1. Introduction
Hibiscus rosa-sinensis L., commonly known as “Chinese Hibiscus”, is an evergreen perennial plant that grows in tropical and sub-tropical regions. It has a charismatic bright red, five-petal, and single layer flower, and the leaves are alternate along the branch.
Pharmacological investigations of the genus Hibiscus indicated the existence of some species with interesting biological activities such as anti-hypertensive [1], anti-inflammatory [2], hepato-protective [3], anti-tumoric [4], anti-diabetic [5], anti-convulsive [6], anti-oxidative [7,8], and anti-mutagenic [9,10].
Traditional propagation of Hibiscus spp. is dependent on vegetative means such as cuttings or grafting. Vegetative propagation can shorten the length of the juvenile period and also allows genotypes combination [11]. However, such traditional asexual propagation cannot circumvent the very fundamental problems of long growing period, large growing space, small plant quantity, and inefficiency. After approximately 100 years of developmentplant tissue culture technique provides an alternative to solving those problems. In this propagation method, only small pieces of plant tissue are required to regenerate on plant tissue culture medium under sterile conditions. The plant tissues can be the internodes, nodes, shoot tips (stems), root tips, calli, leaves, seed embryos, or anthers.
Due to the strikingly encouraging effects of plant growth regulator (PGR) in accelerating, inducing, and maintaining in vitro shoots, direct in vitro shoots establishment and multiplication from explants often involve the application of PGRs such as 6-benzylaminopurine (BAP) [12, 13], zeatin [14], BAP plus kinetin (KIN) [15], BAP plus indole-3-acetic acid (IAA) [16], or BAP plus naphthalene-3-acetic acid (NAA) [17]. Christensen et al. [13]) reported that the most suitable multiplication medium for H. rosa-sinensis L. was demonstrated to be a modified Murashige and Skoog (MS) medium containing 2.2 μM BAP and increased concentrations of calcium at 9 mM and iron at 295 μM provided as ethylenediamine di-2-hydroxyphenyl acetate ferric (Fe-EDDHA). Bhalla et al. [18] modified the MS medium strength coupled with BAP in inducing direct shooting from H. rosa-sinensis but concluded that BAP was not suitable in their study. While in other hibiscus species, H. cannabinus (kenaf), Herath et al. [12] reported that 8.8 μM of BAP was the best treatment, but was contradicting Zapata et al. [19] who revealed BAP at 4.4 μM completely suppressed shoot growth of kenaf. Both reports again contradicted Ayadi et al. [20] who found that the additions of PGRs [BAP, NAA, and indoleacetic acid (IBA)] to the MS medium were detrimental to the cultures as they reduced buds formation, inhibited shoots growth and roots induction. Hence, it seems crucial that focus be targeted at the medium ingredients rather than exogenous supplementation of PGRs in inducing shoots formation or elongation, as an alternative to optimize direct in vitro shoot establishment and multiplication of hibiscus explants.
In this paper, we present the results on the effectiveness of shoot induction through modification of the MS medium ingredients, without involving any PGRs. We also report the effectiveness of sodium hypochlorite (NaOCl) in controlling the balance between contamination and survival levels for three types of H. rosa-sinensis L. vegetative explants, and highlight the optimized conditions for explants sterilization of this plant species, which were harvested from open field. Since most of the reported studies on hibiscus species were focused on samples obtained from plants grown in greenhouses, this paper provides alternative reference for plants grown in the open fields.
2. Materials and Methods
2.1. Culture Medium
All the media used were based on MS basal salts and vitamins [21]. No PGR was added. For media used in the sterilization process, 20 g/L of sucrose was added to half strength MS (1/2 MS) basal medium while for subsequent direct shoot induction, different sucrose concentrations (10, 20, 30, 40, 50 g/L), activated charcoal [0.1, 0.2, 0.3, 0.4 and 0.5% (w/v)] and different combinations of organic ingredients [myoinositol + thiamine.HCl, myoinositol + thiamine.HCl + nicotinic acid, myoinositol + thiamine.HCl + pyridoxine.HCl, myoinositol + thiamine. HCl + nicotinic acid + pyridoxine.HCl, and myoinositol + thiamine.HCl + nicotinic acid + pyridoxine.HCl + glycine] were tested. The pH of the medium was adjusted to 5.7 - 5.8 using 1 M NaOH before adding 2.7 g/L gelrite agar (for sterilization study) or 1.6 g/L gelrite agar (for organogenesis). The medium was autoclaved at 121˚C for 15 min. In the sterilization study, the explants were cultured on solid medium in Petri dishes while for shoot induction, the explants were placed on solid medium in culture tubes (diameter: 2.5 cm; height: 10 cm). Each treatment consisted of 50 replicates and the whole experiment was carried out twice.
2.2. Explant Surface Sterilization
Three types of explants—shoot tip, node, and internodewere harvested from young shoots of H. rosa-sinensis L. plants (the shoot harvested contained a maximum of three nodes counting from the shoot tip) that grew beside the Sultan Abdul Samad Library, Universiti Putra Malaysia, Selangor Darul Ehsan, Malaysia, and was authenticated with the Voucher Specimen Number: SK1560/08.
The nodes, internodes and shoot tips were cut into 2 cm long before washing under running tap water for 30 min. One drop of detergent (Dynamo) was added into the water and the washing was continued for an additional min. The detergent was removed under the running tap water and the explants were rinsed with distilled water three times. Commercial Clorox solution [5.25% (w/v) NaOCl] diluted to concentrations ranging from 5 to 50% (v/v), were tested on decontaminating all explants except the shoot tips, which were only subjected to 5% to 20% (v/v) of the Clorox solution. All treatments (except for shoot tips) were subjected to a Clorox exposure time ranging from 5 to 30 min at 5-min intervals; while for shoot tip, it was 10 to 60 min exposure time at 10-min intervals (Table 1). One drop of Tween-20 was added to the Clorox solution prior to sterilization. After each treatment, the explants were thoroughly washed with sterile deionized water 3 times [22], each comprising 10 min. After the sterilization steps above and prior to culturing on the nutrient medium, each node, internode and shoot tip explants were trimmed into 1 cm length. Each treatment for the node and internode explants, respectively, consisted of 45 replicates, while shoot tip comprised of 25 replicates due to limited samples. All cultures were maintained at 27˚C ± 1˚C under a 16 h-photoperiod provided by cool-white fluorescent tubes at 25 mMol photon/m2/s.
For sterilization, observation was taken daily for 35 days to record the percentages of contamination and survival of the explants. All experiments were carried out twice.
2.3. Direct Organogenesis
Sterile nodal explants were cultured in tubes containing the relevant MS medium formulation (as described previously in culture medium). The nodal explants were first subjected to treatment of different concentrations of sucrose. Following which, the optimized sucrose concentration was chosen for subsequent assessment of the organic ingredients and activated charcoal. The explants were maintained at 27˚C ± 1˚C under a 16 h-photoperiod provided by cool-white fluorescent tubes at 25 mMol photon/m2/s. Observation was taken weekly for 6 weeks to
Table 1. Explants treatments at different Clorox concentrations and exposure times. Data were taken after 35 days of culture which were displayed as survival and contamination percentages: (a) Node; (b) Internode; (c) Shoot tip. “C” denotes control. The numbers followed by different superscript letters (a, b, c, d, e) within a column are significantly different at p < 0.05 by Duncan’s multiple range test (DMRT). Data is the mean ± standard deviation (SD). Means are the results of 2 experiments.
record the percentages of survival and regeneration of explants, mean leaf length (cm), and mean number of leaf. All experiments were carried out twice.
2.4. Statistical Analysis
The experiments were performed in a completely randomized design (CRD). Data were subjected to one-way analysis of variance (ANOVA) using SPSS version 16 software (SPSS Inc., Chicago, USA). Multiple comparisons among means were performed using Duncan’s multiple range test with the level of significance at p = 0.05.
3. Results and Discussion
3.1. Explant Surface Sterilization
Three types of explants (node, internode and shoot tip) were obtained from young hibiscus stems and subjected to different surface sterilization conditions as summarized in Table 1. The best sterilization condition for each explant type was scored based on the highest survival rate with minimal contamination.
The results show that nodal explants is the most difficult to sterilize, followed by shoot tip and internode. The nodal explant (node) bears an axillary bud located in a “V” shape trough, formed between the main stem and leaf petiole. Such shape easily traps contaminants and poses a barrier to water current during sterilization. The internodal explant has a smooth and small surface area compared to the other two explants (node and shoot tip) used in this study. A smooth surface is a poor “landing site” for microbial attachment because they are often easily ousted under strong water current, and hence, a lower chance for the explants to get contaminated. Both of these characteristics seem to contribute to a low contamination percentage (<10%) and high survival rate (>80%) as observed for 90% of the treatments (Table 1(b)).
For the shoot tip and nodal explants, the results show that increasing Clorox concentration with short exposure time was not effective in removing contaminants. For a 5-min exposure time, the contamination percentage using 5% (v/v) Clorox is comparable to almost all the Clorox levels tested. However, increasing the exposure time seems to be more favorable. Indeed, most researchers used longer exposure time (≥10 min) for nodal explant sterilization from varying plant species [23-25]. If a shorter exposure time is required, usually HgCl2 is used [26,27]. In this study, 75% of the treatments were able to confine the contamination percentages within 20%, and the explants survival percentages within the range of 30% - 70%. The best treatment for the node is 40%—20 min [2.1% (w/v) NaOCl)], a concentration comparable to that of the seeds from other plants [28,29]. It is interesting to find that Christensen et al. [13] applied 0.01% (w/v) NaOCl for H. rosa-sinensis nodal explants sterilization, a dose 210 times lower than the best treatment for the nodal explants found in this study. Such discrepancies could be attributed to the location of the sampling site—greenhouse versus open environment. This indicates that by controlling the plants’ exposure to outside environment can limit the level of contamination on the plant itself.
By taking into account of both the contamination and survival percentages, 10% - 15% min is the best treatment for the internode. Internodal explants subjected to this treatment did not show any contamination and almost all survived (Table 1(b)). However, under a situation where both the nodal and internodal explants were to be subjected to the disinfectant treatment simultaneously, 40% - 20% min is applicable because both the contamination and survival percentages are not affected significantly (Tables 1(a) and (b)).
The shoot tip was found to be susceptible to dehydration after being excised from the mother plant. We found that the shoot tips did not survive with 30% (v/v) Clorox or higher and also when the sterilization time was 10 min or more. The best treatment for shoot tip is 5%—40 min [0.2625% (w/v) NaOCl], a treatment comparable to Jo et al. [30] who used about 0.15% (w/v) of NaOCl with 30 min exposure for shoot tip of Alocasia amazonica. In contrast, Misra and Chakrabarty [22] used higher concentration4% (w/v) NaOCl, and shorter exposure time, 5 min, to sterilize Rosa clinophylla shoot tip.
3.2. Direct Organogenesis
Apart from exogenous supply of PGRs, growth and induction of in vitro shoots are influenced by exogenous carbon source. The in vitro plants are either heterotrophic or semi-autotrophic, and hence an external supply of carbon is necessary. Sucrose is readily hydrolysed into glucose and fructose during autoclave, with the former being used up first and then fructose. Sucrose at 30 g/L (standard MS medium) was used for H. rosasinensis [13,18], H. cannabinus [12,20], H. sabdariffa [31,32] and other in vitro cultures. From the results obtained (Figure 1(a)), 10 and 20 g/L of sucrose were unsuitable for shoot induction. Growth of the shoots improved significantly at 30 g/L or higher. Further increment at 40 g/L showed that 30% of the explants regenerated, and the mean number of leaves produced and mean leaf length achieved were the highest. However, sucrose of more than 40 g/L did not improve the regeneration or the growth rates of the explants.
Four types of vitamins (myo-inositol, thiamine, pyridoxine, and nicotinic acid) and one amino acid, glycine were present in the standard MS medium formulation. Of the five supplements, myo-inositol and thiamine are essential for the culture of plant cells in vitro. Thiamine is an essential co-factor in carbohydrate metabolism and is involved in the biosynthesis of certain amino acids in its active form, thiamin diphosphate [33]. Plant cells and tissues could produce some essential vitamins in vitro but at a sub-optimal level, hence an exogenous supply of vitamin is always crucial. Similar to other plant species, all vegetative propagations of H. rosa-sinensis as reported involved the complete MS organic supplementations [13, 18,34]. In contrast to previous reports, the results obtained in this study (Figure 1(b)) revealed that shoots induction with myoinositol and thiamine (MT) supplementations only were achieved at a percentage higher than that with myoinositol, thiamine, and nicotinic acid (MTN). However, the shoots grown with organic supplements consisted of MTN gave better qualitative results of greenier and healthier-looking shoots (result not shown).
Activated charcoal or carbon (AC) had been reported to be a useful supplement in the plant tissue culture medium for several purposes such as improving rooting [35], shoot elongation [36], preventing necrosis [37], and preventing browning [38]. The fine network of pores and large surface area of AC serves as a useful scavenger to adsorb inhibitory phenolic compounds. As shown in Figure 1(c), nodal explant cultured on medium augmented with 0.3% (w/v) of activated charcoal achieved the highest shoot regeneration rate (40%) at the 3rd week. Leaf abscission and shoot necrosis were delayed until the 6th week,
Figure 1(c). However, further increment of AC concentration did not improve the observable growth performance of the shoots as shown in Figure 1(c). This may be due to adsorption of the nutrient ions (Cu2+ or Zn2+) and other organic supplements (vitamins) in the medium by the excess amount of AC resulting in lower amounts of nutrients and supplements being made available to the growing cultures [39].