Acute toxicity of jalawure ( Tacca leontopetaloides (L.) Kuntze) and gadung tikus ( Tacca palmata Blume) using zebra(cid:976)ish ( Danio rerio ) embryos as a model

jalawure leaves extract expressed moderate toxicity level.

gadung tikus, jalawure, Tacca, toxicity, zebra ish A Tacca is a genus of several species reported to have potential as a new therapeutic agent with toxic properties for several cells. Jalawure and gadung tikus are two species from the Tacca genus that can be found in Indonesia. The aim of this study was to determine the level of acute toxicity of jalawure and gadung tikus by using zebra ish (Danio rerio) embryos as a model. The sample was extracted by maceration using ethanol 96%. The acute toxicity test was carried out by using ish embryo acute toxicity (FET) test protocol No. 236, Organisation for Economic Co-Operation and Development (OECD), 96 hr of static exposure using the negative control group (medium embryo), the test solution group (extract) and the positive control group (3,4-dichloroaniline 4 µg/ml). The result of acute toxicity of extract against zebra ish embryos demonstrated that LC 50 of jalawure leaf extract 26.06 ± 0.31 µg/ml, jalawure stem extract 251.52 ± 6.15 µg/ml, jalawure corm extract 463.24 ± 9.68 µg/ml, gadung tikus leaf extract 15.04 ± 0.15 µg/ml, gadung tikus stem extract 263.73 ± 6.58 µg/ml, and gadung tikus corm extract 17.71 ± 0.12 µg/ml. Embryo coagulation was the endpoint that was most commonly found in almost all extracts. Gadung tikus leaves extract, gadung tikus corm extract and jalawure leaves extract expressed moderate toxicity level.

INTRODUCTION
Various plants have been widely used as medicine and therapy in most parts of human life. Research has succeeded in obtaining information about the therapeutic effects, use and development of plants into herbal medicine (Yin et al., 2013;Jamshidi-Kia et al., 2018).
In 1963, Scheuer puri ied a compound called taccalin, which was isolated from the jalawure corm. Taccalin is a compound with bitter yellow powder and has a tetracyclic structure. Then in 1988, several taccalonolides compounds were isolated from the Tacca genus. Taccalonolide is a group of highly oxidized steroid-derived compounds. In addition, the withanolides compounds and their glycosides were also isolated. These compounds have been shown to have cytotoxic effects on several cancer cell line by different mechanisms. The compound group was isolated from Tacca plantaginea (Hance) Drenth, Tacca sub labellata PP Ling & CT Ting and Tacca integrifolia Ker Gawl (Jiang et al., 2014;Risinger and Mooberry, 2010).
Based on the concept of Linnaeus in the 18 th cen-tury, which stated that plants, especially those that have similar morphological characteristics, generally also contained similar chemical substances. The discovery of these compounds from several types of Tacca with cytotoxic effects is possible for several other types, such as Tacca leontopetaloides and Tacca palmata, which belong to the same family also contain compounds that have the potential to have toxic effects.
Zebra ish (Danio rerio) is now widely used as a powerful research model in biology and medicine. Zebra ish could be used as a model organism for toxicity screening before the more expensive mammalian models will use. Zebra ish embryos and larvae are small in size and transparent, so they are very easy to test using multi-wells and observe embryo and larval development (Belyaeva et al., 2009;Kanungo et al., 2014). Based on the zebra ish genome sequencing of TuAB strains, in 2001 (Sanger Institute) informed that more than 71% of the genes encoding proteins in humans have at least 1 gene that is orthologous in zebra ish (Avdesh et al., 2012;Howe et al., 2013). So, this study aims to determine the acute toxicity of the jalawure and gadung tikus using zebra ish embryos as a model.

MATERIALS AND METHODS
Jalawure (Tacca leontopetaloides (L.) kuntze) was obtained from the BP3K Cikelet Garut, West Java and was determined at the Bandungese Herbarium, School of Biological Science and Technology -Bandung Institute of Technology. Gadung Tikus (Tacca palmata Blume.) was obtained and was determined at Bogor Botanical Garden, West Java, meanwhile zebra ish (Danio rerio) was obtained from Laksana aquarium Bandung and was determined at the Museum of Zoology, School of Biological Science and Technology -Bandung Institute of Technology.

Extraction process
One hundred gram crude drug of jalawure and gadung tikus parts (leaves, stem and corm) were macerated with one liter of 95% ethanol for 24 hr at room temperature, the macerate was iltered and the residue was re-extracted twice using the same method. The macerate was collected and then concentrated with a rotary evaporator.

Zebra ish maintenance and embryos handling
This study used zebra ish (Danio rerio) embryos less than 3 hpf (hours post fertilization), which were cultured in the laboratory. These embryos were obtained from adult male and female zebra ish aged 4-5 months, healthy and normal. The male and female zebra ish were separated for at least 1 week before mating.
The water circulation in the aquarium was continuously regulated by means of an aerator and ilter system. Room temperature and water temperature were around 26-28.5 • C with a pH between 6.8-7.5 and the lighting conditions 14 hr light and 10 hr dark. If necessary, the pH can be adjusted by adding sodium bicarbonate. Aquarium was cleaned regularly about 1-2 times a week, with a replacement of water 2/3 the volume of the aquarium. Fish were fed about 1-2 times a day and if the ish are to be spawned, they were fed 2-3 times a day about 1-5% of the bodyweight of the ish (Avdesh et al., 2012;Harper and Lawrence, 2011).
Zebra ish embryos were produced through spawning groups. Male and female zebra ish (2:1) in the spawning group were placed in the spawning aquarium several hours before the dark phase. Embryos were collected from a minimum of three spawning groups, mixed and randomly selected to avoid a genetic bias. If deemed necessary, arti icial plants made of an inert material (e.g. plastic or glass) can be attached to the spawning aquarium as a stimulus. Mating, spawning and fertilization take ± 30 min after the light phase and the spawning nets were carefully removed. The collected embryos can be cleaned carefully. It is recommended to rinse embryos with medium after collection from the spawning aquarium (Busquet et al., 2013).

Preparation of medium zebra ish embryos
The embryo medium (E3) was used as a medium to deliver the test extract solution during testing. Prepare E3 medium by making a stock solution (60x concentration) consisting of 34.8 g NaCl; 1.6 g KCl; 5.8 g CaCl 2 .2H 2 O and 9.78 g MgCl 2 .6H 2 O were dissolved in 2 liters of distilled water and adjusted the pH to 7.2 with NaOH solution. E3 60x medium stock solution was stored at 4 • C. The solution was diluted to E3 1x solution by taking 16.5 ml of stock solution 60x with distilled water to 1 liter and added 100 µl 1% methylene blue as a fungicide (Cold Spring Harbor Protocols, 2019).

Acute toxicity test using zebra ish embryos
The test referred to the protocols from the Organization for Economic Co-operation and Development (OECD) No. 236, 2013. Acute toxicity test of zebra ish embryos using ive test concentration. The highest concentration should give a 100% mortality after 96 hr of exposure and the lowest concentration should give a 0% mortality. The inding range test aims to determine the appropriate concentration.
Zebra ish embryos (0.5-2 hpf) were collected and acclimatized for 2-3 hours in E3 1x medium at room temperature 28 • C. Selection of zebra ish embryos, 20 zebra ish embryos were inserted into well plates-24 (capacity 2.5 -5 ml). The medium was carefully exchanged with the test sample (1 concentration/well plate-24), covered the well plate-24 with aluminum foil then incubated at 28 • C. The observation was carried out for 96 hr (static exposure) and observed every 24 hr using a stereomicroscope (Olympus CKX41) at 4-10X magni ication. Four endpoints were observed, 1. Coagulated embryo, 2. Lack of somite formation, 3. Non-detachment of the tail, and 4. Lack of heartbeat.
After 96 hr of observation, data from the four endpoints above were recorded and calculated to determine the LC 50 value. 3,4-dichloroaniline 4 µg/ml per well plate-24 with 20 embryos was used as a positive control. Meanwhile, E3 medium with 24 embryos per well plate-24 as a negative control (Busquet et al., 2013).

Data analysis
A probit analysis was performed on the percent embryo mortality data. The probit value of percent mortality is plotted as the Y and the log of concentration as the X. From this data, a line plot is obtained with the equation Y = aX + b and linearity (R 2 )
All extracts positive contained saponins. It was similar to the previous study by (Abdel-Aziz et al., 1990), with identi ied the presence of steroidal sapogenin compounds from acid hydrolysis in jalawure leaves extract. Saponins had toxic properties to the embryo based on Hassan et al. (2008) research that saponin isolated from Quilajja Saponaria at a concentration above 5 µg/ml caused 100% zebra ish embryo mortality.

Finding range
Finding range is used to determine the ive test concentration. The highest concentration should give a 100% mortality after 96 hr of exposure and the lowest concentration should give a 0% mortality (Figure 1). The inding range test aims to determine the appropriate concentration. Five test concentrations were calculated by arithmetic methods from the highest and the lowest concentration.

Lethal concentration 50% (LC 50 ) of extract
Previous studies presented that several plants from the Tacca family have the potential to be developed as anticancer agents (Tinley et al., 2003;Peng et al., 2011;Li et al., 2014), but the safety effect of the compounds has not been reported. Exposure jalawure extracts and gadung tikus extracts at certain concentrations caused embryotoxicity, as assessed from the hatching rate and defects in the zebra ish embryo. In this study, the effects of exposure of some jalawure extracts and gadung tikus extracts will be exposed, which cause death and malformation of zebra ish embryos as a test model. The percentage of zebra ish embryo mortality increased with increasing concentration of the test sample ( Figure 2).
Four endpoint observations were made to determine lethality. If one of these four endpoints was found, it indicated embryonic death. Coagulation is characterized by the embryo appearing white in color and black clumps under the microscope. Damage to the somite form of the embryo can be characterized by the absence of somite formation after 48 hr of exposure. Somite deformities and nondetachment of the tail are almost never found in this test. Heart rate can be observed after 48 hr of exposure, normal embryo heart rate > 80 times per min. If no heart rate or less than 80 times per min, it indicated embryo death.
The LC 50 value indicated the concentration of the extract that caused 50% mortality in zebra ish embryos, which was obtained from the results of the probit regression analysis during 96 hr of exposure (Table 2). Kovriznych et al. (2013) referred to the guideline ON 46 6807 (1988) classi ied the level of toxicity based on the LC 50 value of a substance namely, concentration <1 µg/ml (high toxic), concentration 1-10 µg/ml (toxic), concentration 10-100 µg/ml (moderate toxic), concentration 100-1000 µg/ml (low toxic).

Coagulated embryo
Embryo coagulation was the endpoint that was most commonly found ( Figure 3). Some extracts also provided an endpoint in the form of cessation of embryo development due to weakness and even loss of heart rate and failure of embryo hatching. Lack of pigment, swelling of the abdomen and malformation of the tail also occurred at a certain concentration, but these data were not calculated as the endpoint for the lethal concentration of 96 hr of exposure.

Extract characterization
The three extracts with moderate toxicity then were tested for characterization. The characterization was included, determination of water content, total ash content and acid insoluble ash content (Table 3).
Characterization was carried out in order to ascertain the character of each extract with a speci ic pharmacological effect. The total ash content indicated minerals from combustion either as natural minerals needed by plants or as environmental contaminants. GTLE, as the sample with the smallest LC 50 value, had the highest total ash content and acid insoluble ash value than the other two samples. The possibility of mineral oxides as insoluble acid ash also affected the level of extract toxicity. In addition, differences in plant parts also affect the amount of extract water content. Where both leaves extracts had higher water content compared to corm extract.