The History of Licorice Applications in Maruzen Pharmaceuticals Co., Ltd.

Yukiyoshi Tamura

doi:10.5772/65962

Abstract

Licorice is the root and stolon of the genus Glycyrrhiza plants. Licorice has a long and storied history of use in both Eastern and Western cultures for over 4000 years. Licorice extracts and its principal component, glycyrrhizin, have been used extensively in foods, tobacco, and cosmetics and in both traditional and herbal medicines. Since its start-up in 1938, our company has been working on extracting and purifying the flavoring, sweetening, cosmetic, and medicinal constituents from licorice. At first, we were manufacturing licorice extracts for soy sauce. Recently, our company has developed new licorice products, such as antioxidative and antimicrobial products for foods from hydrophobic licorice extracts; whitening, antioxidative, and antityrosinase products for cosmetics from hydrophobic licorice extracts; antiaging products for cosmetics from licorice leaves; and some disease-suppression products for agriculture and fishery by water-soluble licorice flavonoids. This chapter presents the history of several kinds of food and cosmetic applications from many extracts and purified constituents from licorice plants in our company.

Keywords

Glycyrrhiza plants
glycyrrhizin
flavonoids
application
foods
cosmetic

Author Information

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Yukiyoshi Tamura*
- Research Center, Maruzen Pharmaceuticals Co., Ltd., Fukuyama, Hiroshima, Japan

*Address all correspondence to: y-tamura@maruzenpcy.co.jp

1. Introduction

Licorice (liquorice in British English, Gancao in Chinese, the leguminous plant (Fabaceae)) is a perennial plant grown in the Mediterranean region, the Middle East, Central Asia, Russia, and China. Licorice is the root and stolon of the genus Glycyrrhiza plants. Licorice has a long and storied history of use in both Eastern and Western cultures for over 4000 years. Licorice extracts and its principle component, glycyrrhizin, have been used for extensive use in foods, tobacco, and cosmetics and in both traditional and herbal medicines [1–3]. As for the components of Glycyrrhiza species, about 100 kinds of triterpenoid saponins and sapogenins and about 300 kinds of phenolic compounds have been reported [4]. Since its start-up in 1938, our company has been working on extracting and purifying the flavoring, sweetening, cosmetic and medicinal constituents from licorice. In the early days, the licorice extracts have been used in the food industry, which includes soy sauce and salted foods. Also the licorice extracts and glycyrrhizin have been used in the cosmetic industry. Recently, our company has developed new licorice products, such as antioxidative and antimicrobial products for foods from hydrophobic licorice extracts; whitening, antioxidative and antityrosinase products for cosmetics from hydrophobic licorice extracts; antiaging products for cosmetics from licorice leaves; and some-disease suppression products for agriculture and fishery by water-soluble licorice flavonoids. Our company is a world-leading company to supply a high quality of licorice products and has a historical know-how of licorice-derived product manufacturing (Figure 1). This chapter presents the history of several kinds of food and cosmetic applications from many extracts and purified constituents from licorice plants in our company.

Figure 1.
Maruzen Pharmaceuticals profile, licorice plants, and its formulated finished products.

2. Glycyrrhizin-producing Glycyrrhiza plants

Licorice is applied to the root and stolon of some Glycyrrhiza species. Among around 30 species of genus Glycyrrhiza [5], the three species of genus Glycyrrhiza are commercially used, because they contain glycyrrhizin, which is the main sweetening and bioactive agent. The water-soluble constituents of the three Glycyrrhiza species, G. uralensis, G. glabra, and G. inflata are almost same. On the other hand, the hydrophobic extract from the three Glycyrrhiza species contains the species-specific flavonoids (Table 1) [6]. The structures of these compounds are shown in Figure 2. Glycyrrhizin is a conjugate of two molecules, glucuronic acid and glycyrrhetic acid, an oleanane-type triterpene. Glycyrrhizin is found in the thickening root and the stolon, but not in the seed, leaf, and stem. Hydrophobic flavonoids are found in the peel of the root and stolon.

Glycyrrhiza plant	Distribution	Water soluble constituents		Hydrophobic flavonoids
Glycyrrhiza plant	Distribution	Saponin	Flavonoids	Hydrophobic flavonoids
G. uralensis	China, Mongolia, Kazakhstan	Glycyrrhizin	Liquiritigein and its glycosides isoliquiritigenin and its glycosides	Glycycoumarin licocoumarone
G. glabra	Mediterranean region Middle East Central Asia	Glycyrrhizin	Liquiritigein and its glycosides isoliquiritigenin and its glycosides	Glabridin glabrene
G. inflata	Xinjiang(China)	Glycyrrhizin	Liquiritigein and its glycosides isoliquiritigenin and its glycosides	Licochalcone A licochalcone B

Table 1.

Distribution and constituents of the three kinds of Glycyrrhiza species.

Figure 2.
Structures of the constituents of the three kinds of Glycyrrhiza species.

3. Application of licorice products for foods

Pontefract cakes are made of licorice extract, molasses, sugar, and flour in the Yorkshire town of Pontefract, England, during the seventeenth century. In the nineteenth century, it was used extensively for confectionery [7]. Licorice extracts and glycyrrhizin have the following properties [8]:

High-intensity sweetener, glycyrrhizin possesses about 200 times the sweetness potency of sucrose
Improving foam stabilization and head-forming characteristics
Masking effect of bitter aftertaste
Flavor-enhancing effect
Nonfermented sweetener
Noncaramelization
Heat stable
Soften the saltiness
Depression of freezing point
Full-bodied umami and sweetening

Therefore, licorice extracts and glycyrrhizin are used as food additives in a variety of foods such as alcohol beverages, nonalcohol beverages, chewing gum, candy, chocolate, sweet snacks, ice cream, soy sauce, Japanese pickled vegetables, seafood delicacies, steamed fish paste, and sausages in Japan.

Research work by our company in 1994 resulted in a yeast that selectively hydrolyzed the terminal β-glucuronyl linkage of glycyrrhizin to yield glycyrrhetic acid 3-O-mono-glucuronide (MGGR), a potent sweetener (relative sweetness to sucrose: ×950, Table 2) [9, 10]. Moreover, MGGR has a flavor-enhancing property (Table 3) [11].

Comparable sucrose concentration (%)	In water		In 5% salt solution
Comparable sucrose concentration (%)	Glycyrrhizin	MGGR	Glycyrrhizin	MGGR
2	250	1400	－	－
4	170	950	500	2800
6	170	950	500	2800
8	150	730	440	2400
10	100	500	320	1400

Table 2.

Relative sweetness intensity in water or 5% salt solution.

	Cocoa	Chocolate	Whipped cream
Blank	2*	2*	16**
MGGR	7*	8*	27**
Same	1*	0*	17**

Table 3.

Flavor-enhancing effect of MGGR against cocoa, chocolate, and whipped cream.

*

No. of panelist felt delicious.

**

Delicious score.

4. Application of licorice products for pharmaceuticals and cosmetics

Glycyrrhizin has also demonstrated antiviral, antimicrobial, anti-inflammatory, antiallergy, antiulcer, antitussive, hepatoprotective, and blood pressure-increasing effects in vitro and in vivo. In addition, glycyrrhizin is effective in treating hyperlipidemia and inflammation-induced skin hyperpigmentation and is effective in preventing neurodegenerative disorders and dental caries [2].

Therefore, licorice extract, glycyrrhizin, and its derivatives are extensively used in the preparation of cosmetics in Japan. Glycyrrhizin as well as licorice extracts, glycyrrhetin, stearyl glycyrrhetinate, and succinyloxy -glycyrrhetinate (carbenoxolone) are used in drugs, quasi-drugs, and cosmetics. Glycyrrhizin and its salts are used in eye drops, lotions, and tonics as they are soluble in water. On the other hand, glycyrrhetic acid and its derivatives are used in creams, milky lotions, and sun oils as they are soluble in oil.

5. Application of hydrophobic extract of licorice for cosmetics and foods

Recently, the species-specific flavonoids from hydrophobic extracts of G. uralensis, G. glabra, and G. inflata were found. The primary active ingredient isolated from G. uralensis was glycycoumarin, that isolated from G. glabra was glabridin, and that isolated from G. inflata was licochalcone A (Figure 1). In the course of our studies on the further application of licorice as a cosmetic ingredient, we studied new dermatological availabilities in the hydrophobic extracts of licorice containing licochalcone A isolated from G. inflata and glabridin isolated from G. glabra.

5.1. Efficacies of hydrophobic extract from G. inflata (HPGI)

The primary active ingredient isolated and extracted from G. inflata is licochalcone A, an oxygenated retrochalcone that exhibits antimicrobial, antioxidative, anti-inflammatory, antiparasitic activity, and antitumorigenic activity [12, 13].

We indicate several efficacies of hydrophobic extracts from G. inflata (HPGI), especially in dermatological uses. The efficacy of HPGI against sebum-induced skin trouble was assessed in several experiments (Table 4) [14]. An androgenic hormone, testosterone, is converted into a pharmacologically active compound, dihydrotestosterone, by an intracellular enzyme, testosterone 5α-reductase. Dihydrotestosterone combines with the androgen receptor of the sebaceous gland to increase the sebum. Ultimately, the increase of sebum-secretion promotes skin trouble through the oxidative damage and increase of acne fungus.

Tests	Inhibitory effect (IC₅₀: ppm)
Testosterone 5α-reductase activity	18.7
Androgen receptor	5.8
Lipase activity	43.6
Phospholipase A activity	0.38
SOD-like activity	7.0
Antimicrobial activity against P. acnes	15.6 (MIC)

Table 4.

Inhibitory effects of HPGI on sebum-induced skin trouble experiments.

(1) Inhibitory test of testosterone 5α-reductase. As shown in Table 4, in an assay of the inhibitory effect against testosterone 5α-reductase activity, HPGI demonstrated the potent inhibitory activity. The inhibitory ability was more effective than positive controls (ethynyl estradiol (IC₅₀: 31.5 ppm) and benzyl peroxide (IC₅₀: 129 ppm)).

(2) Inhibitory effect against androgen receptor.

In this assay, HPGI inhibited the binding of dihydrotestosterone on the receptor at a low concentration and its IC₅₀ was 5.8 ppm (Table 4). From this result, it was indicated that HPGI has a binding ability in the androgen receptor and works an androgen antagonist.

(3) Inhibitory effect against lipase and phospholipase A_2.

HPGI indicated the inhibition of lipase (IC₅₀: 43.6 ppm) and phospholipase A₂ (IC₅₀: 0.38 ppm). In this case, the potency of HPGI against phospholipase A₂ was remarkable.

(4) Superoxide dismutase (SOD) like activity.

The suppressant effect of HPGI on active oxygen generation was examined by the reduction of nitro blue tetrazolium (NBT) in a xanthine-xanthine oxidase system. In this assay, HPGI suppressed the generation of active oxygen at low concentration (IC₅₀: 7.0 ppm).

(5) Antimicrobial activity against Propionibacterium acnes.

In the hair follicle and the sebaceous gland, P. acnes produces the chemotactic factor that enhances the migration of neutrophils toward the hair follicle or the sebaceous gland, and causes the development of acne. In addition, P. acnes is considered to increase the release of cytokine and T-lymphocyte. These cells and the sebaceous gland also promote damage by acne through allergic reaction. Furthermore, P. acnes can multiply in the hair follicle by using the sebum as a nutriment and enhance the production of enzyme, such as lipase, protease, and hyaluronidase. Among these enzymes, lipase attacks sebum to give free fatty acid and promotes the formation of the primary eruption, comedo. Besides, free radicals generated from fatty acid attack phospholipid in cell membranes result in the formation of chemical mediators, such as prostaglandins and leukotrienes. These mediators derived by the action of phospholipase A₂ enhance the development of acne through inflammatory reaction.

HPGI has antimicrobial activity against P. acnes at a low concentration (MIC: 31.3 ppm).

(6) Efficacy assessment in acne patient.

From the above-mentioned results in vitro assays, HPGI expected following four actions: (1) inhibitory action of sebum production, (2) antimicrobial action, (3) inhibitory action of allergic and inflammatory response, and (4) suppressant action of oxidative damage.

Therefore, we assessed the efficacy of HPGI in acne patients.

Twenty female acne patients received anti-acne gel containing HPGI. All patients applied anti-acne gel onto the whole face twice or three times daily for 2 weeks.

Table 5 shows the result of efficacy assessment in acne patients. In 17 of the 20 patients tested, the improvement effect was recognized [13].

Efficacy	No. of patients
Marked improvement	6
Improvement	5
Slightly improvement	6
No effect	3
Worse	0

Table 5.

Result of efficacy assessment of HPGI preparation in acne patients (n = 20).

5.2. Efficacies of hydrophobic extracts from G. glabra (HPGG)

The hydrophobic extract from G. glabra (HPGG) contains various flavonoids such as glabridin, glabrene, and glabrol (Figure 3). HPGG has been known to have antimicrobial and antioxidant activities [15]. In addition, glabridin has the inhibitory effects on melanogenensis and inflammation [16]. In this section, a depigmenting effect of HPGG in vitro and in vivo studies was examined [17].

Figure 3.
Structure of flavonoid in HPGG.

(1) Inhibitory effect of tyrosinase activity.

We found that HPGG and its constituents had inhibitory effects on tyrosinase activity by absorbance measurement. Their tyrosinase inhibition doses (IC₅₀: mg/mL) were as follows: glabridin 0.0003, HPGG 0.031, glabrene 0.0046, hydroquinone 0.016, and ascorbic acid 0.21 (Table 6) [15]. The latter two compounds are commonly known as depigmenting agents.

Sample	IC₅₀ (mg/mL)
HPGG	0.0031
Glabridin	0.0003
Glabrene	0.0046
Glabrol	>0.1
Ascorbic acid	0.21
Kojic acid	0.058
Hydroquinone	0.016

Table 6.

Inhibition against tyrosinase activity.

(2) Melanization assay by 14C-thiouracil uptake.

Melanization was assayed by the incorporation of ¹⁴C-thiouracil into B-16 melanoma cells. Melanization was inhibited by HPGG and glabridin dose-dependently, although glabridin more strongly inhibited it than HPGG (Figure 4) [15].

Figure 4.
Melanization assayed by ¹⁴C-thiouracil uptake of B-16 melanoma cells.

(3) Application in patients with melasma.

We have first synthesized an HPGG that contains 40% of glabridin and using this HPGG, 0.1 or 0.2% HPGG creams were made. An open study has been carried out with application of 0.1 or 0.2% HPGG cream twice a day in patients with melasma, senile pigment freckle, and postinflammatory pigmented lesions for 4 months. The efficacy was evaluated by measuring skin lightness (L value) with colorimeter before and after the application. The L value has a theoretical value ranging from of 0 (pure black) to 100 (pure white).

L value was significantly improved after the therapy with 0.1% HPGG cream in patients with melasma only (Table 7) [15]. However, with 0.2% HPGG cream, not only patients with melasma, but also with the two lesions showed significantly improvement in L values (Table 8) [15].

Disease	No. of cases	L value before and after the 4 month therapy
Chloasma	20	Before 58.28 ± 4.06 p < 0.05 After 59.25 ± 3.61
Postinflammatory pigmentation	6	Before 57.56 ± 3.44 NS After 58.22 ± 2.46
Chloasma + PIP	7	Before 60.26 ± 2.09 NS After 60.62 ± 3.44
Total	33	Before 58.57 ± 3.65 p < 0.05 After 59.35 ± 3.39

Table 7.

Changes in L values by application with 0.1% GPGG cream.

Disease	No. of case	L value before and after the 4 month therapy
Chloasma	12	Before 55.80 ± 3.09 p < 0.01 After 57.37 ± 2.68
Postinflammatory pigmentation	8	Before 56.34 ± 3.84 p < 0.05 After 57.94 ± 3.06
Senile pigment freckle	15	Before 55.75 ± 3.48 p < 0.05 After 56.99 ± 2.63
Total	35	Before 55.90 ± 3.34 p < 0.01 After 57.33 ± 2.69

Table 8.

Changes in L values by application with 0.2% GPGG cream.

6. Application of licorice leaf extract for cosmetics

The aerial parts of licorice are less used in cosmetics. A few phytochemical investigations on the G. glabra leaves have reported the presence of several phenolic constituents that are not present in the root [18–20].

We found that licorice extract from G. glabra has antiaging effect on human skin [21]. Skin hydration is one of the most important claims in cosmetics as hydrated skin gives an impression of healthy skin. Intracellular lipids in stratum corneum (SC), which are composed mainly of cholesterol, fatty acids, and ceramide, play a crucial role for both water-holding and permeability barrier function in SC. Hyaluronan (HA) is also known to have high water-retaining capacity released to skin hydration, elasticity, and plasticity. It has been reported that HA decreased and was found to be changed in aged skin. Therefore, materials that can modulate ceramide and HA contents in SC could be very effective for aging skin.

6.1. Isolation of licorice leaf components

Ten components were isolated from 70% ethanol extract of licorice leaf from G. glabra. Three active components out of 10 are shown in Figure 5 [19].

Figure 5.
Structure of isolated active components from licorice leaf extract. (1) Pinocembrin, (2) 6-prenyl-naringenin, (3) angophorol.

6.2. Effects of licorice leaf extract on mRNA expressions of ceramide-related enzymes

To examine the effects of plant extracts on ceramide synthesis, real-time quantitative RT-PCR analysis was performed on gene expressions of serine palmitoyltransferase long chain base subunit 1 (SPTLC1) and SPTLC2, which were two subunits of serine palmitoyltransferase (SPT) and acid sphingomyelinase (SMPD1). SPT is known to catalyze the rate-limiting step of de novo ceramideynthesis. Acid sphingomyelinase (SMPD1) is also known to convert sphingomyelin into ceramide and plays an important role in ceramide generation for permeability barrier function. Licorice leaf extract and 6-prenyl-naringenin showed the promoting activity on mRNA expressions of SPTLC1, SPTLC2, and SMPD1 in a dose-dependent manner (Table 9) [19].

	mRNA expressions (% of control)
	Licorice leaf extract (μg/mL)		6-prenyl-naringenin (μg/mL)
	5	20	2.5	5
SPTLC1	113.3 ± 3.5*	132.9 ± 2.7***	113.7 ± 3.7*	148.4 ± 3.7***
SPTLC2	108.8 ± 3.9	127.6 ±11.6	113.9 ±14.5	93.8 ±12.4
SMPD1	117.3 ± 4.1	132.9 ± 8.1*	153.8 ± 9.4**	353.3 ± 5.9***

Table 9.

Effects of licorice leaf extract on the mRNA levels of SPTLC, SPTLC2, and SMPD1.

*

p < 0.05

**

p < 0.01

***

p < 0.001

These results indicate that licorice leaf extract may increase de nove biosynthesis of ceramide and hydrolysis of sphingomyelin to ceramide.

6.3. Effect of licorice leaf extract on ceramide production in skin-equivalent models and human skin

To examine whether licorice leaf extract has an efficacy on the production of ceramide in skin-equivalent models. The extract dramatically promoted the production of ceramide in skin-equivalent models (Figure 6) [19]. For further research to determine the efficacy on the production of ceramide in human skin, 1% licorice leaf extract or placebo lotion was topically applied on healthy volunteers (n = 10). The amount of ceramide by the topical application of 1% licorice leaf extract lotion (1.58 μg/mg) was increased as compared to that of placebo lotion (0.56 μg/mg) (Figure 7) [19].

Figure 6.
Effects of licorice leaf extract lotion on ceramide production. *p < 0.05 compared with the control.

Figure 7.
Effects of licorice leaf extract lotion on ceramide production. Placebo lotion (A) and 1% licorice leaf extract lotion (B). Values were the mean SEM; n = 10.

These results suggested that licorice leaf extract has an efficacy on the synthesis of ceramide.

6.4. Effects of licorice leaf extract on mRNA expression of 3-hydroxy-3-methylglutaryl-CoA reductase (HMGCR), a key enzyme on cholesterol biosynthesis

To examine whether licorice leaf extract has a promoting effect on other stratum corneum lipids, real-time quantitative RT-PCR analysis was performed on mRNA expression of HMGCR, the key enzyme for de novo cholesterol synthesis. Treatment with licorice leaf extract showed a significant increase in the expression of HMGCR mRNA by 150% compared with the controls (Figure 8(A)). Among three components tested, especially 6-prenyl-naringenin enhanced the expression of HMGCR mRNA in the dose-dependent manner (Figure 8(B)) [19]. These results indicate that licorice leaf extract and its components may increase biosynthesis of cholesterol as well as ceramide. Further studies will be needed to determine the promoting activity on cholesterol synthesis.

Figure 8.
Effects of licorice leaf extract (A) and the components (B) on the mRNA level of HMGCR. *p < 0.05; **p < 0.01; ***p < 0.001, compared with the controls.

6.5. Effects of licorice leaf extract on HA production

Gene expression of HAS3 that relates to hyaluronan biosynthesis was upregulated by the treatment of licorice leaf extract in the dose-dependent manner in normal human epidermal keratinocytes (NHEK) (Figure 9(A)). Three components tested also enhanced the hyaluronan synthase 3 (HAS3) mRNA expression (Figure 9(B)) [19]. All-trans retinoic acid that is known as a stimulator of HA synthesis in NHEK also showed a strong increase in the expression of HAS3 mRNA by 400% compared with the control. To examine whether licorice leaf extract has a promoting activity on HA production, ELISA analysis was performed using cell culture supernatant. These results indicate that licorice leaf extract and its components have a potent stimulation activity for HA production.

Figure 9.
Effects of licorice leaf extract (A) and the components (B) on the mRNA level of HAS3 in NHEK. *p < 0.05; **p < 0.01; ***p < 0.001, compared with the control.

These results indicate that licorice leaf extract may be a useful ingredient for skin hydration and barrier repair because of their ability to synthesize ceramide through the enhancement of mRNA expressions of SPT and SMPD1 and the increase of mRNA of HMGCR related to cholesterol biosynthesis and the increase of HA production through the enhancement of mRNA levels of HAS3 by its active principles.

7. Application of flavonoid-rich water-soluble licorice flavonoids (WSLF) for agriculture and fishery

Table 10 shows the flavonoid composition of water-soluble licorice flavonoids (WSLF) tested. WSLF contains about 10% of the total flavonoids and 10% of glycyrrhizin. General water extracts of licorice contain 2% of the total flavonoids and 10% of glycyrrhizin. WSLF tested has five times higher content of total flavonoids [22].

Compounds	Contents (%)
Flavonoids
Liquiritin	4–8
Isoliquiritin	1–3
Liquiritigenin	0.5–2.0
Isoliquiritigenin	0.5–2.0
Saponin
Glycyrrhizin	8–13

Table 10.

Contents of flavonoids and saponin of water-soluble licorice flavonoids (WSLF).

7.1. Control of some fungal foliage diseases of vegetables using WSLF

7.1.1. In vitro test of WSLF

The antifungal activity in vitro of WSLF was evaluated by culture tests using the PDA agar medium. The antifungal activity of WSLF among various pathogens causing fungal foliage diseases on vegetables was investigated. WSLF exhibited the antifungal activity against 15 fungi tested (Table 11) [23].

Plants	Diseases	Pathogen	% Inhibition of mycerial growth
			100 μg/mL	1000 μg/mL
Rice	Blast	Magnaporthe grisea	14	61
	Bakanae disease	Gibberella fujikuroi	37	84
	Sheath blight	Thanatephorus cucumeris	16	71
	Seed and seedling rot	Pythium graminicola	16	17
Tomato	Late blight	Phytothora infestans	18	55
	Gray mold	Botrytis cinerea	18	45
	Corynespora target spot	Corynespora cassicola	34	67
	Leaf mold	Passalora fulva	29	60
Egg plant	Leaf mold	Mycovellosiella nattrassii	19	58
Sweet pepper	Frogeye leaf spot	Cercospora capsici	11	42
Cucumber	Corynespora leaf spot	Corynespora cassicola	20	51
	Anthracnose	Colletotrichum orbiculare	11	71
Melon	Gummy stem blight	Didymella bryoniae	50	50
Spinach	Fusarium wilt	Fusarium oxysporum f. spinaciae	38	59
Potato	Late blight	Phytothora infestans	29	43

Table 11.

The antifungal activity of WSLF.

WSLE solution of 20 μL of spore solution and 20 μL was mixed on the slide maintained at 25°C for 20 h. The germinated spores were counted under a microscope. WSLE at 0.1 and 1% inhibited the germination of spores in three kinds of fungi (Table 12) [23].

Plants	Diseases	Concentration (%)	Inhibition rate (%)
			No. 1	No. 2
Sweet pepper	Frogeye leaf spot	0.1	48.4	50.1
		1	87.8	94.2
Water			2.3	5.9
Egg plant	Leaf mold	1	76.2	72.3
Water			2.9	4.4
Cucumber	Corynespora Leaf spot	1	62.4
Water			26.4

Table 12.

Effect of WSLE on the germination of spores.

7.1.2. Control of fungal foliage diseases in vivo

Control efficacy of WSLE against seven pathogens was evaluated in pot tests. WSLE solutions were sprayed onto young plants. After air-drying the solutions, the plants were artificially inoculated with the spore suspension on the test pathogen, and incubated at 25°C for a given period. Percent of disease control was assessed after the inoculation of 9–12 days by visually measuring the number of diseasing spot.

Control efficacy of WSLE among seven pathogens exhibited 80–100% at 1% (Table 13) [24]. In the pot test, WSLE showed excellent control of diseases caused by various pathogens.

Plant disease	No. of disease spot	Inhibition rate (%)
Tomato Corynespora target spot
WSLE 1%	30	98
Water	1926
Tomato late blight (no. 1)
WSLE 1%	0	100
Water	9.3
Tomato late blight (no. 2)
WSLE 1%	0	100
Water	22.8
Cucumber Corynespora leaf spot
WSLE 1%	506.0	80
Water	2541.0
Cucumber anthracnose
WSLE 1%	4.0	97
Water	134.5
Cucumber downy mildew
WSLE 1%	0	100
Water	31.1
Sweet pepper frogeye leaf spot
WSLE 1%	17.5	97
Water	520.0

Table 13.

Efficacy of WSLE against 6 pathogens.

7.2. Efficacy of WSLE on fish diseases

7.2.1. Antibacterial activity of WSLE against fish disease causing bacteria in vitro

The antibacterial activity of WSLE was examined by the agar dilution method, which ranged from 32 to 1024 μg/mL against 33 kinds of bacteria. As shown in Table 14, WSLE inhibited the growth of Gram-positive bacteria with MIC values of 128–512 μg/mL. Whereas of the Gram-negative bacteria 17 kinds of bacteria were sensitive and nine kinds of bacteria were insensitive to the inhibitory effect [25].

Bacteria	MIC (μg/mL)	Bacteria	MIC (μg/mL)
Gram-positive bacteria
Carnobacterium pisciicola	256	Staphylococcus epidermidis	512
Nocardia asteroides	256	S. aureus	256
Bacillus cereus	256	Lactococcus garvieae	128
B. brebis	256
Gram-negative bacteria
Aeromonas hydrophila	>1024	Vibrio. damsela	1024
A. salmonicida	1024	V. fisheri	128
Flavobacterium columnare	64	V. fluviaris	>1024
F. psychrophilum	64	V. carchariae	>1024
Flexibacter maritimus	256	V. harveyi	1024
Pseudomonas chloraruphis	>1024	V. ichthyoenteri	512
Photobacterium damsela	1024	V. ordalli	256
Enterococcus cloacae	>1024	V. parahaemolyticus	1024
Escherichia coli	>1024	V. penaeicida	256
Klebsiella planticola	>1024	V. proteolitycus	>1024
Salmonella typhimurium	1024	V. splendidus	512
Vibrio alginolyticus	>1024	V. tubiashii	256
V. anguillarum	1024	V. vulnificus	256

Table 14.

Antibacterial activity of WSLE.

The MICs of constituents, liquiritigenin, and isoliquiritigenin are shown in Table 15. Isoliquiritigen demonstrated significant antibacterial activity against all bacteria tested. In contrast, liquiritigenin exhibited no antibacterial activity against six kinds of bacteria tested [23].

Bacteria	MIC（μg/mL）
	Liquiritigenin	Isoliquiritigenin
Gram-positive bacteria
Nocardia asteroides	128	<32
Staphylococcus epidermidis	>128	64
S. aureus	>128	128
Gram-negative bacteria
Aeromonas salmonicida	>128	>128
Photobacterium damsela	>128	128
Vibrio anguillarum	>128	128
V. harveyi	>128	>128

Table 15.

Antibacterial activities of constituents in WSLE.

7.2.2. Effects of WSLE on nonspecific immune responses and disease resistance against Edwardsiella tarda infection in Japanese flounder, Paralichthys olivaceus

7.2.2.1. Effects of WSLE on nonspecific immune responses in Japanese flounder, P. olivaceus

Healthy Japanese flounder, each weighting about 56 g, was divided into three groups used in 0, 5, and 50 mg/kgBW/day of WSLE. Each diet was fed to three groups once a day for 2 weeks. After 1 and 2 weeks of feeding, five fishes from each group were randomly collected. Blood was drawn from the caudal vein and used for hemolytic and lysozyme activities. Hemolytic activity of WSLE-treated fish was significantly higher (P < 0.05) than that of the control fish after 1 and 2 weeks (Figure 10) [24]. On the other hand, lysozyme activity showed little change (Figure 11) [24].

Figure 10.
Hemolytic activity of Japanese flounder serum.

Figure 11.
Lysozyme activity of Japanese flounder serum.

Leukocytes were collected from the head kidney and the intestinal tract and used for superoxide anion release and phagocytic activities. The production of the superoxide anion was quantified by the reduction of nitro blue tetrazolium (NBT). WSLE showed significant higher activity than the control group after 1 and 2 weeks (Figure 12) [25]. The activity increased according to time in most groups. The production of the superoxide anion is a method for destroying intracellular bacteria. Phagocytic activities of head-kidney and intestinal tract leukocytes were determined under a microscope by the zymosan-NBT method. Supplementation of WSLE significantly (p < 0.05) enhanced the phagocytic activity after 1 and 2 weeks (Figure 13) [26].

Figure 12.
NBT reduction activity of Japanese flounder leukocytes.

Figure 13.
Phagocytic activity of Japanese flounder leukocytes.

7.2.2.2. Effects of WSLE on disease resistance against Edwardsiella tarda infection in Japanese flounder, P. olivaceus

Healthy Japanese flounder, each weighing about 53 g, was divided into three groups of 33 fishes fed with 0, 5, and 10 mg/kgBW/day of WSLE, respectively. These three groups were fed with each supplementation diet once a day for 10 days. On the 10th day of feeding, these groups were injected intraperitoneally with 8.0 × 10² CFU of E. tarda.

The cumulative survival rate of the experimental fish following E. tarda intraperitoneal challenge is shown in Figure 14 [27, 28]. The cumulative survival rate was high 48 and 44% when infected fish were fed with 5 and 10 mg/kgBW/day diet and low as 20% in 0 mg/kgBW/day diet fed group, respectively.

Figure 14.
Effect of WSLE administration on the survival of Japanese flounder experimentally infected with E. tarda.

Oral administration of WSLE caused enhancement in humoral (hemolytic and lysozyme) and cellular (phagocytic and superoxide anion release) activities. After 10 days of dietary treatment with WSLE, the fish were challenged by intraperitoneal injection with E. tarda, WSLE-treated fish demonstrated increased survival rate.

8. Conclusion

Licorice has been used for pharmaceuticals, cosmetics, and food products as water-soluble licorice extract that contains glycyrrhizin, the primary constituent having sweet-taste and various biological activities. Recently, many studies have focused on the licorice ingredients except glycyrrhizin, about 300 phenolic compounds were found from licorice. We investigated licochalcone A extracted from G. inflata and glabridin from G. glabra in particular. The primary active ingredient isolated and extracted from G. inflata is licochalcone A, an oxygenated retrochalcone, which has been associated with various biological properties such as an antioxidant, antimicrobial, as well as anti-inflammatory. As a result, licochalcone A showed several activities such as inhibitory effects of testosterone 5α-reductase, lipase, and phospholipase A₂, as well as androgen receptor antagonist, antimicrobial and SOD-like activities, which relate to skin care, especially the suppression of acne formation and development. On the basis of this evidence, a trial of licochalcone A with acne patients was carried out and the efficacy was demonstrated clinically. The primary active ingredient of G. glabra is glabridin, a prenylated isoflavonoid, which is one of the most studies licorice flavonoids, a comprehensive literature survey linked to its bioactivities. Glabridin has inhibitory effects on tyrosinase activity, a key enzyme in the production of melanins and melanization using cultured B16 melanoma cells. An open study of glabridin with melasma patients was conducted. The efficacy was evaluated by measuring skin lightness before and after therapy. Glabridin significantly improved after the therapy not only in melasma but also in lesions. The aerial parts of licorice have received scant interest. The few phytochemical investigations on the G. glabra leaves have shown the presence some flavonoids that are not in the roots. We found licorice leaf extract and its component, 6-prenyl-naringenin upregulated both SPTLC1 and SMPD1 mRNA expression related to ceramide synthesis as well as HMGCR mRNA expression related to the cholesterol synthesis. In addition, licorice leaf extract stimulated ceramide production in skin-equivalent models and human skin and promoted HA synthesis by a mechanism that involves upregulation of HAS3 mRNA expression. These results suggested that the licorice leaf extract may be a useful ingredient for skin hydration and barrier repair. There are few reports on licorice extract and glycyrrhizin used in agriculture and fishery. We examined flavonoid-rich water soluble licorice extract (WSLE) in agriculture and fishery uses. In agriculture, WSLE suppressed hyphal elongation of 12 kinds of plant pathogenic fungi and zoospore release from the conidia. In the pot test, WSLE suppressed the number of lesions in six kinds of plant diseases. As a result, we suggested WSLE has the control effects on some fungal diseases of vegetables such as cucumber, tomato, and sweet pepper. In fishery, WSLE and isoliquiritigenin inhibited the fish disease caused by bacteria, especially Gram-positive bacteria. Effects of WSLE on nonspecific immune response of Japanese flounder were investigated. Oral administration of 5 or 50 mg/kgBW/day of WSLE for 2 weeks showed some significant enhance in humoral (hemolytic and lysozyme activities) and cellular (super oxide anion release and phagocytic activities) activities. After 10 days dietary treatment with WSLE, the fishes were challenged by intraperitoneal injection with E. tarda, WSLE-treated fish demonstrated increased survival rate.

9. Future direction

As for licorice resources, licorice plants are widely found growing wild in regions along the Silk Road. However, according to the recent overharvesting of wild licorice, its habitants are severely disturbed and many of them are degraded or undergoing desertification, especially in China. Therefore, licorice cultivation has been undertaken in China. However, in the present glycyrrhizin and flavonoid content of the cultivated licorice is lower than wild one. In the aim of securing a stable source of licorice, we have to study to obtain the cultivated licorice with same quality of wild licorice.

Over the past half-century, we have been engaged in the development of licorice extracts and its components, and have been offering a number of useful and unique materials to our customers in medicinal, cosmetic, functionary food, and food industries. Elucidation of the constituents and biological activities of both underground and aerial parts in licorice plants have led to the development of many valuable licorice products for various industries. We are further expanding the potential of licorice.

References

1. Shibata S. A Drug over the Millennia: Pharmacognosy, Chemistry and Pharmacology of Licorice. Yakugaku Zasshi. 2000;120:849–862.
2. Isbrucker RA, Burdock GA. Risk and Safety Assessment on the Consumption of Licorice Root (Glycyrrhiza sp.), Its Extract and Powder as a Food Ingredient, with Emphasis on Pharmacology and Toxicology of Glycyrrhizin. Regulatory Toxicology and Pharmacology. 2006;46:167–192.
3. Hayashi H, Sudo H. Economic Importance of Licorice. Plant Biotechnology. 2009;26:101–104.
4. Nomura T, Fukai T. Phenolic Constituents of Licorice (Glycyrrhiza species), In: Herz W, Kirby GW, Moore RE, Steglich W, Tamm Ch (eds.), Progress in the Chemistry of Organic Natural Products 73. Springer Wien, New York; 1998. pp. 1–140.
5. Satake M. Glycyrrhiza Plants. In: Records of Lecture in 2nd Meeting on Crude Drug; December 6; Tokyo. 1986. pp. 1–21.
6. Tamura Y. New Developments in Licorice. Bokin Bobai. 2005;33:127–136.
7. Nieman C. Licorice. Advances in Food Research. 1959;7:339–381.
8. Fenwick GR, Lutomski J, Nieman C. Licorice, Glycyrrhiza glabra L.—Composition, Uses and Analysis. Food Chemistry. 1990;38:119–143.
9. Kuramoto T, Ito Y, Oda M, Tamura Y, Kitahata S. Microbial Production of Glycyrrhetic Acid 3-O-Mono-β-D-Glucuronide from Glycyrrhizin by Cryptococcus Magnus MG-27. Bioscience, Biotechnology and Biochemistry. 1994;58:455–458.
10. Mizutanii K, Kuramoto T, Tamura Y, Ohtake N, Doi S, Nakaura M, Tanaka O. Sweetness of Glycyrrhetic Acid 3-O-β-Monoglucuronide and the Related Glycosides. Bioscience, Biotechnology and Biochemistry. 1994;58:554–555.
11. In-house Data. Application of Glycyrrhizin and Stevioside in Foods. 1994; pp.1–12.
12. Tsukiyama R, Katsura H, Tokuriki N, Kobayashi M. Antibacterial Activity of Licochalcone A Against Spore-Forming Bacteria. Antimicrobial Agents and Chemotherapy. 2002;46:1226–1230.
13. Baumann LS. Less-Known Botanical Cosmeceuticals. Dermatologic Therapy. 2007;20:330–342.
14. Kambara T, Zhou YY, Kawashima Y, Kishida N, Mizutani K, Ikeda T, Kameyama K. A New Dermatological Availability of the Flavonoids from Licorice Roots-Effect on Acne. Journal of Society Cosmetic Chemists Japan. 2003;37:179–186.
15. Okada K, Tamura Y, Yamamoto M, Inoue Y, Takagaki R, Takahashi K, Demizu S, Kajiyama K, Hiraga Y, Kinoshita T. Identification of Antimicrobial and Antioxidant Constituents from Licorice of Russian and Xinjiang Origin. Chemical and Pharmaceutical Bulletin. 1989;37:2528–2530.
16. Yokota T, Nishio H, Kubota Y, Mizoguchi M. The Inhibitory Effect of Glabridin from Licorice Extracts on Melanogenesis and Inflammation. Pigment Cell Research. 1998;11:355–361.
17. Haramoto I. Licorice Extract has an Inhibitory Effect on Melanogenesis and Improves Melasma Other Pigmented Lesions by Its Topical Use. The St. Marianna Medical Journal. 1994;22:941–948.
18. Fukui H, Goto K, Tabata M. Two Antimicrobial Flavanones from the Leaves of Glycyrrhiza glabra. Chemical and Pharmacological Bulletin. 1998;36:4174–4176.
19. Biondi DM, Rocco C, Ruberto G. New Dihydrostilbene Derivatives from the Leaves of Glycyrrhiza glabra and Evaluation of Their Antioxidant Activity. Journal of Natural Products. 2003;66:477–480.
20. Siracusa L, Saija A, Cristani M, Cimino F, D'Arrigo M, Trombetta D, Rao F, Ruberto G. Phytocomplexes from Liquorice (Glycyrrhiza glabra L.) Leaves—Chemical Characterization and Evaluation of Their Antioxidant, Anti-genotoxic and Anti-inflammatory Activity. Fitoterapia. 2011;82:546–556.
21. Kiso A, Kawashima Y, Ohto N, Zhou YY, Tohi K, Murakami T, Araho D, Kambara T, Mizutani K. The Effects of Licorice Leaf Extract on Ceramide and Hyaluronan Synthesis. Journal of Society Cosmetic Chemists Japan. 2009;43:267–273.
22. Miyagawa H. Control of Foliage Diseases of Vegetables by Using a New Licorice Extract, Licorice Extract MZ-1. Food Research. 2009;653:36–39.
23. Miyagawa H, Ohno H. Control of Some Fungal Foliage Diseases of Vegetables Using Purified Licorice Extract. Bulletin of the National Agricultural Research Center for Western Region. 2007;6:55–69.
24. Miyagawa H, Ohno H. Studies on the Mechanism of Cucumber Downy Mildew and Anthracnose Suppression by Licorice Extract. Bulletin of NARO Western Region Agricultural Research Center. 2014;13:71–106.
25. Furushita M, Maeda T, Shiba T, Ohno H, Yamamoto M, Tamura Y. Antimicrobial Activity of a New Licorice Extract-Flavolicorice. Gekkan Aqua Culture. 2005;42:76–77.
26. Miyoshi Y, Fukuda Y, Ohno H, Kawahara E, Kusuda R. Effect of Oral Administration of Licorice Extract on Non-Specific Immune Response of Japanese Flounder, Paralichthys olivaceus. In: Annual Meeting of the Japanese Society of Fish Pathology; September; Nagasaki. 2006.
27. Miyoshi Y, Kawahara E, Fukuda Y. Effect of Oral Administration of Licorice Extract on the Non-Specific Immunodefense Activity of Japanese Flounder, Paralichthys olivaceus. Oita Fisheries Experimental Station Research Report. 2009;1–4.
28. Miyoshi Y, Ohno. Effect of a New Licorice Extract on Disease Resistance in Marine Fishes. Aqua Culture. 2010;47:57–59.

[1] 1. Shibata S. A Drug over the Millennia: Pharmacognosy, Chemistry and Pharmacology of Licorice. Yakugaku Zasshi. 2000;120:849–862.

[2] 2. Isbrucker RA, Burdock GA. Risk and Safety Assessment on the Consumption of Licorice Root (Glycyrrhiza sp.), Its Extract and Powder as a Food Ingredient, with Emphasis on Pharmacology and Toxicology of Glycyrrhizin. Regulatory Toxicology and Pharmacology. 2006;46:167–192.

[3] 3. Hayashi H, Sudo H. Economic Importance of Licorice. Plant Biotechnology. 2009;26:101–104.

[4] 4. Nomura T, Fukai T. Phenolic Constituents of Licorice (Glycyrrhiza species), In: Herz W, Kirby GW, Moore RE, Steglich W, Tamm Ch (eds.), Progress in the Chemistry of Organic Natural Products 73. Springer Wien, New York; 1998. pp. 1–140.

[5] 5. Satake M. Glycyrrhiza Plants. In: Records of Lecture in 2nd Meeting on Crude Drug; December 6; Tokyo. 1986. pp. 1–21.

[6] 6. Tamura Y. New Developments in Licorice. Bokin Bobai. 2005;33:127–136.

[7] 7. Nieman C. Licorice. Advances in Food Research. 1959;7:339–381.

[8] 8. Fenwick GR, Lutomski J, Nieman C. Licorice, Glycyrrhiza glabra L.—Composition, Uses and Analysis. Food Chemistry. 1990;38:119–143.

[9] 9. Kuramoto T, Ito Y, Oda M, Tamura Y, Kitahata S. Microbial Production of Glycyrrhetic Acid 3-O-Mono-β-D-Glucuronide from Glycyrrhizin by Cryptococcus Magnus MG-27. Bioscience, Biotechnology and Biochemistry. 1994;58:455–458.

[10] 10. Mizutanii K, Kuramoto T, Tamura Y, Ohtake N, Doi S, Nakaura M, Tanaka O. Sweetness of Glycyrrhetic Acid 3-O-β-Monoglucuronide and the Related Glycosides. Bioscience, Biotechnology and Biochemistry. 1994;58:554–555.

[11] 11. In-house Data. Application of Glycyrrhizin and Stevioside in Foods. 1994; pp.1–12.

[12] 12. Tsukiyama R, Katsura H, Tokuriki N, Kobayashi M. Antibacterial Activity of Licochalcone A Against Spore-Forming Bacteria. Antimicrobial Agents and Chemotherapy. 2002;46:1226–1230.

[13] 13. Baumann LS. Less-Known Botanical Cosmeceuticals. Dermatologic Therapy. 2007;20:330–342.

[14] 14. Kambara T, Zhou YY, Kawashima Y, Kishida N, Mizutani K, Ikeda T, Kameyama K. A New Dermatological Availability of the Flavonoids from Licorice Roots-Effect on Acne. Journal of Society Cosmetic Chemists Japan. 2003;37:179–186.

[15] 15. Okada K, Tamura Y, Yamamoto M, Inoue Y, Takagaki R, Takahashi K, Demizu S, Kajiyama K, Hiraga Y, Kinoshita T. Identification of Antimicrobial and Antioxidant Constituents from Licorice of Russian and Xinjiang Origin. Chemical and Pharmaceutical Bulletin. 1989;37:2528–2530.

[16] 16. Yokota T, Nishio H, Kubota Y, Mizoguchi M. The Inhibitory Effect of Glabridin from Licorice Extracts on Melanogenesis and Inflammation. Pigment Cell Research. 1998;11:355–361.

[17] 17. Haramoto I. Licorice Extract has an Inhibitory Effect on Melanogenesis and Improves Melasma Other Pigmented Lesions by Its Topical Use. The St. Marianna Medical Journal. 1994;22:941–948.

[18] 18. Fukui H, Goto K, Tabata M. Two Antimicrobial Flavanones from the Leaves of Glycyrrhiza glabra. Chemical and Pharmacological Bulletin. 1998;36:4174–4176.

[19] 19. Biondi DM, Rocco C, Ruberto G. New Dihydrostilbene Derivatives from the Leaves of Glycyrrhiza glabra and Evaluation of Their Antioxidant Activity. Journal of Natural Products. 2003;66:477–480.

[20] 20. Siracusa L, Saija A, Cristani M, Cimino F, D'Arrigo M, Trombetta D, Rao F, Ruberto G. Phytocomplexes from Liquorice (Glycyrrhiza glabra L.) Leaves—Chemical Characterization and Evaluation of Their Antioxidant, Anti-genotoxic and Anti-inflammatory Activity. Fitoterapia. 2011;82:546–556.

[21] 21. Kiso A, Kawashima Y, Ohto N, Zhou YY, Tohi K, Murakami T, Araho D, Kambara T, Mizutani K. The Effects of Licorice Leaf Extract on Ceramide and Hyaluronan Synthesis. Journal of Society Cosmetic Chemists Japan. 2009;43:267–273.

[22] 22. Miyagawa H. Control of Foliage Diseases of Vegetables by Using a New Licorice Extract, Licorice Extract MZ-1. Food Research. 2009;653:36–39.

[23] 23. Miyagawa H, Ohno H. Control of Some Fungal Foliage Diseases of Vegetables Using Purified Licorice Extract. Bulletin of the National Agricultural Research Center for Western Region. 2007;6:55–69.

[24] 24. Miyagawa H, Ohno H. Studies on the Mechanism of Cucumber Downy Mildew and Anthracnose Suppression by Licorice Extract. Bulletin of NARO Western Region Agricultural Research Center. 2014;13:71–106.

[25] 25. Furushita M, Maeda T, Shiba T, Ohno H, Yamamoto M, Tamura Y. Antimicrobial Activity of a New Licorice Extract-Flavolicorice. Gekkan Aqua Culture. 2005;42:76–77.

[26] 26. Miyoshi Y, Fukuda Y, Ohno H, Kawahara E, Kusuda R. Effect of Oral Administration of Licorice Extract on Non-Specific Immune Response of Japanese Flounder, Paralichthys olivaceus. In: Annual Meeting of the Japanese Society of Fish Pathology; September; Nagasaki. 2006.

[27] 27. Miyoshi Y, Kawahara E, Fukuda Y. Effect of Oral Administration of Licorice Extract on the Non-Specific Immunodefense Activity of Japanese Flounder, Paralichthys olivaceus. Oita Fisheries Experimental Station Research Report. 2009;1–4.

[28] 28. Miyoshi Y, Ohno. Effect of a New Licorice Extract on Disease Resistance in Marine Fishes. Aqua Culture. 2010;47:57–59.