Ovarian Development of Conger Eel in Korea, Conger myriaster, in Captivity.

Effects of water temperature and hormones on ovarian development of conger eel in Korea were investigated. Ovarian development was analyzed by measuring gonadosomatic index (GSI) and oocyte diameter with histological methods. At rearing water temperatures of 12°C, 14°C, and 16°C, GSI value increased from 3.66 at the start of the experiment to 7.44, 8.82, and 7.34 at the end of the experiment, respectively. At rearing water temperatures of 12°C, 14°C, and 16°C, egg diameter increased from 245.11-300.25 µm at the start of the experiment to 377.62-480.27 µm, 396.72-498.54 µm, and 382.29-475.69 µm at the end of the experiment, respectively. Follicular oocyte development revealed that primary yolk globule stage observed from January to March. It entered to secondary yolk globule stage in April and remained at the same stage until July. As a result of examining effects of three hormones (human chorionic gonadotropin (HCG), luteinizing hormone releasing hormone analogue (LHRHa), and salmon pituitary extraction (SPE) on ovarian development, HCG was found to be the most effective one. The progress from diapause of the secondary yolk globule stage to migratory nucleus stage of oocytes could be induced by treating fish with HCG at 1,000 IU/kg. The effect of hormone treatment on ovarian development of conger eel in Korea was the most effective at water temperature of 14°C. © Copyright 2021 The Korean Society of Developmental Biology.

INTRODUCTION

The conger eel, Conger myriaster, is a marine eel species widely distributed in temperate regions from East China Sea to coastal waters of Korea and Japan (Park, 2001; Tokimura, 2001). It is mainly inhabited in shallow coastal waters to the continental shelf of the East China Sea (Ochiai & Tanaka, 1986). C. myriaster is an important fishery resource in Korea, Japan, and China. In Japan, resource of C. myriaster has recent decreased, emphasizing the necessity of management and conservation of major fishing grounds. There is a need for enhanced management to ensure the maintenance of resources with sustainable supply. Proper management of C. myriaster stock needs to enable understating of its population dynamics. Reproduction of the fish is the only way to provide a new generation necessary to sustain its population. Therefore, understanding the reproduction of a stock is essential to unravel population dynamics.

Mature individuals of C. myriaster in natural population have not been collected from coastal waters to the continental margin, where many adults are caught commercially. Knowledge on the reproduction of Japanese C. myriaster has been rapidly increasing from studies of fish in captivity. The Japanese conger eel puberty begins at the age of 2 years. Its annual reproductive cycle progresses even in cultured conditions, although oocyte maturation and ovulation have not occurred yet (Utoh et al., 2004, 2005). Oocyte maturation and ovulation of Japanese conger eel can be induced by repeated injections of human chorionic gonadotropin (HCG) as an exogenous hormone in two weeks interval followed by an injection of maturation inducing steroids (Horie et al., 2001, 2003). Maturation and ovulation of female conger eel can also be induced by manipulation of water temperature manipulation without exogenous hormone treatment (Utoh et al., 2013). It is also reported that oocyte maturation and ovulation in female conger eel can be induced by single injections of HCG followed by a booster injection of HCG and then an injection of maturation inducing steroids (Fueda et al., 2019). Although these reports demonstrated the possibility of developing seed production in this species, successful fertilization of eggs for seed production were rare. To develop a seed production technique for this species, it is necessary to improve the method for obtaining fertilized eggs in terms of quality and quantity.

C. myriaster is one of most important commercial fish species in Korea. The annual yield of fisheries were 12,600 tons in 2015 and 11,992 tons in 2020 (Statistics Korea, 2015, 2020). The conger eel is a species of high value not only as a major fishery species, but also as a new aquaculture species in Korea. Despite its importance, studies on the reproduction of conger eel in Korea have not been reported yet. To develop a method to obtain fertilized eggs, the present study examined ovarian development and performed induction of oocyte maturation and ovulation of Korean C. myriaster in captivity.

MATEIALS AND METHODS

Experimental fish

A total of 250 female conger eels (61–87 cm in total length, 343–1,381 g in weight) were obtained from an aquafarm in Goheung-gun, Jeonnam province, Korea in January 2021. They were transported to maritime and fisheries museum in Yeosu-city Jeonnam province, divided into three groups, and kept in three indoor tanks (3×3×1.5 m) containing seawater. They were fed with commercial pellets for Japanese eel throughout the experimental period.

Temperature effect on ovarian development

To examine effects of water temperatures on ovarian development of female conger eels, they were divided into three water temperature (12°C, 14°C, and 16°C) groups and reared for six months. The objective water temperature was reached by increasing the temperate at 0.5°C per day from 7°C at the commencement of the experiment. From January to July 2021, we conducted monthly sampling until April and then carried out the last sampling in July (three months later). Ten females were sacrificed after anesthetizing them with 0.1% (v/v) 2-phenoxy-ethanol (Sigma-Aldrich, St. Louis, MO, USA). Ovaries were removed and weighed to determine the gonadosomatic index (GSI=100 gonad weight/body weight). These dissected ovaries were measured to determine the diameter of the largest group of oocytes, fixed in Bouin’s solution for 24 hours, embedded in paraffin, sectioned serially at 5 μm in thickness, and then double stained with hematoxylin and eosin. Oocyte developmental stages were determined histologically as reported previously for the common Japanese conger eel (Utoh et al., 2003).

Exogenous hormonal injection

To induce oocyte maturation and ovulation of female conger eels, we conducted two experiments. Fish were anesthetized with 0.1% (v/v) 2-phenoxy-ethanol (Sigma-Aldrich) and their body weights were measured. In the first experiment, each of 10 females were intraperitoneally injected with HCG (Daesung Microbiological Labs, Korea) at 100 IU/kg or 500 IU/kg weekly for 9 weeks followed by booster injections with HCG at 1,000 IU/kg until 10–13 weeks, luteinizing hormone releasing hormone analogue (LHRHa; Sigma-Aldrich) at 400 μg/kg weekly for 13 weeks, and Salmon pituitary extract (SPE; Syndel, Nanaimo, BC, Canada) at 25 mg/fish weekly for 13 weeks. A Pit tag (Destron technologies, USA) was embedded in the muscle of the hormone treated fish for individual identification. Fishes were reared at water temperature of 16°C in FRP tank containing 3,000 liters of seawater during the experimental period. Measurement of body weight to determine the rate of increased body weight (RIW = 100 − initial body weight / initial body weight) was conducted under anesthesia once a week until 13 weeks after exogenous hormonal injection. After 9 weeks of hormone injection, developmental stages of ovaries were investigated by performing cannulation biopsies on individuals whose body weights was increased by more than 10%. In the second experiment, each of 20 females maintained at water temperature of 12°C, 14°C, and 16°C were injected intraperitoneally with HCG 1,000 IU/kg weekly for 8 weeks. Other procedure and methods of the second experiment were the same as the first experiment.

RESULTS

Effects of water temperature on ovarian development

Fig. 1 shows changes in GSI of female conger eels at water temperatures of 12°C, 14°C, and 16°C. At the start of the experiment, the value of GSI was 3.66. The value of GSI of the fish reared at water temperature of 12°C increased gradually to 4.27, 4.96, 6.29, and 7.44 in February, March, April, and July, respectively. The value of GSI of the fish reared at water temperature of 14°C increased gradually to 4.65, 4.97, 6.16, and 8.82 in February, March, April, and July, respectively. The value of GSI of fish reared at water temperature of 16°C increased gradually to 5.07, 5.75, 7.17, and 7.34 in February, March, April, and July, respectively.

Fig. 1.

Changes in gonadosomatic index (GSI) of female conger eels at water temperatures of 12°C, 14°C, and 16°C.

Fig. 2 shows changes in oocyte diameter of female conger eel at water temperatures of 12°C, 14°C, and 16°C. At the start of experiment, the range of oocyte diameter was 245.11–300.25 μm. This range of oocyte diameter of fish reared at water temperature of 12°C increased gradually to 275.34–310.71 μm, 301.68–353.45 μm, 320.27–378.24 μm and 377.62–480.27 μm in February, March, April and July respectively. The range of oocyte diameter of fish reared at water temperature of 14°C increased gradually to 293.52–327.88 μm, 331.63–344.97 μm, 334.72–381.54 μm, and 396.72–498.54 μm in February, March, April and July respectively. The range of oocyte diameter of the fish reared at water temperature of 16°C increased gradually to 257.41–330.41 μm, 346.31–373.69 μm, 384.69–469.81 μm and 382.29–475.69 μm in February, March, April and July respectively. Histological examination revealed that the follicular oocyte development was in primary yolk globule stage from January to March, and in secondary yolk globule stage from April to July until end of the experiment (Fig. 3 A and 3B).

Fig. 2.

Changes in oocyte diameters of female conger eels at water temperatures of 12°C, 14°C, and, 16°C.

Fig. 3.

Photomicrographs showing development of oocyte.

(A) PY, primary yolk globule stage. Scale bars=100 μm. (B) SY, secondary yolk globule stage. Scale bars=100 μm. (C) MN, migratory nucleus stage. Scale bars=500 μm.

Effects of exogenous hormones on ovarian development

For the first experiment, each of 10 females were intraperitoneally injected with exogenous hormones weekly for 10–13 weeks. Table 1 shows the number of individuals at different levels of RIW and stage of ovarian development after injection with various hormones. The number of individuals in 100%–110% and 110%–120% of RIW with the HCG 100 IU/kg was 3 specimens and 4 specimens, respectively after 9 weeks injection (3 specimens died), and then the number of fishes after booster injection of HCG 1,000 IU/kg changed to 2 specimens in 100%–110%, 2 specimens in 110%–120%, 1 specimen in 120%–130% and 2 specimens in 130%–140%. The number of individuals in below 100% and 100%–110% of RIW with HCG 500 IU/kg was 1 specimens and 7 specimens, respectively after 9 weeks injection (2 specimens died) and then the number of fishes after booster injection of HCG 1,000 IU/kg changed to 4 specimens in 110%–120%, 3 specimens in 120%–130% and 1 specimen in 130%–140%. The number of individuals in 110%–120% and 120%–130% of RIW with SPE 25 mg/fish was 3 specimens and 1 specimen (6 specimens died), respectively after 9 week later and then changed to 1 specimen in 100%–110%, 1 specimen in 110%–120%, 1 specimen in 120%–130% and 1 specimen in 130%–140% after 13 weeks injection. The number of individuals in below 100% and 100%–110% of RIW with LHRHa 400 μg/kg was 5 specimens and 1 specimen (4 specimens died), respectively after 9 week later and then changed to 5 specimens in below 100% and 1 specimen in 110%–120%.

Table 1.

Effects of exogenous hormones on ovarian development of Conger myriaster developmental stages of the largest oocytes

Treatment	No of individuals after 9th (10–13th) injection					No of individuals in the end of experiment
	Rate of increased body weight (%)					Developmental stage of the large oocytes (Oocyte Diameter, μm)
	100 below	100–110	110–120	120–130	130–140	PY	SY	TY	MN	GVBD
HCG (100 IU/kg)+ (1,000 IU/kg) from the 9th injection		3 (2)	4 (2)	0 (1)	0 (2)	2 (370–470)	2 (570–667)		3 (1,029–1,297)
HCG (500 IU/kg)+(1,000 IU/kg) from the 9th injection	1 (0)	7 (0)	0 (4)	0 (3)	0 (1)		7 (530–720)		1 (851–987)
SPE (25 mg/fish)		0 (1)	3 (1)	1 (1)	0 (1)	1 (250–324)	2 (481–685)		1 (837–890)
LHRHa (400 µg/kg)	5 (5)	1 (0)	0 (1)			6 (92–350)

Fishes injected with HCG 100 IU/kg and booster shot of HCG 1,000 IU/kg showed different ovarian developmental stages at the end of experiment; 2 specimens (oocyte diameter 370–470 μm) were at the primary yolk globule, 2 specimens (570–667 μm) were at the secondary yolk globule and 3 specimens (1,029–1,297 μm) were at the migratory yolk globule (Fig. 3C). However, fishes injected with HCG at 500 IU/kg and booster shot of HCG 1,000 IU/kg showed slower rate of gonadal development at the end of the experiment than previous treatment, 7 specimens (530–720 μm) at the secondary yolk globule and 1 specimen (851–987 μm) at the migratory yolk globule. After injecting SPE at 25 mg/fish, the primary yolk globule, the secondary yolk globule and the migratory yolk globule stages of ovarian development were found in 1 specimen (oocyte diameter 250–324 μm), 2 specimens (481–685 μm) and 1 specimens (837–890 μm), respectively. After injecting LHRHa at 400 μg/kg, the stages of ovarian of all experimental fishes were in the primary yolk globule (oocyte diameter 92–350 μm).

Effects of water temperature on ovarian development after injection with human chorionic gonadotropin (HCG) 1,000 IU/kg

Table 2 shows numbers of individuals at different levels of RIW and stages of ovarian development at water temperatures of 12°C, 14°C, and 16°C after injecting HCG at 1,000 IU/kg. Each of 20 females was intraperitoneally injected with HCG at 1,000 IU/kg weekly for 8 weeks. At water temperature of 12°C, 2, 10 and 7 specimens had RIW of 110%–120%, 120%–130%, and 130%–140%, respectively. At water temperature of 14°C, 1, 9, and 8 specimens had RIW of 110%–120%, 120%–130%, and 130%–140%, respectively. At water temperature of 16°C, 5, 10, and 5 specimens had RIW of 110%–120%, 120%–130% and 130%–140%, respectively. On regarding ovarian development at water temperatures of 12°C, 14°C, and 16°C, 19, 18 and 20 specimens were found to be in secondary yolk globule stage, migratory nucleus stage, and secondary yolk globule stage respectively.

Table 2.

Effects of HCG at 1,000 IU/kg on ovarian development of Conger myriaster at various water temperatures

Temp.	No of individuals after 8th injection					No of individuals in the end of experiment
	Rate of increased body weight (%)				Developmental stage of the large oocytes (Oocyte diameter, μm)
	100–110	110–120	120–130	130–140	PY	SY	TY	MN	GVBD
12°C	0	2	10	7		19 (552–790)
14°C	0	1	9	8				18 (890–1,303)
16°C	0	5	10	5		20 (564–729)

DISCUSSION

Research on conger eels is mainly conducted in the field of ecology and biological resources such as feeding ecology (Huh & Kwak, 1998; Jeong et al., 2002; Choi et al., 2008), age and growth (Kim et al., 2011), diet compositions (Kim et al., 2020), and so on. There are very little information on the reproduction of Korean conger eels. Thus, we conducted this experiment.

The reproduction of teleost fishes is controlled by environmental factors such as day length and water temperature (De Vlaming, 1972; Munro, 1990). Manipulation of these environmental factors are proven and useful tool for managing egg production in aquaculture (Pankhurst et al., 1996). In Japanese conger eels that reared in captivity, ovarian development of female progresses to secondary yolk globule stage without exogenous hormone treatment when maintained at water temperature from 10 to 20°C (Kajimura et al., 2001; Utoh et al., 2003, 2004, 2005; Chiba et al., 2005). However, ovarian development in all females was halted at the secondary yolk globule stage. In the cultured conger eels of korea, the ovarian development of female progressed to the secondary yolk globule stage without exogenous hormone treatments when reared at water temperatures that varied from 12 to 16°C. It also halted for four months. During the ovarian development of conger eels, diapause of oogenesis in the secondary yolk globule stage in varied range of water temperature needs to be solved in terms of evolutionary strategy of the species.

Values of GSI and oocyte diameter provide valuable information about ovarian development of females. Values of GSI in the primary yolk globule stage and the secondary yolk globule stage were 3.66–5.07 and 5.75–8.82 for conger eels of Korea and 4.33 and 9.70 for Japanese conger eels (Utoh et al., 2003), respectively. Oocyte diameter in the primary yolk globule stage and the secondary yolk globule stage were 245.11–330.41 μm and 320.27–498.54 μm for conger eels of Korea and 200–350 μm and 300–500 μm for Japanese conger eels (Utoh et al., 2003), respectively. These GSI values and oocyte diameters of conger eels of Korea were not significantly different from those of Japanese conger eels in captivity, suggesting that our experimental system was successfully established to study ovarian development of conger eels in Korea.

For Japanese conger eels, oocyte maturation and ovulation can be successfully induced by solely changing the water temperature without exogenous hormone treatments (Utoh et al., 2013). However, the rate of ovulation induction was very low and more fertilization was not successful. Horie et al. (2001; 2003) reported that maturation and ovulation of oocytes of female conger eels can be induced by repeated injections of HCG at 0.1 IU/g BW, 17, 20β-dihydroxy-4-prognen-3-one, 17α-hyroxyprogesterone (17α-OHP). The progress from the secondary yolk globule stage to maturation of oocyte can be induced by injecting fishes with HCG at 100 IU/kg every two weeks. However, in female conger of Korea, ovarian development of fish treated with HCG at 100 IU/kg or 500 IU/kg for 9 weeks remained at the secondary yolk globule stage. The progress from diapause of the secondary yolk globule stage to migratory nucleus stage of oocytes can be induced by HCG at 1,000 IU/kg. Differences in effects of these hormones might be due to differences of products from different companies. However, further studies are needed to explore other possibilities. SPE is the most effective one among hormones used for inducing ovarian development in female Japanese eels. HCG induced the maturation of oocytes more effectively in both conger eels in Korea and Japanese conger eels than SPE.

The vitellogenesis, maturation and ovulation of oocytes are regulated by a cascade of hormones along the brain–pituitary–gonad (BPG) axis. In this axis, secretion of pituitary gonadotropins is controlled by gonadotropin releasing hormones (GnRHs) from the hypothalamus (Peter & Yu, 1997; Yu et al., 1997). It is known that synthetic GnRHs are an order of magnitude more potent than their native peptides. The use of GnRH peptides for ovarian development induction has important advantages over the use of GTH preparations. GnRH and its agonists are small decapeptides that do not trigger an immune response. Thus, they can be used repeatedly without reduction in their efficacy (Zohar & Mylonas 2001). Female conger eels in Korea treated with LHRHa at 400 μg/kg did not show any response to the hormone. Instead, regression of ovarian development was found. This phenomenon is very rare. Further research is needed to clarify it.

It has been reported that conger eels are very sensitive to handling stress. Many females (between 50% and 81%) will die during the handling associated with repeated injections necessary for inducing maturation. Fertilizable eggs could not be obtained from females that had been handled >12 times (Horie et al., 2003). In the present study, ovarian development stage proceeded only to the migration nucleus stage. It was highly likely to be caused by the handling stress.

Anguilla species have similar reproductive life cycles such as extensive oceanic migration for maturity and spawning with leptocephalus stages and metamorphosis to glass eels (Miller et al., 2011). The spawning area of Japanese conger eels based on the survey of preleptocephalus larvae has been suggested to be the area along the Kyushu-Palau Ridge approximately 380 km south of Okinotorishima Island (Kurogi et al., 2012). However, it is still unknown whether conger eels in Korea spawn in the same sea area. The effect of hormone treatment on ovarian development in Japanese conger eel was the most effective at a water temperature of 10°C. In conger eels of Korea, the effect of hormone treatment on ovarian development was the most effective at a water temperature of 14°C. In the future, more precise research on breeding water temperature during hormone treatment is needed.

It is the first report on effect of water temperature and hormones on ovarian development of conger eel in Korea. In the future, more effort is needed to obtain high-quality ovulated eggs from female conger eels, but this study is the beginning of a meaningful challenge.