27 March 2012

EMA/HMPC/232100/2011

Committee on Herbal Medicinal Products (HMPC)

Assessment report on Rhodiola rosea L., rhizoma et radix

Based on Article 16d(1), Article 16f and Article 16h of Directive 2001/83/EC as amended (traditional
use)
Final
Herbal substance(s) (binomial scientific name of

Rhodiola rosea L., rhizoma et radix

the plant, including plant part)

Herbal preparation(s)

Dry extract (DER 1.5-5:1), extraction solvent

ethanol 67-70% v/v

Pharmaceutical forms

Herbal preparations in solid dosage forms for oral

use.

Rapporteur

R. Lnger

7 Westferry Circus Canary Wharf London E14 4HB United Kingdom

Telephone +44 (0)20 7418 8400 Facsimile +44 (0)20 7523 7051
E-mail [email protected] Website www.ema.europa.eu

An agency of the European Union

European Medicines Agency, 2012. Reproduction is authorised provided the source is acknowledged.

Table of contents
Table of contents ................................................................................................................... 2
1. Introduction ....................................................................................................................... 3

1.1. Description of the herbal substance(s), herbal preparation(s) or combinations thereof .. 3

1.2. Information about products on the market in the Member States ............................... 5
Regulatory status overview .......................................................................................... 5
1.3. Search and assessment methodology ..................................................................... 6
2. Historical data on medicinal use ........................................................................................ 6

2.1. Information on period of medicinal use in the Community ......................................... 6

2.2. Information on traditional/current indications and specified substances/preparations .... 6
2.3. Specified strength/posology/route of administration/duration of use for relevant
preparations and indications ......................................................................................... 7
3. Non-Clinical Data ............................................................................................................... 7

3.1. Overview of available pharmacological data regarding the herbal substance(s), herbal
preparation(s) and relevant constituents thereof ............................................................. 7
Pharmacological data regarding the herbal preparation: .................................................. 7
Pharmacological data regarding isolated constituents: ................................................... 15
3.2. Overview of available pharmacokinetic data regarding the herbal substance(s), herbal
preparation(s) and relevant constituents thereof ........................................................... 22
3.3. Overview of available toxicological data regarding the herbal substance(s)/herbal
preparation(s) and constituents thereof ....................................................................... 23
3.4. Overall conclusions on non-clinical data ................................................................ 24
4. Clinical Data ..................................................................................................................... 24

4.1. Clinical Pharmacology ......................................................................................... 24

4.1.1. Overview of pharmacodynamic data regarding the herbal substance(s)/preparation(s)
including data on relevant constituents ........................................................................ 24
4.1.2. Overview of pharmacokinetic data regarding the herbal substance(s)/preparation(s)
including data on relevant constituents ........................................................................ 26
4.2. Clinical Efficacy .................................................................................................. 26
4.2.1. Dose response studies...................................................................................... 26
4.2.2. Clinical studies (case studies and clinical trials) ................................................... 26
4.2.3. Clinical studies in special populations (e.g. elderly and children) ............................ 31
4.3. Overall conclusions on clinical pharmacology and efficacy ........................................ 31
5. Clinical Safety/Pharmacovigilance ................................................................................... 31

5.1. Overview of toxicological/safety data from clinical trials in humans ........................... 31

5.2. Patient exposure ................................................................................................ 31
5.3. Adverse events and serious adverse events and deaths .......................................... 32
5.4. Laboratory findings ............................................................................................. 32
5.5. Safety in special populations and situations ........................................................... 32
5.6. Overall conclusions on clinical safety ..................................................................... 32
6. Overall conclusions .......................................................................................................... 32
Annex .................................................................................................................................. 33

List of references ...................................................................................................... 33

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1. Introduction
1.1. Description of the herbal substance(s), herbal preparation(s) or
combinations thereof

Herbal substance(s)

The herbal substance consists of the dried roots and rhizomes of Rhodiola rosea L. (Crassulaceae).
Although the plant part in use is commonly referred to as the root, the anatomy of these parts reveals
that these parts are underground stems (rhizomes) with irregular secondary thickening. The plant is
native throughout the mountains in the Northern Hemisphere. A main source of commercially available
rhizomes is the Altai region in Asia (Panossian et al. 2010).
Common names are: Roseroot, Rosenroot, Golden Root, Arctic Root, Rosenwurz. The name refers to
the rose-like fragrance of the fresh cut underground organs.
Constituents (according to Panossian et al. 2010, Ali et al. 2008, Tolonen et al. 2003):
Phenylalkanoids: Phenylethanoids (e.g salidroside [syn. rhodioloside]: p-hydroxyphenylethyl-O-D-glucopyranoside), phenylpropenoids (e.g. rosin: cinnamyl-O--D- glucopyranoside; rosarin:
(cinnamyl-(6-O--L-arabinofuranosyl)- O--D- glucopyranoside; rosavin: (cinnamyl-(6-O- -Larabinopyranosyl)- O--D- glucopyranoside), phenylpropanes (e.g. tyrosol). Only limited data are
available regarding the quantitative composition. Hellum et al. 2010 report a considerable
variability between clones of Rhodiola rosea in Norway based on data obtained from ethanolic
extracts (primary extraction solvent ethanol 96%). Irrespective of the plant origin (cultivated in
Lithuania or naturally occurring in Altai mountains). Kucinskaite et al. (2007) found in aqueousethanolic extracts 1.35-1.62 mg/ml of salidroside, while the profile of rosavins differed
considerably. Ethanol 70% v/v yields extracts with a low content of salidroside compared to
ethanol 40% v/v; in contrast rosavins are more efficiently extracted by ethanol 70% (Kucinskaite
et al. 2007).
Essential oil: The dried rhizome contains approximately 0.05% of essential oil. Main components
are -pinene, geraniol, limonene, -phellandrene, linalool, n-octanol, n-decanol, dodecanol, 1,4-pmenthadien-7-ol and cumin alcohol (Rohloff 2002). Evstatieva et al. (2010) found considerable
differences in the composition of the essential oil of different origin. In a sample from Bulgaria,
myrtenol and meraniol counted for more than 75%; in an Indian sample, phenethylalcohol was the
main component (56%); in a sample from China, geraniol (57%) and n-octanol were the
dominating components.
Monoterpene derivatives: rosiridol, rosiridin, rhodiolosides A-E.
Cyanogenic glycosides: rhodiocyanoside A, lotaustralin
Proanthocyanidines: prodelphinidine-gallate esters
Flavonolignans: rhodiolin
Flavonoids: Rhodiola-specific flavonoids like rhodionidin, rhodiolgin, rhodalidin, rhodionin,
rhodiolgidin, rhodalin, rhodiosin; tricin and kaempferol derivatives.
Phenolic acids: chlorogenic acid, hydroxycinnamic acid

Herbal preparation(s)

Dry extract (DER 1.5-5:1), extraction solvent ethanol 67-70% v/v

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Combinations of herbal substance(s) and/or herbal preparation(s) including a description of

vitamin(s) and/or mineral(s) as ingredients of traditional combination herbal medicinal products
assessed, where applicable.

Not applicable.

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1.2. Information about products on the market in the Member States

Regulatory status overview
Member State

Regulatory Status

Comments

Austria

MA

TRAD

Other TRAD

Other Specify:

Belgium

MA

TRAD

Other TRAD

Other Specify:

Bulgaria

MA

TRAD

Other TRAD

Other Specify:

Cyprus

MA

TRAD

Other TRAD

Other Specify:

Czech Republic

MA

TRAD

Other TRAD

Other Specify:

Denmark

MA

TRAD

Other TRAD

Other Specify:

Estonia

MA

TRAD

Other TRAD

Other Specify:

Finland

MA

TRAD

Other TRAD

Other Specify:

France

MA

TRAD

Other TRAD

Other Specify:

No product

Germany

MA

TRAD

Other TRAD

Other Specify:

No product

Greece

MA

TRAD

Other TRAD

Other Specify:

No product

Hungary

MA

TRAD

Other TRAD

Other Specify:

No product

Iceland

MA

TRAD

Other TRAD

Other Specify:

Ireland

MA

TRAD

Other TRAD

Other Specify:

Italy

MA

TRAD

Other TRAD

Other Specify:

Latvia

MA

TRAD

Other TRAD

Other Specify:

Liechtenstein

MA

TRAD

Other TRAD

Other Specify:

Lithuania

MA

TRAD

Other TRAD

Other Specify:

Luxemburg

MA

TRAD

Other TRAD

Other Specify:

Malta

MA

TRAD

Other TRAD

Other Specify:

The Netherlands

MA

TRAD

Other TRAD

Other Specify:

Norway

MA

TRAD

Other TRAD

Other Specify:

Poland

MA

TRAD

Other TRAD

Other Specify:

Portugal

MA

TRAD

Other TRAD

Other Specify:

Romania

MA

TRAD

Other TRAD

Other Specify:

Slovak Republic

MA

TRAD

Other TRAD

Other Specify:

Slovenia

MA

TRAD

Other TRAD

Other Specify:

Spain

MA

TRAD

Other TRAD

Other Specify:

Sweden

MA

TRAD

Other TRAD

Other Specify:

United Kingdom

MA

TRAD

Other TRAD

Other Specify:

Food supplements

No product

No product

No product

MA: Marketing Authorisation

TRAD: Traditional Use Registration
Other TRAD: Other national Traditional systems of registration
Other: If known, it should be specified or otherwise add Not Known
This regulatory overview is not legally binding and does not necessarily reflect the legal status of the
products in the MSs concerned.

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1.3. Search and assessment methodology

Search term: Rhodiola rosea
Databases: Pubmed, Medline and Toxnet.
Libraries: University Vienna, centre of pharmacy; Medical University Vienna, central library.

2. Historical data on medicinal use

2.1. Information on period of medicinal use in the Community
Herbal preparations in medicinal use reported from the Member States:
A. Liquid extract of root and rhizome, DER 1:1, extraction solvent ethanol 40%
Saratikov (1974) reports that in 1969, the Ministry of Health of the former USSR recommended to
allow the medical utilisation and industrial production of the liquid extract of the Rhodiola. In this
paper, a herbal tea and a tincture prepared with ethanol 40% (or vodka) are mentioned as
traditional herbal preparations. In 1975, Rhodiola fluid extract was accepted in the former USSR as
a Temporary Pharmacopoeial Article which allowed the large-scale industrial production of a liquid
extract (DER 1:1, extraction solvent ethanol 40%). The products were in use also in those parts of
the former USSR, which now belong to the European Union (Estonia, Latvia, Lithuania), as
confirmed by the National Medicines Agency of Lithuania.
B. Dry extract of root and rhizome, DER 2.5-5:1, first extraction solvent ethanol 70%, second
extraction solvent water. On the market in Sweden since 1987 (in Panossian et al. 2010, the year
1985 is mentioned). The herbal preparation is named SHR-5 in the literature.
C. Dry extract of root and rhizome, DER 1.5-5:1, extraction solvent ethanol 60% m/m. On the market
as traditional herbal medicinal product according to Directive 2004/24/EC in Austria and UK since
2008, in The Netherlands since 2009, in Sweden and Spain since 2010, in Italy since 2011. The
registrations were granted based on the traditional medicinal use of the herbal preparations A and
B.
Based on this information on the medicinal use of more than 30 years within the European Union, the
requirements laid down in Directive 2004/24/EC are fulfilled.
The herbal preparations B and C are at the moment in medicinal use in the European Union, while
there are no reports on the use of the herbal preparation A. Therefore the following specification for
the herbal preparation is found for the monograph: Dry extract (DER 1.5-5:1), extraction solvent
ethanol 67-70% v/v, with a footnote pointing to the requirement that a narrow range of the DER and a
fixed strength for the ethanol used for extraction need to be specified for each herbal medicinal
product.

2.2. Information on traditional/current indications and specified

substances/preparations
Herbal preparation A (Liquid extract, DER 1:1, extraction solvent ethanol 40%): Asthenia, fatigue,
dystonia
Herbal preparation B (Dry extract, DER 2.5-5:1, first extraction solvent ethanol 70%, second
extraction solvent water): Traditional herbal medicinal product used as an adaptogen in case of stress
related decreased performance ability with symptoms such as fatigue, sensation of weakness,
irritability and mild anxiety.
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Herbal preparation C (Dry extract, DER 1.5-5:1, extraction solvent ethanol 60% m/m): Traditional
herbal medicinal product for relief of mental and physical symptoms of stress, such as fatigue,
weakness, exhaustion, irritability and slight anxiety.
Panossian et al. (2010) report traditional use in folk medicine in the indications like headaches, as
astringent, to strengthen the head, to enhance the intellect, for restoration of weak nerves; external
use for hair growth, relieve of swellings, decrease of back pain, pain in joints. It is said that Laplanders
(Smi) chewed on bits of Rhodiola on long journeys.

2.3. Specified strength/posology/route of administration/duration of use

for relevant preparations and indications
Herbal preparation A (Liquid extract, DER 1:1, extraction solvent ethanol 40%):
single dose 5-10 drops, 15-30 minutes before the meal; 2-3 times daily. Duration of use: 10-20 days.
Herbal preparation B (Dry extract, DER 2.5-5:1, first extraction solvent ethanol 70%, second
extraction solvent water): One tablet contains 144 mg dry extract. Dosage: 1 tablet 1-2 times daily.
Not recommended for children under 12 years. Oral use.
Herbal preparation C (Dry extract, DER 1.5-5:1, extraction solvent ethanol 60% m/m): One tablet
corresponds to ca. 600 mg dried root. Dosage: 1 tablet 2 times daily. Not recommended for children
under 12 years. Oral use. Duration of use: 2 weeks.

3. Non-Clinical Data
3.1. Overview of available pharmacological data regarding the herbal
substance(s), herbal preparation(s) and relevant constituents thereof
Pharmacological data regarding the herbal preparation:
Oxidative stress, antioxidative effects:
Battistelli et al. (2005): An aqueous extract (100 mg herbal substance in 2.4 ml water, 3-fold
extraction) was applied in vitro to human erythrocytes, which were exposed to hypochlorous acid
(HOCl)-oxidative stress. The evaluation of the antioxidant capacity of the Rhodiola extract was carried
out by means of scanning electron microscopy and of haemolytic behaviour in the presence of
increasing doses of the aqueous extract in different experimental environments (co-incubation and
subsequent incubations). The results obtained are consistent with a significant protection by the
extract in presence of the oxidative agent.
De Sanctis et al. (2004): An aqueous extract (12 mg dried herbal substance in 2.4 ml final volume)
was tested for its ability to counteract some of the main damages induced by HOCl to human
erythrocytes. Ascorbic acid was used as a reference substance because of its physiological HOClscavenging ability. The extract was able to significantly protect, in a dose-dependent manner, human
red blood cells from glutathione depletion, glyceraldehyde-3-phosphate dehydrogenase inactivation
and haemolysis induced by the oxidant. It was demonstrated that the extract acts from the inside of
the erythrocyte suggesting a probable involvement of cell components.
Calcabrini et al. (2010): The authors investigated the protection afforded by an aqueous extract
(DER 1:1) to reduce glutathione levels, glyceraldehyde-3-phosphate dehydrogenase activity, and
thiobarbituric acid reactive substances levels in cultured human keratinocytes (NCTC 2544) exposed to
different oxidative insults (Fe(II)/ascorbate, Fe(II)/H(2)O(2), and tert-butyl-hydroperoxide) as well as
the influence of the extract on the production of intracellular reactive oxygen species and on the
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activity of antioxidant enzymes (catalase, superoxide dismutase, glutathione peroxidase, and

glutathione reductase). It could be demonstrated that the extract was able to increase in a time- and
dose-dependent manner the activity of the trans-plasma membrane oxido reductase activity as an
indirect evaluation of the intracellular redox status. Keratinocytes of the type NCTC 2544 are able to
better counteract several oxidative insults if incubated with a Rhodiola rosea aqueous extract.
Chen et al. (2008, only abstract available): This study investigated the antioxidant potential of
3 adaptogen extracts, Rhodiola rosea (golden root), Eleutherococcus senticosus (Siberian ginseng) and
Emblica officinalis (Indian gooseberry, Amla). The results of this study showed that Rhodiola rosea had
a higher potential for singlet oxygen scavenging, hydrogen peroxide scavenging, ferric reducing,
ferrous chelating and protein thiol protection than either of the other two extracts. In addition, the
polyphenol content in the three adaptogen extracts followed the order: Rhodiola rosea, Emblica
officinalis and Eleutherococcus senticosus. The data suggest that the antioxidant potential of the
3 adaptogen extracts was proportional to their respective polyphenol content.
Anti-fatigue effects:
Lee et al. (2009): An extract of Rhodiola rosea (no details on extraction solvent and DER,
approximately 1.4% salidroside, 0.4% rosin, 0.4% rosarin, 1% rosavin) was tested on swimminginduced fatigue in rats. The supplementation (dosages from 5 to 125 mg/kg) in water for 2-4 weeks
was evaluated in male Wistar rats with 90-minutes unloaded swimming exercise and 5% body weight
loaded swimming up to fatigue. Blood urea nitrogen (BUN), glutamic oxaloacetic transaminase (GOT),
glutamic pyruvic transaminase (GPT), lactate dehydrogenase (LDH), hepatic glycogen content, the
activity of fat metabolism enzymes, sterol regulatory element-binding protein-1 (SREBP-1) and fatty
acid synthase (FAS), the tissue oxygen content and ratio of red and white skeletal muscle fibres in rats
were measured. The extract significantly increased liver glycogen, SREBP-1, FAS, heat shock protein
70 expression, B-cell lymphoma 2/Bax protein ratio and oxygen content before swimming. Rhodiola
rosea supplementation significantly increased the swimming time in a dose-dependent manner and
reduced swimming-enhanced serum BUN, GOT and GPT levels. The ratio of red and white muscle fibres
was not altered after chronic Rhodiola rosea extract supplementation. Chronic Rhodiola rosea
supplementation significantly improved exhaustive swimming-induced fatigue by the increased
glycogen content, energy supply of lipogenic enzyme expressions and protective defence mechanisms.
Abidov et al. (2003): The effects of oral treatment with an ethanolic extract (ethanol 40%) from
Rhodiola rosea (50 mg/kg) and Rhodiola crenulata (50 mg/kg) roots on the duration of exhaustive
swimming and ATP content in mitochondria of skeletal muscles in rats were investigated. Treatment
with Rhodiola rosea extract significantly (by 24.6%) prolonged the duration of exhaustive swimming in
comparison with control rats and rats treated with Rhodiola crenulata. Rhodiola rosea extract activated
the synthesis or resynthesis of ATP in mitochondria and stimulated reparative energy processes after
intense exercise.
Stress-protective effects:
Mattioli & Perfumi (2007): The aim of this work was to determine whether in rats a hydroalcoholic
Rhodiola rosea extract (no details on the strength of the extraction solvent published; standardised in
3% rosavin and 1% salidroside) reverses hypophagia induced by (1) physical stress due to 60 minutes
immobilisation; (2) intracerebroventricular injection of corticotropin-releasing factor (CRF, 0.2 g/rat),
the major mediator of stress responses in mammals; (3) intraperitoneal injection of Escherichia coli
Lipopolysaccharide (LPS, 100 g/kg); (4) intraperitoneal administration of fluoxetine (FLU, 8 mg/kg).
The effect of the same doses of the plant extract was also tested in freely-feeding and in 20 hours
food-deprived rats. The extract was administered acutely by gavage to male Wistar rats 1 hour before
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the experiments. The results show that, at doses of 15 and 20 mg/kg, the extract reversed the
anorectic effects induced both by immobilisation and by intracerebroventricular CRF injection.
Moreover, at the same doses, the extract failed to reduce the anorectic effect induced both by LPS and
FLU, and did not modify food intake in both freely-feeding and food-deprived rats. The authors
interpret the results that Rhodiola extract is able selectively to attenuate stress-induced anorexia,
providing functional evidence of claimed adaptogen and anti-stress properties of Rhodiola rosea L.
Zhu et al. (2003): Noise is one of the factors that induce critical stress in animals. The contents of
glycogen, lactic acid and cholesterol in the liver of noise-stressed rats were analysed in order to
investigate the alleviation of noise-stress-induced physiological damages by a decoction of the
underground organs of Rhodiola rosea. More than 95 dB noise ranging from 2 to 4 kHz reduced the
contents of these compounds in the liver of rats not injected with the extract, but did not change the
contents in the liver of rats treated with the extract. The results indicate that Rhodiola extract
improved the ability for rats to resist noise stress.
Boon-Niermeijer et al. (2000): The authors examined whether Rhodiola extract SHR-5 (DER 2.5-5:1,
first extraction solvent ethanol 70%, second extraction solvent water) is able to exert a protective
action against stress-induced death of embryos of the pond snail Lymnaea stagnalis, and whether a
possible protective action by the extract can be explained by the induction of heat shock proteins. The
extract was applied, for a period of 20 hours, to 3-day old larvae of the pond snail. Subsequently, they
were exposed to a high and toxic dose of different environmental stressors (heat shock: 43C for
4 minutes, an oxidative stress condition (superoxide radicals induced by menadione 600 M for
2 hours) and heavy metal-induced stress (copper 150 M for 1 hour or cadmium 20 M during 1 hour).
The Rhodiola extract exerted a strong protective action against a lethal heat shock. It also significantly
protected against the negative effect of superoxide radicals as induced by menadione. With respect to
the protective action against exposure to heavy metals, a small but significant protection was observed
against intoxication with copper or cadmium. Although the degree to which resistance is enhanced
appears to depend on the type of stressor applied, the results confirm, in the opinion of the authors,
the definition of phyto-adaptogens as being universal enhancers of non-specific resistance against
different kinds of stress conditions. The extract did not induce the synthesis of any of the heat shock
proteins, nor did it modulate the normal heat shock induced synthesis of these stress proteins.
Therefore it is concluded that it is unlikely that heat shock proteins play a major role in obtaining an
enhanced state of resistance provided by Rhodiola extracts.
Panossian et al.(2007): Blood levels of several mediators were analysed in rabbits subjected to
restraint stress. Beside other herbal preparations, one group of rabbits received orally 1 mg/kg of the
Rhodiola extract SHR-5 for 7 consecutive days. The effect on the blood levels of the mediator
substances were compared between animals receiving placebo and stress, animals receiving study
medication without stress and animals receiving study medication and stress. The stress was induced
by immobilisation of the animals for 2 hours. In the placebo group, the levels of phosphorylated kinase
(p-SAPK/p-JNK), nitric oxide (NO) and cortisol were increased significantly. In animals treated with
Rhodiola, the levels of NO and cortisol remained unchanged.
Mattioli et al. (2009): The aim of this study was to determine whether chronic treatment with a
hydroalcoholic Rhodiola rosea extract (no details on the strength of the extraction solvent published;
containing 3% rosavin and 1% salidroside) can prevent alterations induced in female rats following
6 weeks of a chronic mild stress (CMS) procedure. This was analysed through the behavioural and
physiological parameters of consumption of 1% sucrose solution, locomotor and exploratory activities,
body weight gain and oestrous cycle length. After the first 3 weeks of stress, the extract was
administered daily by gavage at doses of 10, 15 and 20 mg/kg for the remaining 3 weeks. In addition,
fluoxetine (10 mg/kg orally), which has been shown to reverse CMS-induced disruptions, was used as
the reference treatment. Rats subjected to the CMS procedure demonstrated decreased sucrose intake,
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reduced moving behaviour, minimised weight gain and dysregulation of their oestrous cycle. Treatment
with the Rhodiola extract completely reverted all of these changes. The effects of the extract were
comparable to those of fluoxetine. The authors are of the opinion that chronic administration of
Rhodiola extract results in potent inhibition of the behavioural and physiological changes induced by
chronic exposure to mild stressors.
Chen et al. (2008a, only abstract available): The aim of the study was to explore the effects of
Rhodiola rosea on the body weight and the intake of sucrose and water in depressive rats induced by
chronic mild stress. A total of 70 male Sprague-Dawley (SD) rats were divided into 7 groups, including
normal control group (treated with 0.5% sodium carboxymethycellulose), untreated group, negative
control group (treated with 0.5% sodium carboxymethycellulose), positive control group (treated with
fluoxetine), low-, medium- and high-dose Rhodiola rosea group (treated with 1.5, 3 and 6 g/kg
Rhodiola rosea respectively, no details on the type of herbal preparation available). Except for rats in
the normal control group, the other 60 rats endured chronic stress for 4 weeks to establish the
depression model. After that, rats were administered Rhodiola rosea for 3 weeks. After termination of
the stress regime, compared with the normal control group, the body weight and 1% sucrose intake in
depressive rats were decreased. After 3-week Rhodiola rosea treatment, the body weight and 1%
sucrose intake increased in rats of the low-dose Rhodiola rosea group and recovered to the level of the
normal control group.
Cifani et al. (2010): Stress is a key determinant of binge eating (BE). BE for highly palatable food
(HPF) was evoked in female rats by three 8-day cycles of food restriction/re-feeding (for 4 days 66%
of the usual chow intake; for 4 days food ad libitum) and acute stress on the test day (day 25).
Rhodiola rosea dry extract (3% rosavin, 3.12% salidroside; no details on extraction solvent) or its
active principles were given by gavage 1 hour before access to HPF. Only rats exposed to both food
restrictions and stress exhibited BE in the first 15-60 minutes after the stressful procedure. Rhodiola
rosea extract 10 mg/kg significantly reduced and 20 mg/kg abolished the BE episode. Rhodiola rosea
extract 20 mg/kg abolished also stress-induced increase in serum corticosterone levels. The Rhodiola
rosea active principle salidroside, but not rosavin, at doses present in the extract, dose-dependently
reduced or abolished BE for the period in which it was elicited. In conclusion, results indicate that
Rhodiola rosea extracts may have therapeutic properties in bingeing-related eating disorders and that
salidroside is the active principle responsible for this effect.
Effects on nervous system:
Qu et al. (2009): The authors investigated the pre-treatment effects of Rhodiola rosea extract (no
details on extraction solvent published) on cognitive dysfunction, oxidative stress in hippocampus and
hippocampal neuron injury in a rat model of Alzheimer's disease. Male SD rats were pre-treated with
Rhodiola rosea extract at doses of 1.5, 3 and 6 g/kg for 3 weeks by gavage twice daily, followed by
bilateral intracerebroventricular injection with streptozotocin (1.5 mg/kg) on day 1 and 3. Behavioural
alterations were monitored after 2 weeks from the lesion using Morris water maze task. Three weeks
after the lesion, the rats were sacrificed for measuring the malondialdehyde (MDA), glutathione
reductase (GR) and reduced glutathione (GSH) levels in hippocampus and histopathology of
hippocampal neurons. The MDA level was significantly increased while the GR and GSH levels were
significantly decreased with striking impairments in spatial learning and memory and severe damage to
hippocampal neurons in the model rat induced by intracerebroventricular injection of streptozotocin.
These abnormalities were significantly improved by pre-treatment with Rhodiola rosea extract
(3 g/kg).

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Perfumi & Mattioli (2007): The purpose of the study was to re-investigate the effects produced by a
single oral administration of a Rhodiola rosea hydroalcoholic extract (containing 3% rosavin and 1%
salidroside; no information on the extraction solvent published) on the central nervous system in mice.
The extract was tested on antidepressant, adaptogenic, anxiolytic, nociceptive and locomotor activities
at doses of 10, 15 and 20 mg/kg, using predictive behavioural tests and animal models. The results
show that this Rhodiola rosea extract significantly, but not dose-dependently, induced antidepressantlike, adaptogenic, anxiolytic-like and stimulating effects in mice. This study thus provides evidence of
the efficacy of Rhodiola rosea extracts after a single administration.
Van Diermen et al. (2009): In order to investigate the influence of Rhodiola rosea L. roots on mood
disorders, 3 extracts were tested against monoamine oxidases (MAOs A and B) in a microtitre plate
bioassay. Twelve compounds were then isolated by bioassay-guided fractionation using
chromatographic methods. The methanol and water extracts exhibited respectively inhibitions of
92.5% and 84.3% on MAO A and 81.8% and 88.9% on MAO B, at a concentration of 100 g/ml. The
most active compound (rosiridin) presented an inhibition over 80% on MAO B at a concentration of
10(-5) M (pIC50=5.38+/-0.05).
Chen et al. (2009): The purpose of this study was to investigate the effects of Rhodiola rosea extract
(ethanol 70%) on the serotonin (5-HT) level, cell proliferation and quantity of neurons in the cerebral
hippocampus of depressive rats induced by CMS. After 3 weeks of oral administration of 1.5 g up to 6
g/kg per day, 5-HT content had recovered to normal level. In the low dose group, the extract induced
neural stem cell proliferation in the hippocampus to return to normal level, repairing the injured
neurons in the hippocampus.
Qin et al. (2008, only abstract available): The purpose of this study was to investigate the effects of
Rhodiola rosea (no details on the type of the herbal preparation available) on the level of 5-HT, cell
proliferation and differentiation, and number of neurons in the cerebral hippocampus of rats with
depression induced by CMS. After 3 weeks of administration of the preparation, all measured
parameters like 5-HT content, number of bromodeoxyuridine positive cells, percentage of
bromodeoxyuridine and beta-tubulin III double labelled cells and number of neurons in the cerebral
hippocampus returned to normal level.
Panossian et al. (2008): The antidepressant-like activity of an extract of the roots of Rhodiola rosea
(DER 2.5-5:1, no information on the extraction solvent; containing 2.7% rhodioloside, 6% rosavin,
0.8% tyrosol), its combination with piperine, isolated constituents from Rhodiola, such as rhodioloside,
rosavin, rosin, rosarin, tyrosol, cinnamic alcohol, cinnamaldehyde and cinnamic acid has been assessed
in laboratory animals through application of the Porsolt behavioural despair assay. The orally
administered extract in dosages of 10, 20 and 50 mg/kg reduced dose-dependently the immobility
time more strongly compared to Hypericum extract LI160 (20 mg/kg), amitriptyline (3 mg/kg) or
imipramine (30 mg/kg). The combination with piperine was also active in a similar degree, but no
dose-dependence was detectable. Rhodioloside and tyrosol contributed considerably to this effect.
A fixed combination of rhodioloside, rosavin, rosarin and rosin was more active than any of the
individual components alone.
Mattioli & Perfumi (2011): The aim of the study was to investigate the effects of a Rhodiola rosea
hydroalcoholic extract (no details on extraction solvent published; 3% total rosavins, 1% salidroside)
on the prevention of the development of nicotine dependence and for the reduction of abstinence
suffering following nicotine cessation in mice. Dependence was induced in mice by subcutaneous
injections of nicotine (2 mg/kg, 4 times daily) for 8 days. Spontaneous abstinence syndrome was
evaluated 20 hours after the last nicotine administration, by analysis of withdrawal signs, as affective
(anxiety-like behaviour) and physical (somatic signs and locomotor activity). The extract was
administered orally during nicotine treatment (10, 15 and 20 mg/kg) or during nicotine withdrawal
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(20 mg/kg). Both affective and somatic signs (head shaking, paw tremors, body tremors, ptosis,
jumping, piloerection and chewing) induced by nicotine withdrawal were abolished by administration of
the extract in a dose-dependent manner, during both nicotine exposure and nicotine cessation.
Mattioli & Perfumi (2011a): The same extract, as in Mattioli & Perfumi (2011) was investigated for
effects on acquisition and expression of morphine tolerance and dependence in mice. Animals were
injected with repeated administration of morphine (10 mg/kg, subcutaneous) twice daily for 5 or 6
days, in order to make them tolerant or dependent. The extract (0, 10, 15 and 20 mg/kg) was
administered by the intragastric route 60 minutes prior to each morphine injection (for acquisition) or
prior the last injection of morphine or naloxone on test day (for tolerance or dependence expression,
respectively). Morphine tolerance was evaluated by testing its analgesic effect in the tail flick test at
the 1st and 5th days. Morphine dependence was evaluated by counting the number of withdrawal signs
(jumping, rearing, forepaw tremor, teeth chatter) after naloxone injection (5 mg/kg; intraperitoneal)
on the test day (day 6). The Rhodiola rosea L. extract significantly reduced the expression of morphine
tolerance, while it was ineffective in modulating its acquisition. Conversely, the extract significantly and
dose-dependently attenuated both development and expression of morphine dependence after chronic
or acute administration.
Lifespan increasing effects:
Schriner et al. (2009, only abstract available): The extract SHR-5 (DER 2.5-5:1, first extraction solvent
ethanol 70%, second extraction solvent water) could extend both mean (24% in both sexes) and
maximum (16% in males and 31% in females) lifespan in the fly Drosophila melanogaster when
compared to controls. It lowered mitochondrial superoxide levels and afforded elevated protection
against the superoxide generator paraquat in both sexes. The extract did not alter the activities of the
major antioxidant enzymes, the superoxide dismutases or catalase, nor did it afford protection against
hydrogen peroxide H2O2 or soluble iron.
Schriner et al. (2009a): A Rhodiola rosea extract (no details published) could protect cultured cells
against ultraviolet light, paraquat and H2O2. However, it did not alter the levels of the major
antioxidant defences nor did it markedly activate the antioxidant response element or modulate hemeoxygenase-1 expression levels at relevant concentrations. In addition, the Rhodiola rosea extract was
not able to significantly degrade H2O2 in vitro. These results suggest that, in human cultured cells,
Rhodiola rosea does not act as an antioxidant and that its mode of action cannot be sufficiently
explained through a pro-oxidant hormetic mechanism.
Jafari et al. (2007): Using the fly, Drosophila melanogaster, the effects of Rhodiola extract (no details
published) on lifespan was investigated. Rhodiola supplied every other day at 30 mg/ml significantly
increased the lifespan of Drosophila melanogaster. When comparing the distribution of deaths between
Rhodiola-supplemented and control flies, Rhodiola-fed flies exhibited decelerated aging. Although the
observed extension in lifespan was associated with statistically insignificant reductions in fecundity,
correcting for a possible dietary restriction effect still did not eliminate the difference between
supplemented and control flies, nor did the effect of Rhodiola depend on dietary manipulation, strongly
suggesting that Rhodiola is not a mere dietary restriction mimetic.
Wiegant et al. (2009): Extracts of Rhodiola (SHR-5, DER 2.5-5:1, first extraction solvent ethanol 70%,
second extraction solvent water) and of Eleutherococcus increased the mean lifespan of the nematode
Caenorhabditis elegans in a dose-dependent way. In at least 4 independent experiments, 250 g/ml
Eleutherococcus and 10-25 g/ml Rhodiola (SHR-5) significantly increased lifespan between 10 and
20% (P < 0.001), increased the maximum lifespan with 2-3 days and postponed the moment when the
first individuals in a population die, suggesting a modulation of the ageing process. With higher
concentrations, less effect was observed, whereas at the highest concentrations tested (2500 g/ml
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Eleutherococcus and 250 g/ml Rhodiola) a lifespan shortening effect of 15-25% (P < 0.001) was
observed. Both extracts were also able to increase stress resistance in C. elegans against a relatively
short heat shock (35C during 3 hours) as well as chronic heat treatment at 26C. An increase against
chronic oxidative stress conditions was observed in mev-1 mutants, and during exposure of the wild
type nematode to paraquat (10 mM) or UV stress, be it less efficiently. Both extracts induced the
translocation of the DAF-16 transcription factor from the cytoplasm into the nucleus, suggesting a
reprogramming of transcriptional activities favouring the synthesis of proteins involved in stress
resistance (such as the molecular chaperone Heat Shock Protein HSP-16) and longevity.
Cardio protective effects, effects on the vascular system:
Maslov et al. (2009, only abstract available): A course of treatment (16 mg/kg orally during 5 days) by
Aralia mandshurica or Rhodiola rosea extracts (no details available) reduced the incidence of ischemic
and reperfusion ventricular arrhythmias during 10-minute ischemia and 10-minute reperfusion in rats.
Chronic treatment by Aralia, Rhodiola and Eleutherococcus elevated the ventricular fibrillation
threshold in rats with post-infarction cardiosclerosis.
Li et al. (2005, only abstract available): On the basis of successful establishment of myocardial
infarction rat model, the experimental animals were divided into the model group, the Rhodiola group
(no details on the type of herbal preparation and on posology available), the positive control group and
the sham-operated group. They were sacrificed after 6 weeks feeding. The expressions of Flt-1 and
angiopoietin receptor (Tie-2) in myocardial tissue were significantly increased in the Rhodiola treated
group after treatment, showing significant difference as compared with those in the positive control
group and the model group (P < 0.05). The expression of the growth factor KDR in myocardium after
Rhodiola intervention was higher than that in the sham-operated and non-intervened group (P <
0.05), but insignificantly different to that in the positive control group and model group. Therefore it
was concluded that Rhodiola could improve angiogenesis to ameliorate myocardial ischemia by
regulating the expression of Flt-1 and Tie-2 in ischemic myocardium.
Shen et al. (2008, only abstract available): Thirty male New Zealand rabbits were randomly divided
into 3 groups equally, i. e. the control group (A) fed with common diet and treated with distilled water,
the high fat diet group (B) and the Rhodiola group (C, no details on the type of herbal preparation and
on dosage available) fed with diet containing 1.5% cholesterol and treated respectively with distilled
water and Rhodiola (1 ml/kg per day). All the treatments were administered via gastrogavage once
daily for 9 successive weeks. Levels of blood lipids in various groups was determined and compared at
the end of the experiment. Meanwhile, the tissue sample of aorta was taken for observation through
HE and Sudan red staining, for detecting the CD34 positive response intensity by immunohistochemical
staining and the vascular endothelial cell growth factor (VEGF) expression by Real-time fluorescent
quantitative PCR and Western blot. The determination of blood lipids showed that in Group C, TC was
42.01 +/- 1.99 mmol/l, TG 4.83 +/- 0.75 mmol/l and LDL-C 38.40 +/- 0.74 mmol/l, all lower than
those in Group B (70.74 +/- 2.66 mmol/l, 8.75 +/- 0.78 mmol/l and 51.05 +/- 0.34 mmol/l,
respectively), showing statistical difference between groups (P < 0.05). The intima/media tunica
thickness ratio and the CD34 positive area of plaque in Group C were all lower than those in Group B
(0.35 +/- 0.03 vs 0.43 +/- 0.03 and 29.12 +/- 2.56% vs 39.28 +/- 3.48%, P <0.05). Besides, the
VEGF expression in atherosclerotic plaque was also lower in Group C than that in Group B.
Maslov & Lishmanov (2007, only abstract available): The chronic administration of a Rhodiola rosea
extract (no details available) in a single daily dose of 1 ml/kg (p.o.) during 8 days increased the
resistance of myocardium with respect to the cardiotoxic action of isoproterenol and the
arrhythmogenic action of epinephrine in rats. Pre-treatment with the extract prevented the stressor
cardiac damages, as measured by 99mTc-pyrophosphate accumulation in the heart. The

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cardioprotective action of the extract was highest after 5-day administration. The antiarrhythmic effect
of the adaptogen was at a maximum after 8-day administration. It was found that p-tyrosol also
exhibited antiarrhythmic and cardioprotective properties. Pre-treatment with the extract decreased the
infarction size/risk area ratio during the coronary artery occlusion and reperfusion in vivo. The chronic
administration of the extract increased the tolerance of the isolated perfused rat heart to the
pathogenic action of global ischemia and reperfusion. Pre-treatment not only prevented the occurrence
of arrhythmias, but also abolished cardiac electrical instability in rats with postinfarction cardiac
sclerosis. It has been found that the chronic administration of the extract (1 ml/kg, p.o., over 8 days)
increased the level beta-endorphin in rat blood plasma and the content of leu-enkephalin in myocardial
tissue. Naloxone (2 mg/kg) abolished the cardioprotective and antiarrhythmic effect of the extract.
Effects on the blood system:
Provalova et al. (2002, only abstract available): Extracts of Rhodiola rosea did not modulate
granulocytopoiesis (no details available on type of preparation and methods).
Anti-inflammatory effects:
Pooja et al. (2009): The study was undertaken to evaluate the anti-inflammatory effects of a liquid
extract of Rhodiola rosea underground organs (extraction solvent ethanol 40%). The anti-inflammatory
activity was determined through carrageenan-induced paw oedema, formaldehyde-induced arthritis
and nystatin-induced paw oedema in rat model. The liquid extract exhibited inhibitory effect against
acute and subacute inflammation at a dose of 250 mg/kg body weight. Inhibition of nystatin-induced
oedema was also observed in a dose-dependent manner. The extract showed varying inhibitory
activities against enzymes related to inflammation depending on the concentrations. A potent inhibition
was observed against Cox-2 and phospholipase A2. Inhibition of nystatin-induced oedema and
phospholipase A2 suggested that membrane stabilisation could be the most probable mechanism of
action of the extract in anti-inflammation.
Effects on metabolism:
Kim et al. (2006): This study was designed to examine the effects of Cinnamomum cassia and
Rhodiola rosea extracts (dry extract DER 10:1, extraction solvent ethanol 85%) on blood glucose, lipid
peroxidation, the level of reduced glutathione and its related enzymes (glutathione reductase,
glutathione S-transferase) and the activity of the antioxidant enzymes (catalase, superoxide dismutase
and glutathione peroxidase) in the liver of diabetic db/db mice. Diabetic C57BL/Ks db/db mice were
used as experimental models. Mice were divided into control (n=10), Cinnamomum cassia
(200 mg/kg/day, n=10), and Rhodiola rosea (200 mg/kg/day, n=10) treated groups, for 12 weeks of
oral treatment. Both extracts significantly decreased blood glucose, increased levels of reduced
glutathione and the activities of glutathione reductase, glutathione S-transferase, glutathione
peroxidase, catalase and superoxide dismutase in the liver. Extract treatment also significantly
decreased lipid peroxidation.
Effects on the endocrinous system:
Kwon et al. (2006): Two species of the genus Rhodiola (Rhodiola crenulata and Rhodiola rosea) were
investigated for the inhibition of -amylase and -glucosidase. Water extracts of Rhodiola crenulata
had the highest -amylase inhibitory activity (IC50, 98.1 g total phenolic/ml) followed by ethanol
extract of Rhodiola crenulata (IC50, 120.9 g total phenolic/ml) and ethanol extract (ethanol 12%) of
Rhodiola rosea (IC50, 173.4 g total phenolic/ml). Ethanol extract of Rhodiola rosea (IC50, 44.7 g total
phenolic/ml), water extract (macerate DER 1:10) of Rhodiola rosea (IC50, 52.3 g total phenolic/ml),
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water extract of Rhodiola crenulata (IC50, 60.3 g total phenolic/ml) and ethanol extract of Rhodiola
crenulata (IC50, 60.2 g total phenolic/ml) also showed significant -glucosidase inhibitory activity. The
-glucosidase inhibitory activity of the extracts was compared to standard tyrosol, which was
significantly detected in the extracts using HPLC. Tyrosol had strong -glucosidase inhibitory activity
(IC50, 70.8 g total phenolic/ml) but did not have any inhibitory effect on the -amylase activity.
Results suggested that -glucosidase inhibitory activities of both Rhodiola extracts correlated to the
phenolic content, antioxidant activity and phenolic profile of the extracts. The ability of the above
Rhodiola extracts to inhibit rabbit lung angiotensin I-converting enzyme (ACE) was also investigated.
The ethanol extracts of Rhodiola rosea had the highest ACE inhibitory activity (38.5%) followed by
water extract of Rhodiola rosea (36.2%) and Rhodiola crenulata (15.4%).
Ip et al. (2001): Chronic hypoxia significantly increased the mRNA expression for angiotensinogen II
receptor subtypes AT1b and AT2 in the pancreatic renin-angiotensin system. The activation of the
renin-angiotensin system may play an important role in cellular pathophysiological processes.
Angiotensin II enhances the formation of reactive oxygen species (ROS) via the activation of xanthine
oxidase or NAD(P)H oxidase. The reactive oxygen species can cause oxidative damage in the pancreas
and other tissues, either directly or indirectly via the formation of other radicals such as reactive
nitrogen species. Rhodiola therapy may protect hypoxia-induced pancreatic injury in two ways. It
prevents hypoxia-induced biological changes by increasing intracellular oxygen diffusion and efficiency
of oxygen utilisation. Alternatively, it reduces hypoxia-induced oxidative damage by its antioxidant
activities. Additional experimental data are required to fully elucidate the mode of action of this herbal
drug.
Anti-cancer effects:
Majewska et al. (2006): It has been found that the extract of Rhodiola rosea rhizomes (extraction
solvent ethanol 96%) inhibits division of HL-60 cells, which is preceded by an accumulation of cells at
the prophase stage. This leads to induction of apoptosis and necrosis in HL-60 cells, and to marked
reduction of their survival. The cells enter apoptosis from phase G2/M of the cell cycle. After treatment
with the extract, no chromosome aberrations or micronuclei were observed, which indicates the mild
action of the extract.

Pharmacological data regarding isolated constituents:

Salidroside and other phenylalkaloids:
Oxidative stress, antioxidative effects:
Huang et al. (2009, only abstract available): Wistar rats received 5, 25, 125 mg of a Rhodiola extract
per day for 4 weeks. Salidroside, rosin, rosavin and rosarin scavenged O2(-)*, H2O2, and HOCl activity
in a dose-dependent manner. The 90 minutes swimming exercise increased the O2(-)* production in
the order: liver > skeletal muscle > blood, indicating that liver is the most sensitive target organ. The
level of plasma MDA, a lipid peroxidation product, was also increased after exercise. Treatment during
4 weeks of Rhodiola rosea extracts significantly inhibited swimming exercise-enhanced O2(-)*
production in the blood, liver and skeletal muscle and plasma MDA concentration. The expression of
Mn-superoxide dismutase, Cu/Zn-superoxide dismutase and catalase in livers were all enhanced after
4 weeks of Rhodiola rosea supplementation especially at the dose of 125 mg/day/rat. Treatment with
Rhodiola rosea extracts for 4 weeks significantly increased swimming performance.
Li et al. (2011): In the study the protective activity of salidroside against 1-methyl-4-phenylpyridinium
(MPP(+)) -induced apoptosis in PC12 cells was investigated. The incubation of PC12 cells with
salidroside prior to MPP(+) exposure significantly reduced cell apoptosis and attenuated collapse of the
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mitochondrial membrane potential (MMP). Furthermore, salidroside inhibited the MPP(+)-induced NO

increase and overexpression of nNOS (nitric oxide synthase) and iNOS, and suppressed accumulation
of ROS and intracellular free Ca2+. The results show that the protective effects of salidroside on PC12
cells are mediated, at least in part, by inhibition of the NO pathway.
Yu et al. (2010): The aim of this study was to investigate the effects of salidroside on H2O2-induced cell
apoptosis in nerve growth factor (NGF)-differentiated PC12 cells and the possible involvement of the
extracellular signal-regulated protein kinase 1/2 (ERK1/2) signalling pathway. MTT assay, Hoechst
33342 staining, and terminal deoxynucleotidyl transferase TdT-mediated dUTP-biotin nick end labelling
(TUNEL) assay collectively showed that the pre-treatment with salidroside alleviated, in a dosedependent manner, cell viability loss and apoptotic cell death induced by H2O2 stimulation in cultured
NGF-differentiated PC12 cells. According to Western blot analysis, pre-treatment with salidroside
transiently caused the activation of the ERK1/2 pathway; a selective inhibitor of the mitogen-activated
protein (MAP) kinase (MAPKK, MEK) blocked the salidroside-activated ERK pathway and thus
attenuated the influences of salidroside on H2O2-induced increase in the level of cleaved caspase-3, a
major executant of apoptosis cascades. Morphological analysis further indicated that, in the presence
of the MEK inhibitor, the neuroprotective effect of salidroside against H2O2-evoked cell apoptosis was
significantly abrogated. Taken together, the results suggest that the neuroprotective effects of
salidroside might be modulated by the ERK1/2 signalling pathway, especially at the level or upstream
of the caspase-3 activation.
Tan et al. (2009): The protective effects of salidroside on endothelial cells apoptosis induced by the
hypoxia mimicking agent cobalt chloride were investigated. After challenge with cobalt chloride for
24 hours, loss of cell viability and excessive apoptotic cell death were observed in EA.hy926 endothelial
cells, and the level of intracellular ROS increased concentration-dependently. However, the endothelial
cell apoptosis and excessive ROS generation were attenuated markedly by salidroside pre-treatment.
In addition, salidroside inhibited activation of caspase-3 and cleavage of poly(ADP-ribose) polymerase
(PARP) induced by cobalt chloride, decreased expression of Bax and rescued the balance of pro- and
anti-apoptotic proteins. These findings suggest that salidroside protects endothelial cells from cobalt
chloride-induced apoptosis as an antioxidant and by regulating the Bcl-2 family.
Chen et al. (2009a): This study investigated whether salidroside was able to extend its unique
neuroprotection to primary cultured rat hippocampal neurons against H2O2-induced cell damage. Cell
viability tests and cell apoptosis assays confirmed that salidroside pre-treatment attenuated H2O2stimulated apoptotic cell death in primary culture of hippocampal neurons in a concentrationdependent manner. The measurements of caspase-3 activity, NO production, and NOS activity suggest
that the protection of salidroside, shown in this study, might be mediated by inhibiting caspase-3
activity, and antagonising NO production and NOS activity during H2O2 stimulation.
Mao et al. (2010): Salidroside considerably reversed senescence-like phenotypes in the oxidant
challenged model, including alterations of morphology, cell cycle, SA--gal staining, DNA damage, as
well as related molecules expression such as p53, p21 and p16. The protection occurred in a dosedependent manner, with 5 M offering best efficacy. The proposed antioxidant property of the
compound was confirmed in this cellular system, and thus at least partially accounted for the
protection of the compound against premature senescence. Similar protection of salidroside against
replicative senescence was observed as well. The regulation of senescence-related molecules by
salidroside involved ROS-irrelevant mechanisms in both models.
Effects on the endocrinous system:
Wang et al. (2009, only abstract available): The effect of salidroside on the function and ultramicropathological change of the hypothalamic-pituitary-gonadal (HPG) axis of male rats in experimental
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navigation and intensive exercise was investigated. Six-week SD rats were randomised into three
groups: non-stress control (NC, n = 10), training control (TC, n = 12) and salidroside treatment (ST, n
= 12) group. Blood samples were collected from the NC rats that did not receive any stimulus after a
7-day intragastric administration of saline. The TC rats underwent a 10-day running training with
increasing load on the treadmill followed by a 7-day intragastric administration of saline. The ST rats
were subjected to the same process of running training as the TC group and received intragastric
administration of salidroside. Then, blood samples were immediately obtained. The serum testosterone
level was significantly lower in the TC than in the NC group, but showed no significant difference
between the ST and NC groups. HE staining revealed no significant difference in testis histopathology
among the 3 groups. Ultramicro-pathology showed that the secretory granules of the pituitary cells
were significantly reduced in the TC rats compared with the NC ones; the number of the granules
significantly increased in the ST group compared with the TC rats; mitochondrial swelling, increase of
electron density and decrease/disappearance of mitochondrial cristae were observed in the Leydig cells
of the TC rats. No significant differences were found in the testicular cells between the ST and NC
groups. It is concluded that negative psychological stress and intensive exercise can significantly
suppress the function of the HPG axis in rats. Salidroside therapy may have protective effects on the
HPG axis.
Neuroprotective effects:
Chen et al. (2008b): This study aimed to evaluate the inhibitory effects of salidroside on glutamateinduced cell death in a primary culture of rat hippocampal neurons as compared to brain-derived
neurotrophic factor as positive control. MTT and LDH assays, together with Hoechst 33342 staining,
TUNEL assay and flow cytometric analysis using annexin-V and propidium (PI) label, indicated that
salidroside pre-treatment attenuated glutamate-induced apoptotic cell death in primary cultured
hippocampal neurons, showing a dose-dependent pattern. Furthermore, caspase-3 activity assay and
calcium measurements with Fluo 4-AM, respectively, revealed that salidroside pre-treatment
antagonised activation of caspase-3 and elevation of intracellular calcium level, both of which were
induced by glutamate stimulation.
Cao et al. (2006): Salidroside could protect PC12 cell against injuries caused by exposure of PC12 cells
to 2 mmol/l glutamate for 15 minutes followed by incubation with serum-free medium for 24 hours,
which resembled the excitotoxin in vivo system. Furthermore, salidroside could decrease the cytosolic
free calcium concentration [Ca2+]i of PC12 cells in Mg2+-free Hanks' solution and D-Hanks' solution but
there was no effect on basal [Ca2+]i in Hanks' solution. The studies also indicated that salidroside
inhibited the increases of [Ca2+]i induced by KCl and glutamate. In conclusion, salidroside may protect
PC12 cells against glutamate excitotoxic damage through suppressing the excessive entry of Ca2+ and
the release of the calcium stores.
Zhang et al. (2007): In this paper, the neuroprotective effects of salidroside on H2O2-induced apoptosis
in SH-SY5Y cells were investigated. Pre-treatment with salidroside markedly attenuated H2O2-induced
cell viability loss and apoptotic cell death in a dose-dependent manner. The mechanisms by which
salidroside protected neuron cells from oxidative stress included the induction of several antioxidant
enzymes, thioredoxin, heme oxygenase-1 and peroxiredoxin-I, the down regulation of pro-apoptotic
gene Bax and the up regulation of anti-apoptotic genes Bcl-2 and Bcl-X(L). Furthermore, salidroside
dose-dependently restored H2O2-induced loss of mitochondrial membrane potential as well as the
elevation of intracellular calcium level. These results suggest that salidroside has protective effects
against oxidative stress-induced cell apoptosis, which might be a potential therapeutic agent for
treating or preventing neurodegenerative diseases implicated with oxidative stress.

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Zhang et al. (2010): Beta-amyloid (A) peptide, the hallmark of Alzheimer's disease, invokes a
cascade of oxidative damages to neurons and eventually leads to neuronal death. In this study,
salidroside was investigated to assess its protective effects and the underlying mechanisms against
A-induced oxidative stress in SH-SY5Y human neuroblastoma cells. A25-35-induced neuronal toxicity
was characterised by the decrease of cell viability, the release of LDH, morphological alterations,
neuronal DNA condensation, and the cleavage of PARP by activated caspase-3. Pre-treatment with
salidroside markedly attenuated A25-35-induced loss of cell viability and apoptosis in a dose-dependent
manner. The mechanisms of salidroside protection of neurons from oxidative stress included the
induction of antioxidant enzymes, thioredoxin, heme oxygenase-1 and peroxiredoxin-I, the down
regulation of pro-apoptotic protein Bax and the up regulation of anti-apoptotic protein Bcl-X(L).
Furthermore, salidroside dose-dependently restored A25-35-induced loss of MMP as well as suppressed
the elevation of intracellular ROS level. It was also observed that A25-35-stimulated the
phosphorylation of MAP kinases, including c-Jun NH(2)-terminal kinase (JNK) and p38 MAP kinase, but
not ERK1/2. Salidroside inhibited A25-35-induced phosphorylation of JNK and p38 MAP kinase, but not
ERK1/2. In the opinion of the authors, these results suggest that salidroside has protective effects
against A25-35-induced oxidative stress, which might be a potential therapeutic agent for treating or
preventing neurodegenerative diseases.
Yu et al. (2008): The hypoglycaemia and serum limitation-induced cell death in cultured PC12 cells
represents a useful in vitro model for the study of brain ischemia and neurodegenerative disorders. In
this study, MTT assay, Hoechst 33342 staining, and flow cytometry with annexin V/PI staining
collectively showed that pre-treatment with salidroside attenuated, in a dose-dependent manner, cell
viability loss, and apoptotic cell death in cultured PC12 cells induced by hypoglycaemia and serum
limitation. RT-PCR, Western blot analysis, and enzymatic colorimetric assay indicated the changes in
expression levels of Bcl-2, Bax, and caspase-3 in PC12 cells on exposure to hypoglycaemia and serum
limitation with and without salidroside pre-treatment, respectively. Rhodamine 123 staining and flow
cytometry with 2',7'-Dichlorofluorescin diacetate staining revealed the changes in the mitochondrial
membrane potential and radical ROS production in PC12 cells on exposure to hypoglycaemia and
serum limitation with and without salidroside pre-treatment, respectively. The experimental results
suggest that salidroside protects the PC12 cells against hypoglycaemia and serum limitation-induced
cytotoxicity possibly by the way of the modulation of apoptosis-related gene expression, the
restoration of the MMP, and the inhibition of the intracellular ROS production.
Cardioprotective effects:
Wu et al. (2009): The modification of proteins with O-linked N-acetylglucosamine (O-GlcNAc) is
increasingly recognised as an important posttranslational modification that modulates cellular function.
Cardiomyocytes were exposed to 4 hours of ischemia and 16 hours of reperfusion, and then cell
viability, apoptosis, glucose uptake, ATP levels and cytosolic Ca2+ concentration were determined, and
O-GlcNAc levels were assessed by Western blotting. Salidroside (80 M) was added 24 hours before
ischemia/reperfusion was induced. Treatment with salidroside markedly improved cell viability from
64.7+/-4.5% to 85.8+/-3.1%, decreased LDH release from 38.5+/-2.1% to 21.2+/-1.7%, reduced cell
apoptosis from 27.2+/-3.2% to 12.2+/-1.9%, significantly improved cardiomyocytes glucose uptake
by 1.7-fold and increased O-GlcNAc levels by 1.6-fold, as well as reducing cytosolic Ca2+ concentration
compared to untreated cells following ischemia/reperfusion. Furthermore, the improved cell survival
and the increase in O-GlcNAc with salidroside were attenuated by alloxan, an inhibitor of O-GlcNAc
transferase. These results suggested that salidroside significantly enhances glucose uptake and
increases protein O-GlcNAc levels and this is associated with decreased cardiomyocytes injury following
ischemia/reperfusion.

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Zhang et al. (2009): The study was aimed to investigate the cardioprotective role of salidroside and
the underlying mechanisms in hypoxia-induced cardiomyocyte death. Cardiomyocytes pretreated with
or without salidroside for 24 hours were exposed to hypoxic condition for 6 hours and then cell
viability, necrosis, apoptosis, the expressions of hypoxia inducible factor (HIF)-1 and VEGF were
investigated. Pre-treatment with salidroside markedly attenuated hypoxia-induced cell viability loss,
cell necrosis and apoptosis in a dose-dependent manner. Mechanistically, pre-treatment with
salidroside up-regulated the HIF-1 protein expression and induced its translocation. Moreover, the
level of VEGF, a downstream target of HIF, was significantly increased in parallel with the level of HIF1 following pre-treatment with salidroside. However,
2-methoxyestradiol , a HIF-1 inhibitor, attenuated the protection of salidroside and blocked the
increase of HIF-1 and VEGF. These data indicated that salidroside has protective effect against
hypoxia-induced cardiomyocytes necrosis and apoptosis by increasing HIF-1 expression and
subsequently up regulating VEGF levels.
Zhong et al. (2010): The cardioprotective effects of salidroside, isolated from Rhodiola rosea L, on
oxygen-glucose deprivation (OGD)-induced cardiomyocyte death and ischemic injury evoked by acute
myocardial infarction (AMI) was investigated in rats. Pre-treatment with salidroside notably
ameliorated cell viability losses in a dose-dependent manner and in parallel it alleviated morphologic
injury detected by electron microscopy. Mechanistically, diminished OGD-induced cardiomyocyte
apoptosis was shown in salidroside-pre-treated cardiomyocytes, in accordance with minimal ROS burst.
Moreover, salidroside markedly upregulated the Bcl-2/Bax ratio and preserved mitochondrial
transmembrane potential. Salidroside administration also inhibited myocardial apoptosis in AMI rats by
increasing phosphorylation of AKT and decreasing activation of caspase-3. These findings suggest that
salidroside reduced ischemia-mediated myocardial damage.
Effects on the blood system:
Qian et al. (2011): This study attempted to examine the potential erythropoiesis-stimulating and antioxidative effect of salidroside in TF-1 erythroblasts. The erythropoiesis-promoting effect was
determined by treating human TF-1 cells with salidroside in the presence and absence of erythropoietin
(EPO) through the measurement of the expression of a series of erythroid markers such as glycophorin
A (GPA), transferrin receptor (CD71) and hemoglobin (Hb). The potential protective effect of
salidroside against H2O2-induced apoptosis and its underlying mechanism in TF-1 erythroblasts were
examined by flow cytometry and Western blot analysis. Salidroside promotes erythropoiesis in the
EPO-treated cells and it also reduces the number of apoptotic cells in TF-1 erythroblasts after H2O2
treatment probably through the up regulation of protective proteins thioredoxin-1 and glutathione
peroxidase-1.
Effects on metabolism:
Kobayashi et al. (2008): As a methanol extract of the rhizome of Rhodiola rosea inhibits the activity of
lipase in isolated mouse plasma in vitro and in the mouse gastrointestinal tube in vivo, the active
components in this plant were investigated. After fractionation and separation processes, rhodionin and
rhodiosin were isolated as active ingredients. Their IC50 values were 0.093 mM and 0.133 mM in vitro,
respectively. Both compounds significantly suppressed the elevation of the postprandial blood
triglyceride level, e.g., by 45.6% (150 mg/kg, 60 minutes after oral administration) and 57.6%
(200 mg/kg, 180 minutes after oral administration), respectively.
Li et al. (2008): The metabolic effects of salidroside on skeletal muscle cells were investigated.
Salidroside dose-dependently stimulated glucose uptake in differentiated L6 rat myoblast cells.
Inhibition of AMP-activated protein kinase (AMPK) by pre-treating the cells with compound C
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(= dorsomorphin) potently reduced salidroside-stimulated glucose uptake, while inhibition of

phosphatidylinositol 3-kinase (PI3K) by wortmannin exhibited no significant inhibitory effect on
salidroside-mediated glucose transport activation. Western blotting analyses revealed that salidroside
increased the phosphorylation level of AMPK and acetyl-CoA carboxylase (ACC). In addition, salidroside
enhanced insulin-mediated AKT activation and glucose uptake, and such enhancement can be
specifically inhibited by compound C.
Effects on hepatic tissue:
Ouyang et al. (2010, only abstract available): This study aimed to investigate whether salidroside can
induce differentiation of rat mesenchymal stem cells (rMSCs) towards hepatocytes in vitro and the
mechanism of hepatic differentiation of rMSCs. rMSCs were subject to hepatic differentiation. One, two
and 3 weeks later, the expression of -fetoprotein (AFP) and albumin (ALB), cytochrome P450
(CYP450)-dependent activity and inducibility, cellular uptake of low density lipoprotein (LDL) and urea
synthesis were assessed and the hepatic differentiation of rMSCs was evaluated. In order to unravel
the mechanism of hepatic differentiation of rMSCs in vitro, inhibitors of ERK1/2, PI3K and p38 were
applied. When the process of hepatic differentiation was completed, special proteins of hepatic
differentiation were detected and blocking of inhibitors was evaluated. Salidroside significantly induced
the differentiation of rMSCs towards hepatocytes. Differentiated rMSCs have typical functional hepatic
characteristics. The results also showed that the ERK1/2 and PI3K signalling pathways play important
roles in the regulatory effects of salidroside on hepatic differentiation of rMSCs and are involved in cell
fate determinations, while the p38 signalling pathway does not.
Wu et al. (2009a, only abstract available): The aim was to investigate the protective effect of
salidroside on D - galactosamine/lipopolysaccharide-induced fulminant hepatic failure. Hepatotoxicity
was induced by an intraperitoneal injection of D-galactosamine (700 mg/kg) and lipopolysaccharide
(10 g/kg); salidroside (20, 50 and 100 mg/kg) was administered intraperitoneally 1 hour before
induction of hepatotoxicity. Liver injury was assessed biochemically and histologically. Salidroside
attenuated the induced acute increase in serum aspartate aminotransferase and alanine
aminotransferase activities, and levels of tumour necrosis factor-alpha (TNF-) levels and serum NO. It
restored depleted hepatic glutathione, superoxide dismutase, catalase and glutathione peroxidase
activities, decreased MDA levels and considerably reduced histopathological changes. Histopathological,
immunohistochemical and Western blot analyses also demonstrated that salidroside could reduce the
appearance of necrotic regions and expression of caspase-3 and HIF-1 in liver tissue. The authors
conclude that salidroside protected liver tissue from the oxidative stress elicited by D-galactosamine
and lipopolysaccharide. The hepatoprotective mechanism of salidroside appears to be related to
antioxidant activity and inhibition of HIF-1 .
Wu et al. (2008): The protective effect of salidroside was investigated in the acetaminophen (APAP)induced hepatic toxicity mouse model in comparison to N-acetylcysteine (NAC). Drug-induced
hepatotoxicity was induced by an intraperitoneal injection of 300 mg/kg (sub-lethal dose) of APAP.
Salidroside was given orally to mice at a dose of 50 or 100 mg/kg 2 hours before the APAP
administration in parallel with NAC. Mice were sacrificed 12 hours after the APAP injection to determine
aspartate aminotransferase (AST), alanine aminotransferase (ALT), and TNF- levels in serum and
glutathione (GSH) depletion, MDA accumulation, and caspase-3 expression in liver tissues. Salidroside
significantly protected APAP-induced hepatotoxicity, as salidroside improved mouse survival rates
better than NAC against a lethal dose of APAP and significantly blocked not only APAP-induced
increases of AST, ALT, and TNF- but also APAP-induced GSH depletion and MDA accumulation.
Histopathological and immunohistochemical analyses also demonstrated that salidroside could reduce
the appearance of necrosis regions as well as caspase-3 and HIF-1 expression in liver tissue. The

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results indicate that salidroside protected liver tissue from the APAP-induced oxidative damage via
preventing or alleviating intracellular GSH depletion and oxidation damage.
Effects on cancer cells:
Hu et al. (2010): To investigate the cytotoxic effects of salidroside on breast cancer cells and in order
to reveal possible ER-related differences in response to salidroside, MDA-MB-231 cells and MCF-7 cells
(estrogen receptor-positive) were used as models to study possible molecular mechanisms. The effects
of salidroside on cell growth characteristics, such as proliferation, cell cycle duration, and apoptosis,
and on the expression of apoptosis-related molecules were evaluated. The results demonstrated that
salidroside in concentration between 5 M and 80 m dose-dependently induces cell-cycle arrest and
apoptosis in human breast cancer cells.
Hu et al. (2010a): The study focused on evaluating the effects of salidroside on the proliferation of
various human cancer cell lines derived from different tissues, and further investigating its possible
molecular mechanisms. Cell viability assay and [3H] thymidine incorporation were used to evaluate the
cytotoxic effects of salidroside on cancer cell lines, and flow cytometry analysed the change of cell
cycle distribution induced by salidroside. Western immunoblotting further studied the expression
changes of cyclins (cyclin D1 and cyclin B1), cyclin-dependent kinases (CDK4 and Cdc2), and cyclindependent kinase inhibitors (p21(Cip1) and p27(Kip1)). The results showed that salidroside in
concentration between 1 g/ml and 32 g/ml dose-dependently inhibited the growth of various human
cancer cell lines in concentration- and time-dependent manners, and the sensitivity to salidroside was
different in those cancer cell lines. Salidroside could cause G1-phase or G2-phase arrest in different
cancer cell lines, meanwhile, salidroside resulted in a decrease of CDK4, cyclin D1, cyclin B1 and Cdc2,
and upregulated the levels of p27(Kip1) and p21(Cip1). Taken together, salidroside could inhibit the
growth of cancer cells by modulating CDK4-cyclin D1 pathway for G1-phase arrest and/or modulating
the Cdc2-cyclin B1 pathway for G2-phase arrest.
Anti-bacterial activity:
Ming et al. (2005): Bioactivity-guided fractionation of a 95% ethanol extract from the stems of
Rhodiola rosea led to the isolation of 5 compounds: gossypetin-7-O-L-rhamnopyranoside (1),
rhodioflavonoside (2), gallic acid (3), trans-p-hydroxycinnamic acid (4) and p-tyrosol (5). Compounds
1 and 2 were evaluated for their antibacterial and antiprostate cancer cell activities. Compounds 1 and
2 exhibited activity against Staphylococcus aureus with minimum inhibitory concentrations of 50 g/ml
and 100 g/ml, respectively. Cytotoxicity studies of 1 and 2 also displayed activity against the prostate
cancer cell line with IC50 values of 50 g/ml and 80 g/ml, respectively.
Other effects:
Yin et al. (2009): This study aimed to investigate the inhibitory effect of salidroside on high glucoseinduced mesangial cell proliferation and its possible mechanism. Salidroside (in concentrations from 1
to approximately 100 M) dose-dependently inhibited high glucose-induced mesangial cell early
proliferation. Exposure of mesangial cells to high glucose for 24 hours significantly induced ROS
accumulation, ERK1/2 phosphorylation, and p27 (Kip1) expression, and these changes were
dramatically inhibited by salidroside in a dose-dependent manner. High glucose-promoted TGF- 1
secretion was also significantly attenuated by treatment of mesangial cells with salidroside.
Wang et al. (2009a): The aim of this study was to investigate the antiviral effects of salidroside. The
antiviral effects of salidroside against coxsackievirus B3 (CVB3) were determined in vitro and in vivo.
The effect of salidroside on the mRNA expression of some important cytokines was measured in hearts
of infected BALB/c mice by RT-PCR. Salidroside exhibited obvious antiviral effects both in in vitro
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concentrations of 80 and 120 mg/l) and in vivo (concentrations between 20 and 80 mg/kg body
weight) experiments. Salidroside was found to modulate the mRNA expression of interferon-gamma
(IFN-), interleukin-10 (IL-10), TNF-, and interleukin-2 (IL-2).
Flavonoids: effects on neuraminidase
Jeong et al. (2009): The flavonols kaempferol, herbacetin, rhodiolinin, rhodionin and rhodiosin were
isolated from Rhodiola rosea. The compounds showed neuraminidase inhibitory activities with IC50
values ranging from 1.4 to 56.9 M. The in vitro anti-influenza virus activities were evaluated using 2
influenza viral strains, H1N1 (A/PR/8/34) and H9N2 (A/Chicken/Korea/MS96/96), testing their ability
to reduce virus-induced cytopathic effect (CPE) in MDCK cells. The activity of these compounds ranged
from 30.2 to 81.9 M against H1N1- and 18.5 to 49.6 M against H9N2-induced CPE. Activity
depended on the position and number of hydroxy groups on the flavonoids backbone.

Pharmacological data from combinations:

Panossian et al. (2009): Experiments were carried out with BALB/c mice taking ADAPT-232 forte, a
fixed combination of extracts of Eleutherococcus senticosus, Schisandra chinensis and Rhodiola rosea
(extract SHR-5), characterised for the content of active markers eleutherosides, schisandrins,
salidroside, tyrosol and rosavin and in doses of about 30, 90 and 180 mg/kg for 7 consecutive days
followed by forced swimming test to exhaustion. ADAPT-232 forte strongly augments endurance of
mice, increasing the time taken to exhaustion in a dose-dependent manner from 3.0+/-0.5 to 21.1+/1.7 min, approximately seven fold. Serum Hsp72 was measured by EIA both in normal and stressful
conditions before and after the swimming test. Repeated administration of adaptogen dose
dependently increases basal level of Hsp72 in serum of mice from 0.8-1.5 to 5.5-6.3 pg/ml. This effect
is even stronger than the effect of stress, including both physical (swimming) and emotional impacts:
3.2+/-1.2 pg/ml. The cumulative effect of stress and adaptogen was clearly observed in groups of
animals treated with adaptogen after swimming to exhaustion, when serum Hsp72 increased to
15.1+/-1 pg/ml and remained at almost the same level during the 7 days. The authors conclude that
adaptogens induce increase of serum Hsp72, regarded as a defence response to stress, and increase
tolerance to stress (in the model combination of physical and emotional stresses). It can be suggested
that increased tolerance to stress induced by adaptogen is associated with its stimulation of expression
of Hsp70 and particularly with Hsp72 production and release into systemic circulation, which is known
as a mediator of stress response involved in reparation of proteins during physical load.
Panossian et al. (2011) found that adaptogens like the combination ADAPT-232 (a fixed combination
of extracts from Eleutherococcus, Schisandra and Rhodiola) stimulate the expression of the
neuropeptide Y in neuroglia cells.

3.2. Overview of available pharmacokinetic data regarding the herbal

substance(s), herbal preparation(s) and relevant constituents thereof
Panossian et al. (2010) found that in rats the bioavailablity of rhodioloside was high after oral
administration (75-90%) compared to that of rosavin (20-26%). After intravenous application,
rhodioloside was 1 hour after administration no longer detectable in the plasma. After multiple single
doses (50 mg/kg on 5 consecutive days), the maximum concentration of rhodioloside in the plasma
was reached 1-1.5 hours after the administration of the herbal preparation SHR-5. After 5 hours, the
blood level fell below the limit of detection.
Hellum et al. (2010) investigated 6 clones of Rhodiola rosea from different areas in Norway for their in
vitro inhibitory potential on CYP3A4-mediated metabolism and P-gp efflux transport activity. Extracts
were prepared using ethanol 96% as a primary extraction solvent, the dry residue was re-dissolved in
ethanol 50%, the supernatant was used for the experiments. C-DNA baculovirus expressed CYP3A4
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and Caco-2 cells were used for inhibitory assays, and as positive control inhibitors ketoconazole and
verapamil were applied, respectively. Scintillation counting was used to quantify the transport of [3H]digoxin in Caco-2 cells. All clones showed potent inhibition of CYP3A4 and P-gp activities, with IC50
values ranging from 1.7 to 3.1 g/ml and from 16.7 to 51.7 g/ml, respectively. The concentration of
presumed biologically active constituents in the different clones varied considerably, but this variation
was not related to the clones' inhibitory potential on CYP3A4 or P-gp activities.
Panossian et al. (2009a) investigated whether Rhodiola rosea SHR-5 extract (DER 2.5-5:1, first
extraction solvent ethanol 70%, second extraction solvent water) interacts with warfarin and
theophylline when administered concomitantly. The extract used in the theophylline study contained
2.7% rhodioloside (= salidroside), 6% rosavin and 0.8% tyrosol, while that for the warfarin study
contained 2.5% rhodioloside, 3.9% rosavin and 0.8% tyrosol. The Wistar rats received orally 50 mg/kg
daily for 3 days. After the final dose the animals received a single dose of aminophylline or warfarin.
The animals in the placebo group received water by oral gavage. All relevant pharmacokinetic
parameters remained unchanged. The authors conclude that the concomitant treatment of rats with
theophylline and SHR-5 did not give rise to significant effects on the pharmacokinetics of theophylline.
Simultaneous administration of SHR-5 and warfarin did not alter significantly the pharmacokinetics or
the anticoagulant activity of warfarin.

3.3. Overview of available toxicological data regarding the herbal

substance(s)/herbal preparation(s) and constituents thereof
Herbal preparations:
No data published.
The Swedish Herbal Institute supplied unpublished information (Burgos & Hancke 1991) regarding
tests on the subchronic toxicity of the herbal preparation SHR-5. The herbal preparation was
administered orally to rats for 90 days in a dose range from 1.0-3.4 g/kg. The study medication did
not change the development of the body weight, behaviour and appearance of the test animals.
Further parameters were not investigated.
In a subsequent study Hancke & Burgos (1992, unpublished) investigated the same herbal preparation
in dosages of 0.142 1.43 g/kg in piglets for 90 days. No changes in haematological parameters were
observed, also glucose, triglyceride, creatinine kinase and urea levels as well as protein concentrations
remained unchanged. An increase in hepatic transaminases was attributed to the increasing hepatic
enzyme activity during maturation of the piglets.
A possible CNS toxicity was investigated by Hancke et al. (1993, unpublished). Mice received
100 mg/kg or 500 mg/kg of the herbal preparation SHR-5 intraperitoneally. The influence of the study
medication was rated according to the Irwin Method, which utilises several behavioural, neurological
and autonomic parameters as well as mortality. No signs of toxicity were observed.
Unpublished tests on the cytotoxicity (inhibitory cell growth with L1210 cells and colony-forming
efficiency with V79 cells) of the powdered underground organs (Bjellin et al. 1988) revealed a very low
cytotoxic potential.
The considerably high dosages which were used in some of the pharmacological tests (e.g. Chen et al.
2008a, Qu et al. 2009) indicate that dosages up to 6 g herbal preparation per kg body weight per day
were well tolerated in rats.
In a Public Assessment Report of the UK Medicines and Healthcare products Regulatory Agency, it is
stated that an extract prepared with ethanol 68% v/v did not reveal any mutagenic effect up to a
cytotoxic concentration of 3,160 g/plate in an Ames test, with and without metabolic activation.
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Isolated constituents:
Zhu et al. (2010, only abstract available) evaluated the potential genotoxicity of salidroside by using
the standard battery of tests (i.e. bacterial reverse mutation assay, chromosomal aberrations assay,
and mouse micronucleus assay). The results showed that salidroside was not genotoxic under the
conditions of the reverse mutation assay, chromosomal aberrations assay and mouse micronucleus
assay conditions. The anticipated clinical dose seems to be smaller compared to doses administered in
the genotoxicity assays.

3.4. Overall conclusions on non-clinical data

A high number of pharmacological investigations on herbal preparations and isolated constituents from
the underground parts of Rhodiola rosea are published. However, in many of the experiments
supraphysiological concentrations or dosages far exceeding the proposed dose in humans were applied.
Therefore, the relevance of the results of such studies must be questioned.
Some of the studies (e.g. in models investigating anti-fatigue effects, stress-protective effects, effects
on the nervous system) support the medicinal use of herbal preparations from Rhodiola rosea as an
adaptogen and make the use in this indication plausible. Results from studies performed with isolated
constituents suggest that the phenylethanoids like salidroside contribute to these effects.
Only limited data is published on toxicity of preparations of Rhodiola. In vitro data concerning
metabolic and transporter interactions indicated moderate inhibitory effects by Rhodiola extracts,
whereas in vivo animal studies were negative. No final conclusion can be drawn at the moment.

4. Clinical Data
4.1. Clinical Pharmacology
4.1.1. Overview of pharmacodynamic data regarding the herbal
substance(s)/preparation(s) including data on relevant constituents
The purpose of a study by Parisi et al. (2010, only abstract available) was to investigate the effects on
physical performance as well as on the redox status of a chronic Rhodiola rosea supplementation in a
group of competitive athletes during endurance exercise. Following a chronic supplementation with
Rhodiola rosea for 4 weeks (no details on the type of the herbal preparation available), 14 trained male
athletes underwent a cardio-pulmonary exhaustion test, additionally blood samples were evaluated for
antioxidant status and other biochemical parameters. These data were compared with those coming
from the same athletes after an intake of placebo. The supplementation did not affect the maximum
heart rate, Borg Scale level (measure for perceived exertion), peak oxygen uptake, blood antioxidant
status, inflammatory parameters and blood glucose level. The level of plasma free fatty acids was
significantly reduced. Blood lactate and plasma creatine kinase levels were found to be significantly
lower (P<0.05) in treated subjects when compared to the placebo treated group.
Evdokimov (2009, only abstract available, original article in Russian language): Seven-hour continuous
physical loading test (bicycle ergometry) was used to assess the effects of a cryopowder of Rhodiola
rosae on the human cardiorespiratory system. Comparing with the control, the preparation facilitated
activation of the energy-supplying mechanisms in human organism during physical work. In addition, it
increased the efficiency of the cardiovascular and respiration systems and prevented fatigue growth.
Skarpanska-Steijnborn et al. (2009) investigated the effect of Rhodiola rosea supplementation on the
balance of oxidants and antioxidants in the serum and erythrocytes of competitive rowers. The study
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medication contained 100 mg of a Rhodiola rosea concentrate (no more details available) and 5 mg
zinc and was given twice daily for 4 weeks. This double-blinded study included 22 members of the
Polish Rowing Team, who were participating in a preparatory camp. At the beginning and end of the
study, participants performed a 2,000-m maximum test on a rowing ergometer. Blood samples were
taken from the antecubital vein before each exercise test, 1 minute after completing the test, and after
a 24-hour restitution period. The following redox parameters were assessed in erythrocytes:
superoxide dismutase activity, glutathione peroxidase activity, and thiobarbituric-acid-reactive
substances concentrations. In addition, creatine kinase activity and total antioxidant capacity were
measured in plasma samples, lactate levels were determined in capillary blood samples, and uric acid
concentrations were measured in serum. After supplementation, the total plasma antioxidant capacity
was significantly higher (p = 0.0002) in the supplemented group than in the placebo group, and
superoxide dismutase activity in erythrocytes directly after and 24 hours after the ergometry was
significantly (p = 0.0461) lower in athletes receiving Rhodiola rosea concentrate than in the placebo
group.
The purpose of the investigation by Walker et al. (2007) was to examine the effect of Rhodiola rosea
ingestion on human skeletal muscle phopshocreatine recovery after exhaustive exercise. The study
medication was 1500 mg Rhodiola rosea standardised to 3% rosavins (no more details on the herbal
preparation available), divided into 3 doses. Twelve resistance-trained men (19 to 39 years of age)
completed incremental forearm wrist flexion exercise to volitional fatigue, once after ingesting Rhodiola
rosea for 4 days, and once after ingesting an equivalent placebo dose. During exercise and recovery
from exercise, muscle phosphates were examined using

31

P nuclear magnetic resonance spectroscopy.

In summary, there were no significant differences between groups for any of the parameters
measured. The authors conclude that Rhodiola rosea ingestion does not improve ATP turnover during
or immediately after exercise.
Colson et al. (2005, only abstract available) examined the effects of a fixed combination of Cordyceps
sinensis and Rhodiola rosea (no details on the type of herbal preparation and on posology available) on
circulatory dynamics, specifically muscle tissue oxygen saturation in male subjects during maximal
exercise. This study followed a double-blind, randomised, placebo-treatment, pre-post test design.
Capsules were administered to 8 subjects, who were randomly assigned to one of 2 groups. All
subjects performed 2 exercise stress tests to volitional fatigue on a cycle load ergometer. There were
no significant (p </= 0.05) differences between or within the treatment or control group. The
combination did not affect the muscle tissue oxygen saturation.
In a double-blind, placebo-controlled study, Abidov et al. (2004) studied the effect of 30 mg Rhodiola
rosea extract (no details available) twice daily for 30 days before and 6 days after exhausting physical
exercise on the level of C-reactive protein and creatinine kinase. The study medication reduced the
levels of C-reactive protein significantly compared to both placebo and control group.
Wing et al. (2003) investigated the effects of a 7-day supplementation with 447 mg Rhodiola rosea
4 times daily (no details on the herbal preparation) on hypoxia and oxidative stress at a simulated
altitude of 4600 m. Fifteen volunteers (ages 20-33) received 3 separate 60-minute hypoxic exposures
by breathing 13.6% oxygen at an ambient barometric pressure of 633 mm Hg (simulating the partial
pressure of oxygen at 4600 m elevation). Each subject received, in random order, treatments of a
7-day supply of placebo, Rhodiola rosea, and an acute dose of stabilised oxygen dissolved in water.
The supplementation did not have a significant effect on blood oxygenation after 60 minutes of
sedentary hypoxic exposure. Hypoxia-induced oxidative stress was observed in the control group only.
Supplementation appeared not to increase oxidative stress and may decrease free radical formation
after hypoxic exposure compared with the control.

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4.1.2. Overview of pharmacokinetic data regarding the herbal

substance(s)/preparation(s) including data on relevant constituents
16 volunteers received in a single dose 288 mg of the herbal preparation SHR-5 containing 7.26 mg
rhodioloside and 8.4 mg rosavin (Panossian et al. 2010). Rhodioloside was detectable immediately
after oral administration while rosavin could not be detected in the first hour. Maximum concentrations
were reached 2 hours after oral administration (Cmax rhodioloside 948 ng/ml, rosavin 446 ng/ml). After
8 hours, the concentration had fallen below the detection limit.

4.2. Clinical Efficacy

4.2.1. Dose response studies
Darbinyan et al. (2007): see details in 4.2.2.
Shevtsov et al. (2003): see details in 4.2.2.

4.2.2. Clinical studies (case studies and clinical trials)

Clinical trials: Indication mental performance, fatigue
Single preparations:
Olsson et al. (2009): The aim of the study was to assess the efficacy of the extract SHR-5 (DER 2.55:1, first extraction solvent ethanol 70%, second extraction solvent water) in the treatment of
individuals suffering from stress-related fatigue. The phase III clinical trial took the form of a
randomised, double-blind, placebo-controlled study with parallel groups. Participants, males and
females aged between 20 and 55 years, were selected according to the Swedish National Board of
Health and Welfare diagnostic criteria for fatigue syndrome. A total of 60 individuals were randomised
into 2 groups, one of which (N = 30) received 4 tablets daily of SHR-5 extract (576 mg extract/day),
while a second (N = 30) received 4 placebo tablets daily. The effects of the extract with respect to
quality of life (SF-36 questionnaire, a validated scale to assess the quality of life), symptoms of fatigue
(Pines' burnout scale), depression (Montgomery-Asberg depression rating scale - MADRS), attention
(Conners' computerised continuous performance test II - CCPT II), and saliva cortisol response to
awakening were assessed on day 1 and after 28 days of medication. Data were analysed by betweenwithin analyses of variance. Significant post-treatment improvements were observed for both groups
(placebo effect) in Pines' burnout scale, mental health (SF-36), and MADRS and in several CCPT II
indices of attention, namely omissions, commissions and standard error of the reaction time (Hit RT
SE). When the two groups were compared, however, significant effects of the SHR-5 extract in
comparison with the placebo were observed in Pines' burnout scale and the CCPT II indices omissions,
Hit RT SE and variability. Pre- versus post-treatment cortisol responses to awakening stress were
significantly different in the treatment group compared with the control group. No serious side effects
that could be attributed to the extract were reported. It is concluded that repeated administration of
the extract exerts an anti-fatigue effect that increases mental performance, particularly the ability to
concentrate, and decreases cortisol response to awakening stress in burnout patients with fatigue
syndrome.
Schutgens et al. (2009): In a randomised double-blind placebo-controlled study, 30 subjects were
randomly assigned to 3 groups: one group (n = 10) taking placebo pills, one group (n = 10) taking
Rhodiola rosea (144 mg extract SHR-5, DER 2.5-5:1, first extraction solvent ethanol 70%, second
extraction solvent water) pills and one group (n = 10) taking ADAPT-232 supplements (fixed
combination of Eleutherococcus senticosus, Rhodiola rosea (SHR-5 extract, no details on the amount of
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extract per tablet) and Schisandra chinensis). The study medication was given twice daily for 7 days.
All subjects underwent measurements to determine ultra-weak photon emission of the dorsal side of
their hands using a photon-counting device, both before and after a week of taking the supplements.
In addition, the experienced levels of stress and fatigue (tiredness) were evaluated. After 1 week of
supplementation, the Rhodiola group showed a significant decrease (p = 0.027) in photon emission in
comparison with the placebo group. Furthermore, after supplementation, a significant decrease (p =
0.049) concerning the experienced level of fatigue in the Rhodiola group was observed compared with
the placebo group. No significant changes were observed between the ADAPT-232 and the placebo
group.
Darbinyan et al. (2007): The objective of this study was to assess the efficacy and safety of the
standardised extract SHR-5 (DER 2.5-5:1, first extraction solvent ethanol 70%, second extraction
solvent water) in patients suffering from a current episode of mild/moderate depression according to
DSM-IV. The phase III clinical trial was carried out as a randomised double-blind placebo-controlled
study with parallel groups over 6 weeks. The participants were males and females aged 18-70 years.
The severity of the depression was determined by scores gained in Beck Depression Inventory and
Hamilton Rating Scale for Depression (HAMD) questionnaires. Exclusion criteria: previous attempt to
commit suicide, scores on the scales indicating suicidal tendency, total HAMD score above 31,
progressive organic or metabolic brain syndrome, compulsive, schizophrenic or other delusive
disorders. Patients with initial HAMD scores between 21 and 31 were randomised into 3 groups, one of
which (group A: 31 patients) received 2 tablets daily of SHR-5 (340 mg/day), a second (group B: 29
patients) received 2 tablets twice per day of SHR-5 (680 mg/day), and a third (group C: 29 patients)
received 2 placebo tablets daily. The efficacy of SHR-5 extract with respect to depressive complaints
was assessed on days 0 and 42 of the study period from total and specific subgroup HAMD scores. For
individuals in groups A and B, overall depression, together with insomnia, emotional instability and
somatization, but not self-esteem, improved significantly following medication, whilst the placebo
group did not show such improvements. In the group A, the HAMD score improved form 24.52 to
15.97, in group B from 23.79 to 16.72, while it remained nearly unchanged in the placebo group
(24.17 to 23.41). No serious side-effects were reported in any of the groups A-C.
No difference in the clinical outcome was observed between the different dosages.
Assessorss comment:
The observation of nearly an absent placebo-effect (expressed by a nearly unchanged HAMD score in
the placebo group) is untypical for clinical trials with depressant patients. Therefore, the significances
documented in the publication remain questionable.

De Bock et al. (2004): The purpose of this study was to investigate the effect of acute and 4-week
Rhodiola rosea extract (no details on DER and extraction solvent, extract contains 3% rosavin and 1%
salidroside) intake on physical capacity, muscle strength, speed of limb movement, reaction time, and
attention in 24 patients. PHASE I: A double blind placebo-controlled randomised study (n= 24) was
performed, consisting of 2 sessions (2 days per session). Day 1: one hour after acute Rhodiola rosea
intake (R, 200-mg Rhodiola rosea extract) or placebo (P, 700 mg starch) speed of limb movement
(plate tapping test), aural and visual reaction time, and the ability to sustain attention (Fepsy Vigilance
test) were assessed. Day 2: Following the same intake procedure as on day 1, maximal isometric
knee-extension torque and endurance exercise capacity were tested. Following a 5-day washout
period, the experimental procedure was repeated, with the treatment regimens being switched
between groups (session 2). PHASE II: A double-blind placebo-controlled study (n = 12) was
performed. Subjects underwent sessions 3 and 4, identical to Phase I, separated by a 4-week R/P
intake, during which subjects ingested 200 mg R/P per day. RESULTS: PHASE I: Compared with
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placebo the acute intake of Rhodiola extract in Phase I increased (p <.05) time to exhaustion from
16.8 +/- 0.7 min to 17.2+/- 0.8 min. Accordingly, VO2peak (p <.05) and VCO2peak (p<.05) increased
during the study medication compared to placebo from 50.9 +/- 1.8 ml/min/kg to 52.9 +/- 2.7
ml/min/kg (VO2peak) and from 60.0 +/- 2.3 ml/min/kg to 63.5+/- 2.7 ml/min/kg (VCO2peak).
Pulmonary ventilation (p =.07) tended to increase more in the verum group compared to placebo (P:
115.9+/- 7.7 l/min; R: 124.8 +/- 7.7 l/min). All other parameters remained unchanged. PHASE II:
Four-week R intake did not alter any of the variables measured. The authors conclude that acute
Rhodiola rosea intake can improve the endurance exercise capacity in young healthy volunteers. This
response was not altered by prior daily 4-week Rhodiola intake.
Shevtsov et al. (2003): A randomised, double-blind, placebo-controlled, parallel-group clinical study
with an extra non-treatment group was performed to measure the effect of a single dose of
standardised SHR-5 (DER 2.5-5:1, first extraction solvent ethanol 70%, second extraction solvent
water) on capacity for mental work against a background of fatigue and stress. Some physiological
parameters, e.g. pulse rate, systolic and diastolic blood pressure, were also measured. The study was
carried out on a highly uniform population comprising 161 cadets aged from 19 to 21 years. Group 1
(41 subjects) received 370 mg extract per day, group 2 (20 subjects) received 555 mg extract per
day. The study showed a pronounced anti-fatigue effect reflected in an anti-fatigue index defined as a
ratio called AFI. The verum groups had AFI mean values of 1.0385 and 1.0195, 2 and 3 capsules
respectively, whilst the figure for the placebo group was 0.9046. This was statistically highly significant
(p < 0.001) for both doses (verum groups), whilst no significant difference between the 2 dosage
groups was observed. There was a possible trend in favour of the lower dose in the psychometric tests.
No such trend was found in the physiological tests. Only one case of hypersalivation in the placebo
group was reported as undesirable effect.
Ha et al. (2002): The aim of the study was to investigate the changes of sleep architecture and blood
oxygen saturation (SaO(2)) during sleep in men living at high altitude, and to investigate the effect of
Rhodiola and acetazolamide on these sleep indexes. Twenty-four men aged 18 to 21 years, who had
stayed at high altitude (5 380 m above sea level) for 1 year, were randomly divided into groups A
(treated with oral Rhodiola, no information on kind of herbal preparation and on posology), B (treated
with oral acetazolamide 0.25 g twice daily) and C (treated with Rhodiola + acetazolamide). Their sleep
architecture and SaO(2) were recorded for 24 days before and after taking the medicines. The authors
conclude that both Rhodiola and acetazolamide were effective in modulating the sleep architecture and
improving the sleep quality in young men living at high altitude, but there was no synergistic effect
between Rhodiola and acetazolamide.
Assessorss comment:
Because of the lack of any information concerning the type of the herbal preparation and the posology,
the findings cannot be taken into consideration.

Darbinyan et al. (2000): The aim of this study was to investigate the effect of repeated low-dose
treatment with a standardised extract SHR-5 (DER 2.5-5:1, first extraction solvent ethanol 70%,
second extraction solvent water) on fatigue during night duty among a group of 56 young, healthy
physicians. The effect was measured as total mental performance calculated as Fatigue Index. The
tests chosen reflect an overall level of mental fatigue, involving complex perceptive and cognitive
cerebral functions, such as associative thinking, short-term memory, calculation and ability of
concentration, and speed of audio-visual perception. These parameters were tested before and after
night duty during 3 periods of 2 weeks each: a) a test period of one Rhodiola/placebo tablet daily, b) a
washout period and c) a third period of one placebo/Rhodiola tablet daily, in a double-blind cross-over
trial. The verum tablets contained 170 mg extract (with approximately 4.5 mg salidroside) and were
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taken once daily. The perceptive and cognitive cerebral functions mentioned above were investigated
using 5 different tests. A statistically significant improvement in these tests was observed in the
treatment group during the first 2 weeks period. No side-effects were reported for either treatment.
These results suggest that Rhodiola can reduce general fatigue under certain stressful conditions.
Spasov et al. (2000a): The objective was to investigate the stimulating and normalising effect of the
adaptogen Rhodiola rosea extract SHR-5 (DER 2.5-5:1, first extraction solvent ethanol 70%, second
extraction solvent water) in 40 students during a stressful examination period. The study was
performed as a double-blind, randomised and placebo-controlled with low repeated dose regime. One
tablet contained 50 mg of the Rhodiola extract, taken twice daily for 20 days. The physical and mental
performance were assessed before and after the period, based on objective as well as on subjective
evaluation. The most significant improvement in the SHR-5 group was seen in physical fitness, mental
fatigue and neuro-motoric tests (p <0.01). The self-assessment of the general well-being was also
significantly (p < 0.05) better in the verum group. No significance was seen in the correction of text
tests or a neuro-muscular tapping test. The authors conclude that the study medication gave
significant results compared to the placebo group but that the dose level probably was suboptimal.
Spasov et al. (2000b): 60 male students (17-18 years of age) were randomised to 3 groups; the
participants in one group received the study medication (660 mg of Rhodiola, no details on the type of
herbal preparation published) for 20 days. The authors observe in the treatment group improvement of
health and well-being, activeness level, mood, and work stimulation as well as reduced signs of
fatigue. No adverse events in the verum group were observed.
Clinical trials in other indications:
Bystritsky et al. (2008): The goal of this pilot study was to evaluate whether Rhodiola rosea is effective
in reducing symptoms of generalised anxiety disorder (GAD). Ten participants (age 34-55 years) with a
DSM-IV diagnosis of GAD were enrolled in this study. Participants received a total daily dose of 340 mg
of Rhodiola rosea extract (no details of the type of the herbal preparation published) for 10 weeks.
Assessments included the Hamilton Anxiety Rating Scale (HARS), the Four-Dimensional Anxiety and
Depression Scale and the Clinical Global Impressions of Severity/Improvement Scale. Individuals
treated with Rhodiola rosea showed significant decreases in mean HARS scores at endpoint (t=3.27,
p=0.01). Adverse events were generally mild or moderate in severity, the most common being
dizziness and dry mouth.
Reviews:
The current knowledge is summarised in the following review articles: Iovieno et al. (2010), Panossian
et al. (2010), Panossian & Wikman (2009), Walker & Robergs (2006), Tharakan & Manyam (2006),
Panossian & Wagner (2005).
Opinions:
Based on the published clinical data, Zubeldia et al. (2010) propose Rhodiola rosea as a viable
alternative treatment for the symptoms of short-term hypothyroidism in patients with differentiated
thyroid cancer who require hormone withdrawal.
Meta-analyses:
Hung et al. (2011): Eleven RCTs met the inclusion criteria, all were placebo-controlled. (Shevtsov et al.
2003, DeBock et al. 2004, Abodiv et al. 2004, Olsson et al. 2009, Spasov et al. 2000a, Spasoc et al.
2000b, Darbinyan 2007, Darbinyan 2000, Walker 2007, Schutgens 2009, Wing 2003). Six trials
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investigated the effects of Rhodiola rosea on physical performance, four on mental performance, and
two in patients diagnosed with mental health condition. The methodological quality of most trials was
moderate or good. Only a few mild adverse events were reported. Rhodiola rosea may have beneficial
effects on physical performance, mental performance and certain mental health conditions. There is,
however, a lack of independent replications of the single different studies. Five of the 11 RCTs reached
more than 3 points on the Jadad score (i.e., good quality). More research seems warranted.
Blomkvist et al. (2009): With a focus on the statistical methods, the authors found considerable
shortcomings in all but one of the studies that claim significant improvement from roseroot extract.
Overall, the study designs have not been well explained. Experimental results have been confused and
appear to be in some cases incorrect. Some of the conclusions are based on selected results and
contradicting data have not been adequately taken into account. For example, it is criticised that
Darbinyan et al. (2000) claimed significant results while insignificant results are explained away with
unfounded assumptions. In the study of Darbinyan et al. (2007), irrelevant tests and an inappropriate
statistical comparison were used. Bystritsky et al. (2008) and Fintelmann & Gruenwald (2007) claimed
an effect but did not use a placebo control. In the article of Shevtsov et al. (2003) misprints and mixups occur. The authors find it alarming that poorly conceived and performed studies have been
published apparently without adequate scientific and editorial scrutiny. The authors conclude that the
currently available evidence for the claimed effects is insufficient and that the effect of Rhodiola rosea
is in need of further investigation before therapeutic claims can be made.
Sarris (2007): This paper reports a critical review of 27 herbal medicines and formulas in treating a
broad range of psychiatric disorders (in addition to anxiety and depression), including obsessivecompulsive, seasonal affective, bipolar depressive, psychotic, phobic and somatoform disorders. The
author states that Rhodiola rosea might be a promising herb for the treatment of depression. However,
most studies are published in the Russian language and could not be located by the author.
Combination products:
Aslanyan et al. (2010) investigated the fixed combination ADAPT-232 containing Rhodiola rosea L.,
Schisandra chinensis (Turcz.) Baill., and Eleutherococcus senticosus Maxim. The subjects in the
ADAPT-232 received a single dose of the study medication. Quickly after intake (2 hours after verum
was taken) improved attention and increased speed and accuracy during stressful cognitive tasks, in
comparison to placebo was observed. There was also a tendency of ADAPT-232 to reduce percentage
of errors, which means better accuracy, quality of the work, and degree of care in the volunteers under
stressful conditions. No serious side effects were reported, although a few minor adverse events, such
as sleepiness and cold extremities, were observed in both treatment groups.
Dieamant et al. (2008, only abstract available): A double-blind comparative study was conducted on
124 volunteers with sensitive skin, who were selected by their reactivity to stinging test. Two
randomised groups of 62 each received twice daily for 28 consecutive days either a formulation
containing 1% of a combination of Rhodiola extract (no details on the type of the extract and on
posology) and L-carnosine or placebo. One perceptibility questionnaire was completed at the onset and
at the end of the treatment to evaluate the subjective response to test product. Additionally, in vitro
studies were performed to investigate potential neuroimmunomodulatory mechanisms. The verum
treatment produced in vivo protective effects in skin barrier function and a positive subjective response
of sensitive skin volunteers. In vitro treatment promoted the release of proopiomelanocortin peptides
and restored to normal the increased levels of neuropeptides and cytokines produced by keratinocytes
exposed to ultraviolet radiation. Clinical effectiveness was measured by reduction of transepidermal
water loss, positive perceptions of improvements in skin dryness and skin comfort sensation, and
reduction of discomfort sensation after stinging test. The protective effect of the combination in skin

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barrier function and the positive response produced in human subjects with sensitive skin could be
partially explained by the in vitro results showing a significant increase in opioid peptides release, an
inhibitory effect on neuropeptide production and modulation of cytokines production by keratinocytes
under ultraviolet stress.
Fintelmann & Gruenwald (2007) studied a food supplement containing 200 mg Rhodiola extract (no
more details available), magnesium, vitamin E, vitamin B6, folic acid and vitamin B12 in a 12-week
drug monitoring study. The study was neither blinded nor placebo-controlled. The authors state that in
the 120 patients a statistically highly significant improvement in physical and cognitive deficiencies was
observed. No adverse events occurred during the course of the study.

4.2.3. Clinical studies in special populations (e.g. elderly and children)

No data published.

4.3. Overall conclusions on clinical pharmacology and efficacy

The results from trials on clinical pharmacology are contradictory. The number of clinical trials for
clinical efficacy is limited, also the number of included subjects.
Meta-analyses of these clinical trials found considerable shortcomings and deficiencies. Therefore, it
can be concluded that there is not sufficient evidence for a clinical efficacy of herbal preparations of
Rhodiola rosea for the treatment of symptoms of fatigue or mental weakness. Therefore wellestablished use cannot be supported in the monograph.
However, the data support the plausibility of the use of traditional herbal medicinal products of
Rhodiola rosea as adaptogens.

5. Clinical Safety/Pharmacovigilance
5.1. Overview of toxicological/safety data from clinical trials in humans
In the study of Olsson et al. (2009) no serious side effects that could be attributed to the extract (DER
2.5-5:1, first extraction solvent ethanol 70%, second extraction solvent water; 567 mg extract/day,
duration of use: 28 days) were reported. No data on non-serious side effects are mentioned in the
publication.
The same safety profile was observed in the study of Darbinyan et al. (2007) in a posology of 340 mg
or 680 mg per day over 6 weeks.
In the study of Bystritsky et al. (2008), dizziness and dry mouth were observed after oral
administration of 340 mg of extract daily (no details on the type of extract published).
In the SmPC of the registered traditional herbal medicinal products, also hypersensitivity reactions and
hypoglycaemia are mentioned.

5.2. Patient exposure

No data available.

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5.3. Adverse events and serious adverse events and deaths

No additional data compared to those from clinical trials are available.
Assessors comment: The few reported adverse events may also be caused by the underlying disease.
Therefore they should not be included in the monograph.

5.4. Laboratory findings

No data available.

5.5. Safety in special populations and situations

Children and adolescents:
Although the use of registered traditional herbal medicinal products containing Rhodiola extract is
permitted in adolescents, this age group cannot be considered in the monograph since no safety data
from clinical trials in adolescents are available.
Interactions:
Neither clinical data nor case reports on interactions are published.
Pregnancy and lactation:
No data published. The safety during pregnancy and lactation has not been established. In the absence
of data the use during pregnancy and lactation is not recommended.
Overdose:
There are no case reports published.
Effects on ability to drive or operate machinery
No studies on the effect on the ability to drive and use machines have been published.

5.6. Overall conclusions on clinical safety

Although experimental data on genotoxicity are missing the published literature does not give reasons
for safety concerns. The reported adverse events are mild. The use in children and adolescents as well
as during pregnancy and lactation cannot be recommended. Based on the published data it can be
concluded that traditional herbal medicinal products containing Rhodiola rosea are not harmful when
used in the specified conditions.

6. Overall conclusions
Herbal preparations of the underground organs of Rhodiola rosea are used in traditional medicine since
centuries. In the former USSR (including countries which now belong to the European Union like
Estonia, Lithuania and Latvia), a liquid extract (DER 1:1, extraction solvent ethanol 40%) was in
medicinal use and in 1975 it was accepted as a so called Temporary Pharmacopoeia Article which
allowed a large-scale production. Dry extracts (DER 1.5-5:1), extraction solvent ethanol 67-70% v/v,
are in medicinal use within the European Union since 1987. Therefore, the criteria for 30 years of
medicinal use as defined for traditional herbal medicinal products in Directive 2004/24/EC are fulfilled.
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The traditional use as an adaptogen for temporary relief of symptoms of stress such as fatigue and
sensation of weakness is appropriate for traditional herbal medicinal products.
The published clinical trials exhibit considerable deficiencies in their quality. Therefore well-established
use cannot be accepted.
The long-standing use as well as the outcome of the clinical trials support the plausibility of the use of
the mentioned herbal preparation in the proposed indication.
The clinical trials as well as the traditional use do not give reasons for special safety concerns. No
serious adverse events are reported. The in vitro observed inhibition of CYP3A4 and P-glycoprotein was
not confirmed in vivo. Additionally, no case reports on interactions are published. Because of the
limited duration of use of 2 weeks, the in vitro data seem to be of minor clinical relevance.
Therefore the overall benefit/risk balance is positive.
Due to the missing published data on genotoxicity, the development of a Community list entry cannot
be supported.

Annex
List of references

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