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Acute nitrite exposure alters the metabolism of thyroid hormones in grass carp (Ctenopharyngodon idellus)
Accepted Manuscript Acute nitrite exposure alters the metabolism of thyroid hormones in grass carp ( Ctenopharyngodon idellus)
Chen Xiao, Zidong Liu, Dapeng Li, Mohamed M. Refaey, Rong Tang, Li Li, Xi Zhang PII:
S0045-6535(17)31170-0
DOI:
10.1016/j.chemosphere.2017.07.119
Reference:
CHEM 19652
To appear in:
Chemosphere
Received Date:
12 April 2017
Revised Date:
17 July 2017
Accepted Date:
24 July 2017
Please cite this article as: Chen Xiao, Zidong Liu, Dapeng Li, Mohamed M. Refaey, Rong Tang, Li Li, Xi Zhang, Acute nitrite exposure alters the metabolism of thyroid hormones in grass carp ( Ctenopharyngodon idellus), Chemosphere (2017), doi: 10.1016/j.chemosphere.2017.07.119
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ACCEPTED MANUSCRIPT 1
Acute nitrite exposure alters the metabolism of thyroid hormones in
2
grass carp (Ctenopharyngodon idellus)
3 4
Chen Xiao12, Zidong Liu1, Dapeng Li1, *, Mohamed M. Refaey2, Rong Tang1, Li
5
Li1, Xi Zhang1
6 7
1
College of Fisheries, Huazhong Agricultural University, Hubei Provincial
8
Engineering Laboratory for Pond Aquaculture, Wuhan, 430070, P. R. China
9
2
Department of Animal Production, Faculty of Agriculture, Mansoura University,
10
Al-Mansoura 35516, Egypt
11
*Correspondence: E-mail: [email protected]; Tel.: +86-027-87282114
12 13
ABSTRACT: Nitrite has the potential to disturb thyroid hormone homeostasis, but
14
little is known about the underlying mechanisms. In the present study, juvenile grass
15
carp (Ctenopharyngodon idellus) were exposed to various concentrations of nitrite (0,
16
0.5, 1, 4, and 16 mg/L, respectively). Serum concentrations of triiodothyronine (T3),
17
thyroxine
18
triiodothyronine (rT3), thyroid-stimulating hormone (TSH), and the activity of
19
iodothyronine deiodinases were assayed at 0, 12, 24, 48, and 96 h after exposure. It
20
was found that acute nitrite exposure significantly altered the TH levels and
21
iodothyronine deiodinase activities. The rT3 levels were significantly increased in the
22
treatment groups, whereas the concentrations of T3, FT3, FT4, and TSH decreased 1
(T4),
free
triiodothyronine
(FT3),
free
thyroxine
(FT4),
3,3,5ʹ-
ACCEPTED MANUSCRIPT 23
significantly. The concentration of T4 was elevated in the lower-dose exposure group,
24
but was reduced in the higher-dose exposure group. Increases in type I iodothyronine
25
deiodinase (ID1) and type III iodothyronine deiodinase (ID3) activities were observed
26
in the exposure groups. The activity of type II iodothyronine deiodinase (ID2)
27
decreased at 12 and 24 h after exposure. A decrease of colloid in the thyroid follicles
28
was observed in the exposure group. The results indicate that acute nitrite=-0exposure
29
has the potential to disturb the homeostasis of thyroid hormone metabolism, leading
30
to a hypothyroidism state in the juvenile grass carp.
31
Keywords: Ctenopharyngodon idellus; nitrite; thyroid hormone; iodothyronine
32
deiodinase
33 34
1. Introduction
35
Nitrite is part of the nitrogen cycle in ecosystems, and is generally present at low
36
levels in freshwaters. However, high levels of nitrite have been recorded in intensive
37
aquaculture systems (Meybeck, 1982; Avnimelech et al., 1986; Svobodová, 1991).
38
The main reason for the reported increase in the nitrite level is high density farming,
39
with excess feeding leading to high levels of residual protein based feed and
40
nitrogen excretion. When the residual protein based feed supply and nitrogen
41
excretion outstrips the metabolic capability of indigenous flora in aquaculture water,
42
the nitrite continuously accumulates (Tiedje, 1988). Acute toxicity of nitrite has
43
been well documented in a number of fish species (Hilmy et al., 1987; Chin and
44
Shyong, 1998; Huertas, 2002; Das et al., 2004a; Zhang et al., 2012). In addition, 2
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nitrite disrupts various physiological functions, including ion regulation (Doblander
46
and Lackner 1996; Jensen, 2003), hemoglobin oxygen capacity (Cosby et al 2003;
47
Jensen and Rohde 2010), immune system performance (Cheng et al., 2002; Tseng
48
and Chen, 2004; Chand and Sahoo, 2006; Xian et al 2011), physiological
49
metabolism (Woo and Chiu 1997; Das et al., 2004b; Das et al., 2004c; Ciji et al.,
50
2012), and endocrine regulation (Deane and Woo, 2007; Ciji et al., 2012).
51
Moreover, studies have shown that in Sparus sarba (Rhabdosargus sarba) exposed
52
to 25 and 50 mg/L nitrite, the serum thyroxine (T4) levels decreased by 42 and 68%,
53
respectively, suggesting that nitrite may disrupt the thyroid endocrine system of
54
exposed fish (Deane and Woo, 2007).
55
The thyroid hormones (THs) have widespread biological effects on physiological
56
processes (Power et al., 2001; Crane et al., 2004; Porazzi et al., 2009). In fish, THs
57
play a major role in differentiation, growth, metabolism, salinity adaptation, and
58
reproduction (Liu and Chan, 2002; Orozco et al., 2002; Crane et al., 2004). Free
59
triiodothyronine (FT3), free thyroxine (FT4), and the thyroid-stimulating hormone
60
(TSH) are the current front line tests for evaluating thyroid functional status (Yeasmin
61
et al., 2016). The plasma concentrations of free THs, FT4, and FT3, are preferred
62
clinically as indices of thyroidal status, because they are not influenced by the degree
63
of protein binding, which can be affected by numerous factors (Lazarus, 2005;
64
Refetoff, 1979).The predominant TH synthesized from the thyroid tissue is T4, and
65
the TSH regulates the synthesis of THs secreted by the thyroid gland. However, T4
66
has little biological activity, whereas T3 has considerable biological activity. The 3
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conversion of T4 to T3 is catalyzed by the iodothyronine deiodinases in the peripheral
68
tissues (Liu et al., 2011). Three types of iodothyronine deiodinase,—type I
69
iodothyronine deiodinase (ID1), type II iodothyronine deiodinase (ID2), and type III
70
iodothyronine deiodinase (ID3)—has beenidentified in fish. Each iodothyronine
71
deiodinase can convert THs to more or less active forms. For the effective functioning
72
of THs, T4 should be converted to the more active T3 by molecular deiodination in the
73
outer ring (ORD), which is catalyzed by ID1 and ID2 (Orozco and Valverde, 2005).
74
The inner ring deiodination (IRD) catalyzed by ID3 produces 3,3,5ʹ-triiodothyronine
75
(rT3), which has no biological activity from T4, and the less active diiodotyrosine (T2)
76
from T3 (Gai, 2012). ID1 plays a minimal role in plasma TH homeostasis, this
77
enzyme has a considerable influence on iodine recovery and TH degradation (Van der
78
Geyten et al., 2001; Yu et al., 2010). Thus, ID2 and ID3 play the leading roles in
79
adjusting the content of T3 (Orozeo et al., 2002; Brown et al., 2004).
80
Because of the key role of THs in fish, it is important to identify environmental
81
chemicals that may disturb thyroid function, and then evaluate the risk to aquatic
82
organisms (Brucker-Davis, 1998). Although nitrite can alter the concentrations of TH
83
in Sparus sarba, the mechanisms underlying the changes in TH levels are still
84
unclear. We hypothesized that nitrite may alter the morphology of thyroid follicles,
85
change the activities of iodothyronine deiodinases and the peripheral circulating
86
content of THs, to ultimately influence the TH metabolism. Therefore, the objective
87
of this study was to determine the possible mechanisms for changes in TH levels in
4
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fish exposed to nitrite by investigating the effects of nitrite on TH metabolism in grass
89
carp.
90
2. Materials and Methods
91
2.1 Toxin and fish administration
92
The experimental drug was analytical grade NaNO2 (purity ≥99.0%), which was
93
purchased from the Sinopharm Chemical Reagent Co. Ltd (Shanghai, China). The
94
nitrite was dissolved in double distilled water as a stock solution. The concentrations
95
required for exposure were achieved by diluting the stock solution into aquarium
96
water.
97
The experimental animals were healthy grass carp (mean mass ± S.D., 65.82 ±
98
5.53 g), which were obtained from Tuanfeng Fish Farm in Wuhan City, China and
99
then transported to the laboratory at the College of Fisheries in Huazhong Agricultural
100
University. The fish were acclimated for one week before the start of the experiment.
101
During the acclimation and experimental period, fish were maintained in 200 L glass
102
tanks, with a natural photoperiod. Dechlorinated aeration water was used in the
103
experiment to achieve the aquaculture water standard, with water quality parameters
104
as follows, NH4+-N + NO3--N <0.1 mg/L, dissolved oxygen (7.0 ± 0.5 mg/L),
105
temperature (26.0 ± 2°C), and pH (7.0–7.6). Nitrite concentrations were checked daily
106
during the acclimation and experiment, as well as the dissolved oxygen, temperature,
107
and pH. The fish were fed with a commercial diet twice a day, and the supply was
108
stopped during the period from two days before the start to the end of experiment.
5
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Fish were exposed to various concentrations (0, 0.5, 1, 4, and 16 mg/L) of nitrite
110
for 96 hours. During the exposure period, 50% of the exposure solution was renewed
111
every day. There were fifteen grass carp specimens in each group, which were
112
distributed equally among tanks, with three replicate tanks used for each group. Dead
113
fish were removed from the tank daily.
114
2.2 Sample collection Blood, liver, and the tissues from the first branchial arch to the third branchial
115 116
arch
of six fish in each group were taken after exposures of 0, 12, 24, 48, and 96 h.
117
At each sampling, the fish were anaesthetized with tricaine methanesulfonate
118
(MS222, Sigma-Aldrich, Louis, MO, USA).
119
from the caudal vein with a syringe.
120
4°C and then was used for hormone assay.
121
nitrogen and then kept at -80°C until assay
122
2.3 Hormone content measurement
Blood sample (2 mL) was collected
Serum was centrifuged at 3000 ×g for 15 min at Liver samples were frozen in liquid
123
Serum T3, T4, rT3, FT3, FT4 and TSH levels were measured by radioimmunoassay
124
(RIA) using commercial kits purchased from the Beijing North Institute of
125
Biotechnology, China. The RIA kits for hormones were validated for use with serum
126
samples by demonstrating parallelism between a series of diluted and spiked samples
127
in relation to the standard curve. The catalog number (standard limits) of T3, T4, rT3,
128
FT3, FT4 and TSH kits were A01TFB (0-7.5 ng/mL ), A02TFB (0-360 ng/mL),
129
A06TBB (0.075-3.0 ng/mL), A03TFB (1-54 fmol/mL or 0.651-35.15 *10-3 ng/mL),
6
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A04TFB (6-100 pmol/mL or 4.66-77.7 *10-6 ng/mL), A05TFB (0-50 μ IU /mL),
131
respectively. In addition, T3/T4 ratios were calculated for each individual.
132
2.4 Deiodinase activity assay
133
The liver was homogenized in buffer solution (0.1 M PBS, 1 mM DTT, 2 mM
134
EDTA, pH 7.0) and centrifuged at 12,000 ×g for 20 min, and then the insoluble
135
particles were removed. The homogenates were quickly frozen in liquid nitrogen and
136
stored at –80°C prior to the assay. Enzyme activities were measured using a
137
modification of the radiolabeled iodine release method (Van der Geyten et al., 1998;
138
Coimbra, 2005; Liu et al., 2015; Liu et al., 2016 ).
139
The protein concentration was determined by a Bradford Protein Assay (Bio-rad,
140
Hercules, CA, USA). The activity of ID1 was measured by incubating 200 μL liver
141
homogenate at 37°C for 120 min with 200 μL of
142
50,000 cpm of 125I-rT3, 0.1 μM unlabeled rT3, and 15 mM DTT. The activity of ID2
143
and ID3 were similar to that of ID1, and were measured by incubating 200 μL of liver
144
homogenate at 37°C for 120 min with 50,000 cpm of
145
mM DTT in 200 μL of 0.1 M PBS (pH 7.0); and 150,000 cpm of
146
unlabeled T3, 30 mM DTT in 200 μL of 0.1 M PBS (pH 7.0), respectively. All
147
reactions were stopped by adding 200 μL 5% (w/v) bovine serum albumin (Sigma-
148
Aldrich) successively, and 400 μL 10% (w/v) trichloroacetic acid at 4°C. The
149
radioactivity in the supernatant was counted using a GC-911 γ-counter (Zhong Jia,
150
Tianjin, China) after centrifuging at 3500 ×g for 30 min. Instead of liver homogenate,
7
0.1 M PBS (pH 7.0), containing
125I-T , 4
1 nM unlabeled T4, 30 125I-T , 3
1 nM
ACCEPTED MANUSCRIPT 151
0.1 M PBS was used as a blank control. The iodothyronine deiodinase activity was
152
calculated using the following formula: Iodothyronine deiodinase activity [SCc (cpm) × SA
153
(
)
pmol/fmol × 1000] cpm
= [homogenate volume (μL) × protein content
( )
mg × incubation time (min)] mL
154
Where SCc is sample counts minus blank counts, and SA is total moles (rT3, T4 or T3)
155
in the incubation solution/total counts. Therefore, the units of iodothyronine
156
deiodinase activity are expressed as pmol I– released/mg protein per min.
157
2.5 Thyroid histology
158
The organizations from the first branchial arch and the third branchial arch were
159
severed from the fish and fixed in Bouin’s fixative for 48 h. Following fixation, the
160
samples were washed in water and stored in 70% ethanol. The organizations were
161
embedded in paraffin and serial transverse cross-sections (5 μm) were made using a
162
tissue processor (Leica RM 2135, Germany). Dewaxed and rehydrated sections were
163
stained with hematoxylin and eosin. The photograph was taken by NIS-Element BR
164
3.0 software.
165
2.6 Statistical analysis
166
Experimental data were expressed as a mean ± SD, inputted using EXCEL
167
software and performed using SPSS 13.0 software. The differences between the
168
control group and each exposure group were evaluated by one-way analysis of
169
variance (ANOVA) followed by Duncan’s multiple comparison tests where
8
ACCEPTED MANUSCRIPT 170
differences were found. A value of p<0.05 was considered statistically significant and
171
indicated with *.
172
3. Results
173
3.1 Mortality
174
No fish died in the control and lower concentration groups (0.5 and 1 mg/L)
175
during the experimental period. Mortalities of 4.76 and 9.52% were found in the 4 and
176
16 mg/L groups, respectively, at 96 h after exposure.
177
3.2 Serum TSH level
178
After the administration of nitrite, serum TSH levels decreased significantly as the
179
nitrite concentration increased, with the largest decrease observed 48 h after exposure,
180
before rising again at 96 h after exposure (Figure. 2).
181 182
Figure 1. Serum thyroid-stimulating hormone (TSH) concentration of grass carp,
183
exposed to nitrite (0 mg/L, 0.5 mg/L, 1 mg/L, 4 mg/L, 16 mg/L). The values are
184
expressed as mean±SD. Significant differences obtained by one-way analysis of
185
variance followed by Duncan’s multiple comparison test are indicated from value at 0
186
h: *p<0.05.
187
3.3 Serum levels of thyroid hormones 9
ACCEPTED MANUSCRIPT 188
After the exposure, the T4 level initially displayed an upward trend before later
189
descending. The T4 content increased when the nitrite concentration increased from 0
190
to 1 mg/L. The T4 content rose significantly in the 0.5 mg/L group at 12 and 48 h after
191
exposure. When the nitrite concentration increased further, the T4 content fell
192
significantly (Figure. 2A).
193
The FT4 levels decreased significantly with an increase in the exposure
194
concentration. A significant drop in serum FT4 was found in the 1, 4, and 16 mg/L
195
groups 12 h after exposure; in the 1 and 4 mg/L groups 24 h after exposure; and in the
196
4 and 16 mg/L groups 48 h after exposure There was a tendency for a decrease in the
197
0 to 4 mg/L groups, and an increase in the 16 mg/L group (Figure. 2B).
198
During the nitrite administration, serum T3 levels decreased significantly as the
199
nitrite concentration increased and exposure time lengthened, with the largest
200
decrease observed 96 h after exposure (Figure. 2C).
201
After exposure, serum FT3 displayed a similar trend to that of TSH, with a
202
significant decrease as the nitrite concentration increased. At 24 h after exposure, the
203
serum FT3 levels in the 1, 4, and 16 mg/L groups decreased significantly. At 48 and
204
96 h after exposure, a significant decrease was observed in every nitrite group
205
(Figure. 2D).
206
When the nitrite concentration was increased from 0 to 0.5 mg/L, rT3 levels
207
increased significantly. However, when the nitrite concentration was further increased
208
to 1 mg/L, the concentration of rT3 fell at 24 and 48 h after exposure, with the
209
opposite result observed at 12 and 96 h after exposure. At 12 and 96 h after exposure, 10
ACCEPTED MANUSCRIPT 210
the concentration of rT3 decreased in the two higher nitrite concentration groups. At
211
24 and 48 h after exposure, the concentration of rT3 increased significantly (Figure.
212
2E).
213
During the exposure period, T3 /T4 ratio decreased significantly as the nitrite
214
concentration increased and exposure time lengthened, with the largest decrease
215
observed 96 h after exposure (Figure. 2F).
11
(A)
(B)
(C)
(D)
(E)
(F)
ACCEPTED MANUSCRIPT 216
Figure 2.
217
triiodothyronine (FT3), 3,3,5ʹ-triiodothyronine (rT3) concentration and T3/T4 ratio of
218
grass carp, exposed to nitrite (0 mg/L, 0.5 mg/L, 1 mg/L, 4 mg/L, 16 mg/L). The
219
values are expressed as mean±SD. Significant differences obtained by one-way
220
analysis of variance followed by Duncan’s multiple comparison test are indicated
221
from value at 0 h: *p<0.05.
222
3.4 Deiodinase activity In all treatment groups, the ID1 activity increased significantly in a dose-
223 224
Serum thyroxine (T4), free thyroxine (FT4) triiodothyronine (T3), free
dependent manner as the nitrite concentration increased (Figure. 3A).
225
Nitrite exposure significantly affected the ID2 activity. The ID2 activity was
226
significantly decreased in the 0.5 and 1 mg/L groups after 12 h exposure and in the
227
0.5, 1, and 4 mg/L groups 24 h after exposure (Figure. 3B).
228
At 12 and 96 h after exposure, the activity of ID3 significantly increased in the
229
0.5, 1, and 4 mg/L groups. However, there was no significant difference in ID3
230
activity at the other time points. No significant change in ID3 activity occurred in the
231
16 mg/L nitrite exposure group (Figure. 4C).
(A)
12
(B)
ACCEPTED MANUSCRIPT
(C)
232
Figure 3. The activity of type I iodothyronine deiodinase (ID1), type II iodothyronine
233
deiodinase (ID2) and type III iodothyronine deiodinase (ID3) in grass carp, exposed
234
to nitrite (0 mg/L, 0.5 mg/L, 1 mg/L, 4 mg/L, 16 mg/L).The values are expressed as
235
mean±SD. Significant differences obtained by one-way analysis of variance followed
236
by Duncan’s multiple comparison test are indicated from value at 0 h: *p<0.05.
237
3.5 Histopathology
238
The thyroid follicles were observed in the 0 and 16 mg/L treatment groups 96 h
239
after exposure. Representative images of the control and treatment groups are shown
240
in Figure. 4. The thyroid follicles in the control group had varying sizes, linked the
241
simple cuboidal epithelium, and were filled with colloid within the lumen. The
242
follicles typically had a slightly oval appearance (Figure. 4A). In the 16 mg/L nitrite
243
exposure group, the amount of colloid was diminished in the thyroid follicles. This
244
phenomenon was widespread, and the image shown in Figure. 4B was typical.
13
ACCEPTED MANUSCRIPT
(A)
(B)
245
Figure 5. Histologic section of thyroid in grass carp, exposed with nitrite, A --
246
histologic section of thyroid in 0 mg/L; B -- histologic section of thyroid in 16 mg/L
247
after 96 hours of exposure (CO--colloid).
248
4. Discussion
249
In this study, treatment with nitrite significantly altered T4 levels, increased rT3
250
levels, and decreased TSH, T3, FT4, and FT3 levels. Moreover, significant changes in
251
the histology of thyroid follicle and the activity of iodothyronine deiodinase were also
252
observed after exposure to nitrite. Thus, our results showed that exposure to nitrite
253
under laboratory conditions had an adverse effect on the TH metabolism of grass carp.
254
Chemical contaminants have been reported to affect thyroidal hormone function
255
in many fish species (Xu et al., 2002; Brown et al., 2004; Scott and Sloman, 2004;
256
Van der Ven et al., 2006), but the effect of nitrite on THs in fish has received little
257
attention, especially in grass carp (Deane, 2007; Hinther et al., 2012). The
258
histopathology of thyroid follicles is frequently used as an indicator of thyroid
259
function (Brown et al., 2004; Liu et al., 2011). In this study, the thyroid follicles in the
260
control group were filled with colloid within the lumen, whereas the amount of 14
ACCEPTED MANUSCRIPT 261
colloid was diminished in the thyroid follicles 96 h after exposure in the 16 mg/L
262
nitrite exposure group. Severity of colloid depletion is a routinely employed marker
263
for thyroid disruption (Liu et al., 2006).There was a general decrease pattern of
264
colloid area in chemical treatment, the result indicated high concentration nitrite
265
exposure altered TH levels by changing colloid size in thyroid follicles.
266
The changes in TH levels are usually used as direct endpoints to assess the thyroid
267
disruption (Liu et al., 2011). In this study, the T4 levels were increased in the 0.5 and
268
1 mg/L treatment and decreased in 4 and 16 mg/L treatment. The alteration in T4
269
levels may be caused by variations in the colloid size of thyroid follicles, regulation of
270
TSH, and change in ID activity. In fish, T4 is the only TH secreted in the thyroid
271
follicle and is stimulated by TSH (Chiamolera et al., 2009; MacKenzie et al., 2009).
272
In the present study, serum TSH levels decreased significantly with increasing nitrite
273
concentration. The minimum of reduction was appeared at 96 h after exposure which
274
may cause by the adaptation of fish to their environment. Thus, the results indicate
275
that the stress response was induced by nitrite and may contribute to the decrease of
276
TSH levels, leading to a depressed synthesis of T4 in thyroid follicles. In this study,
277
the ID1 activity was significantly increased as the nitrite concentration increased, and
278
the ID2 activity was significantly decreased after exposure in first 24 hours and
279
returned to normal level in last 24 hours. ID1 and ID2 can catalyze the outer ring
280
deiodination of thyroid hormones (Van der Geyten et al., 2001; Yu et al., 2010).
281
plays a minimal role in thyroid hormone homeostasis, ID2 is the main iodothyronine
282
deiodinase of T3 production which operates by metabolizing T4 into active T3 (Berry, 15
ID1
ACCEPTED MANUSCRIPT 283
1991; Orozco et al., 2002; Larsen et al., 1981 Liu et al., 2011). These data suggest that
284
the decreased ID2 activity resulting from nitrite exposure contribute to a reduced rate
285
of conversion from T4 to T3, which leads to a decrease in T4 decomposition and T3
286
production (Liu et al., 2011). The depressed composition and decomposition during
287
the period of the experiment resulted in changes in the T4 levels. T4 levels depend on
288
the quantity of composition and decomposition. The depressed TSH levels leads to
289
the decrease in T4 production. On the contrary, the reduced ID2 activities resulting
290
from nitrite exposure contribute to the reduced rate of conversion from T4 to T3,
291
which result in the decrease in T4 decomposition. In lower nitrite groups the quantity
292
of reduced composition is less than the quantity of reduced decomposition, the T4
293
levels show an increased observation and vice versa. During the nitrite administration,
294
T3 /T4 ratio decreased significantly and the largest decrease observed 96 h after
295
exposure. In 0.5 and 1 mg/L groups, the reducion of T3/T4 ratios caused by increased
296
T4 levels and decreased T3 levels; in higher nitrite groups, deceased T4 levels and
297
more seriously decreased T3 levels leaded to the reducion of T3/T4 ratios.
298
Furthermore, the T3/T4 ratio is an index which reflects thyroid function and the action
299
of hormones on the tissues. T3/T4 ratios in grass carp indicated the alteration of
300
peripheral deiodinase activity (Brar et al., 2010). In this study, the reducion of T3/T4
301
ratios may point to nitrite decreased the conversion of T4 into T3 in the
302
peripheral.The result was in a good agreement with the tendency of ID2 actvity. FT4,
303
a free form of T4 in serum, can be transported to target tissues and directly induce
304
biological activity (Lazarus, 2005). The decline of FT4 levels were closely related to 16
ACCEPTED MANUSCRIPT 305
the depressed synthesis of T4 observed in the study. Significant decreases in FT4 and
306
FT3 levels were detected after exposure to nitrite.. The decrease in T3 and FT3 levels
307
is mostly due to changes in the peripheral TH metabolism, especially the decline of
308
ID2 activity. (Liu et al., 2015). In our study, a decline of FT4 may be one of the
309
reasons for the decrease in the FT3 level. Increased rT3 levels were observed in the
310
experiment during the experimental period and the maximum of augment was
311
appeared at 48 h after exposure. These results were due to the increased ID3 activities.
312
ID3 was the main physiological inactivator of THs, and acted by metabolizing T4 and
313
T3 into the inactive compounds, rT3 and T2 (Gereben et al., 2007). ID3 activity was
314
significantly increased at 12 and 96 h after nitrite exposure in 0.5,1 and 4 mg/L group.
315
The increase in ID3 activity means that more T4 was catalyzed to rT3 rather than T3.
316
Thus, a rise in ID3 activity can result in a decrease in FT4 and FT3 levels, and can also
317
increase the rT3 level (Orozco and Valverde, 2005). These data suggest that the
318
observed changes in the activities of ID2 and ID3 could contribute to reduced FT4 and
319
FT3 levels, as well as promoting the rT3 levels following the nitrite treatments. The
320
exposure of grass carp to nitrite significantly altered iodothyronine deiodinase
321
activity.
322
Iodothyronine deiodinases are crucial regulators of the concentrations of
323
peripheral circulating THs in fish (Zhang et al., 2013). The detection of changes in
324
iodothyronine deiodinase activity caused by environmental contaminants can reflect
325
the mechanisms of interference more clearly and suggest a possible pathway toward
326
poisoning (Blanton et al., 2007). Because of its toxicity, nitrite is undesirable in 17
ACCEPTED MANUSCRIPT 327
environment water, especially in aquaculture water. In intensive fish culture, for the
328
preservation of grass carp’s health, the water must maintain low nitrite concentration
329
Conclusion
330
This study suggests that nitrite altered iodothyronine deiodinases activity and
331
thyroid follicle morphology, which in turn resulted in the change of serum THs level.
332
The changes also revealed a disturbance in thyroid hormone synthesis and metabolism
333
in fish exposed to nitrite, leading to a decline in FT4 and FT3 production. Thus, acute
334
nitrite exposure disturbs thyroid hormone homeostasis and results in a hypothyroidism
335
state in juvenile grass carp.
336
Acknowledgments
337
This study was supported by the Earmarked Fund for China Agriculture
338
Research System (Project no. CARS-46), the National Natural Foundation of China
339
(Project no. 31502140), the Fundamental Research Funds for the Central Universities
340
(Project no. 2662015PY119).
341
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26
(Carassius
auratus).
General
&
Comparative
Endocrinology,
ACCEPTED MANUSCRIPT 3.2 Serum TSH level
Figure 1. Serum thyroid-stimulating hormone (TSH) concentration of grass carp, exposed to nitrite (0 mg/L, 0.5 mg/L, 1 mg/L, 4 mg/L, 16 mg/L). The values are expressed as mean±SD. Significant differences obtained by one-way analysis of variance followed by Duncan’s multiple comparison test are indicated from value at 0 h: *p<0.05.
3.3 Serum levels of thyroid hormones
(A)
(B)
ACCEPTED MANUSCRIPT
Figure 2.
(C)
(D)
(E)
(F)
Serum thyroxine (T4), free thyroxine (FT4) triiodothyronine (T3), free
triiodothyronine (FT3), 3,3,5ʹ-triiodothyronine (rT3) concentration and T3/T4 ratio of grass carp, exposed to nitrite (0 mg/L, 0.5 mg/L, 1 mg/L, 4 mg/L, 16 mg/L). The values are expressed as mean±SD. Significant differences obtained by one-way analysis of variance followed by Duncan’s multiple comparison test are indicated from value at 0 h: *p<0.05.
3.4 Deiodinase activity
ACCEPTED MANUSCRIPT (A)
(B)
(C)
Figure 3. The activity of type I iodothyronine deiodinase (ID1), type II iodothyronine deiodinase (ID2) and type III iodothyronine deiodinase (ID3) in grass carp, exposed to nitrite (0 mg/L, 0.5 mg/L, 1 mg/L, 4 mg/L, 16 mg/L).The values are expressed as mean±SD. Significant differences obtained by one-way analysis of variance followed by Duncan’s multiple comparison test are indicated from value at 0 h: *p<0.05.
3.5 Histopathology
(A)
(B)
Figure 4. Histologic section of thyroid in grass carp, exposed with nitrite, A -histologic section of thyroid in 0 mg/L; B -- histologic section of thyroid in 16 mg/L after 96 hours of exposure (CO--colloid).
ACCEPTED MANUSCRIPT Highlight: 1. Acute nitrite exposure alters iodothyronine deiodinase activities of grass carp. 2. Acute nitrite exposure destroys homeostasis of thyroid hormones in grass carp. 3. High dose of nitrite leads to decline in collide size of thyroid follicles in fish.
Chen Xiao, Zidong Liu, Dapeng Li, Mohamed M. Refaey, Rong Tang, Li Li, Xi Zhang PII:
S0045-6535(17)31170-0
DOI:
10.1016/j.chemosphere.2017.07.119
Reference:
CHEM 19652
To appear in:
Chemosphere
Received Date:
12 April 2017
Revised Date:
17 July 2017
Accepted Date:
24 July 2017
Please cite this article as: Chen Xiao, Zidong Liu, Dapeng Li, Mohamed M. Refaey, Rong Tang, Li Li, Xi Zhang, Acute nitrite exposure alters the metabolism of thyroid hormones in grass carp ( Ctenopharyngodon idellus), Chemosphere (2017), doi: 10.1016/j.chemosphere.2017.07.119
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ACCEPTED MANUSCRIPT 1
Acute nitrite exposure alters the metabolism of thyroid hormones in
2
grass carp (Ctenopharyngodon idellus)
3 4
Chen Xiao12, Zidong Liu1, Dapeng Li1, *, Mohamed M. Refaey2, Rong Tang1, Li
5
Li1, Xi Zhang1
6 7
1
College of Fisheries, Huazhong Agricultural University, Hubei Provincial
8
Engineering Laboratory for Pond Aquaculture, Wuhan, 430070, P. R. China
9
2
Department of Animal Production, Faculty of Agriculture, Mansoura University,
10
Al-Mansoura 35516, Egypt
11
*Correspondence: E-mail: [email protected]; Tel.: +86-027-87282114
12 13
ABSTRACT: Nitrite has the potential to disturb thyroid hormone homeostasis, but
14
little is known about the underlying mechanisms. In the present study, juvenile grass
15
carp (Ctenopharyngodon idellus) were exposed to various concentrations of nitrite (0,
16
0.5, 1, 4, and 16 mg/L, respectively). Serum concentrations of triiodothyronine (T3),
17
thyroxine
18
triiodothyronine (rT3), thyroid-stimulating hormone (TSH), and the activity of
19
iodothyronine deiodinases were assayed at 0, 12, 24, 48, and 96 h after exposure. It
20
was found that acute nitrite exposure significantly altered the TH levels and
21
iodothyronine deiodinase activities. The rT3 levels were significantly increased in the
22
treatment groups, whereas the concentrations of T3, FT3, FT4, and TSH decreased 1
(T4),
free
triiodothyronine
(FT3),
free
thyroxine
(FT4),
3,3,5ʹ-
ACCEPTED MANUSCRIPT 23
significantly. The concentration of T4 was elevated in the lower-dose exposure group,
24
but was reduced in the higher-dose exposure group. Increases in type I iodothyronine
25
deiodinase (ID1) and type III iodothyronine deiodinase (ID3) activities were observed
26
in the exposure groups. The activity of type II iodothyronine deiodinase (ID2)
27
decreased at 12 and 24 h after exposure. A decrease of colloid in the thyroid follicles
28
was observed in the exposure group. The results indicate that acute nitrite=-0exposure
29
has the potential to disturb the homeostasis of thyroid hormone metabolism, leading
30
to a hypothyroidism state in the juvenile grass carp.
31
Keywords: Ctenopharyngodon idellus; nitrite; thyroid hormone; iodothyronine
32
deiodinase
33 34
1. Introduction
35
Nitrite is part of the nitrogen cycle in ecosystems, and is generally present at low
36
levels in freshwaters. However, high levels of nitrite have been recorded in intensive
37
aquaculture systems (Meybeck, 1982; Avnimelech et al., 1986; Svobodová, 1991).
38
The main reason for the reported increase in the nitrite level is high density farming,
39
with excess feeding leading to high levels of residual protein based feed and
40
nitrogen excretion. When the residual protein based feed supply and nitrogen
41
excretion outstrips the metabolic capability of indigenous flora in aquaculture water,
42
the nitrite continuously accumulates (Tiedje, 1988). Acute toxicity of nitrite has
43
been well documented in a number of fish species (Hilmy et al., 1987; Chin and
44
Shyong, 1998; Huertas, 2002; Das et al., 2004a; Zhang et al., 2012). In addition, 2
ACCEPTED MANUSCRIPT 45
nitrite disrupts various physiological functions, including ion regulation (Doblander
46
and Lackner 1996; Jensen, 2003), hemoglobin oxygen capacity (Cosby et al 2003;
47
Jensen and Rohde 2010), immune system performance (Cheng et al., 2002; Tseng
48
and Chen, 2004; Chand and Sahoo, 2006; Xian et al 2011), physiological
49
metabolism (Woo and Chiu 1997; Das et al., 2004b; Das et al., 2004c; Ciji et al.,
50
2012), and endocrine regulation (Deane and Woo, 2007; Ciji et al., 2012).
51
Moreover, studies have shown that in Sparus sarba (Rhabdosargus sarba) exposed
52
to 25 and 50 mg/L nitrite, the serum thyroxine (T4) levels decreased by 42 and 68%,
53
respectively, suggesting that nitrite may disrupt the thyroid endocrine system of
54
exposed fish (Deane and Woo, 2007).
55
The thyroid hormones (THs) have widespread biological effects on physiological
56
processes (Power et al., 2001; Crane et al., 2004; Porazzi et al., 2009). In fish, THs
57
play a major role in differentiation, growth, metabolism, salinity adaptation, and
58
reproduction (Liu and Chan, 2002; Orozco et al., 2002; Crane et al., 2004). Free
59
triiodothyronine (FT3), free thyroxine (FT4), and the thyroid-stimulating hormone
60
(TSH) are the current front line tests for evaluating thyroid functional status (Yeasmin
61
et al., 2016). The plasma concentrations of free THs, FT4, and FT3, are preferred
62
clinically as indices of thyroidal status, because they are not influenced by the degree
63
of protein binding, which can be affected by numerous factors (Lazarus, 2005;
64
Refetoff, 1979).The predominant TH synthesized from the thyroid tissue is T4, and
65
the TSH regulates the synthesis of THs secreted by the thyroid gland. However, T4
66
has little biological activity, whereas T3 has considerable biological activity. The 3
ACCEPTED MANUSCRIPT 67
conversion of T4 to T3 is catalyzed by the iodothyronine deiodinases in the peripheral
68
tissues (Liu et al., 2011). Three types of iodothyronine deiodinase,—type I
69
iodothyronine deiodinase (ID1), type II iodothyronine deiodinase (ID2), and type III
70
iodothyronine deiodinase (ID3)—has beenidentified in fish. Each iodothyronine
71
deiodinase can convert THs to more or less active forms. For the effective functioning
72
of THs, T4 should be converted to the more active T3 by molecular deiodination in the
73
outer ring (ORD), which is catalyzed by ID1 and ID2 (Orozco and Valverde, 2005).
74
The inner ring deiodination (IRD) catalyzed by ID3 produces 3,3,5ʹ-triiodothyronine
75
(rT3), which has no biological activity from T4, and the less active diiodotyrosine (T2)
76
from T3 (Gai, 2012). ID1 plays a minimal role in plasma TH homeostasis, this
77
enzyme has a considerable influence on iodine recovery and TH degradation (Van der
78
Geyten et al., 2001; Yu et al., 2010). Thus, ID2 and ID3 play the leading roles in
79
adjusting the content of T3 (Orozeo et al., 2002; Brown et al., 2004).
80
Because of the key role of THs in fish, it is important to identify environmental
81
chemicals that may disturb thyroid function, and then evaluate the risk to aquatic
82
organisms (Brucker-Davis, 1998). Although nitrite can alter the concentrations of TH
83
in Sparus sarba, the mechanisms underlying the changes in TH levels are still
84
unclear. We hypothesized that nitrite may alter the morphology of thyroid follicles,
85
change the activities of iodothyronine deiodinases and the peripheral circulating
86
content of THs, to ultimately influence the TH metabolism. Therefore, the objective
87
of this study was to determine the possible mechanisms for changes in TH levels in
4
ACCEPTED MANUSCRIPT 88
fish exposed to nitrite by investigating the effects of nitrite on TH metabolism in grass
89
carp.
90
2. Materials and Methods
91
2.1 Toxin and fish administration
92
The experimental drug was analytical grade NaNO2 (purity ≥99.0%), which was
93
purchased from the Sinopharm Chemical Reagent Co. Ltd (Shanghai, China). The
94
nitrite was dissolved in double distilled water as a stock solution. The concentrations
95
required for exposure were achieved by diluting the stock solution into aquarium
96
water.
97
The experimental animals were healthy grass carp (mean mass ± S.D., 65.82 ±
98
5.53 g), which were obtained from Tuanfeng Fish Farm in Wuhan City, China and
99
then transported to the laboratory at the College of Fisheries in Huazhong Agricultural
100
University. The fish were acclimated for one week before the start of the experiment.
101
During the acclimation and experimental period, fish were maintained in 200 L glass
102
tanks, with a natural photoperiod. Dechlorinated aeration water was used in the
103
experiment to achieve the aquaculture water standard, with water quality parameters
104
as follows, NH4+-N + NO3--N <0.1 mg/L, dissolved oxygen (7.0 ± 0.5 mg/L),
105
temperature (26.0 ± 2°C), and pH (7.0–7.6). Nitrite concentrations were checked daily
106
during the acclimation and experiment, as well as the dissolved oxygen, temperature,
107
and pH. The fish were fed with a commercial diet twice a day, and the supply was
108
stopped during the period from two days before the start to the end of experiment.
5
ACCEPTED MANUSCRIPT 109
Fish were exposed to various concentrations (0, 0.5, 1, 4, and 16 mg/L) of nitrite
110
for 96 hours. During the exposure period, 50% of the exposure solution was renewed
111
every day. There were fifteen grass carp specimens in each group, which were
112
distributed equally among tanks, with three replicate tanks used for each group. Dead
113
fish were removed from the tank daily.
114
2.2 Sample collection Blood, liver, and the tissues from the first branchial arch to the third branchial
115 116
arch
of six fish in each group were taken after exposures of 0, 12, 24, 48, and 96 h.
117
At each sampling, the fish were anaesthetized with tricaine methanesulfonate
118
(MS222, Sigma-Aldrich, Louis, MO, USA).
119
from the caudal vein with a syringe.
120
4°C and then was used for hormone assay.
121
nitrogen and then kept at -80°C until assay
122
2.3 Hormone content measurement
Blood sample (2 mL) was collected
Serum was centrifuged at 3000 ×g for 15 min at Liver samples were frozen in liquid
123
Serum T3, T4, rT3, FT3, FT4 and TSH levels were measured by radioimmunoassay
124
(RIA) using commercial kits purchased from the Beijing North Institute of
125
Biotechnology, China. The RIA kits for hormones were validated for use with serum
126
samples by demonstrating parallelism between a series of diluted and spiked samples
127
in relation to the standard curve. The catalog number (standard limits) of T3, T4, rT3,
128
FT3, FT4 and TSH kits were A01TFB (0-7.5 ng/mL ), A02TFB (0-360 ng/mL),
129
A06TBB (0.075-3.0 ng/mL), A03TFB (1-54 fmol/mL or 0.651-35.15 *10-3 ng/mL),
6
ACCEPTED MANUSCRIPT 130
A04TFB (6-100 pmol/mL or 4.66-77.7 *10-6 ng/mL), A05TFB (0-50 μ IU /mL),
131
respectively. In addition, T3/T4 ratios were calculated for each individual.
132
2.4 Deiodinase activity assay
133
The liver was homogenized in buffer solution (0.1 M PBS, 1 mM DTT, 2 mM
134
EDTA, pH 7.0) and centrifuged at 12,000 ×g for 20 min, and then the insoluble
135
particles were removed. The homogenates were quickly frozen in liquid nitrogen and
136
stored at –80°C prior to the assay. Enzyme activities were measured using a
137
modification of the radiolabeled iodine release method (Van der Geyten et al., 1998;
138
Coimbra, 2005; Liu et al., 2015; Liu et al., 2016 ).
139
The protein concentration was determined by a Bradford Protein Assay (Bio-rad,
140
Hercules, CA, USA). The activity of ID1 was measured by incubating 200 μL liver
141
homogenate at 37°C for 120 min with 200 μL of
142
50,000 cpm of 125I-rT3, 0.1 μM unlabeled rT3, and 15 mM DTT. The activity of ID2
143
and ID3 were similar to that of ID1, and were measured by incubating 200 μL of liver
144
homogenate at 37°C for 120 min with 50,000 cpm of
145
mM DTT in 200 μL of 0.1 M PBS (pH 7.0); and 150,000 cpm of
146
unlabeled T3, 30 mM DTT in 200 μL of 0.1 M PBS (pH 7.0), respectively. All
147
reactions were stopped by adding 200 μL 5% (w/v) bovine serum albumin (Sigma-
148
Aldrich) successively, and 400 μL 10% (w/v) trichloroacetic acid at 4°C. The
149
radioactivity in the supernatant was counted using a GC-911 γ-counter (Zhong Jia,
150
Tianjin, China) after centrifuging at 3500 ×g for 30 min. Instead of liver homogenate,
7
0.1 M PBS (pH 7.0), containing
125I-T , 4
1 nM unlabeled T4, 30 125I-T , 3
1 nM
ACCEPTED MANUSCRIPT 151
0.1 M PBS was used as a blank control. The iodothyronine deiodinase activity was
152
calculated using the following formula: Iodothyronine deiodinase activity [SCc (cpm) × SA
153
(
)
pmol/fmol × 1000] cpm
= [homogenate volume (μL) × protein content
( )
mg × incubation time (min)] mL
154
Where SCc is sample counts minus blank counts, and SA is total moles (rT3, T4 or T3)
155
in the incubation solution/total counts. Therefore, the units of iodothyronine
156
deiodinase activity are expressed as pmol I– released/mg protein per min.
157
2.5 Thyroid histology
158
The organizations from the first branchial arch and the third branchial arch were
159
severed from the fish and fixed in Bouin’s fixative for 48 h. Following fixation, the
160
samples were washed in water and stored in 70% ethanol. The organizations were
161
embedded in paraffin and serial transverse cross-sections (5 μm) were made using a
162
tissue processor (Leica RM 2135, Germany). Dewaxed and rehydrated sections were
163
stained with hematoxylin and eosin. The photograph was taken by NIS-Element BR
164
3.0 software.
165
2.6 Statistical analysis
166
Experimental data were expressed as a mean ± SD, inputted using EXCEL
167
software and performed using SPSS 13.0 software. The differences between the
168
control group and each exposure group were evaluated by one-way analysis of
169
variance (ANOVA) followed by Duncan’s multiple comparison tests where
8
ACCEPTED MANUSCRIPT 170
differences were found. A value of p<0.05 was considered statistically significant and
171
indicated with *.
172
3. Results
173
3.1 Mortality
174
No fish died in the control and lower concentration groups (0.5 and 1 mg/L)
175
during the experimental period. Mortalities of 4.76 and 9.52% were found in the 4 and
176
16 mg/L groups, respectively, at 96 h after exposure.
177
3.2 Serum TSH level
178
After the administration of nitrite, serum TSH levels decreased significantly as the
179
nitrite concentration increased, with the largest decrease observed 48 h after exposure,
180
before rising again at 96 h after exposure (Figure. 2).
181 182
Figure 1. Serum thyroid-stimulating hormone (TSH) concentration of grass carp,
183
exposed to nitrite (0 mg/L, 0.5 mg/L, 1 mg/L, 4 mg/L, 16 mg/L). The values are
184
expressed as mean±SD. Significant differences obtained by one-way analysis of
185
variance followed by Duncan’s multiple comparison test are indicated from value at 0
186
h: *p<0.05.
187
3.3 Serum levels of thyroid hormones 9
ACCEPTED MANUSCRIPT 188
After the exposure, the T4 level initially displayed an upward trend before later
189
descending. The T4 content increased when the nitrite concentration increased from 0
190
to 1 mg/L. The T4 content rose significantly in the 0.5 mg/L group at 12 and 48 h after
191
exposure. When the nitrite concentration increased further, the T4 content fell
192
significantly (Figure. 2A).
193
The FT4 levels decreased significantly with an increase in the exposure
194
concentration. A significant drop in serum FT4 was found in the 1, 4, and 16 mg/L
195
groups 12 h after exposure; in the 1 and 4 mg/L groups 24 h after exposure; and in the
196
4 and 16 mg/L groups 48 h after exposure There was a tendency for a decrease in the
197
0 to 4 mg/L groups, and an increase in the 16 mg/L group (Figure. 2B).
198
During the nitrite administration, serum T3 levels decreased significantly as the
199
nitrite concentration increased and exposure time lengthened, with the largest
200
decrease observed 96 h after exposure (Figure. 2C).
201
After exposure, serum FT3 displayed a similar trend to that of TSH, with a
202
significant decrease as the nitrite concentration increased. At 24 h after exposure, the
203
serum FT3 levels in the 1, 4, and 16 mg/L groups decreased significantly. At 48 and
204
96 h after exposure, a significant decrease was observed in every nitrite group
205
(Figure. 2D).
206
When the nitrite concentration was increased from 0 to 0.5 mg/L, rT3 levels
207
increased significantly. However, when the nitrite concentration was further increased
208
to 1 mg/L, the concentration of rT3 fell at 24 and 48 h after exposure, with the
209
opposite result observed at 12 and 96 h after exposure. At 12 and 96 h after exposure, 10
ACCEPTED MANUSCRIPT 210
the concentration of rT3 decreased in the two higher nitrite concentration groups. At
211
24 and 48 h after exposure, the concentration of rT3 increased significantly (Figure.
212
2E).
213
During the exposure period, T3 /T4 ratio decreased significantly as the nitrite
214
concentration increased and exposure time lengthened, with the largest decrease
215
observed 96 h after exposure (Figure. 2F).
11
(A)
(B)
(C)
(D)
(E)
(F)
ACCEPTED MANUSCRIPT 216
Figure 2.
217
triiodothyronine (FT3), 3,3,5ʹ-triiodothyronine (rT3) concentration and T3/T4 ratio of
218
grass carp, exposed to nitrite (0 mg/L, 0.5 mg/L, 1 mg/L, 4 mg/L, 16 mg/L). The
219
values are expressed as mean±SD. Significant differences obtained by one-way
220
analysis of variance followed by Duncan’s multiple comparison test are indicated
221
from value at 0 h: *p<0.05.
222
3.4 Deiodinase activity In all treatment groups, the ID1 activity increased significantly in a dose-
223 224
Serum thyroxine (T4), free thyroxine (FT4) triiodothyronine (T3), free
dependent manner as the nitrite concentration increased (Figure. 3A).
225
Nitrite exposure significantly affected the ID2 activity. The ID2 activity was
226
significantly decreased in the 0.5 and 1 mg/L groups after 12 h exposure and in the
227
0.5, 1, and 4 mg/L groups 24 h after exposure (Figure. 3B).
228
At 12 and 96 h after exposure, the activity of ID3 significantly increased in the
229
0.5, 1, and 4 mg/L groups. However, there was no significant difference in ID3
230
activity at the other time points. No significant change in ID3 activity occurred in the
231
16 mg/L nitrite exposure group (Figure. 4C).
(A)
12
(B)
ACCEPTED MANUSCRIPT
(C)
232
Figure 3. The activity of type I iodothyronine deiodinase (ID1), type II iodothyronine
233
deiodinase (ID2) and type III iodothyronine deiodinase (ID3) in grass carp, exposed
234
to nitrite (0 mg/L, 0.5 mg/L, 1 mg/L, 4 mg/L, 16 mg/L).The values are expressed as
235
mean±SD. Significant differences obtained by one-way analysis of variance followed
236
by Duncan’s multiple comparison test are indicated from value at 0 h: *p<0.05.
237
3.5 Histopathology
238
The thyroid follicles were observed in the 0 and 16 mg/L treatment groups 96 h
239
after exposure. Representative images of the control and treatment groups are shown
240
in Figure. 4. The thyroid follicles in the control group had varying sizes, linked the
241
simple cuboidal epithelium, and were filled with colloid within the lumen. The
242
follicles typically had a slightly oval appearance (Figure. 4A). In the 16 mg/L nitrite
243
exposure group, the amount of colloid was diminished in the thyroid follicles. This
244
phenomenon was widespread, and the image shown in Figure. 4B was typical.
13
ACCEPTED MANUSCRIPT
(A)
(B)
245
Figure 5. Histologic section of thyroid in grass carp, exposed with nitrite, A --
246
histologic section of thyroid in 0 mg/L; B -- histologic section of thyroid in 16 mg/L
247
after 96 hours of exposure (CO--colloid).
248
4. Discussion
249
In this study, treatment with nitrite significantly altered T4 levels, increased rT3
250
levels, and decreased TSH, T3, FT4, and FT3 levels. Moreover, significant changes in
251
the histology of thyroid follicle and the activity of iodothyronine deiodinase were also
252
observed after exposure to nitrite. Thus, our results showed that exposure to nitrite
253
under laboratory conditions had an adverse effect on the TH metabolism of grass carp.
254
Chemical contaminants have been reported to affect thyroidal hormone function
255
in many fish species (Xu et al., 2002; Brown et al., 2004; Scott and Sloman, 2004;
256
Van der Ven et al., 2006), but the effect of nitrite on THs in fish has received little
257
attention, especially in grass carp (Deane, 2007; Hinther et al., 2012). The
258
histopathology of thyroid follicles is frequently used as an indicator of thyroid
259
function (Brown et al., 2004; Liu et al., 2011). In this study, the thyroid follicles in the
260
control group were filled with colloid within the lumen, whereas the amount of 14
ACCEPTED MANUSCRIPT 261
colloid was diminished in the thyroid follicles 96 h after exposure in the 16 mg/L
262
nitrite exposure group. Severity of colloid depletion is a routinely employed marker
263
for thyroid disruption (Liu et al., 2006).There was a general decrease pattern of
264
colloid area in chemical treatment, the result indicated high concentration nitrite
265
exposure altered TH levels by changing colloid size in thyroid follicles.
266
The changes in TH levels are usually used as direct endpoints to assess the thyroid
267
disruption (Liu et al., 2011). In this study, the T4 levels were increased in the 0.5 and
268
1 mg/L treatment and decreased in 4 and 16 mg/L treatment. The alteration in T4
269
levels may be caused by variations in the colloid size of thyroid follicles, regulation of
270
TSH, and change in ID activity. In fish, T4 is the only TH secreted in the thyroid
271
follicle and is stimulated by TSH (Chiamolera et al., 2009; MacKenzie et al., 2009).
272
In the present study, serum TSH levels decreased significantly with increasing nitrite
273
concentration. The minimum of reduction was appeared at 96 h after exposure which
274
may cause by the adaptation of fish to their environment. Thus, the results indicate
275
that the stress response was induced by nitrite and may contribute to the decrease of
276
TSH levels, leading to a depressed synthesis of T4 in thyroid follicles. In this study,
277
the ID1 activity was significantly increased as the nitrite concentration increased, and
278
the ID2 activity was significantly decreased after exposure in first 24 hours and
279
returned to normal level in last 24 hours. ID1 and ID2 can catalyze the outer ring
280
deiodination of thyroid hormones (Van der Geyten et al., 2001; Yu et al., 2010).
281
plays a minimal role in thyroid hormone homeostasis, ID2 is the main iodothyronine
282
deiodinase of T3 production which operates by metabolizing T4 into active T3 (Berry, 15
ID1
ACCEPTED MANUSCRIPT 283
1991; Orozco et al., 2002; Larsen et al., 1981 Liu et al., 2011). These data suggest that
284
the decreased ID2 activity resulting from nitrite exposure contribute to a reduced rate
285
of conversion from T4 to T3, which leads to a decrease in T4 decomposition and T3
286
production (Liu et al., 2011). The depressed composition and decomposition during
287
the period of the experiment resulted in changes in the T4 levels. T4 levels depend on
288
the quantity of composition and decomposition. The depressed TSH levels leads to
289
the decrease in T4 production. On the contrary, the reduced ID2 activities resulting
290
from nitrite exposure contribute to the reduced rate of conversion from T4 to T3,
291
which result in the decrease in T4 decomposition. In lower nitrite groups the quantity
292
of reduced composition is less than the quantity of reduced decomposition, the T4
293
levels show an increased observation and vice versa. During the nitrite administration,
294
T3 /T4 ratio decreased significantly and the largest decrease observed 96 h after
295
exposure. In 0.5 and 1 mg/L groups, the reducion of T3/T4 ratios caused by increased
296
T4 levels and decreased T3 levels; in higher nitrite groups, deceased T4 levels and
297
more seriously decreased T3 levels leaded to the reducion of T3/T4 ratios.
298
Furthermore, the T3/T4 ratio is an index which reflects thyroid function and the action
299
of hormones on the tissues. T3/T4 ratios in grass carp indicated the alteration of
300
peripheral deiodinase activity (Brar et al., 2010). In this study, the reducion of T3/T4
301
ratios may point to nitrite decreased the conversion of T4 into T3 in the
302
peripheral.The result was in a good agreement with the tendency of ID2 actvity. FT4,
303
a free form of T4 in serum, can be transported to target tissues and directly induce
304
biological activity (Lazarus, 2005). The decline of FT4 levels were closely related to 16
ACCEPTED MANUSCRIPT 305
the depressed synthesis of T4 observed in the study. Significant decreases in FT4 and
306
FT3 levels were detected after exposure to nitrite.. The decrease in T3 and FT3 levels
307
is mostly due to changes in the peripheral TH metabolism, especially the decline of
308
ID2 activity. (Liu et al., 2015). In our study, a decline of FT4 may be one of the
309
reasons for the decrease in the FT3 level. Increased rT3 levels were observed in the
310
experiment during the experimental period and the maximum of augment was
311
appeared at 48 h after exposure. These results were due to the increased ID3 activities.
312
ID3 was the main physiological inactivator of THs, and acted by metabolizing T4 and
313
T3 into the inactive compounds, rT3 and T2 (Gereben et al., 2007). ID3 activity was
314
significantly increased at 12 and 96 h after nitrite exposure in 0.5,1 and 4 mg/L group.
315
The increase in ID3 activity means that more T4 was catalyzed to rT3 rather than T3.
316
Thus, a rise in ID3 activity can result in a decrease in FT4 and FT3 levels, and can also
317
increase the rT3 level (Orozco and Valverde, 2005). These data suggest that the
318
observed changes in the activities of ID2 and ID3 could contribute to reduced FT4 and
319
FT3 levels, as well as promoting the rT3 levels following the nitrite treatments. The
320
exposure of grass carp to nitrite significantly altered iodothyronine deiodinase
321
activity.
322
Iodothyronine deiodinases are crucial regulators of the concentrations of
323
peripheral circulating THs in fish (Zhang et al., 2013). The detection of changes in
324
iodothyronine deiodinase activity caused by environmental contaminants can reflect
325
the mechanisms of interference more clearly and suggest a possible pathway toward
326
poisoning (Blanton et al., 2007). Because of its toxicity, nitrite is undesirable in 17
ACCEPTED MANUSCRIPT 327
environment water, especially in aquaculture water. In intensive fish culture, for the
328
preservation of grass carp’s health, the water must maintain low nitrite concentration
329
Conclusion
330
This study suggests that nitrite altered iodothyronine deiodinases activity and
331
thyroid follicle morphology, which in turn resulted in the change of serum THs level.
332
The changes also revealed a disturbance in thyroid hormone synthesis and metabolism
333
in fish exposed to nitrite, leading to a decline in FT4 and FT3 production. Thus, acute
334
nitrite exposure disturbs thyroid hormone homeostasis and results in a hypothyroidism
335
state in juvenile grass carp.
336
Acknowledgments
337
This study was supported by the Earmarked Fund for China Agriculture
338
Research System (Project no. CARS-46), the National Natural Foundation of China
339
(Project no. 31502140), the Fundamental Research Funds for the Central Universities
340
(Project no. 2662015PY119).
341
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(Carassius
auratus).
General
&
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Endocrinology,
ACCEPTED MANUSCRIPT 3.2 Serum TSH level
Figure 1. Serum thyroid-stimulating hormone (TSH) concentration of grass carp, exposed to nitrite (0 mg/L, 0.5 mg/L, 1 mg/L, 4 mg/L, 16 mg/L). The values are expressed as mean±SD. Significant differences obtained by one-way analysis of variance followed by Duncan’s multiple comparison test are indicated from value at 0 h: *p<0.05.
3.3 Serum levels of thyroid hormones
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(B)
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Figure 2.
(C)
(D)
(E)
(F)
Serum thyroxine (T4), free thyroxine (FT4) triiodothyronine (T3), free
triiodothyronine (FT3), 3,3,5ʹ-triiodothyronine (rT3) concentration and T3/T4 ratio of grass carp, exposed to nitrite (0 mg/L, 0.5 mg/L, 1 mg/L, 4 mg/L, 16 mg/L). The values are expressed as mean±SD. Significant differences obtained by one-way analysis of variance followed by Duncan’s multiple comparison test are indicated from value at 0 h: *p<0.05.
3.4 Deiodinase activity
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(B)
(C)
Figure 3. The activity of type I iodothyronine deiodinase (ID1), type II iodothyronine deiodinase (ID2) and type III iodothyronine deiodinase (ID3) in grass carp, exposed to nitrite (0 mg/L, 0.5 mg/L, 1 mg/L, 4 mg/L, 16 mg/L).The values are expressed as mean±SD. Significant differences obtained by one-way analysis of variance followed by Duncan’s multiple comparison test are indicated from value at 0 h: *p<0.05.
3.5 Histopathology
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(B)
Figure 4. Histologic section of thyroid in grass carp, exposed with nitrite, A -histologic section of thyroid in 0 mg/L; B -- histologic section of thyroid in 16 mg/L after 96 hours of exposure (CO--colloid).
ACCEPTED MANUSCRIPT Highlight: 1. Acute nitrite exposure alters iodothyronine deiodinase activities of grass carp. 2. Acute nitrite exposure destroys homeostasis of thyroid hormones in grass carp. 3. High dose of nitrite leads to decline in collide size of thyroid follicles in fish.