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Bitter orange (Citrus aurantium), also known as sour orange and Seville orange, is a citrus fruit with a multitude of uses. It’s commonly used in complementary medicine, herbal weight loss supplements, and certain foods and toppings like marmalade (1, 2, 3).
Thought to have originated in Southeast Asia, it’s now found throughout Latin America and the Caribbean, the South Sea Islands, Europe, and Western and Southern Africa (2).
This article covers all you need to know about bitter orange, including its role in weight loss and skin health, as well as its overall safety as a supplement.
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Tim Platt/Getty ImagesThe bitter orange plant thrives in subtropical regions but can withstand adverse environmental conditions like frost for short periods (2).
Oval or oblong in shape, the fruit is red-orange when ripe and has a distinctively thick, dimpled skin. True to its name, it’s very bitter (2).
There are 23 cultivars of the fruit, the most prominent of which is Bergamot. You can expect some varieties to be more bitter than others.
Bitter orange contains several potent plant compounds that are sometimes extracted from the dried peel to make dietary supplements. The patented extract of bitter orange, p-synephrine, is sold in capsule form as the herbal weight loss supplements Advantra Z and Kinetiq (4).
Essential oils and powdered and liquid supplement forms are available as well.
SummaryBitter orange is a citrus fruit with dimpled skin and potent plant compounds that are extracted and used in a variety of supplements.
The plant compounds in bitter orange, which are called protoalkaloids, have been used for over 20 years in supplements for weight loss, athletic performance, skin care, appetite control, and brain health, as well as perfumery (1, 2, 3, 5, 6, 7, 8).
P-synephrine, the main extract from bitter orange, has a similar structure to ephedrine, the main component of the herbal weight loss supplement ephedra (8).
This supplement was banned by the U.S. Food and Drug Administration (FDA) because it raised blood pressure, increased heart rate, and caused heart attacks and stroke among some consumers (1, 3, 7).
In addition, p-synephrine is structurally similar to your flight-or-fight hormones, epinephrine and norepinephrine, which also increase your heart rate (1, 4).
As such, the safety of bitter orange extract has been called into question.
However, several studies have shown that bitter orange extracts and the plant’s natural uses neither harm your heart and nervous system nor excite nervous system activity, as some stimulants do (3, 4, 5, 6, 7, 9).
Furthermore, at least one study has claimed that p-synephrine shouldn’t be classified as a stimulant (4).
P-synephrine is also found in other citrus fruits and their juices, such as mandarins and clementines (4, 7).
Like other citrus fruits, bitter orange provides limonene — a compound shown to have anti-inflammatory and antiviral properties (10, 11, 12).
Population studies suggest that limonene may prevent certain cancers, namely colon cancer. However, more rigorous human research is needed (13).
An ongoing study is also exploring the use of limonene as a treatment for COVID-19. However, the results are not yet known. Bear in mind that limonene cannot prevent or cure COVID-19 (12).
Another protoalkaloid found in bitter orange is p-octopamine. However, little to no p-octopamine exists in bitter orange extracts. Moreover, it’s thought to be metabolized very rapidly in your liver when consumed from the whole fruit (3, 5).
Likewise, it doesn’t appear to exert any beneficial or adverse effects on your body.
The leaves of the bitter orange plant are rich in vitamin C, which acts as an antioxidant. What’s more, its peel has a high content of flavonoids, which are potent antioxidants with high medicinal value (2, 14).
Antioxidants are substances that may protect your body from disease by preventing cell damage. They work by deactivating free radicals, which are unstable compounds that damage your cells, increasing inflammation and your disease risk (15, 16).
SummaryProtoalkaloids are plant compounds found in bitter orange that have anti-inflammatory and antiviral properties. They have been shown to be safe for consumption.
Bitter orange and other citrus varieties show potential for weight loss, but there’s limited evidence on their effectiveness (1, 5, 6, 8, 17, 18).
Many weight loss supplements use bitter orange extracts in combination with other ingredients. However, scientific studies have not thoroughly examined the composition of these supplements to determine which ingredient, if any, supports weight loss.
Notably, p-synephrine has been shown to increase fat breakdown, raise energy expenditure, and mildly suppress appetite, all of which may contribute to reduced weight.
Yet, these effects occur at high doses that are discouraged due to the lack of safety information (4, 8, 18).
Thus, more studies on bitter orange’s weight loss properties are needed.
SummaryAlthough bitter orange extracts are often included in weight loss supplements, there’s limited evidence to support their effectiveness.
Bitter orange and its extracts are used in Traditional Chinese Medicine (TCM) to treat indigestion, diarrhea, dysentery, and constipation. In other regions, the fruit is used to treat anxiety and epilepsy (3).
Nonetheless, there’s limited evidence to support these uses.
There’s also insufficient evidence to support any uses for symptoms of premenstrual syndrome (PMS) (1).
Although a study in older rats suggested that flavanone compounds in citrus fruits and juices may improve thyroid function, it cannot be assumed that they’ll exert the same effects in humans (19).
All the same, given the high vitamin C content of bitter orange, it’s presumed that this fruit may improve skin health. Vitamin C’s role in wound healing and collagen formation is well established (16).
Another study noted that the bitter orange compound p-synephrine may improve athletic performance though by increasing total reps and volume load, or your ability to train harder (20).
SummaryThere’s insufficient evidence to support the effectiveness of bitter orange and its extracts for its numerous medicinal uses.
There’s conflicting information about whether synephrine, one of bitter orange’s natural compounds, should be considered a stimulant. A stimulant is a substance that increases your heart rate and blood pressure (1).
Several sports organizations, such as the National Collegiate Athletic Association (NCAA), list synephrine as a stimulant. Thus, it’s regarded as a banned substance in athletics (1, 21).
Furthermore, one study determined that bitter orange juice contains furanocoumarin, a compound that may cause the same medication interactions as grapefruit juice (22).
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Therefore, people taking decongestants or those who have high blood pressure, an irregular heartbeat, or glaucoma should avoid the juice and fruit of bitter oranges. It’s unclear whether bitter orange supplements pose this risk (5).
SummaryDespite numerous studies showing that bitter orange extracts are not stimulants, widespread controversy exists, and the NCAA has listed it as a banned substance. Bitter orange may also interact with certain medications.
Generally, bitter orange extracts in dietary supplements are safe to consume in doses of 50–98 mg per day (1, 23).
One study showed that 40 mg of synephrine combined with 320 mg of caffeine is a safe dose of these combined ingredients (3).
In another study, eating a whole bitter orange containing 30.6 mg of p-synephrine revealed no interactions with medications (24).
Still, people who are pregnant or breastfeeding should avoid bitter orange due to a lack of safety information (1).
summaryBitter orange is likely safe in doses ranging from 30.6 mg of synephrine in the fruit itself to 98 mg in dietary supplements, although additional research is required.
Bitter orange is quite tart and unlikely to be eaten raw.
Naturally high in pectin, a gelling agent, the fruit’s primary culinary application is for making marmalade (2, 25).
Bitter orange oil is also used as a flavoring or additive for the following:
The juice of the bitter orange can be used as a marinade to flavor fish and meat. In some regions, it’s used similarly to vinegar (2).
What’s more, the extracted oils give a distinctive flavor to liqueurs like Grand Marnier (2).
In China, bitter orange is used to make herbal teas and medicines.
Bitter orange has several other household uses outside of the kitchen. These include (2):
SummaryBitter orange is a citrus fruit with several household and industrial uses, ranging from food additives to perfumery. It’s primarily used to make marmalades and jellies due to its high pectin content.
Bitter orange is a citrus fruit that’s often processed into an extract. It has several culinary uses as well, though it’s rarely eaten whole.
Although bitter orange supplements are widely considered safe at common doses, there’s inconclusive evidence for their efficacy for weight loss, thyroid health, and skin care.
You may want to avoid this fruit and its extracts if you have high blood pressure, an irregular heartbeat, or glaucoma. Likewise, bitter orange supplements are banned for NCAA athletes.
Citrus aurantium L. (Rutaceae), commonly known as bitter orange, possesses multiple therapeutic potentials. These biological credentials include anticancer, antianxiety, antiobesity, antibacterial, antioxidant, pesticidal, and antidiabetic activities. The essential oil of C. aurantium was reported to display marked pharmacological effects and great variation in chemical composition depending on growing locations but mostly contained limonene, linalool, and β-myrcene. Phytochemically, C. aurantium is rich in p-synephrine, an alkaloid, and many health-giving secondary metabolites such as flavonoids. Animal studies have demonstrated a low affinity of p-synephrine for adrenergic receptors and an even lower affinity in human models. The present review focuses on the different biological activities of the C. aurantium in animal and human models in the form of extract and its pure secondary metabolites. Finally, it is concluded that both the extract and isolated compounds have no unwanted effects in human at therapeutic doses and, therefore, can confidently be used in various dietary formulations.
In the last years, phytopharmaceuticals have shown an outstanding role in new drug discovery [ 18 – 20 ]. Both in the crude form as well as pure chemical entities, a large population around the globe are getting therapeutic benefits from them [ 21 – 23 ]. In this review article, we have aimed to overview the bioactivity studies performed on C. aurantium revealing its therapeutic potential in the light of isolated molecules and/or essential oils.
Citrus aurantium L. (Rutaceae), commonly known as bitter orange, is usually utilized as a flavoring and acidifying agent for food [ 1 ]. Besides the essential oil and its components [ 2 , 3 ], the fruits of C. aurantium are sources of flavonoid-type compounds with diverse biological effects [ 4 – 6 ]. Additionally, it was reported that flavonoid glycosides were isolated from the plant [ 7 ] and the biogenic amine and flavanone contents have been determined [ 8 , 9 ]. Due to the abundance of health-giving secondary metabolites, C. aurantium is also used for the treatment of several ailments such as anxiety [ 10 ], lung and prostate cancers [ 11 ], and gastrointestinal disorders and obesity [ 2 , 12 ]. Due to the prohibition of Ephedra sinica Stapf. in Farw.-containing weight loss products in the market, C. aurantium has found an important place as a preferable agent to replace ephedra, as it contains p-synephrine, a phenylethanolamine type alkaloid, which is chemically similar to adrenergic agents, as appetite suppressants [ 12 – 14 ]. Recently, several scientific studies investigating the potential effects of various parts (including flowers, fruits, and essential oils) of C. aurantium have been conducted [ 15 – 17 ].
Zarrad and coworkers [ 32 ] explored the chemical composition of Tunisian C. aurantium fruits using gas chromatography (GC) and gas chromatography-mass spectroscopy (GC-MS). 25 compounds were identified in 97.696% exploration, but the most prominent one was limonene with 85.52%, followed by linalool and β-myrcene with 3.365% and 1.628%, respectively. The remaining compounds were in traces. Earlier, Villafane et al. [ 33 ] reported the presence of D-limonene and nootkatone in the essential oil of the plant. Similarly, Sanei-Dehkordi et al. [ 34 ] identified 21 compounds in peel essential oil of the plant. Of the total explored 98.62% composition, the quantity of limonene was 94.81% while the LC 50 was 31.20 ppm against Anopheles stephensi. However, the concentration of limonene was only 0.5–2.5% in C. aurantium from Algeria and linalool and α-terpineol were 18.6% and 15.1%, respectively [ 35 ]. Thus, overall considerable variation was observed in the concentration of these major components in C. aurantium grown in different parts of the world [ 36 – 41 ]. Carvalho-Freitas and Costa observed strong anxiolytic and sedative-like effects of the essential oil derived from C. aurantium [ 42 ].
Another class of compounds contained in C. aurantium are phenylethylamine alkaloids with p-synephrine being the most abundant. This compound has a hydroxyl group in the para position on the benzene ring and has some structural similarity to ephedrine. The peel of unripe fruits is the part of the plant which has the highest level of p-synephrine [ 31 ].
The second class of secondary metabolites found in C. aurantium are the limonoids ( ). The latter were considered as oxygenated triterpenoids as they contain relatively high numbers of oxygen atoms (7–11) in their structures. All components have a furan ring attached to the D-ring at C-17. Limonoids occur both in glucosidic and aglyconic form. Limonoid aglycones are water-insoluble and responsible for a bitter taste of the Citrus fruits, while limonoid glucosides are water-soluble and tasteless [ 28 ]. Among limonoids, the most important one is limonin, known as Citrus constituent since 1841. Limonoid glucosides are more abundant in juices and pulps, such as limonin glucoside, nomilin glucoside, obacunone glucoside, nomilinic acid glucoside, and deacetylnomilinic acid glucoside, because they are water-soluble, while limonoid aglycones such as limonin, nomilin, obacunone, ichangin, and deacetyl nomilin are water-insoluble and are present mainly in seeds and peels [ 29 , 30 ].
In C. aurantium, the flavones may be present also in the methoxylated form, in which all or almost all hydroxyls are capped by methylation, as nobiletin and tangeretin [ 27 ]. Furthermore, the C. aurantium may contain low amounts of flavonols, as kaempferol and quercetin, mainly in glycosidic form.
The flavones in aglycon or/and glycosidic form are the second major group of flavonoids in C. aurantium. The most commonly detected free flavones are apigenin, luteolin, and diosmetin. O-Glycosides and C-glycosides are the two main forms of flavone glycosides, and the most common linked sugar moieties include glucose, rutinose, and neohesperidose [ 26 ].
Flavanones are the main flavonoids contained in C. aurantium [ 25 ]. The most abundant detected free flavanones are hesperetin (4′-methoxy-3′,5,7-trihydroxyflavanone) and naringenin (4′,5,7-trihydroxyflavanone) [ 26 ]. Hesperetin and naringenin present a common skeleton: two hydroxyl group in positions C-5 and C-7, respectively, and they can be found as aglycone and/or as glycosides [ 25 ]. The most widely distributed glycosides of hesperetin are hesperidin and neohesperidin, which are conjugates with rutinose and neohesperidose, respectively, while, for naringenin, the most abundant glycosyl derivatives are naringin (naringenin-7-neohesperidoside) and narirutin (naringenin-7-rutinoside) [ 25 ].
Flavonoids are mainly present in Citrus fruits as glycosyl derivatives. Aglycones are mainly present in specific parts of the fruit as peel and seeds, owing to their lipophilic nature and consequently their low solubility in water [ 21 – 23 ]. For glycoside forms, O-glycosides, C-glycosides, rutinosides, glucosides, and neohesperidosides are common [ 21 – 23 ]. The presence of a relatively large number of glycosylated flavonoids in Citrus is a result of many different combinations possible between polyhydroxylated aglycones and a limited number of mono- and disaccharides [ 24 ].
The chemical composition of C. aurantium is responsible for health-promoting effects. The chemical composition includes vitamins, minerals, phenolic compounds, and terpenoids [ 21 – 23 ]. Among the diverse chemical components in C. aurantium, flavonoids belonging to phenolics have been recognized as important due to their physiological and pharmacological role and their health benefits [ 21 – 23 ].
The anticancer activity of the plant has been reported in literature [26, 43]. Cytotoxic properties of the polysaccharides obtained from C. aurantium were examined. Cytotoxic activity on human breast cancer cells (MCF-7) and lung cancer cells (HCC827) and immune-enhancement effect were examined. The results indicated that C. aurantium var. amara polysaccharides displayed good immune-enhancement activity by stimulating the production of tumor necrosis factor-α (TNF-α) and interleukin-6 (IL-6) in RAW264.7 cells and by promoting the mRNA expression levels of inducible nitric oxide synthase (iNOS), TNF-α, interleukin-1β (IL-1β), and IL-6. Moreover, phosphorylated extracellular signal-regulated kinase (ERK), phosphorylated c-Jun N-terminal kinase (JNK), phosphorylated p38, and phosphorylated p65 were significantly enhanced in C. aurantium var amara polysaccharides-treated RAW264.7 cells [24, 44]. Isolimonic acid and ichanexic acid from ethyl acetate extract of C. aurantium were isolated by using chromatographic methods. The compounds for their inhibitory action on human colon cancer cells (HT-29) proliferation, apoptosis, and on noncancerous (COS-1 fibroblast) cells were investigated. The compounds displayed an increment in the cell counts in G2/M stage, demonstrating a potential effect in the cell-cycle arrest [25].
Protective activity of the extract obtained from the peels of C. aurantium against apoptosis in cholestatic liver fibrosis-induced mice was investigated. As part of the experiment, cholestatic liver injury was induced by bile duct ligation and the mice were treated with C. aurantium peel extract. According to the histopathological analysis, the administration of C. aurantium peel extract significantly decreased liver fibrosis. Biochemical analysis revealed that the extract reduced the concentrations of alanine transaminase (ALT), aspartate transaminase (AST), gamma-glutamyl transferase, total bilirubin, nitric oxide, and thiobarbituric acid reactive substances (TBARS), suggesting C. aurantium can efficiently regulate bile duct ligation-induced liver injury by displaying antioxidant, anti-inflammatory, and antiapoptotic effects [27].
C. aurantium was shown to possess antimetastasis activities in in vitro assays. A study by Park et al. evaluated the antimetastatic effect of flavonoids, isolated from Korean C. aurantium in mice models. Flavonoids were shown to prevent cancer cell infiltration and localization to the lungs. Moreover, through the regulation of caspase-3 and phospho-p53, the flavonoids induced cancer cell apoptosis. In vitro tests demonstrated that flavonoids inhibited A549 cells metastasis and induced apoptosis and downregulation of the Ddx3x and ANP43B proteins, supporting the use of C. aurantium flavonoids in human lung cancer treatment. According to the bioactivity assays conducted on the major compounds of C. aurantium var. amara, namely, 5-hydroxy-6,7,30,40-tetramethoxyflavone (HTF) and limonexic acid (LA), both compounds showed remarkable antioxidant effects and notable inhibitory action on the B16 and SMCC-7721 cell lines, at a concentration between 6.25 and 50 μg/mL and between 12.5 and 200 μg/mL, respectively [28]. illustrates the cytotoxic effects and mechanisms of C. aurantium extracts.
Open in a separate windowMiyazawa et al. [45] isolated three polymethoxy flavonoid-type compounds, namely, tetra-O-methylscutellarein, sinensetin, and nobiletin from C. aurantium. These compounds caused marked downstream regulation of a variety of gene expressions and thus showed strong antimutagenic activity. Wang and coworkers [46] summarized the anticancer effects of polymethoxyflavones with detailed molecular mechanisms. The various amines and flavonoids have been quantitatively analyzed in C. aurantium using liquid chromatography [47, 48]. Hesperidin has been isolated from C. aurantium [49]. It displayed a significant apoptotic effect against liver cell lines, HepG2 cells, by mediating through the upstream regulation of mitogen-activated protein kinase ERK1/2 [50].
The anxiolytic and sedative effects of C. aurantium by in vivo light-dark box and the marble-burying assays were evaluated. C. aurantium essential oil enhanced the period the mice spent in the light chamber, as well as the number of transitions between the two compartments in the light-dark box test [29]. Moreover, single and repeated treatments with the essential oil were reported to suppress marble-burying behavior [10]. The anxiolytic activity of the blossom of C. aurantium was also evaluated clinically on 60 patients undergoing minor surgical operation with no organic pathology. Two hours before the anesthesia induction, two groups consisting of 30 patients were administered at 1 mL/kg of either C. aurantium distillate or saline solution. Anxiety was assessed by using the Spielberger state-trait anxiety inventory, the Amsterdamd preoperative anxiety, and information scale. The outcome of this study revealed that C. aurantium could be active by reducing preoperative anxiety before minor operation [30].
In traditional Chinese medicine (TCM), the combination of the aqueous extracts of the fruits of Gardenia jasminoides Ellis, C. aurantium, and the bark of Magnolia officinalis Rehd. et Wils. is called Zhi-Zi-Hou-Po (ZZHPD) and has been used to treat depression-like symptoms. Xing et al. [51] explored in vivo antidepressant activity of ZZHPD in rats, by using coat state test, sucrose preference test, forced swimming test, and open-field test. The effects of ZZHPD on hypothalamic-pituitary-adrenal (HPA) axis were determined by measuring the hormone levels. The results showed that ZZHPD improved depressive behaviors and normalized the adrenocorticotropic hormone (ACTH) and corticosterone levels, by restoring the function of HPA axis, and increasing brain-derived neurotrophic factor expression in hippocampus and promoting hippocampal neurogenesis [51]. ACTH/corticotropinis a peptidic hormone secreted from the anterior pituitary, which regulates glucocorticoid cortisol production from the adrenals [52]. Stress increases ACTH release, which induces the stress hormone cortisol, together they cause numerous diseases [53].
Letie et al. [54] conducted another study in vivo, where rat models were exposed to the essential oil of C. aurantium at 1.0%, 2.5%, and 5.0% concentrations by inhalation, in acrylic boxes before employing elevated plus maze and open-field assays. C. aurantium essential oil increased the time of the animals in the open arms of the elevated plus maze test and the time of active social interaction in the open field [54].
Wolfenbuttel et al. [55] investigated the influence of C. aurantium essential oil on melatonin and corticosterone in mice after inhalation for 30 min. Melatonin provides protective effects on neuronal cells and acts as an antidepressant by restoration of corticosterone levels. After treatment, the hormone levels did not present variation, whereas behavioral tests showed that the inhalation of 10% essential oil causes an anxiolytic-like and sedative effect. From these data, Citrus essential oil represents a valuable tool for the treatment of the anxiety disturbs, apparently without interference with melatonin and corticosterone physiological levels [55].
Several reports have been cited in literature regarding the antidiabetic effects of C. aurantium [56–58]. An in vivo study was performed to evaluate the antidiabetic effect and to reveal the toxicity profile of the aqueous extract of the fruits of C. aurantium and the leaves of Rauwolfia vomitoria. In this study, NMRI lean mice (6-week-old) and C57BL/6J lean mice (6- or 11-week-old) were used. A single dose, which corresponds to seventy-fold of a human daily dose, was detected to be nontoxic to the animals. A significant weight loss was determined when the dosage, which corresponds to tenfold of a human daily dose, was administered to C57BL/KsBom-db (db/db) genetic diabetic mice for 6 weeks. These mice were maintained on the carbohydrate-deficient diet during the treatment period. The food intake was not significantly different from the control group animals; however, the serum triglyceride levels of the treated animals were significantly higher suggesting the lipid mobilization from internal stores. The fatty acid levels of the eyes of the treated mice remarkably reduced along with stearoyl-CoA desaturase activity [59]. A possible effect of the extract obtained from C. aurantium and p-synephrine on liver metabolism was evaluated. In order to measure catabolic and anabolic pathways, an isolated perfused rat liver was used. Both the extract and the compound were found to enhance glycolysis, glycogenolysis, oxygen uptake, and perfusion pressure. p-Synephrine increased the glucose output at 200 μM concentration. C. aurantium extract enhanced gluconeogenesis at low concentrations, however, inhibited at high concentrations. The effects of C. aurantium extract on liver metabolism was found to be similar to those of adrenergic agents, and p-synephrine could be responsible from the activity [14].
Besides its scientifically proven antimicrobial, antioxidant, cytotoxic, anxiolytic, and antidiabetic effects, C. aurantium extract has been commonly utilized for the weight loss and as sports performance enhancer, in dietary supplements [60–62]. Therefore, the use of C. aurantium extract and its constituent p-synephrine (C9H13NO2), for the treatment of obesity in 360 subjects, was reviewed. More than 50% of the subjects involved in these clinical studies were overweight, and approximately two-thirds of them consumed caffeine (132–528 mg/day) and p-synephrine (10–53 mg/day). Approximately 44% of the subjects used a C. aurantium/p-synephrine product, while the remaining consumed a combination product containing multiple ingredients with p-synephrine. The results showed that C. aurantium extract alone or in combination with other ingredients did not cause significant adverse effects including an increase in heart rate or blood pressure or change in electrocardiographic data, serum chemistry, blood cell counts, or urinalysis. p-Synephrine, alone or in combination products, was demonstrated to enhance metabolic rate and energy expenditure and to promote weight loss when given for six to 12 weeks [63].
The study by Verpeut et al. [64] investigated the effect of the combination of C. aurantium (standardized to 6% p-synephrine) and Rhodiola rosea L. (golden root) (standardized to 3% rosavins and 1% salidroside) on diet-induced obesity in Sprague-Dawley rats. Acute administration of C. aurantium (1–10 mg/kg) or R. rosea (2–20 mg/kg) alone did not decrease food intake in normal weight animals; however, the combination of C. aurantium (5.6 mg/kg) and R. rosea (20 mg/kg) provided a 10.5% feeding suppression. On the other hand, 10 days of treatment with C. aurantium (5.6 mg/kg) or R. rosea (20 mg/kg) alone, or in combination, to the animals fed on a high-fat diet (60% fat) during the 13-week period led to a 30% decline in visceral fat weight, compared with other treatments. Coadministration of C. aurantium and R. rosea also resulted in an elevation in hypothalamic norepinephrine and frontal cortex dopamine, indicating the beneficial role of C. aurantium and R. rosea in the treatment of obesity [64]. illustrates the various pharmacological effects of C. aurantium extracts.
Open in a separate windowThe cardiovascular toxicity of C. aurantium extracts with different concentrations of protoalkaloid p-synephrine (4 and 6%) was reported by Calapai et al. in 1999 in rats. Authors showed an antiobesity effect by the administration of C. aurantium but also possible cardiovascular toxicity. The cardiovascular effects have not been confirmed by studies using much higher doses of p-synephrine [65].
Another study was carried out to evaluate the cardiovascular effects of different doses of C. aurantium and pure p-synephrine in rats. C. aurantium extract and pure p-synephrine enhanced the heart rate and blood pressure. Higher activities were obtained with C. aurantium extract than p-synephrine, suggesting that other compounds in the extract can alter physiological parameters [13]. The effect of p-synephrine on heart rate and blood pressure in female Sprague-Dawley rats was assessed. During 28 days, two types of extracts, one of which contained 6% and other 95% p-synephrine, were administered daily by gavage at 10 or 50 mg/kg, doses for a 60 kg human equal to 600 and 3000 mg/kg. The outcome of the study showed that both p-synephrine and C. aurantium extract resulted in clinically insignificant increases in heart rate and blood pressure at doses many times greater than used in humans. p-Synephrine and bitter orange extract exhibited little or no effect on the cardiovascular effects of caffeine [13].
Safety of p-synephrine was investigated by Ratamess et al. [66] on humans, animals, and in vitro. Authors reported over 30 human studies indicating that the cardiovascular effects of p-synephrine and bitter orange extracts are clinically insignificant. p-Synephrine showed a greater ability to bind adrenergic receptors in rodents than in humans, and the data in literature on its effects on animals cannot be indicative for men at commonly used doses.
This review concluded that C. aurantium extract and p-synephrine are safe for use in dietary supplements and foods at commonly used doses. Also, other authors reported similar conclusions [67, 68]. While p-synephrine alone seems to have low toxicity, when it is formulated in combination with other ingredients such as caffeine (Paullinia cupana, Cola nitida, Cola acuminata, and Camellia sinensis), salicin (Salix sp.), and ephedrine (ma huang, Ephedra sinica, and Ephedra sp.) in weight loss products, the mixture could induce some cardiovascular effects. However, the study did not demonstrate that p-synephrine contributed to cardiovascular effects.
Schmitt et al. [69] reported clear signs of toxicity of this mixture in mice of both sexes as reduction in locomotor activity, ptosis, seizures, salivation, agitation, piloerection, and deaths after acute oral administration of 300, 350, and 400 mg/kg total of p-synephrine, ephedrine, salicin, plus caffeine in a 10 : 4 : 6 : 80 w/w ratio.
The volatile oil obtained from the flowers of C. aurantium var. amara, namely, neroli oil, is used to reduce heart rate and palpitations, to encourage sleep, and to soothe the digestive tract. Kang et al. [15] investigated the activity mechanism of neroli in mouse aorta. Neroli was found to exert vasodilator activity in mice precontracted with prostaglandin (PG)-F2α. Nevertheless, the relaxation was reduced in the endothelium-denuded ring or preincubation with the nitric oxide synthase inhibitor by neroli treatment. Moreover, the relaxation induced by neroli was partially reversed by soluble guanylyl cyclase inhibitor. Neroli also inhibited extracellular Ca2+-dependent and depolarization-induced contraction in a dose-dependent manner. Nonselective cation channel blocker, Ni2+, decreased neroli-induced relaxation. On the other hand, a K+ channel blocker, tetraethylammonium chloride, did not alter the relaxation. In order to prevent Ca2+ influx through the smooth muscle voltage-gated Ca2+ channels, verapamil was added. In this case, the ryanodine (a class of intracellular calcium channels) receptor inhibitor reduced neroli-induced relaxation. All these data indicated that neroli-induced relaxation might be partly mediated by the nitric oxide-soluble guanylyl cyclase, and ryanodine receptor signaling pathway [15].
Antimicrobial activity of C. aurantium was investigated by using several in vitro assays [70–72]. For instance, Karabıyıklı et al. [1] explored the antimicrobial action of C. aurantium juice against Salmonella enterica Typhimurium and Listeria monocytogenes. For this purpose, both neutralized and unneutralized juice samples with various concentrations were tested for the inoculation of the microorganisms at 4°C and 37°C temperatures, during a period of seven days. The results showed that Salmonella enterica Typhimurium and Listeria monocytogenes not only survived but also grown for two days in neutralized juice at 37°C. On the other hand, on day 7, none of them survived. The results also revealed that L. monocytogenes was less resistant than S. enterica Typhimurium. The low pH of C. aurantium juice was suggested to be responsible for its antimicrobial potential along with the duration of the incubation period as well as the temperature [1]. In another research, the antimicrobial potential of C. aurantium was investigated, and high antimicrobial activity was recorded against Bacillus subtilis and Staphylococcus aureus (among 12 microorganisms tested), with the minimum inhibition concentration (MIC) values of 2.7 mg/mL and 4.8 mg/mL. Moderate effects were detected against Saccharomyces cerevisiae and Mucor ramannianus with the values of 9.2 mg/mL and 5 mg/mL, respectively. In the same study, radical scavenging and antibacterial effects of the essential oil obtained from the leaves of C. aurantium were evaluated. Weak antioxidant effect was detected against 1,1-diphenyl-2-picrylhydrazyl (DPPH) and 2,2′-azinobis-3-ethylbenzothiazoline-6-sulphonate (ABTS) radicals [73].
Previous in vitro investigations on the essential oil of C. aurantium peels and its isolated component limonene have demonstrated their pest fumigant activity against Bemisia tabaci (silverleaf whitefly). In 24 h exposure, insect mortality between 41.00 and 47.67% was determined at 2.5 and 20.0 μL/L air concentrations. In the same study, the authors conducted another assay, investigating the anticholinesterase effect of the oil itself, as well as that of the pure compound. Both exerted anticholinesterase effect with the IC50 values of 2.94 mM and 3.54 mM, respectively [74–76]. Other studies investigated the larvicidal effect of the essential oils of C. aurantium against Anopheles labranchiae. After 24 h, the mortality counts were carried out, and LC50 and LC90 values were determined. The outcome of this study demonstrated that the essential oils exerted significant larvicidal potential. C. aurantium essential oil was found to be the most active by the LC50 and LC90 values of 22.64 mg/L and 83.77 mg/L, respectively [13, 77]. The essential oil extract from the fresh peeled ripe fruit of Citrus aurantium showed also good larvicidal effect against mosquito vector Anopheles stephensi (LC50 values, 31.20 ppm) The main constituent of the leaf oil was limonene (94.81).
DPPH, ABTS, and ferric-reducing antioxidant power assays were used for the determination of the antioxidant potential of the macerate of the albedo layers of C. aurantium fruits obtained by protopectinase-SE (produced by Geotrichum klebahnii and hydrolyzed selectively the intercellular protopectin of plant tissues). Moreover, the levels of total phenols, reducing sugars, vitamin C, total flavonones, naringin, and galacturonic acid and total acidity were detected. Antioxidant activity, vitamin C, and total flavonone levels were found to be the highest with the greatest degree of tissue maceration [78–81]. In vivo and in vitro antioxidant activities of polysaccharide fractions from C. aurantium were evaluated. The most active fraction was subjected to ion exchange and gel-filtration chromatography to obtain four purified polysaccharides. Upon the evaluation of their antioxidant effect, it was found that C. aurantium can be utilized as an antioxidant in the food and medical industries [82, 83].
In a study by Lagha-Benamrouche et al. [84], the antioxidant potentials of the peels and leaves of seven orange varieties obtained from Algeria were investigated by linoleic acid and β-carotene oxidation assays. The presence of phenolic compounds was also investigated. C. aurantium cv. Bigarade was found to have the highest phenol level. The antioxidant activity assay was in accordance with the phytochemical findings. C. aurantium displayed the highest action on slowing down the rate of linoleic acid and β-carotene oxidation [84, 85]. An antioxidant study was performed on the C. aurantium fruits on different ripening stages. According to the outcome obtained from DPPH free radical-scavenging and β-carotene/linoleic acid systems, the antioxidant activity was found to be varied related to the amount of the phenolic components [86]. Another antioxidant activity study revealed that during dehydration, different air-drying temperature affected the antioxidant effect of the C. aurantium by-products, including peel and pulp remaining after juice extraction [79]. C. aurantium peel and juice were suggested as a new potential source of natural antioxidants; although, they were found to be less effective than butylated hydroxytoluene (BHT), butylated hydroxyanisole (BHA), and ascorbic acid, used as antioxidant standards [87, 88]. Anti-inflammatory activity of the flavonoid-type compounds of Korean C. aurantium, namely, nobiletin, naringin, and hesperidin was investigated. Inhibition of proinflammatory mediators by blocking nuclear factor-kappa B (NF-ƘB) and mitogen-activated protein kinase (MAPK) signaling in lipopolysaccharide- (LPS-) stimulated RAW 264.7 macrophages was assessed [89]. The flavonoids were found to have the capacity to suppress the mRNA and protein expression of COX-2 and iNOS, by clarifying their anti-inflammatory action [4]. A polymethoxy flavonoid-rich C. aurantium extract was shown to have a protective effect on alcohol-induced liver injury in an animal study via AMPK and Nrf2-related signal regulation [90].
In order to assess the effect of C. aurantium essential oil and its main compound limonene on gastric mucosa, Moraes et al. [2] conducted a study in vivo. The essential oil and its compound limonene were found to possess protective activity in the gastrointestinal system against lesions, which were induced by ethanol and nonsteroidal anti-inflammatory drugs in rats, at doses of 250 mg/kg and 245 mg/kg, respectively. The essential oil and limonene increased the production of gastric mucus. The findings revealed that C. aurantium essential oil and its main compound limonene can be used as a promising target for the development of a novel gastroprotective drug [2]. In another study, the gastroprotective effect of β-myrcene, a monoterpene-type compound of C. aurantium, was evaluated. Experimental models of ulcer, induced by ethanol, NSAID stress, Helicobacter pylori, ischemia-reperfusion injury (I/R), and cysteamine (a drug used to treat cystinosis) was used to assess the ameliorative activity. β-Myrcene was administered at dose of 7.5 mg/kg. The results showed a potential role for β-myrcene against peptic ulcer disease. β-Myrcene contributed to the maintenance of integrity of the gastric mucosa with a significant decrease of ulcerative lesions, attenuating lipid peroxidative damage and preventing depletion of GSH, GR, and GPx [91].
Polo et al. confirmed the healing properties of C. aurantium essential oil on gastric ulcers after treatment in middle-aged Wistar rats. They showed a significant reduction of the lesion area (76%) within the gastric mucosa that appears regenerated (59%) when compared to the negative control group [92].
On the other hand, Hamdan et al. assessed the effects of hesperidin and neohesperidin, important flavonoid-type components of C. aurantium. For this purpose, indomethacin-induced ulcer models of rats were used. Omeprazole was administered as a reference standard for the comparison. The parameters analyzed in the present study were ulcer index, gastric cyclooxygenase-2 (COX-2) gene expression, TNF-α, MDA, and GSH levels. Histopathalogical analysis was also performed. The findings of the study revealed that hesperidin and neohesperidin notably aggravated indomethacin-induced gastric damage as evidenced by increased ulcer index and histopathological alteration [93]. Recently, hesperidin showed strong inhibition against ovarian cancer cell viability and caused apoptosis mediated through endoplasmic reticulum stress signaling pathways [94]. Hafidh et al. [95] observed the potent anticancer effects of limonene in hepatocellular carcinoma and HepG2, and the cell line caused the modulation of cancer-inducing genes. These data confirmed the antioxidant and prooxidant behavior of flavonoids showing the potential benefits and adverse effects of these opposing events.
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