Submitted Successfully!
To reward your contribution, here is a gift for you: A free trial for our video production service.
Thank you for your contribution! You can also upload a video entry or images related to this topic.
Version Summary Created by Modification Content Size Created at Operation
1
Choon Young Kim
 + 4812 word(s) 4812 2021-04-14 07:32:44 |
2 format correct
Conner Chen
 -36 word(s) 4776 2021-04-26 08:22:32 |

Video Upload Options

Do you have a full video?
Send video materials Upload full video

Confirm

Are you sure to Delete?
Yes No
Cite
If you have any further questions, please contact Encyclopedia Editorial Office.
Kim, C.Y. Adipocyte Browning. Encyclopedia. Available online: https://encyclopedia.pub/entry/8992 (accessed on 25 April 2024).
Kim CY. Adipocyte Browning. Encyclopedia. Available at: https://encyclopedia.pub/entry/8992. Accessed April 25, 2024.
Kim, Choon Young. "Adipocyte Browning" Encyclopedia, https://encyclopedia.pub/entry/8992 (accessed April 25, 2024).
Kim, C.Y. (2021, April 26). Adipocyte Browning. In Encyclopedia. https://encyclopedia.pub/entry/8992
Kim, Choon Young. "Adipocyte Browning." Encyclopedia. Web. 26 April, 2021.
Adipocyte Browning
Edit
This entry is adapted from the peer-reviewed paper 10.3390/antiox10020308

The role of brown adipocytes in thermogenesis is a potential target for preventing obesity. Obesity results from adipocyte hypertrophy and hyperplasia caused by a severe energy imbalance between food intake and energy expenditure. To achieve both safety and multifunctionality, many in vitro and in vivo studies have focused on finding food extracts or natural products for stimulating adipocyte browning (elevating beige adipocyte differentiation and functions) and combating obesity and related metabolic diseases.

adipocyte browning edible dietary extracts plant extracts marine product extracts

1. Edible Dietary Extracts That Stimulate Adipocyte Browning

Antiobesity properties and multiple target mechanisms of edible dietary extracts have been reported. Recently, adipocyte browning is considered as one of the pivotal underlying mechanisms of antiobesity activities of extracts from fruits, tea, and legumes (Table 1).

Table 1. Stimulatory effects of edible extracts on adipocyte browning.

Extract
(Part/Solvent)		 Model Conc. Effects Active
Component		 Ref.
Red raspberry
(fruit/hot water)		 C57BL/6J mice 100 mg/kg/day ↓obesity
(↓body/ WAT weights)
↑thermogenesis
(↑ucp1, pgc1α, Cidea)		 ellagic acid [1]
↑mitochondrial biogenesis
(↑Sirt3, Nrf1)
Primary brown preadipocytes 100 μg/mL ↑mitochondrial activity
↑brown adipogenesis
(ap2, adiponectin, resistin)
↑thermogenesis
(↑ucp1, pgc1α, Cidea)
↑p-AMPK, p-ACC
Black raspberry
(fruit/hot water)		 hMSCs 5–10 μg/mL ↓adipogenesis ellagic acid [2]
zebrafish 100 μg/mL (↓PPARγ, C/EBPα)
3T3-L1 cells 5–10 μg/mL ↓adipogenesis
(↓PPARγ, C/EBPα)
↑thermogenesis
(↑UCP1, PGC1α)
↑mitochondrial function
(↑CIDEA, Nrf1, CPT1B)
C57BL/6J mice 100 mg/kg/day ↑thermogenesis
(↑body temperature in cold-exposure, ↑UCP1, PGC1α, PRDM16, TBX1)
Strawberry
(fruit/80% MeOH)		 3T3-L1 cells 5–10 μg/mL ↓adipogenesis
(↓PPARγ, C/EBPα, resistin)
↑thermogenesis
(↑UCP1, PDK4)
↑mitochondrial biogenesis
(↑AMPK, Sirt1, PGC1α)		 ND [3]
Omija fruit
(fruit/50% EtOH)		 3T3-L1 cells
Sprague–Dawley rats		 20, 150 μg/mL
5, 200 mg/kg/day		 ↓adipogenesis
(↓C/EBPβ, PPARγ, C/EBPα)
↓obesity
(↓body/ WAT weights)		 ND [4]
C57BL/6J mice 500 mg/kg/day ↓WAT /↑BAT weights
↑energy expenditure
↑thermogenesis
(↑Pparα, Cidea, and COX8β.)		 ND [5]
Green Tea
(leaf/water)		 C57BL/6J mice 0.5% ↓obesity
(↓body/ WAT/ BAT weights)
↑brown-specific markers (↑Ucp1, Prdm16, and CIDEA)
↑mitochondrial activity
(↑Pgc1α and Cpt1B)		 Catechin
EGCG		 [6]
Cinnamon
(bark/70–80% EtOH)		 3T3-L1 cells 80 μg/mL ↑brown-specific markers (↑Cidea, Prdm16Pgc, Cpt-1 and ↑PRDM16), cAMP
↓white adipocyte markers
(↓Dpt and Igf)		 Catechin
Quercetin
Icariin
Chlorogenic acid
Protocatechuic acid
asculetin		 [7]
ex vivo adipocytes isolated from db/db mice 80 μg/mL ↑brown-specific markers (↑Ucp-1, Cidea, Prdm16 and ↑UCP1)
C57BL/6J mice fed with high fat diet 500 mg/kg/day ↑brown-specific markers (↑Ucp-1, Cidea, Prdm16 and ↑UCP1)
↓white adipocyte markers
(↓Dpt)
Kunming mice 90, 180, 360 mg/kg/day ↑thermogenesis
(↑body temperature in cold-exposure, ↑Ucp1, Ppargc1 α, Prdm16 in BAT)
↑energy expenditure
(↑VO2 and VCO2)
Uncoupling ATP production, AMPK-SIRT1 pathway in BAT		 Cinnamaldehyde
Cinnamic acid
2-methoxycinnamaldehyde
coumarin		 [8]
Geminated soy germ(germ/EtOH) 3T3-L1 cells 0.1–10 μg/mL ↓adipogenesis, lipogenesis
↑Lipolysis, β-oxidation		 Soya saponin Ab [9]
C57BL/6J mice 1 mg/kg ↓obesity
(↓body/ WAT weights)
↑thermogenesis
↑mitochondrial biogenesis
Ganoderma tsugae
(fruiting body/EtOH)		 3T3-L1 cells 0.2 mg/mL ↑small lipid droplets formation
↑intracellular lipid metabolism flux/flexibility
↑UCP1, Cidea, HSP60, cyto c
↓NADH/NAD+ ratio, NADH content		 Triterpenoid [10]
C57BL/6Narl 150, 300 mg/kg/day ↑WAT browning
(↑UCP1)↓glucose/lipid disorders
↑SIRT1, p-AMPK		  

hMSCs, human mesenchymal stem cells; WAT, white adipose tissue; BAT, brown adipose tissue; UCP1, uncoupling protein-1; PGC-1α, peroxisome proliferator-activated receptor-gamma coactivator-1-alpha; CIDEA, cell-death-inducing DFFA-like effector-a; Sirt3, sirtuin 3; NRF1, nuclear respiratory factor 1; p-AMPK, phosphorylated AMP-activated protein kinase; p-ACC, phosphorylated acetyl-CoA carboxylase; PPARγ, peroxisome proliferator-activator receptor gamma; C/EBPα, CCAT/enhancer-binding protein alpha; PRDM16, PR domain zinc finger protein 16; TBX1, t-box protein 1; PDK4, pyruvate dehydrogenase lipoamide kinase isozyme 4; COX8β, cytochrome c oxidase subunit 8B; EGCG, epigallocatechin gallate; cAMP, cyclic AMP; CPT-1, carnitine palmitoyltransferase; Dpt, dermatopontin; Igf, insulin-like growth factor; HSP60, heat shock protein 60; cyto c, cytochrome c; NADH, nicotinamide adenine dinucleotide; ND, not determined.

1.1. Berries

Red and black raspberry (Rubus coreanus Miquel) is rich in health-beneficial phytochemicals with antioxidant activities [11]. Among the various health benefits, the antiobesity activity of raspberry has been reported.

In high-fat diet (HFD)-induced obese mice supplemented with red raspberry extract for 10 weeks, the extract inhibited body weight gain and white adipose tissue (WAT) accumulation but activated thermogenic gene (Ucp1Pgc1α, and CIDEA) expression in brown adipose tissue (BAT) [1]. In addition, adipogenic and mitochondria-related genes were upregulated in BAT of mice administrated with red raspberry extracts. Moreover, this extract induced brown adipogenesis and thermogenic gene expression in primary brown preadipocytes.

The activation of adipocyte browning by black raspberry has been reported in both in vitro and in vivo models [2]. While black raspberry extract suppressed white adipocyte differentiation in human mesenchymal cells, murine 3T3-L1 preadipocyte, and zebrafish, adipocyte browning was activated by upregulating beige adipocyte-specific markers, including UCP1, PGC1α, NRF1, CIDEA, and CPT1B. Similarly, the gene expression of beige-specific markers such as UCP1, PRDM16, PGC1α, and TBX1 was induced in inguinal WAT in cold-stressed mice fed with black raspberry extract for 2 weeks. Based on HPLC-MS/MS analysis, 4-hydroxybenzoic acid, ellagic acid, gallic acid, and salicylic acid were identified in black raspberry extract. Among them, ellagic acids in black raspberry responsible for adipocyte browning as demonstrated by the 3T3-L1 cell experiment.

Strawberry (Fragaria × ananassa) exhibits health-promoting and preventive activities against various diseases, including cancer, cardiovascular diseases, type 2 diabetes, and obesity [12]. Inhibition of lipid accumulation and induction of adipose browning by strawberry extract was demonstrated in 3T3-L1 cells [3]. Strawberry extract reduced intracellular lipid accumulation by downregulating adipogenic transcription factors such as PPARγ and C/EBPα. Meanwhile, BAT-specific genes (Pdk4 and Ucp1) were stimulated, suggesting adipocyte browning. Furthermore, strawberry extract elevated the levels of proteins related with mitochondrial biogenesis such as AMPKα, sirtuin 1, and PGC-1α [3]. Consistent with these gene and protein expression profiles, oxygen consumption rate and uncoupled respiration were also increased by strawberry.

1.2. Omija Fruit

Omija (Schisandra chinesis), a magnolia berry with five different distinct flavors (sourness, sweetness, bitterness, pungentness, and saltiness) showed antioxidant and anti-inflammatory activities [13]. The inhibitory effects of omija extract on obesity have been shown in 3T3-L1 cells and rats [4]. Since the adipogenic transcription factors of C/EBPβ, PPARγ, and C/EBPα were significantly decreased, omija extract treatment suppressed adipogenesis, and HFD-induced adipose tissue accumulation and body weight gain. Park et al. [5] showed that omija supplementation (500 mg/kg body weight) for 16 weeks reduced epididymal and visceral WAT but increased BAT in HFD-induced obese mice. Indirect calorimetry analysis also showed significant energy expenditure in omija-treated mice [5]. Consistent with these results, epididymal WAT exhibited beiging indicated by the expression of BAT-specific genes, such as PparαCIDEA, and cytochrome c oxidase subunit 8 B (COX8β). In addition, omija feeding improved hepatic steatosis, dyslipidemia, and glucose tolerance. These results suggest that omija extract helps to prevent obesity and metabolic disturbances by activating the browning of white adipocytes.

1.3. Green Tea

Green tea (Camellia sinensis), the second most popular consumed drinks in the world, showed potent antiobesity effects through the suppression of food intake, dietary fat bioavailability, adipogenesis, fat synthesis, together with accelerated fat oxidation, fecal lipid excretion, and energy expenditure by thermogenesis [14]. Neyrinck et al. [6] demonstrated the antiobesity activity of green tea extract by activating adipocyte browning. HFD-fed mice supplemented with 0.5% green tea leaf extract for 8 weeks had significantly lower body weight and white and brown adipocytes weights [6]. In addition, the levels of genes related to mitochondrial activity (Pgc1α and Cpt1b) and brown-specific markers (Ucp1Prdm16, and CIDEA) were higher in the subcutaneous WAT of mice fed with green tea and HFD compared with mice fed with HFD [6]. Additionally, immunohistological analysis of UCP1 in the subcutaneous WAT of the green tea-supplemented mice showed a significantly higher staining area than that of untreated mice, confirming the browning of WAT.

1.4. Cinnamon

Cinnamon is a spice derived from the inner bark of trees from the genus Cinnamomum cassia belongs to the Lauraceae family. Cinnamon has been used as a culinary ingredient and traditional medicine due to its antioxidant, anti-inflammatory, antihyperglycemic, and antihyperlipidemic activities [15]. Recently, the stimulatory effect of cinnamon extract on the activation of BAT and the browning of WAT. Kwan et al. showed that the treatment of cinnamon extract elevated the gene expression of brown adipocyte markers (Cidea, Prdm16Pgc, and Cpt-1) while reduced that of white adipocyte markers (Dpt and Igf) in 3T3-L1 adipocytes and WAT from db/db mice. In the same study, HFD-induced obese mice were fed with cinnamon extract exerted significantly lower body weight and elevated brown adipocyte marker genes such as Ucp1Cidea, and Prdm16 in WAT. Another study showed that cinnamon extract stimulates thermogenesis in mice under cold exposure by the activation of brown adipose tissue [8]. While mice placed in cold environments reduced body temperature and energy expenditure, mice fed with cinnamon extract increased those by activation of BAT (upregulation of UCP1 and PGC-1α) and browning of WAT (upregulation of Ucp1Ppargc1α, and Prdm16). The underlying mechanisms of cinnamon extract were determined as the activation of the AMPK/SIRT1 pathway [8].

1.5. Germinated Soybean Germ

Germination enhances phytochemicals’ health-promoting activities such as antioxidant and anti-inflammatory properties [16]. Kim et al. [9] reported that germinated soy germ extract prevents obesity through adipocyte browning in vitro and in vivo. In 3T3-L1 cells, germinated soybean germ treatment lowered accumulation of lipids and expression levels of genes involved in adipogenesis (C/EBPβ, PPARγ, and C/EBPα) and lipogenesis (SREPB1c, ACC, FAS, and SCD1) but elevated those of genes involved in lipolysis, β-oxidation, and thermogenesis. Consistent with the in vitro results, germinated soybean germ extract reduced body weight gain and adipose tissue accumulation in mice by inhibiting genes related to adipogenesis and lipogenesis. Germinated soybean germ extract also induced adipocyte browning by upregulating UCP1, CPT1, PGC-1α, and PPARα.

1.6. Ganoderma Tsugae

Ganoderma tsugae Murrill is an edible fungi in the family Ganodermataceae. It is also known as lingzhi or reishi and is a traditional Chinese medicinal mushroom used as a popular functional food worldwide [17]. Various pharmacologically active ingredients, such as polysaccharides, triterpenoids, nucleosides, proteins/peptides, organic germanium compounds, and other trace elements, have been isolated from G. tsugae extracts and characterized [17]. These active ingredients have demonstrated several therapeutic effects, including antioxidant, anti-inflammatory, antibacterial, antitumor, anti-HIV, blood pressure regulatory, hepatoprotective, and immunomodulatory, cardioprotective properties and can act as a nerve tonic [18][19][20].

In addition to these therapeutic effects, Tseng et al. [10] recently demonstrated that triterpenoid-rich G. tsugae ethanol extract (GTEE) could improve obesity by promoting intracellular metabolic flexibility and plasticity and inducing adipocyte browning. The data showed that low-dose GTEE (0.2 mg/mL) in 3T3-L1 cells induced adipogenesis and small lipid droplet formation and promoted intracellular lipid metabolism flux and flexibility [10]. It also induced the browning of 3T3-L1 adipocytes by upregulating UCP1, CIDEA, HSP60, and cytochrome c proteins while downregulating the NADH/NAD+ ratio and NADH content [10]. Furthermore, in vivo investigations of GTEE administration to male C57BL/6Narl HFD-fed mice upregulated UCP1 in the inguinal WAT to induce browning while reducing fasting blood glucose, triglyceride, and LDL cholesterol levels, thereby improving glucose intolerance and lipid dysfunction [10]. These effects of GTEE were accompanied with increased expression level of SIRT1 and threonine-172 phosphorylation of AMPK. This indicates GTEE as a prospective treatment strategy for obesity.

2. Plant Extracts That Stimulate Adipocyte Browning

Emerging research indicates that plant extracts can be important environmental regulators of WAT browning and energy homeostasis. Therefore, various in vitro and in vivo studies have investigated the effects of plant extracts on adipocyte metabolism and obesity (Table 2).

Table 2. Plant extracts to induce adipocyte browning.

Extract
(Part/Solvent)		 Model Conc. Effects Active
Component		 Ref.
Panax ginseng
(root and leaf/ND)		 3T3-L1 cells 25–100 μg/mL ↓adipogenesis
(↓C/EBPα, SREBP1-c)
↑mitochondrial activity
↑brown-adipocyte-specific markers
(↑UCP1, PRDM16, PGC-1 α)
↑p-AMPK		 Gensenoside Rb1
Rb2
Rg1
Rg3		 [21][22][23][24][25]
primary white adipocytes
Phyllostachys pubescens
and
Scutellaria baicalensis
(root and leaf/70% EtOH)		 3T3-L1 cells 60–480 μg/mL ↓adipogenesis
(↓PPARγ, C/EBPα)
↓lipogenesis
(↓SREBP-1c, FAS)
↑fatty acid oxidation, lipolysis
(↑p-ACC, CPT1)
↑BAT markers
(↑UCP1, PRDM16, PGC1α)
↑thermogenesis
(↑UCP2)
↑p-AMPK		 Chlorogenic acid
Orientin
Isoorientin
Baicalin
Wogonoside
Baicalein
Tricin
Wogonin
Chrysin		 [10]
Humulus japonicas
(leaf/water)		 3T3-L1 cells 20, 100 μg/mL ↑thermogenesis, browning
(↑UCP1, PRDM16, PGC-1 α)
↑fatty acid oxidation, lipolysis
↓lipogenesis, lipid accumulation
↓oxidative stress/↑SOD1, catalase, GPx1
↑AMPK/PPARδ signaling pathway		 ND [26]
Immature
Citrus reticulate
(fruit/hot water)		 C57BL/6
mice		 1% ↓body/visceral fat weights, adipocyte size
↓fatty livers, insulin resistance, dyslipidemia
↑cold tolerance in cold exposure
↑thermogenesis
(↑UCP1, PRDM16, NRF1)
↑beige adipocyte-selective markers
(↑TEME26, CD137, Cidea)		 Synephrine
Narirutin
Hesperidin
Nobiletin
tangeretin		 [27]
Broccoli Seeds
(sprout/water)		 C57BL/6JSlc mice 0.3% ↓body weight gain, fat mass
↑energy expenditure
↑major browning marker
(↑UCP1)
↓insulin resistance, glucose tolerance
↓plasma lipopolysaccharide
↓relative abundance of Desulfovibrionaceae bacteria
↓oxidative stress, inflammation		 Glucoraphanin [28]

C/EBPα, CCAT/enhancer binding protein alpha; SREBP1-c, sterol regulatory element-binding protein 1; UCP1, uncoupling protein 1; PRDM16, PR domain zinc finger protein 16; PGC-1α, peroxisome proliferator-activated receptor gamma coactivator-1-alpha; p-AMPK, phosphorylated AMP-activated protein kinase; CIDEA, cell-death-inducing DFFA-like effector-A; HSP60, heat shock protein 60; cyto c, cytochrome c; NADH, nicotinamide adenine dinucleotide; WAT, white adipose tissue; Sirt1, sirtuin 1; SOD1, superoxide dismutase 1; GPx1, glutathione peroxidase 1; PPARδ, peroxisome proliferator-activated receptor delta; NRF1, nuclear respiratory factor 1; TEME26, transmembrane protein 26; CD137, cluster of differentiation 137; FAS, fatty acid synthase; p-ACC, phosphorylated acetyl-CoA carboxylase; CPT-1, carnitine palmitoyltransferase; BAT, brown adipose tissue; ND, not determined.

2.1. Panax Ginseng

Ginseng (Panax ginseng Mayer) of the Araliaceae family is a traditional medicinal herb registered in the Chinese classic oriental herbal dictionary as “shin-nong-bon-cho-kyung” with various pharmacological properties [29]. Depending on the processing method, ginseng can be classified into three types: white, red, and black [29][30]. Among these, black ginseng (BG), a ginseng product prepared by the steaming-and-drying process for nine times, exhibits more potent pharmacological and biological activity than either white or red ginseng [29][30][31]. This difference may be because of the conversion of ginsenosides from fresh ginseng into less polar forms during steaming [31]. To date, 19 types of ginsenosides (F4, Rb1, Rb2, Rc, Rd, Re, Rf, Rg1, Rg5, Rg6, Rh4, Rk1, Rk3, Rs4, Rs5, 20(R)-Rg3, 20(R)-Rs3, 20(S)-Rg3, and 20(S)-Rs3) have been identified in BG [30][31]. Previous studies have demonstrated that ginsenosides Rb1, Rb2, Rg1, and Rg3 exhibit antiobesity activity [21][22][23][24][25].

Park et al. [25] showed that BG and ginsenoside Rb1 exhibit antiobesity effects by inducing browning in 3T3-L1 adipocytes and primary white adipocytes (PWATs) through activation of the AMPK signaling cascade. BG (25, 50, and 100 μg/mL) and Rb1 (10, 20, and 40 μM) inhibited the early stages of adipogenesis in 3T3-L1 adipocytes and PWATs by lowering the expression levels of C/EBPα and SREBP-1c to reduce lipid accumulation [25]. In addition, BG and Rb1 have been shown to induce browning of 3T3-L1 adipocytes and PWATs through increased mitochondrial activity and expression of BAT-specific markers such as PRDM16, PGC-1α, PPARγ, and UCP1 [25]. However, this phenomenon was abolished in PWATs treated with the AMPK inhibitor dorsomorphin, suggesting that the browning and antiobesity effects of BG and Rb1 are mediated by activation of the AMPK signaling cascade [25].

Another study investigated the antiobesity activity of ginsenoside Rb2 [21]. Data showed that Rb2 (40 mg/kg/day) treatment resulted in lower body weight gain, enhanced insulin sensitivity, and elevated energy expenditure in diet-induced obese (DIO) mice [21]. Additionally, treating mice with Rb2 was shown to induce the activation of BAT and browning of WAT by reducing lipid droplet size, stimulating UCP1 staining, and upregulating thermogenic and mitochondrial gene expression [21]. The authors also reported that activation of the AMPK pathway is responsible for Rb2-mediated upregulation of browning gene expression [21]. Furthermore, in other studies, Lee et al. and Kim et al. [22][23] demonstrated that Rg1 and Rg3 exert anti-obesity effects by upregulating browning-related gene expression and mitochondrial biosynthesis through activation of the AMPK pathway.

These results suggest the potential for BG and ginsenosides to act as browning agents and exert anti-obesity effects, an area that may be explored in future studies. Further investigation is still needed to confirm whether Rb1, Rb2, Rg1, and Rg3, and other ginsenosides, contribute to the browning process.

2.2. Phyllostachys Pubescens and Scutellaria baicalensis

The leaves of Phyllostachys pubescens Mazel (bamboo), a plant of the family Poaceae commonly consumed as a tea, have various biological functions, such as being an antioxidant and anticoagulant [32]. The roots of Scutellaria baicalensis Georgi (Baikal skullcap), a plant of the family Lamiaceae, are widely used in traditional medicine, preventing inflammation, diuresis, and diarrhea [33].

In a recent study, a 2:1 (w:w) mixture of P. pubescens leaf extract and S. baicalensis root extract (BS21) was used to investigate its effects on adipogenesis and browning in vitro [34]. The results showed that BS21 treatment markedly reduced the accumulation and size of lipid droplets and the levels of leptin and adiponectin in 3T3-L1 adipocytes [34]. In addition, treatment with BS21 lowered the expression levels of white adipocyte markers (PPARγ, C/EBPα, and ap2) and lipogenic markers (SREBP1c and FAS), but increased the expression levels of β-oxidation proteins (CPT1 and p-ACC) [34]. Furthermore, BS21 treatment increased the expression of brown adipocyte marker proteins, such as UCP1, PRDM16, and PGC1α, and thermogenesis-related genes such as UCP2 in 3T3-L1 adipocytes, suggesting that BS21 induces adipocyte browning and thermogenesis [34]. These effects were mediated by activation of the AMPK signaling pathway, indicated by Western blot analysis [34]. According to UPLC analysis, chlorogenic acid, orientin, baicalin, wogonoside, baicalein, tricin, wogonin, and chrysin were identified in BS21, of which adipocyte differentiation and leptin level were markedly suppressed in all compounds except for wogonoside [34]. These results suggest that BS21 has antiobesity efficacy by inhibiting adipogenesis and lipogenesis and inducing fat oxidation and browning.

2.3. Humulus Japonicus

Humulus japonicus, also known as “Japanese hop”, is a perennial herb belonging to the Cannabaceae family and is ubiquitously found in Asian countries, including Korea, Japan, and China [35]H. japonicus has long been used in traditional medicine to cure skin diseases, pulmonary tuberculosis, and hypertension [35]. Other biological effects of H. japonicus include antimutagenic, antibacterial, antiatheroma, antioxidant, antitumor, antimycobacterial, and anti-inflammatory effects [35][36][37][38][39].

A recent study has shown that H. japonicus aqueous extract (AH) can suppress obesity by stimulating thermogenesis and improving oxidative stress through a BAT-like phenotype in 3T3-L1 adipocytes [26]. Treatment with AH (20 and 100 μg/mL) upregulated the expression of BAT-specific markers, such as UCP1, PRDM16, and PGC-1α, in 3T3-L1 adipocytes, suggesting that AH stimulates thermogenesis and browning [26]. In addition, AH promoted fatty acid oxidation and lipolysis while notably inhibiting lipogenesis and lipid accumulation [26]. Oxidative stress could influence the development of obesity-related metabolic disorders [40]. AH also improved hydrogen peroxide-induced oxidative stress and markedly increased the expression level of the antioxidant enzymes SOD1, catalase, and GPx1 [26]. The antiobesity process of stimulating browning and lipid metabolism while reducing oxidative stress in WAT has been shown to involve activation of the AMPK and PPARδ signaling pathways [26]. However, more research into the stimulation of thermogenesis and induction of oxidative stress improvement by H. japonicus is needed using in vivo models of obesity.

2.4. Immature Citrus Reticulata

Ponkan (Citrus reticulata) is a commercial Mandarin cultivar belonging to the genus Citrus of the Rutaceae family [41]. Immature C. reticulata contains higher amounts of p-synephrine, nobiletin, and tangeretin than other citrus species, showing diverse biological activities [42].

In rodents, immature C. reticulata extract (ICRE) can exert positive effects on browning of WAT, thereby suppressing obesity and hepatic steatosis [27]. Administration of 1% ICRE for 11 weeks induced body weight loss in HFD-fed mice, accompanied by a decrease in visceral fat (epididymal, retroperitoneal, and mesenteric) weight and adipocyte size [27]. The administration of ICRE also markedly reduced hepatic steatosis, fasting blood glucose, insulin, and homeostatic model assessment for insulin resistance, serum triglyceride, and total cholesterol levels, suggesting that ICRE can improve HFD-induced fatty liver disease, insulin resistance, and dyslipidemia [27]. In particular, the administration of ICRE improved cold tolerance during cold exposure in HFD mice. These effects were associated with the increased expression level of thermogenic genes, such as UCP1PRDM16, and NRF1, and beige adipocyte-selective markers, such as TEME26, CD137, and CIDEA, in inguinal WAT. These results suggest that ICRE has antiobesity efficacy by inducing BAT-like formation. However, more clarity is need on the possible molecular mechanisms involved in ICRE-induced adipocyte browning.

2.5. Glucoraphanin from Broccoli Seeds

Glucoraphanin, a precursor of sulforaphane, is an isothiocyanate derivative found in cruciferous vegetables of the family Brassicaceae, such as cauliflower, collard, and cabbage, and especially highly concentrated in broccoli seeds and sprouts [43]. When plant tissues and cells are destroyed by external stimuli, glucoraphanin is hydrolyzed by myrosinase to produce biologically activated sulforaphane [44]. Sulforaphane is a potent natural nuclear factor (erythroid-derived 2)-like 2 (Nrf2) inducer that has various pharmacological effects, such as antioxidant, anticancer, anti-aging, and anti-inflammatory effects [45].

It has recently been confirmed that glucoraphanin can induce browning of adipose tissue and reduce metabolic endotoxemia, thereby preventing metabolic disorders, such as obesity and type 2 diabetes [28]. In HFD-induced obese mice, administration of 0.3% glucoraphanin for 14 weeks reduced body weight gain and fat mass and increased energy expenditure. Glucoraphanin also increased the expression level of UCP1, a major browning marker, in inguinal and epididymal adipose depots and improved systemic glucose tolerance and insulin sensitivity. However, this phenomenon was abolished in homozygous NRF2-deficient (Nrf2–/–) mice, suggesting that the antiobesity and insulin-sensitizing effects of glucoraphanin are mediated by NRF2. Additionally, glucoraphanin downregulated plasma lipopolysaccharide levels and reduced the relative abundance of Desulfovibrionaceae bacteria, which are major producers of endotoxins in the gut microbiome. It also inhibited hepatic lipogenic gene expression, lipid peroxidation, M1-like macrophage accumulation, and inflammatory signaling pathways, suggesting that glucoraphanin relieves oxidative stress and inflammation caused by HFD.

Taken together, these findings indicate that glucoraphanin may be effective in preventing hepatic steatosis, insulin resistance, and chronic inflammation by promoting energy expenditure and suppressing gut-derived metabolic endotoxemia.

3. Marine Products That Induce Adipose Browning

Marine products have great attention due to their potential applications in functional foods and food additives because of their health-promoting properties, including antiobesity, antioxidant, anti-inflammatory, and anticancer effects [46]. Recent studies have revealed new roles of marine products in adipocyte browning and energy balance (Table 3).

3.1. Sargassum Serratifolium (C. Agardh)

Sargassum serratifolium, a marine brown alga, has been widely utilized as a food and traditional medicine in Asia. A study examined the roles of a meroterpenoid-rich fraction of an ethanolic extract of S. serratifolium (MES) in HFD-induced obesity and related metabolic syndrome C57BL/6J mice. MES administration notably decreased obesity and hepatic steatosis without altering food intake. The beneficial effects of MES are partially ascribed to increased lipid catabolic AMPK signaling pathways and highly elevated UCP1-positive cells in adipose tissue [47], indicative of MES-stimulated adipose tissue browning.

Chemical composition analysis revealed that MES contains a high level of meroterpenoids, including sargachromenol, sargaquinoic acid (SQA), and sargahydroquinoic acid (SHQA) as the most abundant compound [47]. When the direct effects of SHQA on adipocytes were tested in conditions simulating adipocyte browning, lipolysis, and mitochondrial number was increased, but ATP production decreased. The authors further examined uncoupled metabolic signaling and found that SHQA treatment significantly elevated UCP1-positive adipocytes and beige adipocyte markers [48]. The adipose browning effects of SHQA were related to the activation of PPARγ, PPARα, and AMPKα.

The browning effects of SQA were tested using 3T3-L1 adipocytes differentiated under probrowning conditions. SQA treatment stimulated the differentiation of white adipocytes into beige adipocytes and decreased lipid accumulation. SQA activated AMPK and upregulated genes associated with lipid catabolic pathways, including perilipin, carnitine palmitoyltransferase 1, and acyl-CoA synthetase long-chain family member 1 [49]. These findings confirm SHQA and SQA as active MES compounds that stimulate lipid catabolic signaling and facilitate white to beige adipocyte differentiation. Further studies are still required on the adipocyte browning effects of sargachromenol, the remaining major MES compound.

Table 3. Marine products to stimulate adipocyte browning.

Extract
(Part/Solvent)		 Model Conc. Effects Active
Component		 Ref.
Sargassum
Serratifolium
(whole/EtOH)		 C57BL/6J mice 30–120 mg/kg/day ↑AMPK signaling pathway
↑UCP1-positive cells
↓lipogenesis
(↓SREBP1c, SCD-1, FAS)
↑lipolysis
(↑PLIN, CPT1, ACSL1)
↑mitochondria function		 SHQA
SQA		 [49][48]
Spirulina maxima
(whole/EtOH)		 3T3-L1 cells 50, 100 μg/mL ↑lipid accumulation
↓adipogenesis
(↓C/EBPα, PPARγ, aP2)
↓lipogenesis
(↓SREBP1c, ACC, FAS, LPAATβ, Lipin1, DGAT1)		 chlorophyll A
C-phycocyanin		 [50]
ICR mice 150, 450 mg/kg/day ↑p-AMPK
↑adipose browning proteins
(↑PRDM16, PGC1α, UCP1)
Phaeodactylum
Tricornutum
(whole/ND)		 C57BL/6J mice 0.81, 1.62, 3.25 mg/kg/day ↓body weight, organ weight, adipocyte size
↑blood metabolic profile		 fucoxanthin [51]
3T3-L1 cells 20, 40 μM ↑UCP1
Nitzschia laevis
(whole/EtOH)		 C57BL/6J mice 10, 50 mg/kg/day ↓body weight↑BAT cell number
↑thermogenesis
(↑UCP1)		 ND [52]
Undaria pinnatifida
(whole/chloroform/
methanol)		 Wistar rats and KK-Ay mice 0.5 and 2% in diet ↓WAT weight
↑BAT weight
↑UCP1 only in WAT		 fucoxanthin [53]

AMPK, AMP-activated protein kinase; UCP1, uncoupling protein 1; SREBP1c, sterol regulatory element-binding protein 1c; SCD1, stearoyl-CoA desaturase 1; FAS, fatty acid synthase; PLIN, perilipin; CPT1, carnitine palmitoyltransferase 1; ACSL1, acyl-CoA synthetase long-chain family member 1; SHQA, sargahydroquinoic acid; SQA, sargaquinoic acid; C/EBPα, CCAT/enhancer binding protein alpha; PPARγ, peroxisome proliferator-activator receptor gamma; aP2, adipocyte protein 2; ACC, acetyl-CoA carboxylase; LPAATβ, lysophosphatidic acid acyltransferase beta; DGAT1, diacylglycerol acyltransferase 1; PRDM16, PR domain zinc finger protein 16; PGC1α, peroxisome proliferator-activated receptor-gamma coactivator-1-alpha; BAT, brown adipose tissue. ND, not determined.

3.2. Spirulina Maxima

Spirulina maxima is a microalga that is abundant in essential nutrients and includes pigment proteins including chlorophyll a and C-phycocyanin [54][55]. Studies have reported that S. maxima exhibit antioxidant, anticancer, and neuroprotective effects [46] but its potential in obesity and adipose tissues is unclear. A recent study examined the ethanol extract of S. maxima on adipogenesis, lipogenesis, and browning using in vitro and in vivo mouse models [50]. The treatment of the extract decreased intracellular lipid accumulation in 3T3-L1 adipocytes, reduced protein expression levels of the adipogenic genes, including C/EBPα, PPARγ, and aP2, and the lipogenic genes, including SREBP1, ACC, FAS, LPAATβ, Lipin1, and DGAT1 [50]. When the extract was supplemented in HFD-fed male ICR mice, DIO was inhibited at both low and high concentrations (150 and 450 mg/kg, respectively). Furthermore, Spirulina ethanol extract-supplemented mice showed lower adipose tissue mass and blood lipid concentrations than HFD-fed mice. These characteristics are closely related to the activation of AMPK and the upregulation of adipose browning proteins, including PRDM16, PGC1α, and UCP1 [50]. When the index components (chlorophyll A and C-phycocyanin) of the ethanol extract were administered in 3T3-L1 and C3H10T1/2 cells, both compounds decreased the protein expression related to adipogenesis and lipogenesis. However, their effects on browning markers still need to be confirmed in future studies.

3.3. Phaeodactylum Tricornutum

Phaeodactylum tricornutum is a plentiful source of fucoxanthin, a marine carotenoid found in macroalgae, with health-promoting effects, including antiobesity effects. However, fucoxanthin is scarce and requires delicate extraction techniques, limiting the number of applied research studies to date [51]. In one such study, the antiobesity effects of a Phaeodactylum ethanol extract were tested using cell and animal models. In 3T3-L1 adipocytes treated with the extract, UCP1 protein levels were upregulated at 400 μg/mL. When applied to HFD-induced obese mice, the oral injections of Phaeodactylum extract (0.81, 1.62, and 3.25 mg/kg/day) reduced body weight, organ weight, and adipocyte size while ameliorating the blood metabolic profile [51]. In the same study, fucoxanthin treatment at 20 or 40 μM also upregulated the protein levels of UCP1 in adipocytes. When orally injected into the HFD mice, fucoxanthin (0.1 mg/kg/day) ameliorated DIO and metabolic profile. These findings suggest that fucoxanthin mediates the adipose browning and antiobesity effects of Phaeodactylum extract.

3.4. Nitzschia Laevis

The microalga Nitzschia laevis has been reported to contain polyphenols, polyunsaturated fatty acids, and fucoxanthin [52][56][57]Nitzschia laevis extract has great potential as dietary supplement for various health-promoting effects, and its effects on obesity have also recently been confirmed. An ethanol extract of N. laevis (10 or 50 mg/kg/day) was administered orally to HFD-fed C57BL/6J mice, significantly decreasing body weight without altering food intake and lipid accumulation in the liver and WAT [52]. In addition, supplementation with N. laevis significantly elevated the number of BAT cells and the mRNA expression levels of UCP1. In the same study, N. laevis-fed mice maintained gut epithelium integrity and gut microbiota composition against HFD-induced complications. Although the focus of the study was largely on the effects of N. laevis on the composition of the gut microbiota’s role in antiobesity, an UCP1-induced thermogenic effect by N. laevis supplementation is still plausible. Further research into the roles of N. laevis supplementation in the browning of WAT and related signaling pathways are still required.

3.5. Undaria Pinnatifida

Undaria pinnatifida is one of the most consumed edible seaweed in Korea and Japan. A study examined the antiobesity effects of lipids from Undaria pinnatifida using male Wistar rats and female KK-Ay mice. When the animals were fed 2% Undaria lipids mixed with experimental diets, the weight of WAT was significantly reduced while the weight of BAT was greater than in that of control mice [53]. Nevertheless, there was no difference in UCP1 expression in BAT between groups, indicating that the reduction in WAT weight in Undaria lipids-fed mice may not be explained only through the UCP1-dependent thermogenic energy expenditure in BAT. Thus, the authors tested whether Undaria lipids affect thermogenic signaling in WAT of mice [53]. While there was little expression in the WAT of control mice, the protein levels of UCP1 markedly increased in WAT of Undaria lipids-fed mice in a concentration-dependent manner. However, UCP2 expression was reduced by Undaria lipid feeding compared to the control mice, suggesting that UCP1 signaling in WAT contributes to the significant decrease in fat mass in Undaria lipids-fed mice [53]. Fucoxanthin may be involved in the Undaria lipids-mediated antiobesity activity [51][53]. When dried powder of Undaria pinnatifida after removing carbohydrate and protein was extracted with chloroform/methanol (2:1, v/v), the powder contained 15% (w/w) lipids, of which fucoxanthin was quite abundant (9.6%) [53]. However, conflicting results also exist when fucoxanthin was treated in human adipocytes [58]. When human adipocytes were treated with fucoxanthin or fucoxanthinol because fucoxanthin is converted to fucoxanthinol in adipocytes of mice in 48–57 h [59], there were no apparent effects on oxygen consumption rate and the mRNA expression levels of genes related to adipocyte browning including UCP1 and PGC1α [58]. Therefore, further studies are necessary to determine the active components of Undaria lipids that stimulate adipocyte browning and antiobesity effects.

References

  1. Jeong, M.; Kim, H.; Park, J.; Jung, Y.; Youn, D.; Lee, J.; Jin, J.; So, H.; Park, R.; Kim, S. Rubi fructus (rubus coreanus) activates the expression of thermogenic genes in vivo and in vitro. Int. J. Obes. 2015, 39, 456–464.
  2. Park, W.Y.; Choe, S.-K.; Park, J.; Um, J.-Y. Black raspberry (rubus coreanus miquel) promotes browning of preadipocytes and iinguinal white adipose tissue in cold-induced mice. Nutrients 2019, 11, 2164.
  3. Forbes-Hernández, T.Y.; Cianciosi, D.; Ansary, J.; Mezzetti, B.; Bompadre, S.; Quiles, J.L.; Giampieri, F.; Battino, M. Strawberry (fragaria × ananassa cv. Romina) methanolic extract promotes browning in 3t3-l1 cells. Food Funct. 2020, 11, 297–304.
  4. Park, H.J.; Cho, J.-Y.; Kim, M.K.; Koh, P.-O.; Cho, K.-W.; Kim, C.H.; Lee, K.-S.; Chung, B.Y.; Kim, G.-S.; Cho, J.-H. Anti-obesity effect of schisandra chinensis in 3t3-l1 cells and high fat diet-induced obese rats. Food Chem. 2012, 134, 227–234.
  5. Park, H.J.; Kim, H.-J.; Kim, S.R.; Choi, M.-S.; Jung, U.J. Omija fruit ethanol extract improves adiposity and related metabolic disturbances in mice fed a high-fat diet. J. Nutr. Biochem. 2017, 41, 137–141.
  6. Neyrinck, A.M.; Bindels, L.B.; Geurts, L.; Van Hul, M.; Cani, P.D.; Delzenne, N.M. A polyphenolic extract from green tea leaves activates fat browning in high-fat-diet-induced obese mice. J. Nutr. Biochem. 2017, 49, 15–21.
  7. Kwan, H.Y.; Wu, J.; Su, T.; Chao, X.-J.; Liu, B.; Fu, X.; Chan, C.L.; Lau, R.H.Y.; Tse, A.K.W.; Han, Q.B. Cinnamon induces browning in subcutaneous adipocytes. Sci. Rep. 2017, 7, 1–12.
  8. Li, X.; Lu, H.-Y.; Jiang, X.-W.; Yang, Y.; Xing, B.; Yao, D.; Wu, Q.; Xu, Z.-H.; Zhao, Q.-C. Cinnamomum cassia extract promotes thermogenesis during exposure to cold via activation of brown adipose tissue. J. Ethnopharmacol. 2021, 266, 113413.
  9. Kim, H.-J.; Choi, E.-J.; Kim, H.S.; Choi, C.-W.; Choi, S.-W.; Kim, S.-L.; Seo, W.-D.; Do, S.H. Germinated soy germ extract ameliorates obesity through beige fat activation. Food Funct. 2019, 10, 836–848.
  10. Tseng, H.H.; Yeh, W.C.; Tu, Y.C.; Yang, B.F.; Lai, Y.T.; Lee, H.K.; Yang, Y.C.; Huang, H.C.; Lee, Y.J.; Ou, C.C. Proteomic profiling of ganoderma tsugae ethanol extract-induced adipogenesis displaying browning features. FEBS Lett. 2018, 592, 1643–1666.
  11. Rao, A.V.; Snyder, D.M. Raspberries and human health: A review. J. Agric. Food Chem. 2010, 58, 3871–3883.
  12. Giampieri, F.; Forbes-Hernandez, T.Y.; Gasparrini, M.; Alvarez-Suarez, J.M.; Afrin, S.; Bompadre, S.; Quiles, J.L.; Mezzetti, B.; Battino, M. Strawberry as a health promoter: An evidence based review. Food Funct. 2015, 6, 1386–1398.
  13. Han, H.J.; Jung, U.J.; Kim, H.-J.; Cho, S.-J.; Kim, A.H.; Han, Y.; Choi, M.-S. Combined supplementation with grape pomace and omija fruit ethanol extracts dose-dependently improves body composition, plasma lipid profiles, inflammatory status, and antioxidant capacity in overweight and obese subjects. J. Med. Food 2016, 19, 170–180.
  14. Huang, J.; Wang, Y.; Xie, Z.; Zhou, Y.; Zhang, Y.; Wan, X. The anti-obesity effects of green tea in human intervention and basic molecular studies. Eur. J. Clin. Nutr. 2014, 68, 1075–1087.
  15. Singletary, K. Cinnamon: Update of potential health benefits. Nutr. Today 2019, 54, 42–52.
  16. Gan, R.-Y.; Lui, W.-Y.; Wu, K.; Chan, C.-L.; Dai, S.-H.; Sui, Z.-Q.; Corke, H. Bioactive compounds and bioactivities of germinated edible seeds and sprouts: An updated review. Trends Food Sci. Technol. 2017, 59, 1–14.
  17. Chin, S.K.; Law, C.; Supramaniam, C.; Cheng, P.-G.; Mujumdar, A. Convective drying of ganoderma tsugae murrill and effect of temperature on basidiospores. Dry. Technol. 2008, 26, 1524–1533.
  18. Wasser, S.P. Medicinal mushrooms as a source of antitumor and immunomodulating polysaccharides. Appl. Microbiol. Biotechnol. 2002, 60, 258–274.
  19. Mau, J.-L.; Tsai, S.-Y.; Tseng, Y.-H.; Huang, S.-J. Antioxidant properties of hot water extracts from ganoderma tsugae murill. LWT-Food Sci. Technol. 2005, 38, 589–597.
  20. Paterson, R.R. Ganoderma-a therapeutic fungal biofactory. Phytochemistry 2006, 67, 1985–2001.
  21. Hong, Y.; Lin, Y.; Si, Q.; Yang, L.; Dong, W.; Gu, X. Ginsenoside rb2 alleviates obesity by activation of brown fat and induction of browning of white fat. Front. Endocrinol. 2019, 10, 153.
  22. Kim, K.; Nam, K.H.; Yi, S.A.; Park, J.W.; Han, J.W.; Lee, J. Ginsenoside rg3 induces browning of 3t3-l1 adipocytes by activating ampk signaling. Nutrients 2020, 12, 427.
  23. Lee, K.; Seo, Y.J.; Song, J.H.; Chei, S.; Lee, B.Y. Ginsenoside rg1 promotes browning by inducing ucp1 expression and mitochondrial activity in 3t3-l1 and subcutaneous white adipocytes. J. Ginseng. Res. 2019, 43, 589–599.
  24. Mu, Q.; Fang, X.; Li, X.; Zhao, D.; Mo, F.; Jiang, G.; Yu, N.; Zhang, Y.; Guo, Y.; Fu, M.; et al. Ginsenoside rb1 promotes browning through regulation of ppargamma in 3t3-l1 adipocytes. Biochem. Biophys. Res. Commun. 2015, 466, 530–535.
  25. Park, S.-J.; Park, M.; Sharma, A.; Kim, K.; Lee, H.-J. Black ginseng and ginsenoside rb1 promote browning by inducing ucp1 expression in 3t3-l1 and primary white adipocytes. Nutrients 2019, 11, 2747.
  26. Jung, T.W.; Kim, H.C.; Shin, Y.K.; Min, H.; Cho, S.W.; Kim, Z.S.; Han, S.M.; Abd El-Aty, A.M.; Hacimuftuoglu, A.; Jeong, J.H. Humulus japonicus stimulates thermogenesis and ameliorates oxidative stress in mouse adipocytes. J. Mol. Endocrinol. 2019, 63, 1–9.
  27. Chou, Y.-C.; Ho, C.-T.; Pan, M.-H. Immature citrus reticulata extract promotes browning of beige adipocytes in high-fat diet-induced c57bl/6 mice. J. Agric. Food Chem. 2018, 66, 9697–9703.
  28. Nagata, N.; Xu, L.; Kohno, S.; Ushida, Y.; Aoki, Y.; Umeda, R.; Fuke, N.; Zhuge, F.; Ni, Y.; Nagashimada, M.; et al. Glucoraphanin ameliorates obesity and insulin resistance through adipose tissue browning and reduction of metabolic endotoxemia in mice. Diabetes 2017, 66, 1222–1236.
  29. Saba, E.; Jeon, B.R.; Jeong, D.H.; Lee, K.; Goo, Y.K.; Kim, S.H.; Sung, C.K.; Roh, S.S.; Kim, S.D.; Kim, H.K.; et al. Black ginseng extract ameliorates hypercholesterolemia in rats. J. Ginseng. Res. 2016, 40, 160–168.
  30. Sun, B.S.; Gu, L.J.; Fang, Z.M.; Wang, C.Y.; Wang, Z.; Lee, M.R.; Li, Z.; Li, J.J.; Sung, C.K. Simultaneous quantification of 19 ginsenosides in black ginseng developed from panax ginseng by hplc-elsd. J. Pharm. Biomed. Anal. 2009, 50, 15–22.
  31. Hu, J.N.; Liu, Z.; Wang, Z.; Li, X.D.; Zhang, L.X.; Li, W.; Wang, Y.P. Ameliorative effects and possible molecular mechanism of action of black ginseng (panax ginseng) on acetaminophen-mediated liver injury. Molecules 2017, 22, 664.
  32. Cho, E.-A.; Kim, S.-Y.; Na, I.-H.; Kim, D.-C.; In, M.-J.; Chae, H.-J. Antioxidant and anticoagulant activities of water and ethanol extracts of phyllostachys pubescence leaf produced in geoje. J. Appl. Biol. Chem. 2010, 53, 170–173.
  33. Yoon, S.B.; Lee, Y.J.; Park, S.K.; Kim, H.C.; Bae, H.; Kim, H.M.; Ko, S.G.; Choi, H.Y.; Oh, M.S.; Park, W. Anti-inflammatory effects of scutellaria baicalensis water extract on lps-activated raw 264.7 macrophages. J. Ethnopharmacol. 2009, 125, 286–290.
  34. Sung, Y.Y.; Son, E.; Im, G.; Kim, D.S. Herbal combination of phyllostachys pubescens and scutellaria baicalensis inhibits adipogenesis and promotes browning via ampk activation in 3t3-l1 adipocytes. Plants 2020, 9, 1422.
  35. Park, T.S.; Ryu, Y.K.; Park, H.Y.; Kim, J.Y.; Go, J.; Noh, J.R.; Kim, Y.H.; Hwang, J.H.; Choi, D.H.; Oh, W.K.; et al. Humulus japonicus inhibits the progression of alzheimer’s disease in a app/ps1 transgenic mouse model. Int. J. Mol. Med. 2017, 39, 21–30.
  36. Lee, Y.-R.; Kim, K.-Y.; Lee, S.-H.; Kim, M.-Y.; Park, H.-J.; Jeong, H.-S. Antioxidant and antitumor activities of methanolic extracts from humulus japonicus. Korean J. Food Nutr. 2012, 25, 357–361.
  37. Hong, M.-S.; Son, E.-S.; Lee, S.-J.; Lee, S.-K.; Lee, Y.-J.; Song, S.-D.; Cho, S.-N.; Barry, C.; Eum, S.-Y. Anti-mycobacterial effects of the extract of humulus japonicus. Korean J. Food Sci. Technol. 2014, 46, 94–99.
  38. Sung, B.; Chung, J.W.; Bae, H.R.; Choi, J.S.; Kim, C.M.; Kim, N.D. Humulus japonicus extract exhibits antioxidative and anti-aging effects via modulation of the ampk-sirt1 pathway. Exp. Ther. Med. 2015, 9, 1819–1826.
  39. Lim, H.; Noh, J.R.; Kim, Y.H.; Hwang, J.H.; Kim, K.S.; Choi, D.H.; Go, M.J.; Han, S.S.; Oh, W.K.; Lee, C.H. Anti-atherogenic effect of humulus japonicus in apolipoprotein e-deficient mice. Int. J. Mol. Med. 2016, 38, 1101–1110.
  40. Roberts, C.K.; Sindhu, K.K. Oxidative stress and metabolic syndrome. Life Sci. 2009, 84, 705–712.
  41. Dutt, M.; Vasconcellos, M.; Song, K.; Gmitter, F.; Grosser, J. In vitro production of autotetraploid ponkan mandarin (citrus reticulata blanco) using cell suspension cultures. Euphytica 2009, 173, 235–242.
  42. Sun, Y.; Qiao, L.; Shen, Y.; Jiang, P.; Chen, J.; Ye, X. Phytochemical profile and antioxidant activity of physiological drop of citrus fruits. J. Food Sci. 2013, 78, C37–C42.
  43. Lv, X.; Meng, G.; Li, W.; Fan, D.; Wang, X.; Espinoza-Pinochet, C.A.; Cespedes-Acuna, C.L. Sulforaphane and its antioxidative effects in broccoli seeds and sprouts of different cultivars. Food Chem. 2020, 316, 126216.
  44. Garcia-Saldana, J.S.; Campas-Baypoli, O.N.; Lopez-Cervantes, J.; Sanchez-Machado, D.I.; Cantu-Soto, E.U.; Rodriguez-Ramirez, R. Microencapsulation of sulforaphane from broccoli seed extracts by gelatin/gum arabic and gelatin/pectin complexes. Food Chem. 2016, 201, 94–100.
  45. Dinkova-Kostova, A.T.; Fahey, J.W.; Kostov, R.V.; Kensler, T.W. Keap1 and done? Targeting the nrf2 pathway with sulforaphane. Trends Food Sci. Technol. 2017, 69, 257–269.
  46. Gómez-Zorita, S.; Trepiana, J.; González-Arceo, M.; Aguirre, L.; Milton-Laskibar, I.; González, M.; Eseberri, I.; Fernández-Quintela, A.; Portillo, M.P. Anti-obesity effects of microalgae. Int. J. Mol. Sci. 2020, 21, 41.
  47. Kwon, M.; Lim, S.-J.; Joung, E.-J.; Lee, B.; Oh, C.-W.; Kim, H.-R. Meroterpenoid-rich fraction of an ethanolic extract from sargassum serratifolium alleviates obesity and non-alcoholic fatty liver disease in high fat-fed c57bl/6j mice. J. Funct. Foods 2018, 47, 288–298.
  48. Kwon, M.; Lee, B.; Lim, S.-J.; Choi, J.S.; Kim, H.-R. Sargahydroquinoic acid, a major compound in sargassum serratifolium (c. Agardh) c. Agardh, widely activates lipid catabolic pathways, contributing to the formation of beige-like adipocytes. J. Funct. Foods 2019, 58, 355–366.
  49. Kwon, M.; Lee, B.; Lim, S.; Kim, H.-R. Effects of sargaquinoic acid in sargassum serratifolium on inducing brown adipocyte-like phenotype in mouse adipocytes in vitro. Planta Med. 2020, 86, 45–54.
  50. Seo, Y.-J.; Kim, K.-J.; Choi, J.; Koh, E.-J.; Lee, B.-Y. Spirulina maxima extract reduces obesity through suppression of adipogenesis and activation of browning in 3t3-l1 cells and high-fat diet-induced obese mice. Nutrients 2018, 10, 712.
  51. Koo, S.Y.; Hwang, J.-H.; Yang, S.-H.; Um, J.-I.; Hong, K.W.; Kang, K.; Pan, C.-H.; Hwang, K.T.; Kim, S.M. Anti-obesity effect of standardized extract of microalga phaeodactylum tricornutum containing fucoxanthin. Mar. Drugs 2019, 17, 311.
  52. Guo, B.; Liu, B.; Wei, H.; Cheng, K.-W.; Chen, F. Extract of the microalga nitzschia laevis prevents high-fat-diet-induced obesity in mice by modulating the composition of gut microbiota. Mol. Nutr. Food Res. 2019, 63, 1800808.
  53. Maeda, H.; Hosokawa, M.; Sashima, T.; Funayama, K.; Miyashita, K. Fucoxanthin from edible seaweed, undaria pinnatifida, shows antiobesity effect through ucp1 expression in white adipose tissues. Biochem. Biophys. Res. Commun. 2005, 332, 392–397.
  54. Abd El-Baky, H.H.; El-Baroty, G.S. Characterization and bioactivity of phycocyanin isolated from spirulina maxima grown under salt stress. Food Funct. 2012, 3, 381–388.
  55. Choi, W.Y.; Lee, H.Y. Enhancement of chlorophyll a production from marine spirulina maxima by an optimized ultrasonic extraction process. Appl. Sci. 2018, 8, 26.
  56. Guo, B.; Liu, B.; Yang, B.; Sun, P.; Lu, X.; Liu, J.; Chen, F. Screening of diatom strains and characterization of cyclotella cryptica as a potential fucoxanthin producer. Mar. Drugs 2016, 14, 125.
  57. Wen, Z.-Y.; Chen, F. Production potential of eicosapentaenoic acid by the diatom nitzschia laevis. Biotechnol. Lett. 2000, 22, 727–733.
  58. Rebello, C.J.; Greenway, F.L.; Johnson, W.D.; Ribnicky, D.; Poulev, A.; Stadler, K.; Coulter, A.A. Fucoxanthin and its metabolite fucoxanthinol do not induce browning in human adipocytes. J. Agric. Food Chem. 2017, 65, 10915–10924.
  59. Maeda, H.; Hosokawa, M.; Sashima, T.; Takahashi, N.; Kawada, T.; Miyashita, K. Fucoxanthin and its metabolite, fucoxanthinol, suppress adipocyte differentiation in 3t3-l1 cells. Int. J. Mol. Med. 2006, 18, 147–152.
More
© Text is available under the terms and conditions of the Creative Commons Attribution (CC BY) license; additional terms may apply. By using this site, you agree to the Terms and Conditions and Privacy Policy.
Upload a video for this entry
Information
Subjects: Food Science & Technology
Contributor MDPI registered users' name will be linked to their SciProfiles pages. To register with us, please refer to https://encyclopedia.pub/register :
Choon Young Kim
View Times: 567
Revisions: 2 times (View History)
Update Date: 26 Apr 2021
Table of Contents
    1000/1000
    Hot Most Recent
    Feedback