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Article

Enhancing Centelloside Production in Centella asiatica Hairy Root Lines through Metabolic Engineering of Triterpene Biosynthetic Pathway Early Genes

by
Miguel Angel Alcalde
1,2,
Javier Palazon
1,*,
Mercedes Bonfill
1 and
Diego Hidalgo-Martinez
1,*
1
Department of Biology, Healthcare and the Environment, Faculty of Pharmacy and Food Sciences, University of Barcelona, 08028 Barcelona, Spain
2
Biotechnology, Health and Education Research Group, Posgraduate School, Cesar Vallejo University, Trujillo 13001, Peru
*
Authors to whom correspondence should be addressed.
Plants 2023, 12(19), 3363; https://doi.org/10.3390/plants12193363
Submission received: 18 August 2023 / Revised: 20 September 2023 / Accepted: 22 September 2023 / Published: 23 September 2023
(This article belongs to the Special Issue Secondary Metabolites in Plants)
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Abstract

:
Centella asiatica is a medicinal plant with a rich tradition of use for its therapeutic properties. Among its bioactive compounds are centellosides, a group of triterpenoid secondary metabolites whose potent pharmacological activities have attracted significant attention. Metabolic engineering has emerged as a powerful biotechnological tool to enhance the production of target compounds. In this study, we explored the effects of overexpressing the squalene synthase (SQS) gene and transcription factor TSAR2 on various aspects of C. asiatica hairy root lines: the expression level of centelloside biosynthetic genes, morphological traits, as well as squalene, phytosterol, and centelloside content. Three distinct categories of transformed lines were obtained: LS, harboring At-SQS; LT, overexpressing TSAR2; and LST, simultaneously carrying both transgenes. These lines displayed noticeable alterations in morphological traits, including changes in branching rate and biomass production. Furthermore, we observed that the expression of T-DNA genes, particularly aux2 and rolC genes, significantly modulated the expression of pivotal genes involved in centelloside biosynthesis. Notably, the LS lines boasted an elevated centelloside content but concurrently displayed reduced phytosterol content, a finding that underscores the intriguing antagonistic relationship between phytosterol and triterpene pathways. Additionally, the inverse correlation between the centelloside content and morphological growth values observed in LS lines was countered by the action of TSAR2 in the LST and LT lines. This difference could be attributed to the simultaneous increase in the phytosterol content in the TSAR2-expressing lines, as these compounds are closely linked to root development. Overall, these discoveries offer valuable information for the biotechnological application of C. asiatica hairy roots and their potential to increase centelloside production.

1. Introduction

Centella asiatica, commonly known as Gotu Kola, is a renowned medicinal plant with a rich history of traditional use in various cultures for its therapeutic properties [1]. Among its numerous plant secondary bioactive compounds are centellosides, a group of triterpenes that have attracted considerable attention due to their potent pharmacological activities, including anti-inflammatory, antioxidant, and wound-healing effects. The high medicinal value of centellosides has prompted extensive research aimed at understanding their biosynthesis and developing strategies to enhance their production [2].
The biosynthetic pathways of secondary metabolites, including centellosides, are complex and tightly regulated processes. In plants, secondary metabolite production is influenced by various factors, such as gene expression, enzymatic activity, and metabolic flux. Among the key regulatory components are phytosterols; these primary metabolites and membrane constituents serve as precursors for various hormones and play a crucial role in determining the production of specific triterpenes. It has been observed that when sufficient phytosterols have been synthesized to meet the plant’s growth requirements, the biosynthesis of triterpenes takes precedence [3,4].
Metabolic engineering has emerged as a powerful biotechnological tool to manipulate the biosynthetic pathways of secondary metabolites in plants. By introducing specific genes into plant cells, researchers can modulate gene expression and metabolic pathways to enhance the production of desired compounds [5,6]. In the context of centellosides, studies have focused on manipulating key biosynthetic genes to augment their yields in C. asiatica.
One such gene of interest encodes squalene synthase (SQS), a key enzyme in the biosynthesis of triterpenes [4,7]. By overexpressing the SQS gene, it is possible to increase levels of the precursor squalene, potentially leading to higher centelloside production. The engineering of secondary metabolite production also involves transcription factors (TS) [8,9]. For example, TSAR2 (triterpenoid saponin activating regulator 2) has been identified as having a direct effect on the expression of the HMGR gene, which encodes 3-hydroxy-3-methylglutaryl-coenzyme A reductase, an important enzyme in the triterpene biosynthetic pathway [10,11,12]. The overexpression of the HMGR gene has shown promising results in increasing phytosterol and triterpenoid content in different plant species [11,13,14].
Hence, the generation of C. asiatica hairy roots harboring SQS and TSAR2 offers a potential opportunity to enhance centelloside yields. In this study, we explored the impact of these genetic modifications on the expression of centelloside pathway genes and morphological traits in different C. asiatica hairy root lines. Additionally, we examined the correlation between squalene, phytosterol, and centelloside contents in the transformed roots, aiming to elucidate the regulatory mechanisms underlying centelloside biosynthesis in this medicinal plant.
The findings from this study could offer valuable insights into the biotechnological potential of C. asiatica hairy root lines and pave the way for novel approaches to enhance centelloside production. Ultimately, these advancements could provide the pharmaceutical and cosmeceutical industries with a sustainable source of centellosides and help to unlock their therapeutic potential for various health applications.

2. Results

2.1. Integration of Transgenes by PCR

In the present study, we obtained four different types of hairy root lines: LS, carrying the exogenous SQS gene from A. thaliana; LT, which contains the transcription factor TSAR2; LST, with both of the aforementioned genes; and L1, utilized as the control. These hairy root lines harbored all the rol and aux genes from the pRi plasmid of R. rhizogenes.
Genomic DNAs from transformants and C. asiatica leaves were used for PCR analysis of multiple lines (Figure S1). Initially, the rolC gene served as a positive control to confirm the transformed nature of the obtained roots, given its involvement in hairy root formation. Following three rounds of selection with cefotaxime, the VirD gene was utilized to verify the absence of R. rhizogenes in the transformants, as this gene is present in the bacterial plasmid but not in the T-DNA region integrated in plant cells. The results demonstrated the presence of the rolC gene in R. rhizogenes (positive control) and the transformants but not in C. asiatica leaves (negative control). Conversely, the VirD gene was absent in all the lines. Finally, the presence of the target genes, At-SQS and TSAR2, was verified, and the following lines were selected for further analysis: LST(1-3), LS(1-3), and LT(1-3).

2.2. Influence of Transgenes on Endogenous Gene Expression

By conducting a genetic expression analysis, we explored the impact of the At-SQS and TSAR2 transgenes on the centelloside biosynthetic genes. The results, illustrated in Figure 1, depict the expression profiles of the targeted endogenous genes.
The expression of the HMGR and SQS genes differed notably among the examined lines. Specifically, lines overexpressing TSAR2 exhibited significantly elevated expression levels of these two endogenous genes compared with the control. A correlation analysis revealed a strong positive correlation (r = 0.98) between HMGR and SQS, suggesting that TSAR2 enhances the expression of these genes.
Surprisingly, this transcription factor exhibited no remarkable effects on or correlations with other genes involved in centelloside biosynthesis. In addition, the transformants exclusively overexpressing At-SQS had gene expression values on par with those of the control line. Consequently, no conspicuous augmentations or detrimental influences on the expression of the endogenous genes within the pathway were observable.
To examine the impact of the rol and aux transgenes derived from the pRi plasmid of R. rhizogenes on the centelloside biosynthetic genes, we generated multiple regression models using the randomForestSRC R-package (see Section 4). The models treated the endogenous genes HMGR, SQS, β-AS, CYP83, CYP19, CYP11, and UGT as dependent variables, whereas the expression levels of rolA, rolB, rolC, aux1, and aux2 genes were considered independent variables. Among these models, the one pertaining to CYP11 exhibited the highest R-squared value (0.7349), indicating the strongest level of fit. Conversely, the SQS gene model had the smallest R-squared value (0.1387). This suggests that the expression levels of the pRi plasmid transgenes are either unconnected with or exert a very limited influence on the expression behavior of the SQS gene.
The variable importance metric was utilized to compare the impact of pRi plasmid transgenes on the profile of each endogenous gene, aiding in the interpretation of the multivariate regression models. For a comprehensive understanding of the influence of transgene expression, Figure 2 presents a cluster analysis of the pathway genes.
Remarkably, aux2 exhibited a favorable impact on β-AS, CYP83, CYP19, and CYP11, with UGT displaying the least susceptibility and CYP19 showing the most pronounced effect. Following closely, rolC emerged as the subsequent influential factor, specifically influencing CYP83, CYP19, CYP11, and UGT compared with aux2. The influence of rolC was particularly prominent on the UGT gene. The aux1 gene, on the other hand, was notable solely for its impact on β-AS, while rolA exhibited only a marginal effect on HMGR. Among the endogenous genes, SQS was the least susceptible to the influence of the rol or aux genes, closely followed by HMGR.

2.3. Sterols, Squalene, and Centolloside Profiles in Response to Transgenes TSAR2 and At-SQS

Through a comprehensive phytochemical analysis, we examined the effects of the At-SQS and TSAR2 transgenes on centelloside, squalene, and total sterol profiles. Sterols constitute key compounds within a competitive pathway toward centellosides, while squalene serves as a common precursor.
In Figure 3, the upper section illustrates the total content (measured in mg/g DW) of centellosides, sterols, and squalene in the four types of hairy root lines. Notably, the LS lines exhibited the highest centelloside content (6.56 ± 0.26 mg/g DW), differing significantly from the other lines (Figure S2). The direct influence of the At-SQS transgene on production levels was evident.
Greater variability was observed in the sterol content, which ranged from 188.31 to 56.88 mg/g DW among the root lines. Specifically, the LST lines displayed a significant increase compared with the control, whereas a pronounced decrease was observed in the LS lines, resulting in values lower than the control. Conversely, the values of the LT lines did not differ significantly from those of the LST lines. Noteworthy in this context was the clear positive effect of the transcription factor on sterol content, as well as on the HMGR gene, as previously mentioned.
The profile of the squalene content was similar to that of centellosides, with a significant increase in the LS lines (1.56 ± 0.10 mg/g DW), and nearly constant values in the other three lines. Accumulated expression values of native SQS and At-SQS genes in the LS line clearly demonstrated the positive impact of the At-SQS transgene on centelloside production. However, this positive effect was only observed in the absence of the transcription factor, suggesting that the activation of the sterol biosynthetic pathway effectively utilized the additional squalene generated by the heterologous enzyme.

2.4. Influence of Squalene and Sterol Content on Morphological Traits

In this study, we deemed the branching rate, growth rate, and biomass productivity to be pertinent morphological traits owing to their biotechnological implications. The branching rate denotes the number of lateral roots per centimeter, growth rate signifies the elongation of roots in millimeters per day, and biomass productivity quantifies the daily biomass yield for each line. Various morphologies of hairy root lines after 28 days of growth are illustrated in Figure 4 and Figure S3.
By conducting a thorough correlation analysis between the morphological traits and the contents of squalene and sterols, we have unveiled a compelling depiction of how the accrual or depletion of these two distinct compounds intricately interweaves with the measured characteristics (Figure 5). The control line maintained a robustly positive correlation between the variables. However, in the LS line, which yielded significantly diminished levels of sterols yet substantially elevated quantities of squalene and, therefore, centellosides, a different pattern was discernible. Here, it became distinctly apparent that the aggregation of squalene exerted a deleterious impact on the underlying morphological traits.
Intriguingly, in the LST line, this adverse effect appeared to be counterbalanced by the presence of the transcription factor. This regulatory entity seemed to orchestrate a harmonizing influence, fostering amplified sterol production while concurrently addressing the extra squalene availability. This bifaceted mechanism effectively overcame the negative impact observed in the LS line, thus indicating the intricate interplay between genetic modulation and metabolite accumulation.

3. Discussion

This study further elucidates the complex interplay between specific genes and the centelloside biosynthetic pathway. Notably, the C. asiatica hairy root lines harboring TSAR2 exhibited a substantial upregulation of the endogenous genes SQS and HMGR, suggesting they play pivotal roles in the regulation of centelloside biosynthesis. These findings align with those of Xu et al. [12], who observed increased HMGR gene expression in Ganoderma lucidum overexpressing the GlbHLH5 transcription factor under methyl jasmonate elicitation, and Mertens et al. [11], who reported higher transcript levels of the HMGR gene in Medicago truncatula hairy roots overexpressing TSAR2. Moreover, instances of transcription-factor-mediated modulation of SQS gene homolog expression, leading to activated triterpenoid biosynthesis, have been observed in various species such as Ziziphus jujuba and Torreya grand [15,16].
A key factor in triterpenoid structural diversity is the cytochrome P450 family, particularly the CYP716 enzymes. These versatile enzymes, distributed widely across diverse plant species, have the capacity to catalyze triterpene oxidation at various positions [17]. Among the ensemble of genes, CYP16C11 emerges as a significant player and is modulated by the insertion of T-DNA genes (Figure 2). Our findings are in parallel to those of Pandey et al. [18], who investigated the complex interactions of CYP716C55 gene expression and metabolic pathways under Ri-T-DNA-mediated insertional mutagenesis, unraveling the intricacies of gene modulation within the dynamic landscape of Ocimum species hairy roots.
The aux2 gene (1398 bp), a component of TR-DNA, plays a pivotal role in the induction and continuation of hairy root growth [19,20]. This oncogene orchestrates the conversion of naphthalene acetamide into the potent auxin naphthalene acetic acid, a crucial stage in hairy root development [21]. Notably, Srivastava et al. [22] revealed the significant influence of the aux2 gene on 3-indol acetic acid (IAA) levels, morphological traits, and metabolite content in Ocimum basilicum hairy roots, with implications mirroring our own results, as its overexpression had a favorable impact on the expression of β-AS, CYP, and UGT genes.
By boosting beta-glucosidase activity, the rolC gene provides a gateway for the release of active cytokinins from their inactive counterparts [23]. Its versatile effects include roles in nicotine production in Nicotiana tabacum hairy roots [24], ginsenoside synthesis in Panax ginseng hairy roots [25], and resveratrol production in transgenic Vitis amurensis cell cultures [26]. In our study, we observed how the rolC gene positively influences CYP and UGT gene expression. Similarly, Inyushkina [27] noted that rolC gene expression led to increased transcript levels of CYP98A3 subfamily members, crucial genes in rosmarinic acid biosynthesis.
The important role of the rolA gene in triterpenoid production has been reported in Artemisia dubia hairy roots, where it was found to directly enhance artemisinin production [28]. Interestingly, although the influence of the rolA gene in secondary metabolism remains less explored compared with other oncogenes, our work reveals its notable impact on the early triterpene pathway gene HMGR, which encodes an enzyme catalyzing vital steps in IPP biosynthesis [29].
The LST and LT lines stood out for their high phytosterol content, a direct effect of TSAR2. The influence of other transcription factors such as WRKY or MYC2 (WsWRKY1 and WsMYC2) on phytosterol biosynthesis has been demonstrated in studies on Withania somnifera [30,31].
The LS lines exhibited the highest squalene content, mirroring their centelloside content (Figure 3), which illustrates the effect of introducing the SQS gene from A. thaliana into the C. asiatica hairy root lines. This phenomenon has been previously studied in Medicago truncatula [32], P. ginseng [4], W. somnifera [33], Taraxacum koksaghyz [34], and Eleutherococcus senticosus [35], the results attesting to the intriguing connection between squalene synthase overexpression and enhanced triterpene levels.
As well as the highest centelloside content, the LS lines possessed the lowest phytosterol content (Figure 3), which reflects the fact that triterpene biosynthesis occurs once sufficient phytosterol has been synthesized, signaling the end of growth [3,4]. Supporting this observation, studies have shown that inhibiting the phytosterol biosynthetic pathway by antisense cycloartenol synthase led to a notable increase in ginsenosides (triterpenes) in P. Ginseng hairy roots [13]. A similar antagonistic interaction between the triterpene and sterol pathways has been observed in transgenic Buplerum falcatum roots [36] and in methyl-jasmonate-elicited C. asiatica plants, where free sterol decreased while centellosides increased [37].
Furthermore, it has been reported that triterpenic saponins can also contribute to root growth, as demonstrated in the case of a γ-pyronyl triterpenoid saponin, known as chromosaponin 1 in Lactuca sativa [38]. In A. thaliana, this compound interacts with the aux1 protein, regulating the root gravitropic response [39].
Regarding the hairy root morphological traits, the strongest positive correlation between the different growth values with metabolite composition was observed in the control lines (Figure 5a). Conversely, the traits of LS lines exhibited an opposing trend (Figure 5b), which implies that the accumulation of squalene and subsequent elevation in centelloside content functions as a trigger for secondary metabolism, marked by the cessation of cell division and growth [40]. Curiously, in the LST and LT lines, the negative correlation observed in the LS lines disappears (Figure 5c). This remarkable fact finds its origins in the insertion of TSAR2, which directly affects the HMGR gene and, quite possibly, genes of the sterol biosynthetic pathway, resulting in a higher phytosterol content. These effects of the transcription factor contrast with the findings of Hey et al. [14], who observed a 2.44-fold increase in sterol production in transformed A. thaliana compared with the control.
Our findings further highlight the regulatory interplay between the phytosterol and triterpene production pathways, along with their impacts on hairy root morphological traits. Future research should focus on refining the modulation of the transgenes to achieve a harmonious equilibrium between production levels and morphological attributes.

4. Materials and Methods

4.1. Establishment and Selection of C. asiatica Hairy Roots

The protocol followed in this study was based on Alcalde et al. [41] with slight modifications. In vitro cultures of C. asiatica plants were maintained on Murashige and Skoog (MS) medium supplemented with vitamins, 30% (w/v) sucrose, and 2.7% (w/v) gelrite in a controlled growth chamber. The growth chamber provided a constant temperature of 25 °C and a long-day photoperiod of 16 h of light followed by 8 h of darkness.
To initiate the hairy root induction process, leaf segments from the plantlets were wounded and infected with two distinct strains of R. rhizogenes A4. The first strain carried the binary plasmid pBI121_At-SQS, which encodes squalene synthase 1 from A. thaliana [42]. The second strain carried the plasmid pK7WG2D,1_TSAR2, encoding a transcription factor [43]. To achieve a double mutation, a simultaneous infection involving both strains was performed. Prior to infection, these bacterial strains were cultured at 25 °C on solid YEB medium for 48 h, supplemented with 100 mg/L of kanamycin and 50 mg/L of rifampicin.
After the infection, the wounded leaf segments were placed on solid MS medium enriched with 50 mg/L of acetosyringone. Up to four leaf segments were placed per plate, and the plates were then incubated in darkness at 25 °C for 2 days. Subsequently, the explants were transferred to fresh plates with solid MS medium containing 500 mg/L of cefotaxime and incubated at 25 °C for 4 weeks.
Following this incubation period, the roots that developed on the leaf segments were carefully isolated and transferred to new solid MS medium supplemented with 500 mg/L of cefotaxime and 0.1 mg/L of kanamycin. This step was repeated every 2 weeks over a period of about 2 months to eliminate any residual presence of R. rhizogenes. Robustly growing transgenic roots were identified by excising the top 5–7 cm of the root apex along with its lateral branches. These selected root lines were then cultured on fresh solid MS medium at a temperature of 25 °C in darkness, and subculturing of the transgenic root lines was carried out under the same conditions every 2 weeks.

4.2. DNA Isolation and Transgenic Confirmation by PCR Analysis

The DNA isolation protocol, adapted from Alcalde et al. [41], involved several steps. Initially, 200 mg of hairy root tissue was pulverized with liquid nitrogen and combined with 0.75 mL of extraction buffer (containing 50 mM EDTA pH 8.0, 100 mM Tris pH 8.0, and 500 mM NaCl), 0.6 μL of β-mercaptoethanol, and 50 μL of 20% sodium dodecyl sulfate (SDS). This mixture was incubated at 65 °C for 10 min, followed by the addition of 250 μL of 5 M potassium acetate. After an ice incubation for 20 min and centrifugation at 4 °C for 20 min at 9000 g, the supernatant was collected, mixed with 1 mL of isopropanol, and incubated at −20 °C for 1 h. The resulting pellet was centrifuged at 8000 g for 15 min and air-dried, then resuspended in 140 μL of T10E1 buffer (Tris 10 mM, EDTA 1 mM) and centrifuged for 10 min at 14,000 g. To the retained supernatant, 15 μL of 3 M sodium acetate and 100 μL of isopropanol were added. The resulting supernatant was again retained and centrifuged at 15,000 g for 10 min. The genomic DNA within the pellet was air-dried at 37 °C for 10 min and then resuspended in 30 μL of T10E1 buffer. Subsequently, 1 μL of RNAse (10 mg/mL) was added, and the purity of the DNA was assessed using a NanoDrop 2000 Spectrophotometer (Thermo Fisher Scientific, Waltham, MA, USA).
For the purpose of transgenic confirmation, transgenes from R. rhizogenes strains, including rolC, At-SQS, TSAR2, and virD genes, were amplified by PCR within 0.5 mL tubes. To each tube, 12.5 μL of Green taq polymerase, 1 μL of forward primer, 1 μL of reverse primer, 2 μL of DNA, and 8.5 μL of Milli-Q water were added. The specific primers used are detailed in Table S1. The PCR protocol comprised an initial cycle at 94 °C for 5 min, followed by 35 cycles at 94 °C for 1 min, 60 °C for 30 s, and 72 °C for 1 min, with a final extension step at 72 °C for 5 min. The size of the PCR products was determined using agarose gel electrophoresis (1%).

4.3. Analysis of Morphological Traits

To initiate the cultures, an inoculum of 10 mg of fresh weight (FW) was introduced for each hairy root line onto solid MS medium plates. These cultures were consistently maintained through two consecutive subcultures, with intervals of 2 weeks, at a temperature of 25 °C in a dark environment. This approach is in accordance with our established methodology from previous investigations [44].
Following this cultivation period, the assessment of growth parameters was carried out, with three replicates conducted for each distinct line. The evaluated growth parameters included the branching rate, quantified as the number of lateral roots per centimeter of the initial stem root (number of lateral roots/cm). Additionally, the growth rate was calculated by measuring the average length of the lateral roots (mm/day). Finally, biomass productivity was determined by dividing the difference between the final FW and the initial FW by the number of days the growth occurred (mg/day).

4.4. Quantification of Centelloside Production

The determination of centelloside production was conducted in accordance with the method outlined by Alcalde et al. [41]. Initially, 0.5 g of freeze-dried hairy root material (DW) was carefully weighed, followed by the addition of a 10 mL suspension of methanol:H2O (9:1). This suspension was then subjected to sonication for 1 h at room temperature to facilitate extraction. Subsequently, the suspension underwent centrifugation at 2000 g for 10 min to separate the solid and liquid phases. The supernatant obtained from this process was carefully separated, and the centrifugation step was repeated once more to ensure thorough extraction. The supernatants collected from the various samples were placed into porcelain mortars and evaporated at 38 °C for approximately 24 h. Following this, the resulting material was redissolved in 1 mL of methanol.
The methanolic extracts were subsequently filtered using a 0.22 μm filter for HPLC quantification of centellosides. The HPLC system consisted of a Waters 600 Controller pump, a Waters 717 Autosampler automatic injector, a Jasco variable-length (UV) 1570 detector, and Borwin data analysis software version 1.5. A Lichrospher 100 RP18 5 μm column (250 × 0.4 mm) was employed for gradient chromatography at room temperature following the method described by Alcalde et al. [41]. The mobile phase consisted of acetonitrile and ammonium phosphate (10 mM), acidified to a pH of 2.5 with orthophosphoric acid to enhance the definition of compound peaks. The flow rate was maintained at 1 mL/min, with an injection volume of 10 μL. The detector wavelength was set at 214 nm, 1.00 au/v, and the total run time was 45 min.
For the quantification of centellosides, namely asiatic acid, madecassic acid, asiaticoside, and madecassoside, calibration curves were established using standards of these four compounds. Calibration concentrations ranged from 10 to 500 ppm, with specific points at 10, 25, 50, 100, 250, and 500 ppm.

4.5. Expression Analysis of Centelloside Pathway Genes by RT-qPCR

Total RNA extraction was performed as in Alcalde et al. [41]. Trizol reagent was added to an Eppendorf tube with 200 mg of FW material and incubated for 20 min at room temperature. After shaking to mix the contents, the tubes were centrifuged at 7500 g for 10 min at 4 °C. The RNA pellet obtained was subjected to a single wash with 1 mL of 75% ethanol. After gentle shaking to mix the contents, the tubes were centrifuged at 7500 g for 5 min at 4 °C. Following removal of the supernatant, vacuum drying was employed for 10 min to desiccate the tubes. To dissolve the RNA samples, 20 μL of DEPC-treated water was utilized. Subsequent to extraction, RNA samples were assessed for purity and concentration using the NanoDrop 2000 Spectrophotometer (Thermo Fisher Scientific, Waltham, MA, USA).
The treatment with DNAse was administered using the total RNA as a template, employing a fixed concentration (2 μg of RNA). Additionally, the RNA integrity was confirmed via agarose gel electrophoresis. The synthesis of the first-strand cDNA was performed using the SuperScriptTM IV First-Strand Synthesis System (Invitrogen from Thermo Fisher Scientific, Waltham, MA, USA) with 2 μg of RNA, precisely following the manufacturer’s protocols.
After the design of primers via Primer3Plus software (version: 3.3.0) (Table S2), RT-qPCR assays were performed utilizing the QuantStudio3 System (Thermo Fisher Scientific, Waltham, MA, USA). These amplifications were conducted in 10 μL reaction volumes, consisting of 1 μL of first-strand cDNA (25 ng/μL), 2 μL of DEPC-treated water, 5 μL of iTaq Universal SYBR Green Supermix (Biorad, Hercules, CA, USA), and 1 μL of each specific primer at a concentration of 10 μM. The PCR conditions involved an initial phase at 95 °C for 30 s, followed by 40 cycles of 95 °C for 15 s and 60 °C for 30 s. To confirm the specificity of each primer pair, a melting curve analysis was performed, starting at 95 °C for 15 s, followed by a gradual increase from 60 to 95 °C at a rate of 0.1 °C/s, and ending with another step at 95 °C for 15 s.

4.6. Determination of Squalene Content

The quantification of squalene content was conducted following the methodologies of Shen et al. [45] and Rothblat et al. [46], with minor adjustments. In brief, the hairy roots were subjected to overnight drying in an oven set at 60 °C. For the subsequent steps, 200 mg of the dried sample was employed. Extraction was carried out within glass test tubes, utilizing 2 mL of n-hexane, and conducted in a supersonic water bath maintained at 40 °C for a duration of 30 min. The supernatants thus obtained were collected, and the extraction process was repeated once more to ensure thorough extraction. The pooled fractions were subjected to evaporation at 40 °C. Subsequently, 1 mL of concentrated sulfuric acid was added, and the mixture was subjected to a 5 min incubation in a water bath set at 70 °C. Then, 0.5 mL of 37% formaldehyde solution was gradually added, with the tubes being shaken for comprehensive mixing, and the mixture was placed in a water bath set at 95 °C for a 5 min period. Finally, to reach a final volume of 4 mL, 2.5 mL of glacial acetic acid was added promptly, and the mixture was meticulously mixed. After an incubation of 5 min, the absorbance at 400 nm was gauged using a UV2310 spectrophotometer (DINKO instruments, Barcelona Spain).

4.7. Determination of Phytosterol Content

The quantification of phytosterol content was conducted as in Araújo et al. [47], with minor modifications. For the preparation of the Liebermann–Burchard (LB) reagent, 50 mL of acetic anhydride was added to an amber glass bottle, which was maintained at a chilled temperature over ice. After a 30 min period, 5 mL of concentrated sulfuric acid was cautiously added to the bottle.
To establish the phytosterol reference curve, β-sitosterol was employed as the standard. Specifically, 10 mg of β-sitosterol was dissolved within 1 mL of chloroform, yielding a concentration of 10 mg/mL. Gradient concentrations spanning from 0.02 to 0.1 mg/mL of β-sitosterol were generated by diluting the stock solution with chloroform. Within the context of this reference curve, 0.5 mL of each concentration from the gradient was combined with 0.5 mL of LB reagent. Additionally, a blank solution comprising 0.5 mL of chloroform and 0.5 mL of LB reagent was prepared.
To determine the phytosterol content, 0.1 g of the dried sample material was mixed with 5 mL of chloroform within a glass tube. Subsequently, sonication was carried out for 30 min at room temperature. The supernatants thus obtained were collected, and the extraction process was repeated once more. The pooled fractions were subjected to evaporation at 40 °C, and the resulting residues were resuspended within 2 mL of chloroform. A mixture comprising 0.5 mL of the resuspension and 0.5 mL of LB reagent was prepared. The absorbance was measured at 625 nm, ensuring that this measurement was taken within a maximum of 5 min after the addition of LB reagent. For the purpose of comparison, a blank solution was generated, comprising 0.5 mL of chloroform and 0.5 mL of LB reagent.

4.8. Statistical Analysis and Machine Learning Models

Statistical analysis was performed using GraphPad Prism version 6.04 for Windows, developed by GraphPad Software in La Jolla, CA, USA. The data are presented as mean values with standard deviations. To conduct statistical comparisons, a multifactorial ANOVA analysis was employed, followed by Tukey’s multiple comparison tests. A significance level of p ≤ 0.05 was used to indicate statistical significance.
Machine learning models and Pearson correlation analysis were carried out using R Statistical Software (version 4.3.1) [48]. The randomForestSRC package [49] was employed to implement multivariate regression models. The coefficient of determination (R-squared) was used as a metric to evaluate the fitting of each model. The corrplot package [50] was utilized to compute the Pearson correlation coefficient (r). The reduced accuracy values of the multivariate multiple regression model were employed for hierarchical clustering analysis and were visually represented through a heatmap.

5. Conclusions

In this study, we explored the effects of At-SQS and TSAR2 transgenes on the centelloside biosynthetic pathway, revealing distinct impacts on gene expression profiles. TSAR2 overexpression notably elevated HMGR and endogenous SQS expression, demonstrating a strong positive correlation with these two genes. The transcription factor exhibited limited influence on other pathway genes, although its overexpression enhanced sterol production. Overexpression of At-SQS alone had minimal effects on endogenous genes but significantly increased the squalene content. Further investigation of pRi plasmid-derived rol and aux transgenes revealed a significant positive impact of aux2 and rolC genes on centelloside pathway genes, whereas the influence of aux1 and rolA was more restricted. The overarching theme from the findings of this study is the intricate interplay between genetic modulation and gene expression, shedding light on the complex mechanisms governing centelloside biosynthesis. Additionally, a comprehensive phytochemical analysis unveiled the interactions between At-SQS and TSAR2 transgenes and centelloside, sterol, and squalene content. In general, the accumulation of squalene in the absence of TSAR2 had a detrimental effect on the sterol content. Moreover, by measuring the branching rate, growth rate, and biomass productivity of the hairy roots, we revealed that these morphological traits of biotechnological importance are negatively correlated with squalene, whereas their improvement was strongly positively associated with sterol.

Supplementary Materials

The following supporting information can be downloaded at: https://www.mdpi.com/article/10.3390/plants12193363/s1, Figure S1: PCR analysis: detection of SQS, TSAR2, rolC, and VirD genes in different C. asiatic transgenic root lines, Figure S2: statistical differences between different types of lines, Figure S3: morphology of different transformed root lines of C. asiatica on day 14 of their growth, Table S1: quantitative data for gene expression and metabolite profiling, Table S2: primers used for confirmation of transformed roots, Table S3: primers used for gene expression analysis.

Author Contributions

Conceptualization, J.P. and D.H.-M.; methodology, M.A.A.; formal analysis, M.A.A. and D.H.-M.; data curation, D.H.-M.; writing–original draft, M.A.A.; writing–review and editing, J.P., M.B. and D.H.-M.; supervision, J.P., M.B. and D.H.-M.; funding acquisition, J.P. All authors have read and agreed to the published version of the manuscript.

Funding

This research was funded by Agencia Estatal de Investigación, REF: PID2020−113438RB−I00/AEI/10.13039/501100011033, and by the Agència de Gestió d’Ajuts Universitaris i de Recerca (AGAUR) del Departament de Recerca i Universitats de la Generalitat de Catalunya 2021 SGR00693. D.H. is a postdoctoral researcher at María Zambrano at the University of Barcelona. His contract is financed by the Ministry of Universities, the European Union Next GenerationEU/PRTR.i, and the Recovery, Transformation and Resilience Plan.

Data Availability Statement

Data are contained within the article and Supplementary Material.

Conflicts of Interest

The authors declare no conflict of interest.

References

  1. Sabaragamuwa, R.; Perera, C.O.; Fedrizzi, B. Centella asiatica (Gotu Kola) as a neuroprotectant and its potential role in healthy ageing. Trends Food Sci. Technol. 2018, 79, 88–97. [Google Scholar] [CrossRef]
  2. Kunjumon, R.; Johnson, A.J.; Baby, S. Centella asiatica: Secondary Metabolites, biological activities and biomass sources. Phytomed. Plus 2022, 2, 100176. [Google Scholar] [CrossRef]
  3. Rogowska, A.; Szakiel, A. Enhancement of phytosterol and triterpenoid production in plant hairy root cultures-simultaneous stimulation or competition? Plants 2021, 10, 2028. [Google Scholar] [CrossRef] [PubMed]
  4. Lee, M.H.; Jeong, J.H.; Seo, J.W.; Shin, C.G.; Kim, Y.S.; In, J.G.; Yang, D.C.; Yi, J.S.; Choi, Y.E. Enhanced triterpene and phytosterol biosynthesis in Panax ginseng overexpressing squalene synthase Gene. Plant Cell Physiol. 2004, 45, 976–984. [Google Scholar] [CrossRef] [PubMed]
  5. Mehrotra, S.; Rahman, L.U.; Kukreja, A.K. An Extensive Case Study of hairy-root cultures for enhanced secondary-metabolite production through metabolic-pathway engineering. Biotechnol. Appl. Biochem. 2010, 56, 161–172. [Google Scholar] [CrossRef] [PubMed]
  6. Staniek, A.; Bouwmeester, H.; Fraser, P.D.; Kayser, O.; Martens, S.; Tissier, A.; van der Krol, S.; Wessjohann, L.; Warzecha, H. Natural Products–Modifying Metabolite Pathways in Plants. Biotechnol. J. 2013, 8, 1159–1171. [Google Scholar] [CrossRef]
  7. Kim, O.T.; Kim, S.H.; Ohyama, K.; Muranaka, T.; Choi, Y.E.; Lee, H.Y.; Kim, M.Y.; Hwang, B. Upregulation of phytosterol and triterpene biosynthesis in Centella asiatica hairy roots overexpressed ginseng farnesyl diphosphate synthase. Plant Cell Rep. 2010, 29, 403–411. [Google Scholar] [CrossRef]
  8. Yu, H.; Liu, M.; Yin, M.; Shan, T.; Peng, H.; Wang, J.; Chang, X.; Peng, D.; Zha, L.; Gui, S. Transcriptome analysis identifies putative genes involved in triterpenoid biosynthesis in Platycodon grandiflorus. Planta 2021, 254, 34. [Google Scholar] [CrossRef]
  9. Broun, P. Transcription factors as tools for metabolic engineering in plants. Curr. Opin. Plant Biol. 2004, 7, 202–209. [Google Scholar] [CrossRef]
  10. Chezem, W.R.; Clay, N.K. Regulation of plant secondary metabolism and associated specialized cell development by MYBs and BHLHs. Phytochemistry 2016, 131, 26–43. [Google Scholar] [CrossRef]
  11. Mertens, J.; Pollier, J.; Bossche, R.V.; Lopez-Vidriero, I.; Franco-Zorrilla, J.M.; Goossens, A. The BHLH Transcription Factors TSAR1 and TSAR2 regulate triterpene saponin biosynthesis in Medicago truncatula. Plant Physiol. 2016, 170, 194–210. [Google Scholar] [CrossRef] [PubMed]
  12. Xu, J.; Wang, Y.; Zhang, Y.; Xiong, K.; Yan, X.; Ruan, S.; Wu, X. Identification of a novel metabolic target for bioactive triterpenoids biosynthesis in Ganoderma lucidum. Front. Microbiol. 2022, 13, 878110. [Google Scholar] [CrossRef] [PubMed]
  13. Liang, Y.; Zhao, S.; Zhang, X. Antisense suppression of cycloartenol synthase results in elevated ginsenoside levels in Panax ginseng hairy roots. Plant Mol. Biol. Rep. 2009, 27, 298–304. [Google Scholar] [CrossRef]
  14. Hey, S.J.; Powers, S.J.; Beale, M.H.; Hawkins, N.D.; Ward, J.L.; Halford, N.G. Enhanced seed phytosterol accumulation through expression of a modified HMG-CoA Reductase. Plant Biotechnol. J. 2006, 4, 219–229. [Google Scholar] [CrossRef]
  15. Wen, C.; Zhang, Z.; Shi, Q.; Niu, R.; Duan, X.; Shen, B.; Li, X. Transcription Factors ZjMYB39 and ZjMYB4 regulate farnesyl diphosphate synthase- and squalene synthase-mediated triterpenoid biosynthesis in Jujube. J. Agric. Food Chem. 2023, 71, 4599–4614. [Google Scholar] [CrossRef]
  16. Zhang, F.; Kong, C.; Ma, Z.; Chen, W.; Li, Y.; Lou, H.; Wu, J. Molecular characterization and transcriptional regulation analysis of the Torreya grandis squalene synthase gene involved in sitosterol biosynthesis and drought response. Front. Plant Sci. 2023, 14, 1136643. [Google Scholar] [CrossRef]
  17. Miettinen, K.; Pollier, J.; Buyst, D.; Arendt, P.; Csuk, R.; Sommerwerk, S.; Moses, T.; Mertens, J.; Sonawane, P.D.; Pauwels, L.; et al. The Ancient CYP716 family is a major contributor to the diversification of eudicot triterpenoid biosynthesis. Nat. Commun. 2017, 8, 14153. [Google Scholar] [CrossRef]
  18. Pandey, P.; Singh, S.; Negi, A.S.; Banerjee, S. Harnessing the versatility of diverse pentacyclic triterpenoid synthesis through hairy root cultures of various Ocimum species: An unprecedented account with molecular probing and up-scaling access. Ind. Crops Prod. 2022, 177, 114465. [Google Scholar] [CrossRef]
  19. Gaudin, V.; Camilleri, C.; Jouanin, L. Multiple regions of a divergent promoter control the expression of the Agrobacterium rhizogenes aux1 and aux2 plant oncogenes. Mol. Gen. Genet. 1993, 239, 225–234. [Google Scholar] [CrossRef]
  20. Camilleri, C.; Jouanin, L. The TR-DNA region carrying the auxin synthesis genes of the Agrobacterium rhizogenes agropine-type plasmid PRiA4: Nucleotide sequence analysis and introduction into tobacco plants. Mol. Plant Microbe Interact. 1991, 4, 155–162. [Google Scholar] [CrossRef]
  21. Béclin, C.; Charlot, F.; Botton, E.; Jouanin, L.; Dore, C. Potential Use of the aux2 gene from Agrobacterium rhizogenes as a conditional negative marker in transgenic cabbage. Transgenic Res. 1993, 2, 48–55. [Google Scholar] [CrossRef]
  22. Srivastava, S.; Conlan, X.A.; Adholeya, A.; Cahill, D.M. Elite hairy roots of Ocimum basilicum as a new source of rosmarinic acid and antioxidants. Plant Cell Tissue Organ Cult. 2016, 126, 19–32. [Google Scholar] [CrossRef]
  23. Dilshad, E.; Noor, H.; Nosheen, N.; Gilani, S.R.; Ali, U.; Khan, M.A. Influence of rol genes for enhanced biosynthesis of potent natural products. In Chemistry of Biologically Potent Natural Products and Synthetic Compounds; John Wiley & Sons, Ltd.: Hoboken, NJ, USA, 2021; pp. 379–404. ISBN 9781119640929. [Google Scholar] [CrossRef]
  24. Palazon, J.; Cusido, R.M.; Gonzalo, J.; Bonfill, M.; Morales, C.; Pinol, M.T. Relation between the amount of rolC gene product and indole alkaloid accumulation in Catharanthus roseus transformed root cultures. J. Plant Physiol. 1998, 153, 712–718. [Google Scholar] [CrossRef]
  25. Bulgakov, V.P.; Khodakovskaya, M.V.; Labetskaya, N.V.; Chernoded, G.K.; Zhuravlev, Y.N. The Impact of plant rolC oncogene on ginsenoside production by ginseng hairy root cultures. Phytochemistry 1998, 49, 1929–1934. [Google Scholar] [CrossRef]
  26. Dubrovina, A.S.; Manyakhin, A.Y.; Zhuravlev, Y.N.; Kiselev, K.V. Resveratrol content and expression of phenylalanine ammonia-lyase and stilbene synthase genes in rolC transgenic cell cultures of Vitis amurensis. Appl. Microbiol. Biotechnol. 2010, 88, 727–736. [Google Scholar] [CrossRef]
  27. Inyushkina, Y.V.; Kiselev, K.V.; Bulgakov, V.P.; Zhuravlev, Y.N. Specific genes of cytochrome p450 monooxygenases are implicated in biosynthesis of caffeic acid metabolites in rolC-transgenic culture of Eritrichium sericeum. Biochemistry 2009, 74, 917–924. [Google Scholar] [CrossRef]
  28. Amanullah, M.; Mirza, B.; Zia, M. Production of artemisinin and its derivatives in hairy roots of Artemisia dubia induced by rolA gene transformation. Pak. J. Bot. 2016, 48, 699–706. [Google Scholar]
  29. Kalita, R.; Patar, L.; Shasany, A.K.; Modi, M.K.; Sen, P. Molecular cloning, characterization and expression analysis of 3-Hydroxy-3-Methylglutaryl Coenzyme A Reductase Gene from Centella asiatica L. Mol. Biol. Rep. 2015, 42, 1431–1439. [Google Scholar] [CrossRef]
  30. Singh, A.K.; Kumar, S.R.; Dwivedi, V.; Rai, A.; Pal, S.; Shasany, A.K.; Nagegowda, D.A. A WRKY Transcription Factor from Withania somnifera regulates triterpenoid withanolide accumulation and biotic stress tolerance through modulation of phytosterol and defense pathways. New Phytol. 2017, 215, 1115–1131. [Google Scholar] [CrossRef]
  31. Sharma, A.; Rather, G.A.; Misra, P.; Dhar, M.K.; Lattoo, S.K. Jasmonate responsive transcription factor WsMYC2 regulates the biosynthesis of triterpenoid withanolides and phytosterol via key pathway genes in Withania somnifera (L.) Dunal. Plant Mol. Biol. 2019, 100, 543–560. [Google Scholar] [CrossRef]
  32. Suzuki, H.; Achnine, L.; Xu, R.; Matsuda, S.P.T.; Dixon, R.A. A Genomics approach to the early stages of triterpene saponin biosynthesis in Medicago truncatula. Plant J. 2002, 32, 1033–1048. [Google Scholar] [CrossRef]
  33. Patel, N.; Patel, P.; Kendurkar, S.V.; Thulasiram, H.V.; Khan, B.M. Overexpression of squalene synthase in Withania somnifera leads to enhanced withanolide biosynthesis. Plant Cell Tissue Organ Cult. 2015, 122, 409–420. [Google Scholar] [CrossRef]
  34. Unland, K.; Pütter, K.M.; Vorwerk, K.; van Deenen, N.; Twyman, R.M.; Prüfer, D.; Schulze Gronover, C. Functional characterization of squalene synthase and squalene epoxidase in Taraxacum koksaghyz. Plant Direct 2018, 2, e00063. [Google Scholar] [CrossRef]
  35. Seo, J.W.; Jeong, J.H.; Shin, C.G.; Lo, S.C.; Han, S.S.; Yu, K.W.; Harada, E.; Han, J.Y.; Choi, Y.E. Overexpression of Squalene synthase in Eleutherococcus senticosus increases phytosterol and triterpene accumulation. Phytochemistry 2005, 66, 869–877. [Google Scholar] [CrossRef]
  36. Kim, Y.S.; Cho, J.H.; Park, S.; Han, J.Y.; Back, K.; Choi, Y.E. Gene regulation patterns in triterpene biosynthetic pathway driven by overexpression of squalene synthase and methyl jasmonate elicitation in Bupleurum falcatum. Planta 2011, 233, 343–355. [Google Scholar] [CrossRef] [PubMed]
  37. Mangas, S.; Bonfill, M.; Osuna, L.; Moyano, E.; Tortoriello, J.; Cusido, R.M.; Teresa Piñol, M.; Palazón, J. The Effect of Methyl jasmonate on triterpene and sterol metabolisms of Centella asiatica, Ruscus aculeatus and Galphimia glauca Cultured Plants. Phytochemistry 2006, 67, 2041–2049. [Google Scholar] [CrossRef] [PubMed]
  38. Tsurumi, S.; Tsujino, Y. Chromosaponin I stimulates the growth of lettuce roots. Physiol. Plant. 1995, 93, 785–789. [Google Scholar] [CrossRef]
  39. Tsurumi, S.; Ishizawa, K.; Rahman, A.; Soga, K.; Hoson, T.; Goto, N.; Kamisaka, S. Effects of chromosaponin i and brassinolide on the growth of roots in etiolated Arabidopsis seedlings. J. Plant Physiol. 2000, 156, 60–67. [Google Scholar] [CrossRef]
  40. Li, Y.; Kong, D.; Fu, Y.; Sussman, M.R.; Wu, H. The Effect of developmental and environmental factors on secondary metabolites in medicinal plants. Plant Physiol. Biochem. 2020, 148, 80–89. [Google Scholar] [CrossRef]
  41. Alcalde, M.A.; Cusido, R.M.; Moyano, E.; Palazon, J.; Bonfill, M. Metabolic Gene Expression and Centelloside Production in Elicited Centella asiatica hairy root cultures. Ind. Crops Prod. 2022, 184, 114988. [Google Scholar] [CrossRef]
  42. Mirjalili, M.H.; Moyano, E.; Bonfill, M.; Cusido, R.M.; Palazón, J. Overexpression of the Arabidopsis thaliana squalene synthase gene in withania coagulans hairy root cultures. Biol. Plant. 2011, 55, 357–360. [Google Scholar] [CrossRef]
  43. Sanchez-Muñoz, R.; Almagro, L.; Cusido, R.M.; Bonfill, M.; Palazon, J.; Moyano, E. Transfecting Taxus × Media protoplasts to study transcription factors BIS2 and TSAR2 as activators of taxane-related genes. Plant Cell Physiol. 2020, 61, 576–583. [Google Scholar] [CrossRef] [PubMed]
  44. Alcalde, M.A.; Müller, M.; Munné-Bosch, S.; Landín, M.; Gallego, P.P.; Bonfill, M.; Palazon, J.; Hidalgo-Martinez, D. Using machine learning to link the influence of transferred Agrobacterium rhizogenes genes to the hormone profile and morphological traits in Centella asiatica Hairy Roots. Front. Plant Sci. 2022, 13, 1001023. [Google Scholar] [CrossRef] [PubMed]
  45. Sheng, Y.Y.; Xiang, J.; Wang, K.R.; Li, Z.Y.; Li, K.; Lu, J.L.; Ye, J.H.; Liang, Y.R.; Zheng, X.Q. Extraction of squalene from tea leaves (Camellia sinensis) and its variations with leaf maturity and tea cultivar. Front. Nutr. 2022, 9, 755514. [Google Scholar] [CrossRef] [PubMed]
  46. Rothblat, G.H.; Martak, D.S.; Kritchevsky, D. A quantitative colorimetric assay for squalene. Anal. Biochem. 1962, 4, 52–56. [Google Scholar] [CrossRef]
  47. Araújo, L.B.D.C.; Silva, S.L.; Galvão, M.A.M.; Ferreira, M.R.A.; Araújo, E.L.; Randau, K.P.; Soares, L.A.L. Total phytosterol content in drug materials and extracts from roots of Acanthospermum hispidum by UV-VIS Spectrophotometry. Rev. Bras. De Farmacogn. 2013, 23, 736–742. [Google Scholar] [CrossRef]
  48. R Core Team. R: A Language and Environment for Statistical Computing; R Foundation for Statistical Computing: Vienna, Austria, 2021. [Google Scholar]
  49. Ishwaran, H.; Kogalur, U.B. Fast unified random forests for survival, regression, and classification (RF-SRC) 2022. Available online: https://rdrr.io/cran/randomForestSRC/ (accessed on 18 July 2023).
  50. Wei, T.; Simko, V. R Package “Corrplot”: Visualization of a Correlation Matrix 2021. Available online: https://github.com/taiyun/corrplot (accessed on 18 July 2023).
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Figure 1. Overview of the centelloside biosynthetic pathway and gene expression profile. L1 denotes the control line, while LST, LS, and LT represent the transformed lines. The reddish heatmap indicates the upregulation (UP) or downregulation (DOWN) of gene expression for HMGR (encoding the 3-hydroxy-3-methylglutaryl coenzyme A reductase), SQS (encoding squalene synthase), β-AS (encoding beta amyrin synthase), CYP83 (cytochrome CYP716A83), CYP19 (cytochrome CYP714E19), CYP11 (cytochrome CYP716C11), and UGT (UGT73AD1). The bluish heatmap reflects the fold change in gene expression of At-SQS (squalene synthase from Arabidopsis thaliana).
Figure 1. Overview of the centelloside biosynthetic pathway and gene expression profile. L1 denotes the control line, while LST, LS, and LT represent the transformed lines. The reddish heatmap indicates the upregulation (UP) or downregulation (DOWN) of gene expression for HMGR (encoding the 3-hydroxy-3-methylglutaryl coenzyme A reductase), SQS (encoding squalene synthase), β-AS (encoding beta amyrin synthase), CYP83 (cytochrome CYP716A83), CYP19 (cytochrome CYP714E19), CYP11 (cytochrome CYP716C11), and UGT (UGT73AD1). The bluish heatmap reflects the fold change in gene expression of At-SQS (squalene synthase from Arabidopsis thaliana).
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Figure 2. Comprehensive heatmap illustrating the impact of rol and aux genes on the endogenous gene expression profile in Centella asiatica hairy roots.
Figure 2. Comprehensive heatmap illustrating the impact of rol and aux genes on the endogenous gene expression profile in Centella asiatica hairy roots.
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Figure 3. Comparative plot of various types of hairy root lines. The density plot illustrates the profiles of sterols, squalene, and centellosides, while the bar plots display the gene expression profiles of HMGR, SQS, and At-SQS in terms of fold change values. The stacked column highlighted in purple represents the contribution of At-SQS. See Table S1 for more details.
Figure 3. Comparative plot of various types of hairy root lines. The density plot illustrates the profiles of sterols, squalene, and centellosides, while the bar plots display the gene expression profiles of HMGR, SQS, and At-SQS in terms of fold change values. The stacked column highlighted in purple represents the contribution of At-SQS. See Table S1 for more details.
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Figure 4. Average morphology of different hairy root lines of Centella asiatica at day 28 of growth: (a) control, (b) LST, (c) LS, (d) LT. The initial inoculum was a small section of 10 mg of fresh weight.
Figure 4. Average morphology of different hairy root lines of Centella asiatica at day 28 of growth: (a) control, (b) LST, (c) LS, (d) LT. The initial inoculum was a small section of 10 mg of fresh weight.
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Figure 5. Pearson’s correlation analysis of morphological traits and metabolite content. (a) Correlation plot for the control line; (b) correlation plot for the LS lines; (c) correlation plot for the lines overexpressing the transcription factor. Values indicate the Pearson correlation coefficient (r).
Figure 5. Pearson’s correlation analysis of morphological traits and metabolite content. (a) Correlation plot for the control line; (b) correlation plot for the LS lines; (c) correlation plot for the lines overexpressing the transcription factor. Values indicate the Pearson correlation coefficient (r).
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Alcalde, M.A.; Palazon, J.; Bonfill, M.; Hidalgo-Martinez, D. Enhancing Centelloside Production in Centella asiatica Hairy Root Lines through Metabolic Engineering of Triterpene Biosynthetic Pathway Early Genes. Plants 2023, 12, 3363. https://doi.org/10.3390/plants12193363

AMA Style

Alcalde MA, Palazon J, Bonfill M, Hidalgo-Martinez D. Enhancing Centelloside Production in Centella asiatica Hairy Root Lines through Metabolic Engineering of Triterpene Biosynthetic Pathway Early Genes. Plants. 2023; 12(19):3363. https://doi.org/10.3390/plants12193363

Chicago/Turabian Style

Alcalde, Miguel Angel, Javier Palazon, Mercedes Bonfill, and Diego Hidalgo-Martinez. 2023. "Enhancing Centelloside Production in Centella asiatica Hairy Root Lines through Metabolic Engineering of Triterpene Biosynthetic Pathway Early Genes" Plants 12, no. 19: 3363. https://doi.org/10.3390/plants12193363

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