433
affect the absorption of hindgut to antigen, which had been found that the main site of
434
antigen absorption was in hindgut in the study of teleost [52]. Furthermore, a higher
435
percentage of cumulative mortality also indicates that fish were not getting the
436
expected level of protection from vaccination when vaccinated fish kept at
437
intermittent hypoxic under different temperature condition, and the suppression
438
modulation by intermittent hypoxia under different temperature may affect local as
439
well as systemic immunoreaction.
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In conclusion, our findings indicate that intermittent hypoxia at either 30°C or
441
35°C could suppress immune response in vaccinated Nile tilapia. The occurrence of
442
intermittent hypoxia under different temperatures helps to explain why fish are not
443
getting the expected level of protection from vaccination.
444
Acknowledgments
The Oceanic and Fishery Adminictration of Guangdong Province (2015, 2016).
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This work was funded by Special Science Projects for Fish Diseases Control from
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ACCEPTED MANUSCRIPT Table 1 Primers used for RT-PCR analysis. Primer sequence
Source
Product (bp)
β-actin-F β-actin-R IL-1β-F IL-1β-R HSP70-F HSP70-R TNF-α-F TNF-α-R IFN-γ-F IFN-γ-R
5΄-TCCATTGGCCTTCGTTGC-3΄ 5΄-CTATTCTGTGTGACCCAGG-3΄ 5΄-ATTGTCGTCCTGTCTATC-3΄ 5΄-AATGTCATCATGGTATTGC-3΄ 5΄-ACCATCACCAACGATAAG-3΄ 5΄-CGGCTTTGTATTTCTCTG-3΄ 5΄-CTGTAGTCACCTCCATTA-3΄ 5΄-TACTTGTTGTTGCTTCTG-3΄ 5΄-CAGCAGAGATGAACTTGA-3΄ 5΄-CACTAGGAAATACGGGTTT-3΄
EF206801
163
GBAY01004231
126
FJ207463
length
RI PT
Primer name
232
121
KF294754
128
SC
GAID01031494
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EP
TE D
M AN U
Abbreviations- IL-1β: interleukin-1beta; HSP70: heat shock protein 70; TNF-α: tumor necrosis factor alpha; IFN-γ: gamma interferon.
ACCEPTED MANUSCRIPT Table 2 Streptococcus agalactiae burden in blood, spleen, head kidney and brain of tilapia at 1 and 3 days (D) post-challenge. Experimental groups
30 °C Blood (CFU/ml) 35 °C
0.92×102 b
0b
4.0 ± 1.0 mg/L DO Con.
10.23×108 a
7.11×105 a
4.0 ± 1.0 mg/L DO Vac.
2.83×102 b
0b
8.0 ± 0.5 mg/L DO Con.
11.36×108 a'
6.48×105 a'
8.0 ± 0.5 mg/L DO Vac.
1.97×102 b'
0 b'
4.0 ± 1.0 mg/L DO Con.
10.41×108 a'
5.64×105 a'
3.38×102 b'
0 b'
5.58×1010 a
5.74×106 a
30 °C
Brain (CFU/g)
35 °C
M AN U
8.0 ± 0.5 mg/L DO Vac.
2.86×103 b
1.12×103 b
4.0 ± 1.0 mg/L DO Con.
8.16×1010 a
9.78×106 a
4.0 ± 1.0 mg/L DO Vac.
1.27×104 c
1.74×104 c
8.0 ± 0.5 mg/L DO Con.
8.24×1010 a'
6.78×106 a'
8.0 ± 0.5 mg/L DO Vac.
2.32×104 b'
2.80×103 b'
4.0 ± 1.0 mg/L DO Con.
9.38×1010 a'
6.47×106 a'
4.0 ± 1.0 mg/L DO Vac.
1.14×105 c'
3.12×104 c'
8.0 ± 0.5 mg/L DO Con.
4.34×109 a
1.56×106 a
8.0 ± 0.5 mg/L DO Vac.
8.96×103 b
1.69×103 b
4.0 ± 1.0 mg/L DO Con.
7.86×108 c
5.40×105 c
4.0 ± 1.0 mg/L DO Vac.
9.20×105 d
2.24×103 b
8.0 ± 0.5 mg/L DO Con.
6.72×107 a'
1.01×106 a'
8.0 ± 0.5 mg/L DO Vac.
1.68×105 b'
2.38×103 b'
4.0 ± 1.0 mg/L DO Con.
1.74×107 a'
1.87×106 a'
4.0 ± 1.0 mg/L DO Vac.
1.12×106 c'
4.76×103 b'
8.0 ± 0.5 mg/L DO Con.
2.27×108 a
3.62×106 a
8.0 ± 0.5 mg/L DO Vac.
4.32×102 b
2.86×103 b
4.0 ± 1.0 mg/L DO Con.
2.40×108 a
3.83×106 a
4.0 ± 1.0 mg/L DO Vac.
1.10×103 c
5.38×103 b
8.0 ± 0.5 mg/L DO Con.
4.31×108 a'
4.54×106 a'
8.0 ± 0.5 mg/L DO Vac.
2.12×103 b'
1.61×104 b'
4.0 ± 1.0 mg/L DO Con.
6.06×108 a'
2.22×106 a'
4.0 ± 1.0 mg/L DO Vac.
9.40×103 b'
3.28×104 b'
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3.22×105 a
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Head kidney (CFU/g)
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8.0 ± 0.5 mg/L DO Con.
Spleen (CFU/g)
30 °C
1D
8.0 ± 0.5 mg/L DO Con.
4.0 ± 1.0 mg/L DO Vac. 30 °C
Days post challenge
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Notes: Values are given as CFU/ml of blood or CFU/g of tissues, determined by counting bacteria on a BHI plate. At each sampling date, 3 fish were randomly sampled from each group and bacteria counts are the mean of 3 fish. Different superscript letters indicate significant differences (p < 0.05). a/b/c/d denotes the difference among the groups at 30 °C. a'/b'/c'/d' denotes the difference among the groups at 35 °C. (DO = dissolved oxygen; Con. = control; Vac. = vaccinated)
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Fig. 1. The relative expression of IL-1β (A), TNF-α (B), IFN-γ (C) and HSP70 (D) in spleen of Nile tilapia following vaccination under different oxygen (intermittent hypoxia or normoxia) and rearing water temperature (30 °C or 35 °C) conditions. Bars represent the mean ± SD (n=3). Different superscript letters indicate significant differences (p < 0.05). a/b/c/d denotes the difference among the groups at 30 °C. a'/b'/c'/d' denotes the difference among the groups at 35 °C. (DO = dissolved oxygen; Con. = control; Vac. = vaccinated) IL-1β: interleukin-1beta; TNF-α: tumor necrosis factor alpha; IFN-γ: gamma interferon; HSP70: heat shock protein 70.
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Fig. 2. The relative expression of IL-1β (A), TNF-α (B), IFN-γ (C) and HSP70 (D) in head kidney of Nile tilapia following vaccination under different oxygen (intermittent hypoxia or normoxia) and rearing water temperature (30 °C or 35 °C) conditions. Bars represent the mean ± SD (n=3). Different superscript letters indicate significant differences (p < 0.05). a/b/c/d denotes the difference among the groups at 30 °C. a'/b'/c'/d' denotes the difference among the groups at 35 °C. (DO = dissolved oxygen; Con. = control; Vac. = vaccinated) IL-1β: interleukin-1beta; TNF-α: tumor necrosis factor alpha; IFN-γ: gamma interferon; HSP70: heat shock protein 70.
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Fig. 3. (A) superoxide dismutase (SOD) activity, (B) catalase (CAT) activity, (C) glutathione peroxidase (GSH-Px) activity and (D) malondialdehyde (MDA) levels of Nile tilapia following vaccination under different oxygen (intermittent hypoxia or normoxia) and rearing water temperature (30 °C or 35 °C) conditions. Bars represent the mean ± SD (n=3). Different superscript letters indicate significant differences (p < 0.05). a/b/c/d denotes the difference among the groups at 30 °C. a'/b'/c'/d' denotes the difference among the groups at 35 °C. (DO = dissolved oxygen; Con. = control; Vac. = vaccinated)
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Fig. 4. The phagocytic capacity of PBLs was detected under different oxygen (intermittent hypoxia or normoxia) and rearing water temperature (30 °C or 35 °C) conditions by FCM at 28 d post-vaccination. (A) PBLs with FITC-bacteria were gated (P) on forward and side scatter (FS-SS) do plot, Q demonstrated the bacteria distribution (no showed); (B) Phagocytic percentage were statistically calculated. Histograms showed the phagocytic percentage. Bars represent the mean ± SD (n=3). Different superscript letters indicate significant differences (p < 0.05). a/b/c/d denotes the difference among the groups at 30 °C. a'/b'/c'/d' denotes the difference among the groups at 35 °C. (No. = normoxia; In. Hy. = intermittent hypoxia; Con. = control; Vac. = vaccinated)
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Fig. 5. Respiratory burst activity of Nile tilapia primary spleen cells at 30°C (A) or 35°C (B) and primary head kidney cells at 30°C (C) or 35°C (D) after stimulation with NBT, S. agalactiae and PMA was detected at 28 d post-vaccination. Bars represent the mean ± SD (n=3). Different superscript letters (a, b, c and d) indicate significant differences (p < 0.05). (No. = normoxia; In. Hy. = intermittent hypoxia; Con. = control; Vac. = vaccinated)
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Fig. 6. Nitric oxide production of Nile tilapia primary spleen cells (A) and primary head kidney cells (B) after stimulation with S. agalactiae was detected at 28 d post-vaccination. Bars represent the mean ± SD (n=3). Different superscript letters indicate significant differences (p < 0.05). a/b/c/d denotes the difference among the groups at 30 °C. a'/b'/c'/d' denotes the difference among the groups at 35 °C. (DO = dissolved oxygen; Con. = control; Vac. = vaccinated)
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Fig. 7. Histomorphology of distal intestine (In) and head kidney (HK) in vaccinated Nile tilapia under different oxygen (intermittent hypoxia or normoxia) and rearing water temperature (30 °C or 35 °C) at 28 d post-vaccination. In-A: 30 °C and normoxia; In-B: 30 °C and intermittent hypoxia; In-C: 35 °C and normoxia; In-D: 35 °C and intermittent hypoxia; HK-A: 30 °C and normoxia; HK-B: 30 °C and intermittent hypoxia; HK-C: 35 °C and normoxia; HK-D: 35 °C and intermittent hypoxia. Thickness 4 µm. In bar = 100 µm, HK bar = 50 µm.
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Fig. 8. Cumulative mortality (%) of tilapia was recorded daily for 14 d post intraperitoneal challenge with S. agalactiae THN0901 (2×107 CFU/fish). Tilapia mortalities occurred in large quantities during the first week of the challenge. 384 fish were used with 48 per group. Each value represents mean (n=3) and error bars are omitted for clarity. Different superscript letters indicate significant differences (p < 0.05). a/b/c/d denotes the difference among the groups at 30 °C. a'/b'/c'/d' denotes the difference among the groups at 35 °C. (No. = normoxia; In. Hy. = intermittent hypoxia; Con. = control; Vac. = vaccinated)
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Highlights: Intermittent hypoxia at either 30°C or 35°C modulates immune genes expression. Enzymatic activities were lower in vaccinated hypoxia fish at both temperatures. Phagocytosis and ROS production decreased in vaccinated hypoxia fish.
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Cumulative mortality was higher in vaccinated hypoxia fish. Spleen, head kidney and brain bacteria burden was lower in vaccinated normoxic
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fish.
S1050-4648(18)30225-0
DOI:
10.1016/j.fsi.2018.04.040
Reference:
YFSIM 5256
To appear in:
Fish and Shellfish Immunology
Received Date: 22 November 2017 Revised Date:
16 March 2018
Accepted Date: 19 April 2018
Please cite this article as: Wang J, Lu D-Q, Jiang B, Luo H-L, Lu G-L, Li A-X, The effect of intermittent hypoxia under different temperature on the immunomodulation in Streptococcus agalactiae vaccinated Nile tilapia (Oreochromis niloticus), Fish and Shellfish Immunology (2018), doi: 10.1016/ j.fsi.2018.04.040. This is a PDF file of an unedited manuscript that has been accepted for publication. As a service to our customers we are providing this early version of the manuscript. The manuscript will undergo copyediting, typesetting, and review of the resulting proof before it is published in its final form. Please note that during the production process errors may be discovered which could affect the content, and all legal disclaimers that apply to the journal pertain.
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The effect of intermittent hypoxia under different temperature on the
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immunomodulation in Streptococcus agalactiae vaccinated Nile tilapia
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(Oreochromis niloticus)
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Jing Wang a, Dan-Qi Lu a, Biao Jiang a, Heng-Li Luo a, Ge-Ling Lu a, An-Xing Li a, b,
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*
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a
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Aquatic Economic Animals, School of Life Sciences, Sun Yat-Sen University,
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Guangzhou 510275, Guangdong Province, PR China;
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b
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State Key Laboratory of Biocontrol/Guangdong Provincial Key Laboratory for
Laboratory for Marine Fisheries Science and Food Production Processes, Qingdao
National Laboratory for Marine Science and Technology, Qingdao 266235, Shandong
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Province, PR China.
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*Corresponding author: An-Xing Li, State Key Laboratory of Biocontrol/Guangdong
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Provincial Key Laboratory for Aquatic Economic Animals, School of Life Sciences,
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Sun Yat-Sen University, 135 Xingang West Street, Haizhu District, Guangzhou
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510275, Guangdong Province, PR China.
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E–mail address: [email protected] (A.-X. Li)
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ABSTRACT Dissolved oxygen (DO) and temperature are the potential immunomodulators in
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fish and play the important roles in regulating immunity. We studied the effect of
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intermittent hypoxia under different temperature on the immunomodulation in
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vaccinated Nile tilapia (Oreochromis niloticus). The expression of immune-related
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genes, enzymatic activities, histology, cumulative mortality, and S. agalactiae
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clearance were assessed. Study conditions were intermittently hypoxic (4.0 ± 1.0
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mg/L DO) at 30 ± 0.5°C or 35 ± 0.5°C. Interleukin-1beta (IL-1β), tumor necrosis
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factor alpha (TNF-α) and gamma interferon (IFN-γ) mRNA expression in spleen and
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head kidney were significantly lower in vaccinated hypoxic fish compared to the
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vaccinated normoxic fish. Levels of heat shock protein 70 (HSP70) in tissues showed
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an opposite tendency. Superoxide dismutase (SOD), catalase (CAT) and glutathione
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peroxidase (GSH-Px) activities were significantly lower in vaccinated hypoxic fish.
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Malondialdehyde levels were significantly greater under hypoxic conditions. In vitro
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studies evaluated the effects of intermittent hypoxia at different temperatures on cells
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of vaccinated O. niloticus. Phagocytic activity of peripheral blood leucocytes (PBLs)
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and intracellular reactive oxygen species (ROS) production in head kidney cells were
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significantly decreased by intermittent hypoxia at either 30°C or 35°C, while nitric
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oxide levels in tissues cells increased significantly under hypoxic conditions. These
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changes were well reflected by the further suppression modulation on S. agalactiae
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clearance in vaccinated O. niloticus and higher cumulative mortality by intermittent
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hypoxia. Taken together, intermittent hypoxia at either 30°C or 35°C could suppress
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immunomodulation in vaccinated Nile tilapia.
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Keywords: Streptococcus; Intermittent hypoxia; Temperature; Vaccination; Challenge;
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Nile tilapia
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1. Introduction Streptococcus agalactiae is a common pathogen that causes septicemia,
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meningoencephalitis, exophthalmia, anorexia and ascites in many fish species [1, 2].
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High mortality rates caused by S. agalactiae have caused significant economic losses,
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and it has become a major problem in the aquaculture industry, especially in Nile
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tilapia (Oreochromis niloticus) [3–5]. Though S. agalactiae strains isolated from fish
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in China have been found that are resistant to penicillin, ceftriaxone and clindamycin,
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the misuse of antibiotics could provoke the selection of antibiotic resistant bacteria,
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and increased the risk to the environment and human health [6, 7]. Therefore,
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vaccines are considered a promising approach to prevent bacterial diseases, including
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streptococcosis, in fish [8, 9]. Over these years, attempts were made to control
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diseases by immunization, and it has been demonstrated that vaccination can
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effectively prevent S. agalactiae infection [10–12].
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The immune response in fish is regulated by several factors, including
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administration route, endogenous factors and exogenous factors, such as stocking
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densities, pH, salinities, temperature, dissolved oxygen and water quality [13–16].
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Among these factors, dissolved oxygen (DO) level and temperature are especially
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important because they are closely related to disease outbreaks [17–21]. Previous
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studies have found that the innate immunity and specific antibody titer decreased as
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DO level decreased when fish exposed to pathogenic Edwardsiella ictaluri,
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Aeromonas hydrophila or S. agalactiae [22–24]. In addition, the immune response
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and tolerance to various pathogens can also be lowered by temperatures [25]. Most
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outbreaks of streptococcosis in tilapia farms occur during warm months when water
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temperatures were above 26°C [26]. Though S. Gallage et al. (2017) [24] had reported
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that cumulative mortality of vaccinated fish under moderate hypoxia was significantly
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higher than vaccinated fish under normoxic conditions, the water temperature was
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designed at 25 ± 0.5 °C during the study, which is lower than the sensitive
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temperature of S. agalactiae. In fact, high water temperature and/or intermittent
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hypoxia usually occur during the hot months in tilapia farms, and these conditions
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ACCEPTED MANUSCRIPT have some effect on growth performance and innate immunity in fish [20,23].
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However, recent studies were mainly focused on investigating the impact of high
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temperature stress on Nile tilapia infected by S. agalactiae [18, 27] or the impact of
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moderate hypoxia on immunomodulation in vaccinated tilapia at normal temperature
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(~25 °C) [24]. There is little information about the influence of temperature and DO
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on the immunomodulation in S. agalactiae vaccinated Nile tilapia, including high
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temperature with normal oxygen, high temperature with intermittent hypoxia, or
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intermittent hypoxia under different temperature conditions.
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This study is focused on assessing the immunomodulation of S. agalactiae
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vaccinated Nile tilapia under intermittent hypoxia at different temperature conditions
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by testing the expression profile of immune-related genes, enzymatic activities, cell
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abilities, histology, cumulative mortality and S. agalactiae clearance. By discussing
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the possible impact of intermittent hypoxia under different temperature on vaccinated
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tilapia, reminding people the water environment should be attention in vaccinated fish
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and making the vaccine efficacy optimize against S. agalactiae.
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2. Materials and methods
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2.1. The fish and bacterial strain
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Tilapia (Oreochromis niloticus) juveniles were obtained from the Panyu Tilapia
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Breeding Farm of Guangdong Province (China) and transported to the laboratory,
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where they were reared in 1,000 L circulating tanks with constant aeration and a 29 ±
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1°C water temperature. They were acclimatized for 30 d and fed twice daily with
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commercial feed (Guangdong Evergreen Feed Industry Co., Ltd, China). Before
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experiment initiation, all tested fish were confirmed to be S. agalactiae-free following
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bacteriological examination. Approval was obtained from the Animal Ethics
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Committee of the Life Science Institute prior to using the animals for research.
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S. agalactiae strain THN0901 (serotype Ia) was preserved in our lab. THN0901
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was isolated from an intensive tilapia farm with a typical streptococcosis outbreak in
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the Hainan province of China in 2009. Strain THN0901 has been demonstrated to be a
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fatal pathogen of tilapia [28].
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2.2. Vaccine preparation This work was performed by Yongshun Biological Pharmaceutical Co., Ltd
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(Guangzhou China). Briefly, S. agalactiae (THN0901) strains were cultured on
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brain-heart infusion (BHI) agar culture-medium and incubated at 37 °C for 24 h.
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Propagation of bacteria was then done by inoculating into brain-heart infusion broth
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(BHIB) and incubated in shaker bath at 180 rpm at 28 °C for 12 h, and then overnight
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cultured cell were diluted into 1:100 in BHIB medium. The cultured cells were grown
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until the early stationary phase (10h) and harvested centrifugation at 10,000×g for 10
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min at 4 °C. The cell pellet was washed repeatedly with phosphate buffered saline
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(PBS) and then re-suspended with 0.4% buffered formalin overnight at 4°C for
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inactivation. The formalin-killed bacteria were washed and then re-suspended in
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sterile PBS. The suspension was streaked on BHI agar and incubated for 24 h at 30°C
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to ensure that all S. agalactiae cells were killed and there was no contamination.
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Finally, 70 % white oil adjuvant (Yongshun, Guangdong, China) was added to
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improve the immune response and the final inactivated bacterial concentration was
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3×109 CFU/ml. The prepared inactivation vaccine was stored at -4°C until use.
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2.3. Experimental design and sample collection
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The experiment was conducted during August to September in 2017. Intermittent
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hypoxia with flow-through fresh water was delivered at either 30 ± 0.5°C or 35 ±
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0.5°C. A total of 720 Nile tilapia juveniles (mean weight = 20.0 ± 3.0 g) were selected
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for this study. They were acclimatized 14 d to intermittent hypoxic (4.0 ± 1.0 mg/L
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DO) or normoxic (8.0 ± 0.5 mg/L DO) conditions. The rearing water temperature was
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adjusted concurrently. The intermittent hypoxic groups were treated from 7:00-11:00
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am and 18:00-22:00 pm daily. During the other times of the day, oxygen was
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administrated like the normoxic groups. Dissolved oxygen in tanks was adjusted by
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manipulating aeration and injecting N2 into the tanks through aerators connected with
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and temperature in each tank were measured three times per day using an oxygen
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meter (JPB-70A, China). The pH was 6.8 ± 0.3 and nitrite was less than 0.5 mg/L.
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The selected fish were divided evenly into twenty-four floating glass tanks (30
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fish/tank), and there were eight treatments in triplicate. The four control groups were
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administrated intraperitoneally with 100 µl PBS, and the other four treatment groups
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were administrated intraperitoneally with 100 µl of prepared vaccine at 0 d (the day
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when we immunized the fish was defined as day 0). The eight groups were
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administrated as follows, 30°C + normoxic (No.) + PBS, 30°C + No. + vaccination
136
(Vac.), 30°C + intermittent hypoxic (In. Hy.) + PBS, 30°C + In. Hy. + Vac., 35°C +
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No. + PBS, 35°C + No. + Vac., 35°C + In. Hy. + PBS, 35°C + In. Hy. + Vac.. The
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fish were fed with commercial dry feed (Evergreen, Guangdong, China) twice daily
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and feeding was discontinued 24 h before vaccination, challenge or sampling.
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Fish (n = 3) were sampled randomly from each experiment group at different
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sampling points for different purpose. After anesthetization with MS-222, spleen and
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head kidney samples were collected at 48 h post-vaccination from each group for the
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determination of immune-related gene expression. Organ samples were separated
144
immediately under sterile operation and stored in a Sample Protector for RNA/DNA
145
(Takara, Dalian, China) at -80°C until RNA extraction. Peripheral blood, spleens,
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head kidneys and distal intestine were collected at 28 d post-vaccination. The serum
147
of peripheral blood without heparin was isolated by centrifugation (4000 rpm, 10 min)
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for use in determining serum superoxide dismutase (SOD), catalase (CAT),
149
glutathione peroxidase (GSH-Px) activities and malondialdehyde (MDA) levels.
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Peripheral blood mixed with precooled heparin for use leukocytes isolation. The
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peripheral blood leukocytes (PBLs) were isolated immediately for measuring
152
phagocytic activity. The primary spleen cells and primary head kidney cells were
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isolated immediately from spleens and head kidneys at 28 d post-vaccination for
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measuring respiratory burst response and nitric oxide response. Distal intestine and
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head kidneys were obtained at 28 d post-vaccination and were fixed in 4%
156
paraformaldehyde at least 24 h for use histology observation.
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2.4. Expression of immune-related genes Total RNA from collected organs was extracted using TRIzol reagent (Takara)
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and the nucleic acid quality was measured by agarose gel electrophoresis, and the
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concentration was determined by the absorbance at 260 nm using a Nanodrop
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ND-2000 spectrophotometer (Quawell Technology Inc., San Jose, CA, USA). cDNA
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was then synthesized from 1 µg total RNA using a PrimeScript RT reagent Kit with
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gDNA Eraser (Takara). All cDNA samples were preserved at -20°C until quantitative
164
PCR was processed.
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Real-time Quantitative PCR (RT-qPCR) for analysis of gene expression was
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conducted in a LightCycler 480 Real Time System (Roche, Switzerland) with SYBR
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Green Real-time PCR MasterMix (Takara). The relative expression levels of four
168
immune-related genes including interleukin-1beta (IL-1β), tumor necrosis factor alpha
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(TNF-α), gamma interferon (IFN-γ) and heat shock protein 70 (HSP70) in spleen and
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head kidney were examined with RT-qPCR, while β-actin, a housekeeping gene, was
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chosen as an internal standard. All qPCR primers were designed using the software of
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Beacon Designer 17.0 software based on the gene sequences in GenBank and are
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listed in Table 1. The PCR cycles was conducted at 95°C for 30 s, followed by 40
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cycles, each consisting of at 95°C for 5 s, and 60°C for 30 s. Each sample was run in
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triplicate. Additionally, dissociation-curve analysis was performed and showed a
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single peak in all cases. The relative expression was analyzed using the 2
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method according to Livak and Schmittgen [29].
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2.5. Non–specific immune parameters assay
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SOD, CAT, GSH-Px activities and MDA content in serum were measured using
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assay kits (Nanjing Jiancheng Ins., China) according to the manufacturer’s
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instructions. Details of the procedures were described by the previous methods [30–
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2.6. Phagocytosis activity, respiratory burst and nitric oxide assay
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2.6.1. Isolation of PBLs, spleen and head kidney cells Peripheral blood was collected and PBLs were isolated immediately as described
186
by Ding et al. (2012) [33]. Briefly, the blood was diluted with an equal volume of
187
RPMI 1640 (GE, USA) medium. The suspension was transferred to the surface of
188
Ficoll-Paque PLUS (GE, USA) with a pipette, then isolated by centrifugation at 1600
189
rpm for 45 min at 19°C. PBLs collected at the interphase between the first and second
190
gradient interfaces. Then cells were removed and washed by resuspension five times
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with equal volumes of RPMI 1640. The leucocytes were then resuspended with tissue
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culture medium (TCM), which was prepared from RPMI 1640 medium supplemented
193
with 10% fetal bovine serum (FBS) (Sigma, St. Louis, MO, USA) and 1%
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streptomycin/penicillin (Sigma). The quality and quantity of isolated leucocytes were
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tested using a cell counter (Cellometer AUTO 1000, USA) and then adjusted to 1 ×
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10 6 cells/ml for using to phagocytosis activity analysis.
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Primary spleen cells and primary head kidney cells were obtained from tilapia as
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previously described by Peng et al. (2016) [34]. The spleens and head kidneys of
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individual fish were aseptically removed and immediately placed in TCM. The
200
spleens and head kidneys were then ground into pieces with 180 °C-treated frosted
201
glass slides in TCM and were filtered through a 100-µm cell strainer. The obtained
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cells were washed with RPMI 1640 twice, and resuspended in TCM. The quality and
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quantity of cells were tested as above for use in respiratory burst response and nitric
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oxide response.
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2.6.2. Phagocytosis activity
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S. agalactiae strain (THN0901) was killed as described in 2.2. Inactivated bacteria
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(1 × 109 CFU/ml) were resuspended with TCM. The bacteria were incubated 1 h with
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1 mg/ml fluorescein isothiocyanate (FITC) at 30°C. After washing five times with
209
RPMI 1640, 200 µl FITC-bacteria were added into the prepared PBLs (800 µl, 1 × 10
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min and washed three time with RPMI 1640. The precipitate was incubated 5 min
cells/ml) and cultured 1 h at 28°C. Then they were centrifuged at 500 rpm for 10
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three times with PBS, the precipitate resuspended with 0.9% NaCl. The phagocytosis
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activity of resuspended PBLs was analyzed by flow cytometry (FCM) (FC500, USA).
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Side-scatter (SSC) and forward-scatter (FSC) parameters were used to determine cell
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granularity and cell size, respectively.
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2.6.3. Respiratory burst assay
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Intracellular superoxide production was measured using a nitro blue tetrazolium
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assay (NBT assay) as described by Peng et al. (2016) [34]. Briefly, primary spleen
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cells and primary head kidney cells were isolated from three fish of each group
221
respectively. A 100 µl amount of cells suspension was immediately seeded into
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96-well transparent plates at a density of 1 × 106 cells/ml. The plate was incubated for
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5 min and then centrifuged at 1500 rpm for 5 min at room temperature. The
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supernatant was replaced immediately with 100 µl PBS + 100 µl NBT (2 mg/ml,
225
Sigma), 100 µl inactive S. agalactiae (1 × 109 CFU/ml) + 100 µl NBT, and 100 µl
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phorbol ester (PMA) (100 ng/ml, Sigma) + 100 µl NBT, respectively. The production
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in NBT caused by cells alone was used as a base line. The ROS production caused by
228
PMA was used as the positive control. At the end of the 1 h incubation at room
229
temperature, the non-reduced NBT was removed using 70% methanol. The cell button
230
was air dried and the reduced NBT was dissolved using 120 µl KOH (2 M). A total of
231
140 µl DMSO (Sigma) was added to dissolve the blue crystals that had formed in the
232
cytoplasm. Then the OD values were read at 630 nm using a microplate reader
233
(TECAN infinite M200 Pro Nanoquant, Swizerland).
234
2.6.4. Nitric oxide assay
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Primary spleen cells and primary head kidney cells were isolated immediately
236
from three fish of each group respectively as described in 2.6.1. Nitrite concentration
237
in tissue cells was measured as an indicator of NO production according to the Griess
238
reaction using a NO determination kit (Beyotime, Jiangsu, China) as described by Bai
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240
96-well transparent plates at a density of 1 × 106 cells/ml. Then they were mixed with
241
50 µl Griess reagent Ι and 50 µl Griess reagent ΙΙ, and then the absorbance was read at
242
550 nm using a microplate reader (TECAN, Swizerland).
243
2.7. Distal intestine and head kidney histology
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The sections of tissues were made according to standard histological techniques as
245
described by Su et al. (2017) [36]. Fixed samples of the distal intestine and head
246
kidney were routinely dehydrated in ethanol, equilibrated in xylene and embedded in
247
paraffin, and cut into 4 µm thick sections on a rotary microtome RM2135 (Leica,
248
Wetzlar, Germany). The sections were stained with hematoxylin and eosin (HE) for
249
histology observation. Blinded evaluation of the histological samples was performed
250
using an optical microscope DFC495.
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2.8. Experimental challenge
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S. agalactiae (THN0901) strain was cultured as described in 2.2. The median
253
lethal dose (LD50) in a challenge test was determined from a preliminary experiment
254
(data not shown). The final bacterial concentrations were confirmed by plating
255
ten-fold serial dilutions onto BHI agar medium.
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Fish (n=16) from each tank were infected by intraperitoneal injection with live S.
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agalactiae (THN0901, 2×107 CFU/fish) and returned to their original treatment tanks
258
at 29 d following vaccination. 384 fish were used with 48 per group (triplicate tanks).
259
Mortality was recorded for 14 d after challenge and cumulative mortality was
260
statistically calculated. Additionally, the re-isolation of the S. agalactiae strain from
261
all dead fish was confirmed. The relative percentage survival (RPS) was calculated
262
using the following formula:
263
RPS = [1 − (%Mortality in vaccinated group/%mortality in control group)] × 100
264
2.9. Clearance of S. agalactiae
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266
Gallage et al. (2017) [24]. Briefly, fish (n=3) were randomly sampled to collect blood,
267
spleen, head kidney and brain samples from each experimental group at 1 d and 3 d
268
post-challenge. After anesthetization with MS-222, blood was collected from the
269
caudal vein using a 1 ml sterile syringe, mixed with precooled heparin to prevent
270
clotting and kept on ice. Spleen, head kidney and brain were aseptically removed and
271
immediately placed in 5 ml RPMI 1640 medium RPMI 1640 without antibiotic
272
supplement. Samples were kept on ice until use for bacteria re-isolation.
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A 500 µl sample of heparinized blood was added to 500 µl of distilled water to
274
disrupt the cells and release any surviving bacteria within the cells. The suspension
275
was serially diluted in PBS. A 100 µl sample of each dilution was plated on BHI and
276
incubated at 37°C for 24 h prior to CFU determination. CFU was expressed as mean
277
CFU (n=3 from each group at each sampling point) and the bacteria count was given
278
as CFU/ml of blood. Spleen, head kidneys and brains (100 mg from each) were
279
ground into pieces and serially diluted in PBS, separately. A 100 µl sample of each
280
dilution was plated on BHI and incubated at 37°C for 24 h, CFU were calculated as
281
above.
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The CFU /ml of blood = No. of CFU counted on plate × dilution factor
283
The CFU /g of tissue = No. of CFU counted on plate × dilution factor
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2.10.
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Each group in the present experiment was performed in triplicate. Data were
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expressed as means ± SD. The significant values were calculated using ANOVA and
287
Ducan’s test by SPSS 19.0 (IBM, USA). The results were considered as significant at
288
p < 0.05.
289
3. Results
290
3.1. Expression of immune-related genes
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In both tissues, the expression levels of IL-1β, TNF-α, IFN-γ, and HSP70 were all
292
significantly up-regulated (p < 0.05) in vaccinated fish compared to non-vaccinated
293
fish at 48 h post-vaccination at either 30°C or 35°C. In the spleen (Fig. 1), IL-1β (Fig. 1 A), TNF-α (Fig. 1 B) and IFN-γ (Fig. 1 C)
295
mRNA levels were all significantly down-regulated (p < 0.05) in vaccinated hypoxic
296
fish compared to vaccinated normoxic fish at either 30°C or 35°C. However, HSP70
297
(Fig. 1 D) mRNA levels in vaccinated hypoxic groups were significantly up-regulated
298
(p < 0.05) compared to vaccinated normoxic fish at both temperatures. In the head
299
kidney (Fig. 2), the expression levels of IL-1β (Fig. 2 A), TNF-α (Fig. 2 B), IFN-γ
300
(Fig. 2 C) and HSP70 (Fig. 2 D) were similar to the expression levels in spleen.
301
3.2. Non–specific immune parameters assay
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The SOD, CAT, GSH-Px activities and MDA content in the serum of each group
303
at 28 d post-vaccination were studied. Fig. 3 shows that SOD (Fig. 3 A), CAT (Fig. 3
304
B), GSH-Px (Fig. 3 C) activities were significantly higher (p < 0.05) in the
305
vaccination groups than the non-vaccination groups. At 30°C or 35°C, SOD (Fig 3 A),
306
CAT (Fig 3 B) and GSH-Px (Fig. 3 C) activities in vaccinated fish maintained under
307
hypoxic conditions decreased significantly (p < 0.05) compared to vaccinated fish
308
under normoxic conditions. MDA (Fig. 3 D) content increased significantly (p < 0.05)
309
in hypoxic fish, and no significant differences (p < 0.05) were found between
310
vaccinated hypoxic group and non-vaccinated hypoxic group at either 30°C or 35°C.
311
3.3. Phagocytosis activity
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To elucidate the possible impact of intermittent hypoxia at different temperatures
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on cells of the vaccinated fish, phagocytic activity was subsequently determined by
314
flow cytometry at 28 d post-vaccination. Fig. 4 A showed that PBLs with
315
FITC-bacteria were gated (P) on forward and side scatter (FS-SS) do plot, Q
316
demonstrated the bacteria distribution (no showed). Phagocytic percentages from
317
histograms (Fig. 4 A30 – D35) were statistically calculated and showed by bar graph
ACCEPTED MANUSCRIPT (Fig. 4 B). Fig. 4 B shows that the phagocytic percentage of PBLs towards S.
319
agalactiae increased significantly (p < 0.05) in the vaccination groups compared to
320
the PBS groups. The phagocytic capacity of PBLs decreased significantly (p < 0.05)
321
in the intermittent hypoxic and vaccinated groups compared to normoxic and
322
vaccinated groups at 30°C or 35°C.
323
3.4. Respiratory burst assay
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The effects of S. agalactiae on ROS production in tilapia primary spleen cells and
325
head kidney cells are shown in Fig. 5. In primary spleen cells, a significantly lower (p
326
< 0.05) ROS production was observed in vaccinated hypoxic fish compared to
327
vaccinated normoxic fish caused by S. agalactiae at 35°C (Fig. 5 B), but significant
328
differences were not found between these two groups at 30°C (Fig. 5 A). In primary
329
head kidney cells, a significant decrease (p < 0.05) was found in vaccinated hypoxic
330
fish compared to vaccinated normoxic fish caused by S. agalactiae at either 30°C (Fig.
331
5 C) or 35°C (Fig. 5 D).
332
3.5. Nitric oxide assay
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The possibility that intermittent hypoxia under different temperature induced the
334
changes of nitric oxide levels was investigated in primary spleen cells and head
335
kidney cells. Tilapia spleen and head kidney cells were stimulated with S. agalactiae.
336
Nitric oxide levels in spleen cells and head kidney cells are shown in Fig, 6 A and Fig.
337
6 B, respectively. In both tissue cells, nitric oxide levels increased significantly (p <
338
0.05) in vaccinated hypoxic fish compared to vaccinated normoxic fish at either 30°C
339
or 35°C.
340
3.6. Distal intestine and head kidney histology
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The results of HE staining in distal intestine and head kidney of vaccinated fish
342
under different DO and temperature conditions at 28 d post-vaccination show in Fig.7
343
(the tissue sections of non-vaccinated fish under different conditions do not showed
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345
non-vaccinated fish under the same treatment). In distal intestine, villus showed some
346
degree of shedding in vaccinated hypoxic fish at 30°C (Fig. 7 In-B) and 35°C (Fig. 7
347
In-D) compared to vaccinated normoxic fish at 30°C (Fig. 7 In-A) and 35°C (Fig. 7
348
In-C). In head kidney, intercellular hyperplasia and healthy red cells decreasing were
349
found in vaccinated hypoxic fish at 30°C (Fig. 7 HK-B) and 35°C (Fig. 7 HK-D)
350
compared to vaccinated normoxic fish at 30°C (Fig. 7 HK-A) and 35°C (Fig. 7 HK-C).
351
Furthermore, substantial hemosiderin was found in vaccinated normoxic fish and
352
vaccinated hypoxic fish in head kidney at 35°C.
353
3.7. Cumulative mortality following challenge
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To assess the protective efficacy of vaccine in vaccinated fish under different
355
temperature and dissolved oxygen conditions, tilapias were separately immunized
356
with PBS and inactivation S. agalactiae vaccine on day 0, and then challenged with S.
357
agalactiae on day 29. Fig. 8 shows the percentage cumulative mortality of tilapia.
358
Tilapia mortalities occurred in large quantities from 1 to 7 d post-challenge, and
359
vaccinated fish had a significantly lower (p < 0.05) cumulative mortality compared to
360
non-vaccinated fish. The final mortality of each group was 54.17 ± 2.95 % (30°C
361
normoxic control), 10.42 ± 2.95 % (30°C normoxic vaccinated), 58.33 ± 5.89 %
362
(30 °C intermittent hypoxic control), 14.58 ± 2.95 % (30 °C intermittent hypoxic
363
vaccinated), 68.75 ± 5.10 % (35°C normoxic control), 18.75 ± 5.10 % (35°C
364
normoxic vaccinated), 72.92 ± 5.89 % (35°C intermittent hypoxic control) and 27.08
365
± 2.95 % (35°C intermittent hypoxic vaccinated), respectively. The RPSs of normoxic
366
vaccinated fish at 30°C, intermittent hypoxic vaccinated fish at 30°C, normoxic
367
vaccinated fish at 35°C and intermittent hypoxic vaccinated fish at 35°C compared to
368
the PBS groups were 81.02 ± 4.58%, 75 ± 4.08%, 72.32 ± 8.20% and 62.47 ± 6.05%,
369
respectively.
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3.8. Clearance of S. agalactiae in blood, spleen, head kidney and brain
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372
(p < 0.05) in the PBS groups compared to the vaccination groups (Table 2). In blood,
373
culturable S. agalactiae cells were not detected in vaccinated fish at 3 d
374
post-challenge. At 1 d post-challenge, the bacterial burdens in vaccinated fish spleen
375
and head kidney were significantly higher (p < 0.05) in hypoxic groups compared to
376
normoxic groups either at 30°C or 35°C. Furthermore, spleen in non-vaccinated fish
377
kept under 35°C and hypoxic condition contained the highest bacterial burden at 1 d
378
post-challenge.
379
4. Discussion
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Both temperature and DO at the time of vaccination are recognized as important
381
factors in the development of protective immunity in ectothermic vertebrates [18, 22,
382
24]. To address the potential role of intermittent hypoxia at different temperatures on
383
immune adjustment in vaccinated Nile tilapia, in vivo and in vitro experiments were
384
studied. The present study showed that IL-1β, TNF-α and IFN-γ mRNA levels were
385
all strongly down-regulated in vaccinated hypoxic fish at either 30°C or 35°C. This
386
suggests that intermittent hypoxia at either 30°C or 35°C may have an inhibitory
387
effect on the expression of important pro-inflammatory genes (IL-1β, TNF-α and
388
IFN-γ). These results are also supported by recent studies, demonstrating that IL-1β
389
transcription decreases in response to acute hypoxia in Nile tilapia [37] and long-term
390
hypoxia either reduces or delays the expression of IL-1β, TNF-α and IFN-γ genes in
391
Atlantic salmon (Salmo salar L.) [38].The modulated effects by inhibitory
392
immune-related genes were further detected in primary cells from tilapia peripheral
393
blood, spleen and head kidney, including restraining phagocytosis, respiratory burst
394
activities and enhancement of nitric oxide production in vaccinated hypoxic fish at
395
both temperatures in the present study. These changes in vitro are closely related to
396
the functions of pro-inflammatory cytokines because IL-1β can increase yeast
397
phagocytosis by recruiting and proliferating head kidney leukocytes [39], TNF-α can
398
result in priming of the respiratory burst of the peritoneal exudate and head kidney
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ACCEPTED MANUSCRIPT leukocytes [40], and stimulation of peripheral blood leukocytes with IFN-γ-related
400
protein resulted in the activation of IFN-γ receptor and marked induction of inducible
401
nitric oxide synthase gene expression [41], so these three immune-related genes could
402
lead to changes in phagocytosis, respiratory burst and nitric oxide production by
403
above ways. Additionally, HSP70, a member of the HSP protein family, has powerful
404
immune regulatory effects [42, 43]. Under stress such as hypoxia, the anti-apoptosis
405
and synergetic immunity of HSP70 can be strengthened in order to protect cells from
406
environmental stressors [44, 45], this may be the reason why HSP70 mRNA levels
407
were strongly up-regulated in vaccinated hypoxic fish at both temperatures in present
408
study.
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In non-specific immune system, oxygen consumption is necessary to maintain the
410
NADPH oxidase level in phagocytes in order to activate biochemical reactions that
411
generate ROS [46]. SOD, CAT and GSH-Px, as important antioxidants, play vital
412
roles on transferring ROS for protecting membranes and DNA from damage [47,48].
413
However, teleost fish have a low capacity for regulation of internal levels of dissolved
414
oxygen or temperature by adjusting their physiological, biological mechanisms or
415
behavior [49]. When fish are under hypoxic conditions, the immune system may
416
experience a similar phenomenon because their functions may be affected by the level
417
of hypoxia [24]. Furthermore, substantial hemosiderosis were found in head kidney of
418
vaccinated fish at 35°C in present study. Hemosiderin often forms after hemorrhage.
419
When blood leaves a ruptured blood vessel, the red blood cell dies and the
420
hemoglobin of the cell is released into the extracellular space [50]. In this study,
421
excessive hemosiderin to accumulate may be for red blood cell destruction under
422
hypoxic and high temperature condition. This suggests that the ability of transporting
423
oxygen by red blood cells could be weakened in vaccinated fish under these
424
conditions. Therefore, the activities of SOD, CAT and GSH-Px may be weak driven
425
by lower dissolved oxygen level and/or high temperature. Meanwhile, as the
426
breakdown product of lipid peroxides, increasing MDA content due to hypoxia may
427
have strong cytotoxicity [51]. These negative effects could further suppress the
428
phagocytic activity in cells of the immune system.
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430
bacterial burden was present in vaccinated fish under hypoxic conditions. This may
431
relate to the lower phagocytic capacity and ineffective vaccine absorption. The villus
432
showed shedding in vaccinated hypoxic fish in the present study and this can directly
433
affect the absorption of hindgut to antigen, which had been found that the main site of
434
antigen absorption was in hindgut in the study of teleost [52]. Furthermore, a higher
435
percentage of cumulative mortality also indicates that fish were not getting the
436
expected level of protection from vaccination when vaccinated fish kept at
437
intermittent hypoxic under different temperature condition, and the suppression
438
modulation by intermittent hypoxia under different temperature may affect local as
439
well as systemic immunoreaction.
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In conclusion, our findings indicate that intermittent hypoxia at either 30°C or
441
35°C could suppress immune response in vaccinated Nile tilapia. The occurrence of
442
intermittent hypoxia under different temperatures helps to explain why fish are not
443
getting the expected level of protection from vaccination.
444
Acknowledgments
The Oceanic and Fishery Adminictration of Guangdong Province (2015, 2016).
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This work was funded by Special Science Projects for Fish Diseases Control from
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553
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554
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555 556
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ACCEPTED MANUSCRIPT Table 1 Primers used for RT-PCR analysis. Primer sequence
Source
Product (bp)
β-actin-F β-actin-R IL-1β-F IL-1β-R HSP70-F HSP70-R TNF-α-F TNF-α-R IFN-γ-F IFN-γ-R
5΄-TCCATTGGCCTTCGTTGC-3΄ 5΄-CTATTCTGTGTGACCCAGG-3΄ 5΄-ATTGTCGTCCTGTCTATC-3΄ 5΄-AATGTCATCATGGTATTGC-3΄ 5΄-ACCATCACCAACGATAAG-3΄ 5΄-CGGCTTTGTATTTCTCTG-3΄ 5΄-CTGTAGTCACCTCCATTA-3΄ 5΄-TACTTGTTGTTGCTTCTG-3΄ 5΄-CAGCAGAGATGAACTTGA-3΄ 5΄-CACTAGGAAATACGGGTTT-3΄
EF206801
163
GBAY01004231
126
FJ207463
length
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Primer name
232
121
KF294754
128
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GAID01031494
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Abbreviations- IL-1β: interleukin-1beta; HSP70: heat shock protein 70; TNF-α: tumor necrosis factor alpha; IFN-γ: gamma interferon.
ACCEPTED MANUSCRIPT Table 2 Streptococcus agalactiae burden in blood, spleen, head kidney and brain of tilapia at 1 and 3 days (D) post-challenge. Experimental groups
30 °C Blood (CFU/ml) 35 °C
0.92×102 b
0b
4.0 ± 1.0 mg/L DO Con.
10.23×108 a
7.11×105 a
4.0 ± 1.0 mg/L DO Vac.
2.83×102 b
0b
8.0 ± 0.5 mg/L DO Con.
11.36×108 a'
6.48×105 a'
8.0 ± 0.5 mg/L DO Vac.
1.97×102 b'
0 b'
4.0 ± 1.0 mg/L DO Con.
10.41×108 a'
5.64×105 a'
3.38×102 b'
0 b'
5.58×1010 a
5.74×106 a
30 °C
Brain (CFU/g)
35 °C
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8.0 ± 0.5 mg/L DO Vac.
2.86×103 b
1.12×103 b
4.0 ± 1.0 mg/L DO Con.
8.16×1010 a
9.78×106 a
4.0 ± 1.0 mg/L DO Vac.
1.27×104 c
1.74×104 c
8.0 ± 0.5 mg/L DO Con.
8.24×1010 a'
6.78×106 a'
8.0 ± 0.5 mg/L DO Vac.
2.32×104 b'
2.80×103 b'
4.0 ± 1.0 mg/L DO Con.
9.38×1010 a'
6.47×106 a'
4.0 ± 1.0 mg/L DO Vac.
1.14×105 c'
3.12×104 c'
8.0 ± 0.5 mg/L DO Con.
4.34×109 a
1.56×106 a
8.0 ± 0.5 mg/L DO Vac.
8.96×103 b
1.69×103 b
4.0 ± 1.0 mg/L DO Con.
7.86×108 c
5.40×105 c
4.0 ± 1.0 mg/L DO Vac.
9.20×105 d
2.24×103 b
8.0 ± 0.5 mg/L DO Con.
6.72×107 a'
1.01×106 a'
8.0 ± 0.5 mg/L DO Vac.
1.68×105 b'
2.38×103 b'
4.0 ± 1.0 mg/L DO Con.
1.74×107 a'
1.87×106 a'
4.0 ± 1.0 mg/L DO Vac.
1.12×106 c'
4.76×103 b'
8.0 ± 0.5 mg/L DO Con.
2.27×108 a
3.62×106 a
8.0 ± 0.5 mg/L DO Vac.
4.32×102 b
2.86×103 b
4.0 ± 1.0 mg/L DO Con.
2.40×108 a
3.83×106 a
4.0 ± 1.0 mg/L DO Vac.
1.10×103 c
5.38×103 b
8.0 ± 0.5 mg/L DO Con.
4.31×108 a'
4.54×106 a'
8.0 ± 0.5 mg/L DO Vac.
2.12×103 b'
1.61×104 b'
4.0 ± 1.0 mg/L DO Con.
6.06×108 a'
2.22×106 a'
4.0 ± 1.0 mg/L DO Vac.
9.40×103 b'
3.28×104 b'
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35 °C
3.22×105 a
8.0 ± 0.5 mg/L DO Vac.
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35 °C
Head kidney (CFU/g)
3D 8a
9.10×10
8.0 ± 0.5 mg/L DO Con.
Spleen (CFU/g)
30 °C
1D
8.0 ± 0.5 mg/L DO Con.
4.0 ± 1.0 mg/L DO Vac. 30 °C
Days post challenge
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Water temperature
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Tissue
Notes: Values are given as CFU/ml of blood or CFU/g of tissues, determined by counting bacteria on a BHI plate. At each sampling date, 3 fish were randomly sampled from each group and bacteria counts are the mean of 3 fish. Different superscript letters indicate significant differences (p < 0.05). a/b/c/d denotes the difference among the groups at 30 °C. a'/b'/c'/d' denotes the difference among the groups at 35 °C. (DO = dissolved oxygen; Con. = control; Vac. = vaccinated)
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Fig. 1. The relative expression of IL-1β (A), TNF-α (B), IFN-γ (C) and HSP70 (D) in spleen of Nile tilapia following vaccination under different oxygen (intermittent hypoxia or normoxia) and rearing water temperature (30 °C or 35 °C) conditions. Bars represent the mean ± SD (n=3). Different superscript letters indicate significant differences (p < 0.05). a/b/c/d denotes the difference among the groups at 30 °C. a'/b'/c'/d' denotes the difference among the groups at 35 °C. (DO = dissolved oxygen; Con. = control; Vac. = vaccinated) IL-1β: interleukin-1beta; TNF-α: tumor necrosis factor alpha; IFN-γ: gamma interferon; HSP70: heat shock protein 70.
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Fig. 2. The relative expression of IL-1β (A), TNF-α (B), IFN-γ (C) and HSP70 (D) in head kidney of Nile tilapia following vaccination under different oxygen (intermittent hypoxia or normoxia) and rearing water temperature (30 °C or 35 °C) conditions. Bars represent the mean ± SD (n=3). Different superscript letters indicate significant differences (p < 0.05). a/b/c/d denotes the difference among the groups at 30 °C. a'/b'/c'/d' denotes the difference among the groups at 35 °C. (DO = dissolved oxygen; Con. = control; Vac. = vaccinated) IL-1β: interleukin-1beta; TNF-α: tumor necrosis factor alpha; IFN-γ: gamma interferon; HSP70: heat shock protein 70.
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Fig. 3. (A) superoxide dismutase (SOD) activity, (B) catalase (CAT) activity, (C) glutathione peroxidase (GSH-Px) activity and (D) malondialdehyde (MDA) levels of Nile tilapia following vaccination under different oxygen (intermittent hypoxia or normoxia) and rearing water temperature (30 °C or 35 °C) conditions. Bars represent the mean ± SD (n=3). Different superscript letters indicate significant differences (p < 0.05). a/b/c/d denotes the difference among the groups at 30 °C. a'/b'/c'/d' denotes the difference among the groups at 35 °C. (DO = dissolved oxygen; Con. = control; Vac. = vaccinated)
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Fig. 4. The phagocytic capacity of PBLs was detected under different oxygen (intermittent hypoxia or normoxia) and rearing water temperature (30 °C or 35 °C) conditions by FCM at 28 d post-vaccination. (A) PBLs with FITC-bacteria were gated (P) on forward and side scatter (FS-SS) do plot, Q demonstrated the bacteria distribution (no showed); (B) Phagocytic percentage were statistically calculated. Histograms showed the phagocytic percentage. Bars represent the mean ± SD (n=3). Different superscript letters indicate significant differences (p < 0.05). a/b/c/d denotes the difference among the groups at 30 °C. a'/b'/c'/d' denotes the difference among the groups at 35 °C. (No. = normoxia; In. Hy. = intermittent hypoxia; Con. = control; Vac. = vaccinated)
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Fig. 5. Respiratory burst activity of Nile tilapia primary spleen cells at 30°C (A) or 35°C (B) and primary head kidney cells at 30°C (C) or 35°C (D) after stimulation with NBT, S. agalactiae and PMA was detected at 28 d post-vaccination. Bars represent the mean ± SD (n=3). Different superscript letters (a, b, c and d) indicate significant differences (p < 0.05). (No. = normoxia; In. Hy. = intermittent hypoxia; Con. = control; Vac. = vaccinated)
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Fig. 6. Nitric oxide production of Nile tilapia primary spleen cells (A) and primary head kidney cells (B) after stimulation with S. agalactiae was detected at 28 d post-vaccination. Bars represent the mean ± SD (n=3). Different superscript letters indicate significant differences (p < 0.05). a/b/c/d denotes the difference among the groups at 30 °C. a'/b'/c'/d' denotes the difference among the groups at 35 °C. (DO = dissolved oxygen; Con. = control; Vac. = vaccinated)
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Fig. 7. Histomorphology of distal intestine (In) and head kidney (HK) in vaccinated Nile tilapia under different oxygen (intermittent hypoxia or normoxia) and rearing water temperature (30 °C or 35 °C) at 28 d post-vaccination. In-A: 30 °C and normoxia; In-B: 30 °C and intermittent hypoxia; In-C: 35 °C and normoxia; In-D: 35 °C and intermittent hypoxia; HK-A: 30 °C and normoxia; HK-B: 30 °C and intermittent hypoxia; HK-C: 35 °C and normoxia; HK-D: 35 °C and intermittent hypoxia. Thickness 4 µm. In bar = 100 µm, HK bar = 50 µm.
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Fig. 8. Cumulative mortality (%) of tilapia was recorded daily for 14 d post intraperitoneal challenge with S. agalactiae THN0901 (2×107 CFU/fish). Tilapia mortalities occurred in large quantities during the first week of the challenge. 384 fish were used with 48 per group. Each value represents mean (n=3) and error bars are omitted for clarity. Different superscript letters indicate significant differences (p < 0.05). a/b/c/d denotes the difference among the groups at 30 °C. a'/b'/c'/d' denotes the difference among the groups at 35 °C. (No. = normoxia; In. Hy. = intermittent hypoxia; Con. = control; Vac. = vaccinated)
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Highlights: Intermittent hypoxia at either 30°C or 35°C modulates immune genes expression. Enzymatic activities were lower in vaccinated hypoxia fish at both temperatures. Phagocytosis and ROS production decreased in vaccinated hypoxia fish.
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