Yan Hu1†Minzhen Yin1,2,3†Yunjun Bai2
Shanshan Chu1Ling Zhang1*
Mei Yang1Xiaowen Zheng1Zhengyang Yang1Junling Liu4Lei Li5
Luqi Huang2,3*
Huasheng Peng1,2,3*- 1School of Pharmacy, Anhui University of Chinese Medicine, Hefei, China
- 2National Resource Center for Chinese Materia Medica, China Academy of Chinese Medical Sciences, Beijing, China
- 3Research Unit of DAO-DI Herbs, Chinese Academy of Medical Sciences, Beijing, 2019RU57, China
- 4Anhui Provincial Institute for Food and Drug Control, Hefei, China
- 5Jinzhai Senfeng Agricultural Technology Development Co., Ltd., Lu’an, China
Polygonati rhizoma (Huangjing in Chinese) is a traditional and classic dual-purpose material used in food and medicine. Herbalists in China and Japan have noticed several different rhizome types in Huangjing with different qualities. Rhizome of Polygonatum cyrtonema Hua and P. sibiricum Red. is divided into five types: “Jitou-type” Polygonati rhizoma (JTPR), atypical “Jitou-type” Polygonati rhizoma (AJTPR), “Jiang-type” Polygonati rhizoma (JPR), “Cylinder-type” Polygonati rhizoma (CPR), and “Baiji-type” Polygonati rhizoma (BJPR). This study observed the microstructure and histochemical localization of polysaccharides, saponins, and proteins in Huangjing. Nutritional and medicinal component data and antioxidant capacity (DPPH and ABTS) were analyzed to evaluate the quality of different types of Huangjing. The results showed that the comprehensive quality of the rhizomes, BJPR and JTPR, was better, regardless of their nutritional or medicinal values. Altogether, these results could recommend future breeding efforts to produce Huangjing with improved nutritional and medicinal qualities.
Introduction
The genus Polygonatum (Liliaceae) comprises more than 71 species that are widely distributed in China, Japan, Korea, India, Russia, Europe, and North America. More than half of these species have been used in medicine and food (Zhao et al., 2019). Polygonati rhizoma, commonly known as Huangjing in China, is the dried rhizome of Polygonatum sibiricum Red., P. kingianum Coll. et Hemsl., and Polygonatum cyrtonema Hua (The State Pharmacopoeia Committee of China, 2020). In traditional Chinese medicine clinical practice, Huangjing has multiple effects: invigorating Qi and nourishing Yin, moistening the lungs, invigorating the spleen, and benefiting the kidneys. Modern pharmaceutical research has shown that Huangjing has been used for the treatment of delaying aging, enhancing immunity, anti-fatigue effects, lowering blood sugar, anti-tumor effects, protecting the cardiovascular system, and improving memory (Zhang et al., 2018b; Zhao et al., 2018b; Li et al., 2020, 2021b) and has enormous potential in the treatment of COVID-19 (Mu et al., 2021). From ancient times, Huangjing has also been used as food, such as several well-received sweetmeats, functional beverages, and fruit wine (Li et al., 2021c).
Huangjing was first cited in Ming Yi Bie Lu 名医别录 and has been used as a traditional Chinese medicine for more than 2000 years. Previous studies have shown that P. sibiricum and P. cyrtonema were mainly used as the primitive plants of Huangjing before the Ming Dynasty, and the use of P. kingianum was not recorded until the Qing Dynasty (Cheng and Wang, 2009). Traditional Chinese medicine researchers have noticed that there are differences in the morphology of rhizomes between P. sibiricum and P. cyrtonema, known as Jiang Huangjing (the morphology of rhizomes is similar to the rhizome of ginger, which is called Jiang in Chinese) and Jitou Huangjing (the morphology of rhizomes is similar to that of the chicken head, which is called Jitou in Chinese). Ben Cao Yuan Shi 本草原始 (completed in 1612) was the first work in Chinese history to depict the map of medicinal parts, which described three types of Polygonati rhizoma, one of which has a similar morphology to Bletillae rhizoma (the rhizomes of Bletilla striata; Li et al., 2007; Figure 1). Through field investigation, it was found that the rhizomes of P. sibiricum had two types of morphology, one resembling a chicken head, called “Jitou-type” Polygonati rhizoma (JTPR) and the other atypical “Jitou-type” Polygonati rhizoma (AJTPR). Rhizome of P. cyrtonema is divided (Figure 1) into three types: “Jiang-type” Polygonati rhizoma (JPR), similar to ginger, “Cylinder-type” Polygonati rhizoma (CPR), which is nearly regular cylindrical, and “Baiji-type” Polygonati rhizoma (BJPR), consistent with the type of “shape like Bletillae rhizoma” recorded in Ben Cao Yuan Shi. Interestingly, the quality of BJPR was considered excellent by Han Yao Liang Lie Jian Bie Fa (Naotarov, 1955), showing that traditional Chinese medicine experts have focused on the differences in the quality of different types of Polygonati rhizoma. However, the scientific connotation of the superior quality of BJPR has not yet been revealed.
Figure 1. Huangjing recorded in Ben Cao Yuan Shi 本草原始 (A1-A3) and five types of Huangjing (B-F). (A1) Shan Cheng Tang Edition, (A2,A3) Yong Huai Tang Edition, Image courtesy of Chinese—Japanese Library, Harvard University, (B) “BaiJi-type” Polygonati rhizoma, (C) “Jiang-type” Polygonati rhizoma, (D) “Cylinder-type” Polygonati rhizoma, (E) “JiTou-type” Polygonati rhizoma, and (F) atypical “JiTou-type” Polygonati rhizoma. Scale bar = 1 cm.
Huangjing contains various chemical components, such as polysaccharides, saponins, flavonoids, and alkaloids, and other components (Tang et al., 2019; Hu et al., 2021). Huangjing is used as both medicine and food, and its sweet taste and nutritional components, such as free sugars, amino acids, and nucleic acids, have also attracted much attention. However, presently, trait quality is ignored when evaluating the quality of Huangjing. A comprehensive evaluation of quality traits of Huangjing can provide a scientific basis for “assessing quality by distinguishing features” and help researchers identify excellent materials for improved breeding. Therefore, a scientific method for comprehensively evaluating quality traits of Huangjing is needed. In this study, five different types of Huangjing were collected as: two rhizome types of P. sibiricum (JTPR and AJTPR) and three rhizome types of P. cyrtonema (JPR, CPR, and BJPR; Figure 1B). A multivariate statistical analysis was used to comprehensively evaluate the quality of five rhizomes of Huangjing, including appearance, microstructure, medicinal quality, and nutritional quality.
The appearance and microstructure of Huangjing were compared and analyzed using by morphological and microscopic observations and histochemical experiments. Ultraviolet and visible spectrophotometry (UV-Vis) was used to determine the total polysaccharide. The contents of free sugar content were determined using high-performance liquid chromatography coupled with a charged aerosol detector (HPLC-CAD), including fructose, glucose, and sucrose. The contents of amino acids, nucleosides, and nucleobases were determined using ultra-high performance liquid chromatography-Orbitrap-tandem mass spectrometry (UHPLC-Orbitrap-MS/MS). Furthermore, the total saponin represented by the medicinal components of Huangjing were also determined by UV-Vis spectroscopy. The DPPH and ABTS methods were also used to confirm the antioxidant activities in Huangjing. Then, principal component analysis (PCA) and orthogonal partial least squares discrimination analysis (OPLS-DA) were used to illustrate the component difference among the five types of Huangjing. This research aimed to provide a reliable and useful classification for clarifying the differences in plant material of different characters of Huangjing and provide a reference for the breeding of improved varieties and further quality evaluation of Huangjing.
Materials and Methods
Materials
Thirty-six batches (Supplementary Table 1) of P. sibiricum and P. cyrtonema were collected from two producing regions of China, including Jinzhai and Quanjiao of Anhui province. Professor Huasheng Peng authenticated all herbal samples. After collection, fresh rhizome samples were steamed for 2 h at 100°C, dried in a drying oven at 60°C until constant weight, and then ground into a fine powder (100 mesh).
Chemicals and Reagents
Details of standard compounds (purity ≥98%), including two monosaccharides and one disaccharide, sarsasapogenin, 24 amino acids, 11 nucleosides, four nucleobases, and other compounds, are listed in Supplementary Table 2. The chemical structures of the standard compounds are shown in Supplementary Figure 1. MS-grade acetonitrile (ACN) was obtained from Merck (Darmstadt, Germany). Ammonium acetate and acetic acid (MS grade) were acquired from Sigma Chemical Co., Ltd. (St. Louis, MO, United States). Pure water was prepared using a Direct-Pure®Adept water system (RephiLe Bioscience, Ltd., Shanghai, China). All other reagents and chemicals were of analytical grade.
Morphological and Microscopic Observations
Morphological Observation
Five types of Huangjing were observed, and the plant materials were photographed using a digital camera (Canon EOS 70D, EF 24–70 mm f/4 l IS USM, Japan). Data comprising the diameter of the extension segment fine end and thick end, diameter of stem mark, internodal distance, height, and width of buds, annular spacing, and branch angle of rhizomes were measured and recorded.
Microscopic Observation
Microscopic observation was performed using a previously described method (Xie et al., 2019), and paraffin sections were prepared. The fresh samples were fixed in FAA solution (70% ethanol: acetaldehyde: acetic acid = 90:5:5, v/v/v), followed by routine dehydration with a series of ethanol and paraffin embedding. A Leica RM2265 rotary microtome (Leica Microsystems Wetzlar GmbH, Wetzlar, Hessen, Germany) was used to produce sections (15 μm thick) for permanent slide preparation and stained with safranin and fast green. The microscopic characteristics of the rhizomes were examined using an optical microscope (Motic Panthera, China). The percentage of mucilage cells was calculated by freeze sectioning (Leica CM1950, Germany) combined with an ink staining experiment. Briefly, fresh rhizomes were collected, and a section was cut without pretreatment and embedded into a freezing medium; the temperature of the condensation box was −22°C. After 30 min of condensation time, the sections were sliced after trimming with a thickness of 30 μm. Six glass slides were prepared and observed for each type, and the average value was used to calculate the percentage area of mucilage cells.
Histochemical Analyses
Histochemical analyses were performed on polysaccharides, saponins, and proteins. Polysaccharides were stained using periodic acid-Schiff (PAS) reaction, saponins using 5% vanillin-glacial acetic acid-perchloric acid solution (Cheng and Wang, 2013), and proteins using Coomassie brilliant blue test solution (Fazekas de St Groth et al., 1963).
Qualitative Analysis
Total Polysaccharide Content
Total polysaccharide was determined using the anthrone-sulfuric acid method. About 0.25 g of the as-prepared rhizome powder was weighed accurately into a round-bottom flask with 150 ml of 80% ethyl alcohol and boiled for 60 min. After removal of insoluble matter, 150 ml of water was added and boiled again for 60 min. All solutions were collected and diluted in a 250 ml volumetric flask with water. Then, 8.0 ml of 0.2% anthrone-sulfuric acid solution was added to 1 ml of sample solution and 1 ml of water. The absorbance was measured at 620 nm, and D (+)-glucose was used as a reference. Each sample was prepared in triplicate.
Free Sugar Content
Two monosaccharides and one disaccharide were identified using a high-performance liquid chromatography coupled with a charged aerosol detector (HPLC-CAD). The standard stock solution was prepared by adding an appropriate amount of fructose, glucose, and sucrose standards, precision weighing, and 80% ethanol was added to dissolve the stock solutions at concentrations of 2.0890, 1.0071, and 1.0568 mg/ml of stock solution, respectively. One gram of the as-prepared rhizome powders was extracted once with 80% ethanol (30 ml) by simple sonication (500 W, 30 kHz) for 1 h, steamed, and dried. Then, an appropriate amount of 75% ACN was added and dissolved in a 50 ml volumetric flask. The sample solutions were then filtered with a 0.22 μm syringe filter, and the filtrates were collected.
Samples were analyzed on an Ultimate 3,000 Liquid Chromatograph (Corona Ultra Electromist Detector, Dionex, United States); Shodex Asahipak NH2P-50 4E column (4.6 mm × 250 mm, 5 μm) was used for separation. The mobile phase comprised solutions A (deionized water) and B (ACN), and the gradient elution procedure was as follows: 0–20 min, 19–25% A; 20–35 min, 25–30% A; 35–40 min, and 30–19% A. The flow rate of the mobile phase was 1.0 ml/min, and the column temperature was maintained at 25°C. The injection volume was 5 μl. CAD detector settings were as follows: data acquisition frequency 5 Hz; filter 3.6 F; atomizer temperature 35°C; air N2; and pressure 4.328 × 105 Pa.
Amino Acid, Nucleoside, and Nucleobase Content
Stock solutions of the standard compounds (approximately 1 mg/ml) were prepared by dissolving approximately 1 mg of each compound in 1.0 ml of a suitable solvent. Certain amounts of the 24 amino acids and 15 nucleosides, and nucleobases standard stock solutions were mixed and diluted with 50% ACN to obtain a series of solutions at the appropriate concentrations. These solutions were used to construct calibration curves. All standard solutions were filtered through 0.22 μm cellulose membrane filters before analysis and were stored in a refrigerator at 4°C. One gram of the as-prepared sample powder was extracted once with 60% ethanol (20 ml) by sonication (500 W, 30 kHz) for 30 min and cooled to 25°C for 30 min; solvent was again added to compensate for the weight loss. Then, the supernatant was centrifuged at 13000 rpm/min for 15 min and stored at 4°C. The mixture was diluted five times with 50% ACN solution and then centrifuged at 13000 rpm/min for 15 min. The supernatant was removed through a 0.22 μm filter membrane and was injected into an HPLC column.
Chromatographic analysis was conducted on an Ultimate HPLC system (Thermo Fisher Scientific, Waltham, MA, United States). An Acquity UPLC BEH Amide (2.1 × 100 mm, 1.7 μm) column was used for analyzing all the samples. The mobile phase consisted of solutions A (2 mm ammonium acetate and 0.1% acetic acid) and B (ACN; v/v). The gradient elution procedure was as follows: 0–3 min, 10% A; 3–9 min, 10–18% A; 9–15 min, 18–20% A; 15–16 min, 20–46% A; 16–20 min, 46% A; and 20–25 min, 46–10% A. The mobile phase was set at a 0.30 ml/min flow rate, and the injection volume was 2 μl. The column temperature was maintained at 30°C.
Mass spectrometry (MS) was performed on a Q Exactive Focus Orbitrap MS system (Thermo Fisher Scientific, United States) supplied with a heated electrosprayer for ionization. Mass spectra were acquired separately in positive ionization mode in a full mass operation with a mass range of 70.0–1,050 m/z and a spray voltage of 3.4 kV. The temperature of the capillary and source was maintained at 350°C. Pressures of 50 psi and 10 psi were set for the sheath gas (N2) and auxiliary gas (N2), respectively. Sodium trifluoroacetate was used for accurate mass calibration. Mass spectra and chromatograms were acquired and processed using Xcalibur (Thermo Fisher Scientific, Waltham, MA, United States). The chemical formula for precursor and product ions was determined using the Compound Discoverer software (version 2.0).
Total Saponin Content
Total saponin content was analyzed using the 5% vanillin-glacial acetic acid–perchloric acid method (Zhao et al., 2020a). About 1.0 g of the as-prepared rhizome powder was extracted with 25 ml 70% ethanol ultrasonic extract for 30 min, filtered, and spin-dried in a rotary evaporator. The pellet was dissolved using 20 ml of 1% sodium hydroxide solution, and the solution was transferred to a pear-shaped separating funnel. The extract was washed three times with water-saturated n-butyl alcohol and then twice with 15 ml of n-butyl alcohol-saturated water. Furthermore, the solution was spin-dried, and the pellet was dissolved in methanol in a 5-mL volumetric flask. The prepared sample was mixed with the developer for a color reaction, using sarsasapogenin as the reference, and the wavelength was measured at 530 nm. Each sample was prepared in triplicate.
Antioxidant Capacity Evaluation
Antioxidant capacity was evaluated using 2,2-diphenyl-1-picrylhydrazyl (DPPH) and 3-ethyl benzothiazoline-6-sulfonic acid (ABTS) assays. An extraction method with appropriate modification of the total polysaccharide was used for sample extraction.
DPPH free radical scavenging capacity was measured using the method described by Brand-Williams (Blois, 1958) with slight modifications. During the experiment, 0.1 ml of sample extracts with different concentrations (10, 20, 30, 40, and 50 mg/ml) were mixed with DPPH ethanol solution (0.1 mmol/l, 0.1 ml), added to 96-well plates for a dark reaction for 30 min, and the absorption wavelength was measured at 517 nm using a microplate analyzer (Tecan infinite 200, Tecan, China). ABTS was performed according to a previously described method, with slight modifications (Re et al., 1999). To prepare ABTS working solution, 7 mmol/l of ABTS aqueous solution was mixed with 2.45 mmol/l potassium persulfate aqueous solution at a ratio of 1:1. The solution was left to stand in the dark for 12 h and diluted with water. The absorbance value measured at 734 nm was 0.7 ± 0.05 l/(g·cm). During the experiment, 0.1 ml of sample extracts with different concentrations (10, 20, 30, 40, and 50 mg/ml) were mixed with ABTS ethanol solution (0.1 mmol/l and 0.3 ml) and added into 96-well plates for a dark reaction for 6 min. The absorbance wavelength was set to 734 nm.
The DPPH and ABTS free radical scavenging capacities were calculated using the following formula: DPPH radical scavenging ratio (%) = [1 − (Asample − Abackground)/Ablank] × 100%, where Asample is the absorbance of the sample solution and DPPH solution; Abackground the absorbance of the sample solution and ethanol solution; Ablank the absorbance of water and DPPH solution; and ABTS radical scavenging ratio (%) = [1 − (Asample − Abackground)/Ablank] × 100%, where Asample is the absorbance of the sample solution and ABTS solution; Abackground the absorbance of the sample solution and water; and Ablank the absorbance of water and ABTS solution. IC50 was used to represent antioxidant activity using GraphPad Prism 8.0 software (GraphPad, San Diego, United States).
Statistical Analysis
All data are expressed as mean ± SD. Data were statistically evaluated by one-way ANOVA analysis, least significant difference (LSD) test, and principal component analysis (PCA) scores using IBM SPSS 23.0 Statistics (SPSS, Inc., United States). Correlation analysis was performed using Origin 2021 (OriginLab, United States), and partial least squares discriminant analysis (PLS-DA) was performed using SIMCA-P 14.1 (Umetrics Inc., Sweden). Heatmap clustering analysis was performed using TBtools (Chen et al., 2020).
Results
Morphological Characteristics
The rhizomes of Polygonatum plants grow one segment each year, which is called “annual rhizomes.” There are clear differences in the appearance of the annual rhizomes of the five types of Huangjing. The BJPR showed two continuous bifurcating branches, and the annual rhizomes were usually ovoid in shape (Figure 1B). There are two developed latent buds, one of which is long and stout; the other is short and thin, and there is an acute angle between the two buds (57.95 ± 15.56°). JPR showed two or three bifurcating branches. The annual rhizomes are cylindrical, and their latent buds are short, small, and inconspicuous (Figure 1C). CPR with indistinct branching and annual rhizomes with latent buds were underdeveloped (Figure 1D). P. sibiricum showed two rhizome types. One type of annual rhizome has a thick end and changes significantly from the front end, commonly known as JTPR (Figure 1E). Another kind of annual rhizome has no significant change in thickness, which is called AJTPR (Figure 1F). Detailed data of the appearance features of the five types of Huangjing in Supplementary Table 3.
Microscopic Characteristics and Histochemical Localization
The cross-sectional microstructures of the five types of Huangjing exhibited both similarities and differences (Figures 2A–E). P. cyrtonema and P. sibiricum belong to the Liliaceae family and are typical monocotyledonous plants. The epidermis, cortex, and vascular bundle structures were found in the rhizomes of P. cyrtonema and P. sibiricum. In addition, bundles of needle-shaped calcium oxalate crystals were observed within large mucilage cells under the epidermis. The major difference among the five types of Huangjing was the characteristics and distribution of mucilage cells. The mucilage cells of BJPR were round, with a diameter of 30–60 μm, and were mainly distributed in the cortex near the epidermis. The number of mucilage cells in JPR was relatively small, but the individual area was large, and some of the mucilage cells appeared oval with a long diameter of up to 190 μm. The number of mucilage cells in the CPR was the lowest among the five types, and the diameter of the cells was 40–80 μm. The mucilage cells in JTPR were round, with a diameter of approximately 50 μm, and the distribution in the cortex was relatively evenly distributed. In contrast, the mucilage cells of AJTPR had varying sizes, ranging from 30 to 110 μm in diameter.
Figure 2. The cross-sectional microstructures of the five types of Huangjing (A) “BaiJi-type” Polygonati rhizoma, (B) “Jiang-type” Polygonati rhizoma, (C) “Cylinder-type” Polygonati rhizoma, (D) “JiTou-type” Polygonati rhizoma, and (E) atypical “JiTou-type” Polygonati rhizoma, ink dyeing (F), histochemical localization (G) polysaccharides—Periodic Acid-Schiff reaction, (H) saponins—5% vanillin-glacial acetic acid-perchloric acid solution reaction, (I) proteins—Coomassie brilliant blue test reaction, and M: mucilage cell.
To compare the total mucilage cell area/the whole cross-sectional area ratio in the rhizomes of five kinds of Huangjing, frozen sections were used to section the fresh rhizomes, combined with the mucus reaction (ink dyeing), which can easily observe the mucilage cells (Figure 2F). The ratio of mucilage cell area to rhizome cross-sectional area was calculated (Supplementary Figure 2), among which the value of the BJPR was the largest (6.14 ± 1.87%), followed by the JTPR (4.61 ± 2.30%), and the value of CPR (1.17 ± 0.43%) was the lowest.
Histochemical localization techniques can visualize the distribution relationship of tissue structures and chemical components, which play a vital role in verifying the distribution of chemical components in medicinal plants (Souza et al., 2018; Ribeiro and Leitão, 2020). In this study, we used the periodic acid-schiff reaction, 5% vanillin-glacial acetic acid-perchloric acid solution, and Coomassie brilliant blue test solution to study the histochemistry of polysaccharides, saponins, and proteins in the rhizomes of Huangjing, respectively. The results (Figures 2G–I) showed that polysaccharides in the rhizomes of Huangjing were mainly distributed in mucilage cells, and saponins and proteins were mainly distributed in parenchymal cells. There were no saponins or proteins in the mucilage cells. This result is consistent with previous studies (Cheng and Wang, 2013). Thus, it is expected that BJPR may have higher concentrations of polysaccharides (depending on the mucilage cells).
Nutritional and Medicinal Component Analysis
Sugars
There are abundant polysaccharides in Huangjing, which is recognized as the evaluation index quality (Jiang et al., 2017; Li et al., 2018a). The total polysaccharide content of the five different types of Huangjing is shown in Figure 3A.
Figure 3. Total polysaccharide content of the five different types of Huangjing (A); Three sugars (fructose, glucose, and sucrose) content of the five different types of Huangjing (B); total saponin content of the five different types of Huangjing (C); DPPH and ABTS of antioxidant ability of the five different types of Huangjing (D). BJPR, “BaiJi-type” Polygonati rhizoma; JPR, “Jiang-type” Polygonati rhizoma; CPR, “Cylinder-type” Polygonati rhizoma; JTPR, “JiTou-type” Polygonati rhizoma; and AJTPR, atypical “JiTou-type” Polygonati rhizoma (***compared with BJPR, p < 0.05).
Among the five types, the polysaccharides content of the BJPR (70.5 ± 5.37 mg/g) and JTRP (68.8 ± 6.20 mg/g) was relatively higher. In addition, the polysaccharide content was not significantly different between BJPR and JTRP. Furthermore, the polysaccharide content in the CPR was the lowest (48.5 ± 7.75 mg/g). These results indicate that the different types of Huangjing samples are not uniform in polysaccharides. Interestingly, BJPR contains abundant mucilage cells. This further confirms that polysaccharides in the rhizomes of Polygonatum plants are distributed in mucilage cells. Furthermore, the total polysaccharide content showed a positive relationship with the total area of the mucilage cells.
Sweetness can improve flavor when Huangjing is used as a food product. The sensation of “sweetness” is determined by the presence of free sugars. Fructose, glucose, and sucrose have been reported to contribute to the sweetness of foods, and fructose is considered the sweetest sugar (Georgelis et al., 2018). Therefore, these three free sugars were often used as one of the flavor indexes for evaluating fruit (Filip et al., 2016). The HPLC-CAD method was successfully applied to quantify fructose, glucose, and sucrose in five types of Huangjing samples (Supplementary Figure 3). The method was validated by determining linearity, precision, stability, and accuracy. The results are summarized in Supplementary Table 4. The calibration curves exhibited excellent linear regression (R2 > 0.9980). The precision, repeatability, and stability variation (RSD) were all less than 2.98%. The recoveries were between 94.0 and 103.9%, with an RSD of less than 3.35%.
The contents of fructose, glucose, and sucrose were different in the five types of Huangjing, which may be caused by differences in the biosynthesis process, which affects their accumulation (Zhang et al., 2018a). The different types are listed in the order of most to least: fructose content: AJTPR > CPR > JPR > BJPR > JTPR, glucose content: JTPR > BJPR > AJTPR > JPR > CPR, and sucrose content: BJPR > AJTPR > JTPR > CPR > JPR. The total content of the three free sugars was the highest in the AJTPR samples; thus, we speculated that the AJTPR had a relatively sweet taste among the five types, but the specific taste of the five types of Huangjing still needs further flavor research.
Amino Acids, Nucleosides, and Nucleobases
Amino acids, nucleosides, and nucleobases are primary metabolites that play an important regulatory role in human health. The importance of amino acids, nucleosides, and nucleobases is widely recognized in food science and nutrition (Hoffer, 2016; Kuś and Rola, 2021). This study established an ultrahigh-performance liquid chromatography-Orbitrap-tandem mass spectrometry (UHPLC-Orbitrap-MS/MS) method under the positive MS ion mode to analyze 39 compounds, including amino acids, nucleosides, and nucleobases. The method was validated to determine the linearity, limits of detection (LOD) and quantitation (LOQ), precision, stability, and accuracy, and the results are summarized in Supplementary Table 6. Typical chromatograms of the standards are shown in Supplementary Figure 4. These results showed that this method could determine amino acids, nucleosides, and nucleobases in Huangjing.
Among the 24 free amino acids, nine essential amino acids (phenylalanine, methionine, lysine, leucine, isoleucine, tryptophan, threonine, valine, and histidine) are either not synthesized by the human body or synthesized at a rate far from being adapted to the needs of the organism and must be supplied through food (Church et al., 2020). In addition, amino acids are hydrophilic compounds that play a key role in forming umami, sweet, and bitterness in foods (Wang et al., 2021a). The results (Table 1) showed that umami amino acids (glutamate and aspartic acid) accounted for 46.2% of the total content of 24 amino acids, sweet amino acids (threonine, serine, glycine, alanine, and methionine) for 6.4%, and bitter amino acids (valine, isoleucine, leucine, tyrosine, phenylalanine, and lysine) for 3.7% in all Huangjing samples. The total content of 24 amino acids exhibited different patterns and reached the highest in the JTPR (64.3 ± 0.43 mg/g). Among the 24 amino acids from Huangjing samples, aspartic acid and citrulline are the most abundant and play crucial roles in nutrient metabolism pathways such as the ornithine cycle (Sivashanmugam et al., 2017). Interestingly, the content of aspartic acid was highest in JTPR (53.4%), and citrulline was the most abundant in BJPR (46.1%).
Table 1. Contents of 24 amino acids and 15 nucleosides and nucleobases (μg/g) of the five different types of Huangjing.
Studies have reported that nucleosides and nucleotides can bind to taste receptors to improve taste. For example, inosine 5′-monophosphate (IMP) and guanosine 5′-monophosphate (GMP) can cause umami taste and adenosine 5′-monophosphate (AMP) enhances sweetness (Wang et al., 2021c). Coincidentally, with respect to the total contents of 15 nucleosides and nucleotides, the highest concentration was also in the JTPR (478 ± 4.93 μg/g). This provides new insights for further research on the flavor of Polygonatum plants.
Total Saponin
Polygonatum plants have several steroidal saponins and fewer triterpenoid saponins, and total saponin have attracted more attention (Zhao et al., 2018a). The total saponin contents of the samples from different types of Huangjing are shown in Figure 3C. The total content of saponins in the BJPR (6.14 ± 0.237 mg/g) and AJTPR(5.75 ± 0.777 mg/g) was significantly higher than that in the other types. Therefore, it can be intuitively seen that it is impractical to directly compare the quality of different types of Huangjing using an index component.
Antioxidant Capacity Analysis
Huangjing has an antioxidant capacity (Zhang et al., 2019); however, there are few reports on the antioxidation of different types. Based on the results, the contents of primary and secondary metabolites of different types of Huangjing were different, so we speculated that their antioxidant capacities were also different. DPPH and ABTS radicals have been widely used to analyze the preliminary free radical scavenging capacity of plant extracts or antioxidant compounds (Xie et al., 2014). To evaluate the antioxidant capacity of Huangjing more comprehensively, we used rapid DPPH and ABTS radical scavenging assays. DPPH evaluated the antioxidant capacity of fat-soluble components, and ABTS evaluated the antioxidant capacity of water-soluble and fat-soluble components. The DPPH and ABTS radical scavenging activities of the five types of Huangjing were expressed as IC50 values and are shown in Figure 3D. A higher IC50 value indicates weaker antioxidant capacity. In contrast, the lower the IC50 value, the stronger the antioxidant capacity. The values showed that the antioxidant activity gradually increased with increased sample concentration and had a strong scavenging effect on DPPH and ABTS. The scavenging rates were 88.8 and 90.1%, respectively. Combined with the results of the DPPH and ABTS assays, the IC50 values of AJTPR were significantly higher than those of the other four types, indicating that the antioxidant capacity of AJTPR was significantly lower than that of the other four types. BJPR showed the strongest inhibition ability of DPPH, and CPR showed the strongest ABTS radical scavenging ability. Although ABTS and DPPH antioxidant experiments have some limitations, they can also provide a reference for further evaluation of the quality of Huangjing.
Heatmap Cluster Analysis
A heat map can directly show intragroup and intergroup similarities and differences, and cluster analysis is a clustering tool to evaluate the difference through an algorithm to produce a dendrogram (Yang et al., 2021). Thus, heatmap cluster analysis with complete linkage after column scaling with normalization was used in this study to evaluate the similarities and differences of different types of Huangjing. The results (Figure 4A) showed that the five types of Huangjing were classified into two clusters and exhibited significant spatial aggregation. The colors represent the level of accumulation for each metabolite, from low (blue) to high (red). Heat maps show that more than 60% of the compounds were higher in the BJPR and JTPR. The samples of BJPR and JTPR were grouped into Cluster I. The other samples, including those from JPR, CPR, and AJTPR, were grouped into Cluster II and exhibited a lower content of total polysaccharide, total saponin, glucose, sucrose, amino acids, nucleosides, and nucleobases. Based on these results, the comprehensive quality of the BJPR and JTPR is better. Nevertheless, it is necessary to further evaluate the quality characteristics of different Huangjing sample types using chemometrics.
Figure 4. Heatmap cluster analysis and multivariate statistical analysis (A) Hierarchical clustering analysis heat maps, (B) PLS-DA score plot, (C) OPLS-DA score plot, and (D) the VIP plot. BJPR, “BaiJi-type” Polygonati rhizoma; JPR, “Jiang-type” Polygonati rhizoma; CPR, “Cylinder-type” Polygonati rhizoma; JTPR, “JiTou-type” Polygonati rhizoma; and AJTPR, atypical “JiTou-type” Polygonati rhizoma.
Multivariate Statistical Analysis
The analysis of total polysaccharide, total saponin, free sugars, amino acids, nucleosides, and nucleobases contents showed that the differences in various components were found in the five types of Huangjing. Therefore, PCA and OPLS-DA analyses were used to determine which components had the greatest effect on the differences and could be used as differential compounds to distinguish them. However, PCA is an unsupervised multivariate statistical method of pattern recognition, which cannot assign the class membership of unknown test samples; therefore, it has limited practical use. In contrast, OPLS-DA is a multivariate dimensionality reduction tool and a supervised pattern recognition method that is gaining popularity in metabolomics and other integrative omics analyses (Ruiz-Perez et al., 2020).
After the chemical component data were standardized, the principal component score was calculated, which were the major differential compounds with variable importance in projection (VIP) values greater than 1. Through the principal component score, four principal components were extracted with eigenvalues greater than 1. The characteristic values of the four principal components were 7.253, 4.010, 3.665, and 1.563, respectively. The cumulative contribution rate of the four principal components was 82.5%. Four principal components were selected as the main evaluation factors, which comprehensively evaluated the quality of Huangjing (Supplementary Table 8). From the principal component score, the quality of the BJPR is better than that of the other types of Huangjing, followed by the JTPR.
However, because PCA cannot assign the class membership of unknown test samples, critical to validating statistical models, OPLS-DA extends a regression of PCA and uses class information to maximize the separation between groups of observations, thereby allowing better classification and prediction capacity. The OPLS-DA quality of the models was described using the statistical parameters R2Y and Q2. Generally, the value of R2Y varies from 0 to 1, where 1 indicates a model with a perfect fit. Q2 values of >0.5 indicate excellent predictive abilities. The PLS-DA model established in the first step (Figure 4B), the model’s statistical parameters R2Y (0.936) and Q2 (0.907) were significant, and the five types of Huangjing were divided into four groups: BJPR, CPR, and JTPR were clearly separated, but the other two types (JPR and AJTPR) were not. Next, the OPLS-DA model was established (Figure 4C), the OPLS-DA is suitable for modeling between two groups (Ma et al., 2020), and the score plot showed a clear separation between the two types of samples (JPR and AJTPR). In the established statistical model, the R2Y (0.978) and Q2 (0.947) values were greater than 0.9, indicating the excellent quality of the OPLS-DA model. The VIP is an index used to understand the importance of spectral variables in defining the latent variable subspace and was used to evaluate the importance of the variables in the projection of the PLS-DA model. A VIP value >1 was considered to carry the most relevant information for class discrimination (Wang et al., 2021b). The VIP value (Figure 4D) illustrated that threonine (Thr), cysteine (Cys), sucrose, tryptophan (Trp), aspartic acid (Asp), serine (Ser), hydroxyproline (Hyp), inosine 5′-monophosphate (IMP), phenylalanine (Phe), glutamine (Gln), ABTS, arginine (Arg), Histidine (His), glucose, DPPH, Ornithine (Orn), Proline (Pro), Cyclic guanosinc monophosphate (cGMP), Citrulline (Cit), and Methionine (Met) were the main markers discriminating different types of Huangjing and contributing to the differences among the samples from different types (VIP > 1).
Discussion
Rhizoma polygonati (Huangjing) has a long history of medicinal use in China. Ancient Chinese medicine experts had long noticed the diversity of rhizomes of Huangjing. Ben Cao Yuan Shi of the Ming Dynasty painted the rhizome of Huangjing, including BJPR. Japanese scholars regarded as BJPR had excellent quality. According to the 2020 Edition of Chinese Pharmacopoeia, Polygonatum sibiricum Red., P. kingianum Coll. et Hemsl., and P. cyrtonema Hua are the authentic sources of Rhizoma polygonati (The State Pharmacopoeia Committee of China, 2020). On the basis of the textual research records of materia medica, P. kingianum was recorded for the first time on An Illustrated Book on Plants (AD1848), while P. cyrtonema and P. sibiricum had been widely used in the Tang and Song dynasties (Cheng and Wang, 2009; Xu et al., 2022). Based on the records in Ben Cao Yuan Shi and Han Yao Liang Lie Jian Bie Fa, the rhizomes of Huangjing had different types. Recent years, many researchers had studied the chemical constituents of Huangjing (Fan et al., 2020; Zhao et al., 2020b; Hu et al., 2021). Indeed, some scholars have paid attention to the deeper material activity of Huangjing, it contains a significant number of nanoparticles that can be used as herbzymes (Benassi et al., 2021). However, the relationship between rhizome type and its quality and special metabolites was neglected. Anhui Province is one of the main producing areas of Huangjing. This study investigated and collected a variety of rhizomes of P. cyrtonema and P. sibiricum for comparative research of special metabolites, including the BJPR mentioned in these herbal books.
Since ancient times, Huangjing had been suitable for both medicine and food. Its rhizome is rich in chemical ingredients, including nutritional ingredients, such as sugars and amino acids, and medicinal ingredients such as saponins. At present, polysaccharides of Huangjing have attracted much attention of researchers (Jin et al., 2018; Fan et al., 2020; Hu et al., 2021). It had been reported that monosaccharides cannot be detected by a UV detector without derivatization due to the particularity of functional group structure. Fan et al. studied the monosaccharides of mannose, galacturonic acid, glucose, ribose, galactose, fucose, glucose acid, rhamnose, and arabinose in Huangjing by precolumn derivatization integrated with HPLC-MS/MS. However, precolumn derivatization has the limitation of incomplete derivatization reaction. Jin et al. determined fructose, glucose, galactose, sucrose, and 1-kestose in Huangjing by HPLC-QTOF-MS/MS, which can accurately identify the structure of compounds with high sensitivity, but it also has the limitations of complex operation and needs for professional guidance. To avoid the measurement error caused by derivatization for quantitative determination these compounds using UV detector, the detector of CAD has been used as a reliable and highly sensitive detector to low molecular weight non-volatile compounds (Jing et al., 2014). That is why this study chose this detection method, HPLC combined with CAD detector, a simple, easy to operate, high sensitivity, and no need for pre column derivatization and UV detector. In this study, three sugars (fructose, glucose, and sucrose) in Huangjing were determined. In addition, the content of total polysaccharide was also determined by UV-vis spectrophotometry. The results showed that the contents of total polysaccharide and three sugars in rhizomes of different types of Huangjing were different (Figures 3A,B). The content of fructose was the highest in AJTPR, the content of glucose was the highest in JTPR, and the content of sucrose and total polysaccharide was the highest in BJPR. Furthermore, saponin components from Polygonatum plants have important pharmacological effects, such as anti-inflammatory, anti-tumor, hypoglycemic, and hepatoprotective effects and modulation of the intestinal flora (Zhang et al., 2018b; Ma et al., 2019; Luo et al., 2020; Chai et al., 2021; Li et al., 2021b; Wang et al., 2021b). This study analyzed the content of saponins and found that the content of saponins was less in Huangjing. Among the five types of Huangjing, the content of saponins in BJPR was the highest (Figure 3C). It is speculated that BJPR might have better medicinal value.
Amino acids, nucleosides and nucleobases are indispensable to biological cells to sustain life activities and have good physiological activity (Pu et al., 2020). The determination of amino acids has been paid attention to in traditional Chinese medicine such as Goji berries, Angelicae sinensis radix, Semen sojae praeparatum, and Safflower so far (Chai et al., 2017; Qu et al., 2019; Pu et al., 2020; Lu et al., 2021). Therefore, it is meaningful to clarify the composition of nucleosides and amino acids in Huangjing for understanding the edible value of it. Some scholars had quantified seven amino acids in P. verticillatum (Sharma et al., 2021). However, there is no research on determining the nucleosides, nucleobases, and amino acids in P. cyrtonema and P. sibiricum recently. Comparing with various profiling techniques, Orbitrap is one of widely used mass spectrometry technique in metabolomics research, because it has the ability of a non-targeted search and fragmentation (Li et al., 2021a). In this study, UHPLC-Orbitrap-MS/MS was established for comparatively analyzing five types of Huangjing on amino acids, nucleosides, and nucleobases. A method for simultaneous determination of 39 amino acids, nucleosides, and nucleobases was established for the first time. The results (Figure 4A) showed that the contents of amino acids, nucleosides, and nucleobases were different in five types of Huangjing.
Huangjing is often used as food, and its antioxidant capacity has also attracted much attention. Studies had confirmed that polysaccharide of Huangjing has antioxidant capacity (Li et al., 2018b; Zhang et al., 2019). DPPH radical scavenging activity and ABTS radical scavenging activity are widely used for evaluated the activities of antioxidants, which are classified to the electron transfer mechanism. The antioxidant activities of Huangjing were evaluated by DPPH radical scavenging activity assay and ABTS radical scavenging activity assay in vitro. The results (Figure 3D) showed that the antioxidant capacity of different types was various, and the antioxidant capacity of AJTPR was the weakest.
Above all, the nutritional value of Huangjing is as important as its medicinal value. The five rhizome types of Huangjing were compared in sugar, saponins, amino acids, and antioxidant capacity. It was found that BJPR was more prominent in total sugar, total saponins, and most amino acids content. The other rhizome types also have their advantages, such as glucose content, total content of 24 amino acids, and total content of 15 nucleosides, and nucleobases were the highest in JTPR, ABTS radical scavenging activity was the strongest in JTPR. Fructose content was the highest in AJTPR. These also stated different types of rhizomes of Huangjing on chemical component content and antioxidant capacity had different levels, and the rhizome quality of different types also had its own advantages. Therefore, it is necessary to distinguish the rhizome types of Huangjing in medicine and food. This study provides reference basis for further quality breeding and quality improvement of Huangjing.
Conclusion
This study systematically investigated the metabolites using multidimensional analysis technology and comprehensively evaluated the quality of different types of Huangjing, including BJPR, JPR, CPR, JTPR, and AJTPR. Based on the microstructure, the histochemical localization of polysaccharides, saponins, and proteins in Huangjing was conducted. The contents of total polysaccharide and saponin were determined by UV-visible spectroscopy. We found that these contents were related to the mucilage cell area/the whole cross-sectional area ratio. A reliable, simple, and sensitive method capable of quantifying 24 amino acids and 15 nucleosides and nucleobases was established using the UHPLC-Orbitrap-MS/MS method. Meanwhile, an HPLC-CAD method was established to determine the three types of sugars. The antioxidant capacity was investigated using DPPH and ABTS assays. The multidimensional evaluation results indicated that the comprehensive quality of BJPR and JTPR is better, regardless of nutritional or medicinal values. Certainly, other rhizome types also have advantages. AJTPR and CPR were categorized as the high sweet taste rhizomes based on the fructose content. Nevertheless, the perceived flavor of Huangjing resulting from the combination of various taste and mouthfeel sensations and the flavor evaluation indexes need to be further studied. But these results provide new insights for further research on the flavor of Huangjing. In general, this study proposed methods to accurately determine the contents of total polysaccharide, total saponin, three sugars, and 39 metabolites in Huangjing. The quantitative and comparative results revealed the chemical characteristics and differences of different types of Huangjing, providing a basis for germplasm utilization and related food development in Huangjing.
Data Availability Statement
The original contributions presented in the study are included in the article/Supplementary Material, further inquiries can be directed to the corresponding authors.
Author Contributions
YH and MYi performed the experiments and writing—original draft. The experiments were carried out under the supervision of YB, SC, and LZ. YH, MYa, and XZ validated and analyzed the data. ZY investigated and collected the samples. JL and LL provided resources. LH and HP conducted writing—review and editing. All authors contributed to the article and approved the submitted version.
Funding
This study is financially supported by the National Key Research and Development Program of China (grant no. 2017YFC1701601), Scientific and technological innovation project of China Academy of Chinese Medical Sciences (CI2021A04001), CAMS Innovation Fund for Medical Sciences (2019-I2M-5-065), and Innovation Team and Talents Cultivation Program of National Administration of Traditional Chinese Medicine (No: ZYYCXTD-D-202005).
Conflict of Interest
LL was employed by Jinzhai Senfeng Agricultural Technology Development Co., Ltd.
The remaining authors declare that the research was conducted in the absence of any commercial or financial relationships that could be construed as a potential conflict of interest.
Publisher’s Note
All claims expressed in this article are solely those of the authors and do not necessarily represent those of their affiliated organizations, or those of the publisher, the editors and the reviewers. Any product that may be evaluated in this article, or claim that may be made by its manufacturer, is not guaranteed or endorsed by the publisher.
Supplementary Material
The Supplementary Material for this article can be found online at https://www.frontiersin.org/articles/10.3389/fpls.2022.891775/full#supplementary-material
Abbreviation
ABTS, 3-Ethyl Benzothiazoline-6-Sulfonic Acid; ACN, Acetonitrile; AJTPR, Atypical “Jitou-type” Polygonati rhizoma; AMP, Adenosine 5’-Monophosphate; Arg, Arginine; Asp, Aspartic acid; BJPR, “Baiji-type” Polygonati rhizoma; cGMP, Cyclic Guanosinc Monophosphate; Cit, Citrulline; CPR, “Cylinder-type” Polygonati rhizoma; Cys, Cysteine; DPPH, 2,2-Diphenyl-1-Picrylhydrazyl; Gln, Glutamine; GMP, Guanosine 5’-Monophosphate; His, Histidine; HPLC-CAD, High-Performance Liquid Chromatography Coupled with a Charged Aerosol Detector; Hyp, Hydroxyproline; IMP, Inosine 5’-Monophosphate; JPR, “Jiang-type” Polygonati rhizoma; JTPR, “Jitou-type” Polygonati rhizoma; LSD, Least Significant Difference; Met, Methionine; OPLS-DA, Orthogonal Partial Least Squares Discrimination Analysis; Orn, Ornithine; PAS, Periodic Acid-Schiff Reaction; PCA, Principal Component Analysis; Phe, Phenylalanine; Pro, Proline; Ser, Serine; Thr, Threonine; Trp, Tryptophan; UHPLC-Orbitrap-MS/MS, Ultra-High High-Performance Liquid Chromatography-Orbitrap-tandem Mass Spectrometry; UV–Vis, Ultraviolet and Visible Spectrophotometry; VIP, Variable Importance in Projection.
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Keywords: Polygonati rhizoma, different types, nutritional and medicinal qualities, multivariate statistical analysis, quality evaluation
Citation: Hu Y, Yin M, Bai Y, Chu S, Zhang L, Yang M, Zheng X, Yang Z, Liu J, Li L, Huang L and Peng H (2022) An Evaluation of Traits, Nutritional, and Medicinal Component Quality of Polygonatum cyrtonema Hua and P. sibiricum Red. Front. Plant Sci. 13:891775. doi: 10.3389/fpls.2022.891775
Edited by:
Sezai Ercisli, Atatürk University, TurkeyReviewed by:
Zhaojun Wei, Hefei University of Technology, ChinaAmr Amin, The University of Chicago, United States
Copyright © 2022 Hu, Yin, Bai, Chu, Zhang, Yang, Zheng, Yang, Liu, Li, Huang and Peng. This is an open-access article distributed under the terms of the Creative Commons Attribution License (CC BY). The use, distribution or reproduction in other forums is permitted, provided the original author(s) and the copyright owner(s) are credited and that the original publication in this journal is cited, in accordance with accepted academic practice. No use, distribution or reproduction is permitted which does not comply with these terms.
*Correspondence: Huasheng Peng, hspeng@126.com; Luqi Huang, huangluqi01@126.com; Ling Zhang, zhangling407@sina.com
†These authors have contributed equally to this work