pharmaceuticals
Article
Preliminary Biological Activity Screening of Plectranthus spp.
Extracts for the Search of Anticancer Lead Molecules
Epole Ntungwe 1,2 , Eva María Domínguez-Martín 1,2 , Catarina Teodósio 1 , Silvia Teixidó-Trujillo 3 ,
Natalia Armas Capote 3 , Lucilia Saraiva 4 , Ana María Díaz-Lanza 2 , Noélia Duarte 5 and Patrícia Rijo 1,5, *
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Citation: Ntungwe, E.;
Domínguez-Martín, E.M.; Teodósio,
C.; Teixidó-Trujillo, S.; Armas Capote,
N.; Saraiva, L.; Díaz-Lanza, A.M.;
Duarte, N.; Rijo, P. Preliminary
Biological Activity Screening of
Plectranthus spp. Extracts for the
Search of Anticancer Lead Molecules.
Pharmaceuticals 2021, 14, 402. https://
doi.org/10.3390/ph14050402
Academic Editor: Maria Matilde
Soares Duarte Marques
Received: 6 April 2021
Accepted: 20 April 2021
*
CBIOS—Universidade Lusófona Research Center for Biosciences & Health Technologies,
Universidade Lusófona de Humanidades e Tecnologias, Campo Grande 376, 1749-024 Lisboa, Portugal;
ntungweepolengolle@yahoo.com (E.N.); evam.dominguez@uah.es (E.M.D.-M.);
catarina.teodosio@gmail.com (C.T.)
Department of Biomedical Sciences, Faculty of Pharmacy, University of Alcalá de Henares, Ctra. A2,
Km 33.100—Campus Universitario, 28805 Alcalá de Henares, Spain; ana.diaz@uah.es
Centro Atlántico del Medicamento S.A., Avenida Trinidad 61, 7ª Planta, Torre Agustín Arévalo,
38204 La Laguna, Tenerife, Spain; teixido.silvia@gmail.com (S.T.-T.); nataliaarmas@ceamedsa.com (N.A.C.)
LAQV/REQUIMTE, Laboratório de Microbiologia, Departamento de Ciências Biológicas,
Faculdade de Farmácia, Universidade do Porto, Rua de Jorge Viterbo Ferreira n.º 228,
4050-313 Porto, Portugal; lucilia.saraiva@ff.up.pt
Instituto de Investigação do Medicamento (iMed.ULisboa), Faculdade de Farmácia, Universidade de Lisboa,
1649-003 Lisboa, Portugal; mduarte@ff.ulisboa.pt
Correspondence: patricia.rijo@ulusofona.pt
Abstract: Plectranthus species (Lamiaceae) have been employed in traditional medicine and this is
now validated by the presence of bioactive abietane-type diterpenoids. Herein, sixteen Plectranthus
acetonic extracts were prepared by ultrasound-assisted extraction and their biological activity was
screened. The antimicrobial activity of each extract was screened against yeasts, and Gram-positive
and Gram-negative bacteria. The P. hadiensis and P. mutabilis extracts possessed significant activity
against Staphylococcus aureus and Candida albicans (microdilution method). Moreover, all extracts
showed antioxidant activity using the DPPH method, with P. hadiensis and P. mutabilis extracts
having the highest scavenging activities. Selected by the Artemia salina model, P. hadiensis and
P.ciliatus possessed low micromolar anti-proliferative activities in human colon, breast, and lung
cancer cell lines. Furthermore, the most bioactive extract of P. hadiensis leaves and the known
abietane diterpene, 7α-acetoxy-6β-hydroxyroyleanone isolated from this plant, were tested against
the aggressive type triple negative breast cancer (MDA-MB-231S). P. hadiensis extract reduced the
viability of MDA-MB-231S cancer cell line cells, showing an IC50 value of 25.6 µg/mL. The IC50 value
of 7α-acetoxy-6β-hydroxyroyleanone was 5.5 µM (2.15 µg/mL), suggesting that this lead molecule is
a potential starting tool for the development of anti-cancer drugs.
Published: 23 April 2021
Publisher’s Note: MDPI stays neutral
Keywords: Plectranthus; royleanone; 7α-acetoxy-6β-hydroxyroyleanone; ent-abietane; antitumoral
activity; antimicrobial activity; antioxidant
with regard to jurisdictional claims in
published maps and institutional affiliations.
1. Introduction
Copyright: © 2021 by the authors.
Licensee MDPI, Basel, Switzerland.
This article is an open access article
distributed under the terms and
conditions of the Creative Commons
Attribution (CC BY) license (https://
creativecommons.org/licenses/by/
4.0/).
Over the centuries, plants and natural products derived from plants have been the
basis of traditional medicine. Nowadays, plant-based medicines have been playing an
important role in drug discovery and development. They are also widely employed in
various public health practices as they are safe, cost-effective, and possess unique chemical
diversity [1,2]. Cancer remains one of the leading causes of death globally, with approximately 18.1 million new cases and 9.6 million cancer-related deaths in 2018, according to
the World Health Organization [3]. Furthermore, several types of chemotherapies used are
ineffective and generate unwanted adverse side effects [4,5]. Similarly, there is an increasing number of cases of bacterial infections that are resistant to current antibiotics and are
Pharmaceuticals 2021, 14, 402. https://doi.org/10.3390/ph14050402
https://www.mdpi.com/journal/pharmaceuticals
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difficult or impossible to treat [6]. Currently, there is an emerging interest in developing
drugs that overcome the problems stated above by using natural compounds.
Plectranthus L’ Herit. is a major genus of the Lamiaceae family comprising about
300 species mainly distributed in the summer-rainfall savannahs and forested regions of
tropical Africa, Asia, and Australia [7,8]. Most of the Plectranthus species are soft trailing
semi-succulent to succulent herbs or shrubs and their stems, leaves, roots, and tubers are
frequently used as traditional medicines for the treatment of various illnesses, including
respiratory, digestive, and liver ailments [9]. Phytochemical studies on some species of
Plectranthus revealed the presence of a large number of diterpenes and triterpenes [10,11].
Isolated terpenes from Plectranthus species are reported to possess antibacterial [12–14],
antitumoral [15–18], antifungal [12,19], insecticidal [20], and antiplasmodial [20] activities.
Moreover, our group has been focused on the phytochemical study of Plectranthus species
and we have reported abietane diterpenoids with diverse bioactivity [16,17,21–25]. Therefore, the screening of other Plectranthus spp. extracts aiming at finding new sources of
biologically active natural products is warranted.
Herein, sixteen Plectranthus species were screened for their bioactivity (antioxidant,
antimicrobial activities, and general toxicity) and the main compound of the most bioactive
extract was identified. To the best of our knowledge, the scientific literature concerning these species is scarce or even non-existent. P. hadiensis was earlier reported to have
ethnopharmacological activity and to be a rich source of ent-abietane diterpenes [11]. This
work aims to screen the antimicrobial, antioxidant, and cytotoxic properties of several
Plectranthus spp. extracts and identifying the component in the most bioactive extract that
may be responsible for its bioactivity.
2. Results and Discussion
All sixteen Plectranthus spp. extracts were prepared using ultrasound-assisted extraction in acetone. Previous studies of Plectranthus species showed that acetonic extracts
are rich in diterpenoids, and high extraction yields are obtained when the ultrasound
extraction method is carried out [21]. Therefore, using this extraction method, sixteen
acetonic extracts of Plectranthus spp. were prepared. The extraction of all extracts was done
in triplicate under the same conditions. All extracts were solubilized in DMSO (10 mg/mL)
and stored at −20 ◦ C until further analysis for their biological assays. P. mutabilis had the
highest extraction yield (30.00% w/w) (Table 1).
The antioxidant activity of the extracts was quantitatively determined using the DPPH
(2,2-diphenyl-1-picrylhydrazyl) scavenging radical assay. The antioxidant activity of the
extracts was compared with quercetin, a well-known pure compound used as a positive
control to understand the potential antioxidant activity of the extracts screen. The antioxidant activity indicates the capacity to quench reactive oxygen species (ROS), leading
to decreased oxidative stress [26]. The results of the free radical scavenging capacity of
extracts at a concentration of 10 µg/mL are shown in Table 1. P. mutabilis and P. hadiensis
had the highest scavenging activity of 46.14% and 36.24%, respectively. These results
are also in agreement with other studies with Plectranthus extracts, in which P. madagascarensis P. neochilus, P. barbatus and P. verticillatus extracts showed free radical scavenging
abilities [27]. This could be due to the presence of abietane diterpenes known for their
antioxidant activity. Recently, findings concerning the antioxidant activity of abietane
diterpenes isolated from Plectranthus spp. suggest that the quinone moiety present in
these compounds is probably responsible for their biological activity [28]. The presence
of the 12-OH group and the carbonyl group at position C-7 (p-position) could serve as
hydrogen- and/or electron-donating moieties, resulting in the formation of stable quinone
derivatives [29].
To evaluate the antimicrobial activity, the extracts were screened against Gram-positive
(Staphylococcus aureus, Enterococcus faecalis) and Gram-negative (Pseudomonas aeruginosa and
Escherichia coli) bacteria and yeasts (Candida albicans and Saccharomyces cerevisiae) using the
well diffusion assay. The antimicrobial activity of each acetonic extract was first screened by
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the well diffusion method at a concentration of 1 mg/mL. Only P. hadiensis and P. mutabilis
extracts showed antimicrobial activity against S. aureus with inhibition zones of 16 mm
and 15 mm, respectively. None of the extracts showed significant antibacterial activity
against E. faecalis and Gram-negative bacteria. These results are in agreement with previous
works on Plectranthus spp. [17,30] showing that only Gram-positive bacteria are sensitive
to Plectranthus acetonic extracts [27,31]. When the zone of inhibition of the extracts was
compared with the negative control, it was found that nine extracts (P. ciliatus, P. welshii,
P. mzumbulensis, P. inflexus, P. lucidus, P. xerophylus, P. lippio, P. hadiensis, and P. mutabilis.)
exhibited antimicrobial activity against C. albicans (10–11 mm). The remaining did not
display any antimicrobial effects, showing inhibition zones similar to the negative control
(data not shown).
Table 1. Extraction yields (dry weight % w/w), antioxidant activity, and general toxicity of sixteen Plectranthus spp.
acetonic extracts.
Scientific Name
P. swynnertonii S. Moore †
P. ciliatus E. Mey †
P. mutabilis Codd. †
P. hadiensis (Forssk.) Schweinf.
Ex Sprenger †
P. cylindraceus Hochst, ex Benth †
P. lucidus (Benth.) Van Jaarsv.
and T.J. Edwards †
P. inflexus (Thunb.) Vahl ex Benth †
P. lippio. Druce
P. crassus N.E.Br. †
P. mzimvubuensis Van Jaarsv. †
P. xerophylus Codd
P. welshii
P. petiolaris E. Mey ex Benth.
P. woodii Gürke
P. welwitschii (Briq. Codd)
P. spicatus E. Mey
Positive control
DMSO
Yield
(% w/w) a
Antioxidant Activity b (%)
3.89
11.86
30.03
General Toxicity
* Mortality (%)
LC50 (µg/mL) **
20.24 ± 0.01
13.21 ± 0.01
46.14 ± 0.02
65.88 ± 5
60.14 ± 0.44
51.50 ± 0. 07
0.036 ± 1.69
0.504 ± 1.13
0.984 ± 2.92
13.49
36.24 ± 0.04
43.65 ± 3.04
0.88 ± 4.87
9.68
19.19 ± 0.07
43.50 ± 5.66
0.55 ± 1.96
6.29
23.96 ± 0.09
38.81 ± 3.75
1.053 ± 4.61
10.97
2.09
7.77
7.79
10.16
2.15
11.07
8.51
3.59
4.75
N/A
N/A
0.16 ± 0.05
30.5 ± 0.14
27.27 ± 0.01
22.47 ± 0.05
20.15 ± 0.02
15.06 ± 0.03
14.45 ± 0.01
13.04 ± 0.01
12.63 ± 0.03
10.57 ± 0.02
99.47 ± 0.10
N/A
38.70 ± 3.35
24.70 ± 6.22
31.16 ± 1.29
33.95 ± 1.63
30.48 ± 3.24
23.71 ± 0.60
23.42 ± 4.15
29.95 ± 6.01
25.17 ± 5.54
27 ± 0.28
98.89 ± 2.48
21.87 ± 0.44
0.986 ± 2.87
N/A
N/A
N/A
N/A
N/A
N/A
N/A
N/A
N/A
N/A
N/A
a
(mg of extracts/ g of the dried plant). b Antioxidant activity (%): Quercetin a potent free radical scavenging capacity was used as a
positive control. Data are mean ± SD. * Screening of the Plectranthus spp. extracts for general toxicity at a concentration of 10 µg/mL using
the Artemia salina test (24 h). ** LC50 values (µg/mL) for the most active extracts. Positive control = Potassium dichromate (10 µg/mL).
Data are mean ± SD was calculated from three independent experiments and compared to DMSO († p < 0.001). Lethal concentration (%) =
(Total A.salina − Alive A.salina)/(Total A.salina) × 100 was used to calculate the lethal concentration of all extracts. N/A—not applicable.
As the initial screening using the well diffusion assay identified P. hadiensis and
P. mutabilis extracts as possessing the most promising antimicrobial activities, further
studies were carried out to evaluate the minimum inhibitory concentration (MIC) and
minimum bactericidal concentration (MBC) or minimum fungicidal concentration (MFC)
against the susceptible strains (Table 2). The MIC values ranged from 3.91 µg/mL to
125 µg/mL. P. hadiensis was the most active extract, exhibiting a MIC value of 3.91 µg/mL
against the methicillin-resistant S. aureus strain (MRSA), similar to that observed for the
positive control (1.95 µg/mL). The MBC/MFC values ranged from 62.5 to 250 µg/mL. It is
possible to conclude that the extracts are mainly bacteriostatic rather than bactericidal [32].
To identify the most promising extracts with cytotoxic activity, the screening of general
toxicity using the Artemia salina model was carried out. This assay was employed to screen
the sixteen extracts because it is low-cost, rapid, convenient, and requires only a relatively
small amount of sample [31,33]. All of the acetonic extracts were tested at 10 µg/mL with
values ranging from 23.42 to 65.88% mortality (see Table 1). The most active extracts
were further studied to obtain the LC50 values at concentrations of 0.1, 0.5, and 1 mg/mL,
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after 24 h of exposure. The most toxic extracts (P. mutabilis, P. swynnertonii, P. hadiensis,
P. ciliatus, and P. cylindraceus) with LC50 ≤ 1 µg/mL (see Table 1) were then evaluated on
human-derived cancer cell lines.
Table 2. MIC and MBC/MFC (µg/mL) values of the most active acetonic extracts.
Extracts
Positive Control
P. mutabilis
P. hadiensis
MIC (µg/mL)
MBC/MFC (µg/mL)
S. aureus
MRSA
C. albicans
S. aureus
MRSA
C. albicans
3.91
31.25
15.62
1.95
31.25
3.91
<0.48
125
62.5
250
250
250
250
125
62.5
Positive controls (1 mg/mL): Gram-positive = vancomycin, Gram-negative = norfloxacin, yeast = nystatin,
Negative control = DMSO, methicillin-resistant Staphylococcus aureus = MRSA.
The cytotoxic activity was determined by the sulforhodamine B (SRB) assay in three
different cancer cell lines: colon colorectal carcinoma (HCT116), human breast adenocarcinoma (MCF-7), and lung cancer carcinoma (NCI-H460). The IC50 values in all the cell lines
tested ranged from 2.25 µg/mL to 36 µg/mL (Table 3). According to the National Cancer
Institute (NCI), crude extracts that possess IC50 ≤ 500 µg/mL are of potential interest for
further studies [34] and a possible candidate for further development of cancer therapeutic
agents. Thus, most of the selected extracts showed potential values, and P. hadiensis and
P. ciliatus seem to be potential sources of lead anticancer molecules. P. ciliatus extract was
most active against the colon cell line (HCT116), whereas the P. hadiensis extract was the
most active against the breast (MCF-7) and lung (NCI-H460) cell lines with the lowest IC50
value in the MCF-7 cell lines. For this reason, this extract was further tested against the
aggressive type triple-negative breast cancer (MDA-MB-231S). MCF-7 hormone receptors
expressing breast cancers have a more favorable prognosis as opposed to triple-negative
breast cancer (TNBC), which is characterized by a poor treatment outcome [35]. This cell
line is a highly metastatic triple-negative breast cancer cell line that does not display estrogenic receptors (ER), progesterone receptors (PR), or human epidermal growth factor
receptor 2 (HER2), and is thus difficult to treat [21]. P. hadiensis acetonic extract had a
growth inhibition effect on MDA-MB-231 cancer cells (IC50 value of 25.6 µg/mL, Table 3).
Many studies have attributed the cytotoxicity of Plectranthus extracts to the presence
of royleanone-type abietane diterpenoids with known anticancer activities [18,36]. The
abietane-type diterpenoid royleanones are a highly bioactive group of lead molecules,
important for the development of new anticancer drugs [22] Given the good levels of
bioactivity of P. hadiensis extract in all the cell lines tested, it was selected to identify its
main bioactive component.
Table 3. IC50 (µg/mL) values for five selected acetonic extracts in HCT116, MCF-7, H460 and
MDA-MB231S cell lines.
P. hadiensis
P. ciliatus
P. swynnertonii
P. cylindraceus
P. mutabilis
Doxorubicin
HCT116 *
H460 *
MCF-7 *
MDA-MB231S **
3.45 ± 0.35
2.25 ± 0.75
7.95 ± 0.35
10.25 ± 0.75
28.00 ± 2.00
0.05 ± 3.24
3.00 ± 0.10
6.45 ± 0.05
13.50 ± 0.50
12.50 ± 0.50
36.00 ± 2.00
0.29 ± 2.32
2.90 ± 0.10
6.70 ± 0.30
15.05 ± 0.02
12.00 ± 1.00
35.00 ± 1.00
0.08 ± 4.10
25.6
N/A
N/A
N/A
N/A
0.07 ± 0.01
* The concentration that reduces growth by 50% (IC50 ) was determined by sulforhodamine B assay after 48 h
treatment. Data are mean ± SEM of 4–5 independent experiments. ** IC50 (µg/mL) of the most bioactive P. hadiensis
acetonic extract in MDA-MB231S cancer cell lines. DMSO was used as the negative control. N/A—not applicable.
To unveil the chemical profile of the most bioactive P. hadiensis acetonic extract, and
to identify the main compound responsible for the tested bioactivity, an HPLC–DAD
study was carried out. The chromatogram revealed that the known ent-abietane diterpene,
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7α-acetoxy-6β-hydroxyroyleanone, Roy (Figure 1) was the major compound in the extract
(Supplementary Material). To isolate this diterpene, a bio-guided column and the preparative chromatographic procedure were carried out. Its structure was confirmed through
comparison of its spectroscopic data (Supplementary Material) to those described in the
literature [12,29,37].
Figure 1. Chemical structure of 7α-acetoxy-6β-hydroxyroyleanone.
In previous studies, 7α-acetoxy-6β-hydroxyroyleanone showed cytotoxic activity
against three human cell lines, namely, sensitive non-small cell lung carcinoma, NCI-H460
cell line (IC50 2.7 ± 0.4), multidrug-resistant non-small cell lung carcinoma cell line with
P-glycoprotein overexpression. NCI-H460/R (IC50 3.1 ± 0.4), and human embryonal
bronchial epithelial (MCR-5) cells (IC50 8.6 ± 0.4) [21,38]. Given its cytotoxic properties,
the presence of this compound in P. hadiensis acetonic extract may partially explain, the
foreseen properties of the extract. To further explore its cytotoxicity, additional studies
were performed.
The preliminary toxicity of the isolated 7α-acetoxy-6β-hydroxyroyleanone (Roy) was
evaluated using the Brine shrimp lethality bioassay, which gave a percentage mortality
of 30.95%. The cytotoxicity of 7α-acetoxy-6β-hydroxyroyleanone was further tested in
the TNBC, MDA-MB231S cell line using the MTT assay. It had an IC50 value of 5.5 µM =
2.15 µg/mL (Supplementary Information Figure S4), being approximately 12-fold more
active than the corresponding extract (MDA-MB231S IC50 value = 25.6 µg/mL). This
diterpene has also exhibited cytotoxic activity against breast, renal, melanoma, and central
nervous system cancer cell lines [24,29,30]. It was also found to induce apoptosis in
the H7PX glioma cell line, through the G2/M cell cycle arrest and DSBs (double-strand
breaks) [39]. The cytotoxicity of 7α-acetoxy-6β-hydroxyroyleanone could be due to its
royleanone-type scaffold and by its high lipophilicity, which facilitates penetration into the
interior of the cell membrane [21,22,29,39]. Moreover, 7α-acetoxy-6β-hydroxyroyleanone
was found to exhibit better activity against Gram-positive bacteria, and more importantly,
against MRSA strains than some of the existing antibiotics [37]. Roy is found in many
other Plectranthus species like P. madagascariensis, P. grandidentatus, P. actites, P. amboinicus,
P. sanguineus, P. argentatus, and thus can be considered as a chemomarker of the Plectranthus
genus [21,22].
3. Materials and Methods
3.1. Plant Material
All Plectranthus spp. studied in this work (Table 1) were grown in the “Parque Botânico
da Tapada da Ajuda”, Lisbon-Portugal from cuttings provided by the Kirstenbosch National
Botanical Gardens, South Africa. Plants were collected between 2007 and 2008, always
in June and September. Voucher specimens were deposited in the Herbarium “João de
Carvalho e Vasconcellos” of the Instituto Superior de Agronomia, Lisboa (LISI), Portugal.
The plant names were verified with the Plant List [40].
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Extraction Procedure
Plant extracts were obtained by the ultra-sonication method, adding 30 mL of acetone
to 3 g of ground dry plants (P. hadiensis leaves and the whole plant for the remaining
Plectranthus spp.), sonicated for 1 h, and filtered (Whatman No 5 paper, Inc., Clifton, NJ,
USA). The extraction procedure was repeated three times until complete extraction [41].
The liquid samples were evaporated at 40–50 ◦ C using a rotary evaporator (Sigma-Aldrich,
IKA HBR 4 basic heating bath, Essen, Germany). All extracts were solubilized in DMSO
(10 mg/mL, except for the exceptions that are mentioned) and stored at −20 ◦ C until
further analysis.
3.2. Phytochemical Study of P. Hadiensis
3.2.1. HPLC-DAD Fingerprint Analysis
Extract profiling was performed with an Agilent Technologies 1260 Infinity II Series
system with diode array detector (DAD; Agilent, Santa Clara, CA, USA), equipped with an
Eclipse XDB-C18, (250 × 4.0 mm i.d., 5 µm) column, from Merck and ChemStation Software
(Hewlett-Packard, Alto Palo, CA, USA). Four detection wavelengths were selected: 254,
270, 280, and 360 nm. The mobile phase consisted of a mixture of methanol (A), acetonitrile
(B), and 0.3% (w/v) trifluoroacetic acid in ultrapure water (C). The employed method
was modified from the one previously published Matías et al. [21] as follows: 0 min, 15%
A, 5% B, and 80% C; 10 min, 70% A, 30% B, and 0% C; 25 min, 70% A, 30% B, and 0%
C; and 28 min, 15% A, 5% B, and 80% C. The flow rate was set at 1 mL/min at room
temperature and the injection volume was 20 µL. Solvents were previously filtered and
degassed through a 0.22 µm membrane filter. The major peak from the P. hadiensis leaves
extract was identified by co-elution, comparing the retention time and UV-vis spectrum
overlayed with an authentic standard (Supplementary Materials Figures S2 and S3).
3.2.2. Isolation and Structural Characterization of 7α-Acetoxy-6β-Hydroxyroyleanone
The P. hadiensis extract was fractionated by normal phase column chromatography
over silica gel using mixtures of n-hexane: EtOAc (8: 2) as eluents to give 3 fractions (A, B,
and C) in order of increasing polarity. Fraction B was further studied using preparative
thin-layer chromatography (n-hexane/AcOEt 7:3) on pre-coated TLC sheets (Merck 7747,
Darmstadt, Germany) giving 4 fractions B1 to B4. Visualization of spots was performed
under visible light and UV light (λ 254 and 366 nm) followed by spraying with a mixture of
H2 SO4 : AcOH: H2 O (4:80:16) and heating. Fraction B2 was further purified by preparative
chromatography affording its major compound, 7α-acetoxy-6β-hydroxyroyleanone. The
NMR spectra were collected on a Bruker Fourier 300 spectrometer (1 H 300 MHz, 13 C
75 MHz) using CDCl3 as the solvent. 1 H and 13 C chemical shifts are expressed in δ (ppm)
and the proton coupling constants (J) in hertz (Hz) Supplementary Materials Table S1.
3.3. DPPH Radical Scavenging Assay
The free radical scavenging activity was measured by the DPPH method, as described
by Rijo et al. [26]. Briefly, 10 µL of each extracted sample (1 mg of dry plant extract/mL)
were added to a 990 µL solution of DPPH (0.002% in methanol). The mixture was incubated
for 30 minutes in the dark, at room temperature. The absorbance (Abs) was measured at
517 nm (U-1500 Hitachi Instruments, Inc; USA). The positive control used was quercetin
(10 mg/mL in methanol). An absorbance control (Abscontrol ) containing 10 µL of methanol
and 990 µL of DPPH was also prepared. Assays were carried out in triplicate and the free
radical scavenging activity was calculated using Equation (1):
Scavenging activity (%) =
Abscontrol − Abssample
× 100
Abscontrol
(1)
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3.4. Antimicrobial Screening Assays
3.4.1. Microorganism Used
The microorganisms used in this study were obtained from the American Type Culture
Collection (ATCC). They included five strains Enterococcus faecalis ATCC 29212, Escherichia
coli ATCC 25922, Pseudomonas aeruginosa ATCC 27853, Staphylococcus aureus ATCC 25923,
Saccharomyces cerevisiae ATCC 2601, Staphylococcus aureus. CIP were obtained from the
CIP 106760, and the yeast strain Candida albicans ATCC 10231.
3.4.2. Well Diffusion Method
The antimicrobial activity of each obtained extract was evaluated against two Grampositive bacteria (E. faecalis and S. aureus), two Gram-negative bacteria (E. coli and P. aeruginosa), and two yeasts (S. cerevisiae and C. albicans), according to Rijo et al. [41]. The extracts
were diluted in DMSO from 10 mg/mL to a final concentration of 1 mg/mL. Stock solutions of reference antibiotics (vancomycin, norfloxacin, and nystatin) were also prepared at
1 mg/mL in DMSO.
In aseptic conditions, Petri dishes containing 20 mL of solid Mueller–Hinton for bacteria, or Sabouraud Dextrose Agar culture medium (from Biokar Diagnostics), for yeasts, were
inoculated with 0.1 mL of bacterial suspension matching a 0.5 McFarland standard solution
and uniformly spread on the medium surface using a sterile swab. Wells of approximately
5 mm in diameter were made in the medium, using a sterile glass Pasteur pipette, and
50 µL of each extract were added into the wells. A positive control of vancomycin for
Gram-positive bacteria, norfloxacin for Gram-negative bacteria, and nystatin for yeasts,
and a negative control of DMSO, were used in the assay. Plates were incubated at 37 ◦ C
for 24 h. The antimicrobial activity was evaluated by measuring the diameter (mm) of the
inhibition zone formed around the wells and compared to controls.
3.4.3. Minimum Inhibitory Concentration (MIC) and Minimum Bactericidal Concentration
(MBC)/ Minimum Fungicidal Concentration (MFC)
The MIC and MBC/MFC were determined using the microdilution technique proposed by National Committee for Clinical Laboratory Standards (NCCLS) [42]. Briefly,
100 mL of Mueller–Hilton broth for bacteria and Sabouraud for yeasts was placed into each
well of a 96 microplate, under aseptic conditions. Each extracted sample (100 µL), the appropriate positive control of each microorganism, and negative controls at a concentration
of 1 mg/mL, were added to the first well. Using a multichannel micropipette, a 1:2 microdilution series was made. A standardized bacterial suspension (10 µL), corresponding
to 0.5 McFarland of each microorganism, was then placed in all wells. Finally, the plates
were incubated at 37 ◦ C for 24 h. The MIC was determined when no growth was detected
in the well of the microplate. Each measurement was performed in triplicate using 96 well
microtiter plates with enrichment. A total of 10 µL was withdrawn from the microplate
and sown in a Petri dish to verify the MBC/MFC, which was determined when there was
no visible microbial growth on the plates [43].
3.5. Evaluation of General Toxicity on Artemia salina Model
To evaluate the general toxicity of the different extracts and ent-abietane diterpene
7α-acetoxy-6β-hydroxyroyleanone, a test of lethality to Artemia salina (brine shrimp) was
performed as described by Ntungwe et al. [31]. A. salina eggs, dry cyst (JBL GmbH and
Co. KG, D-67141 Neuhofen Germany), were hatched in artificial seawater at 25–30 ◦ C
under aeration with a concentration of 35 g/L. A handmade container with two connected
chambers was used for brine shrimp hatching. The eggs were placed in one of two
compartments of a container separated by a boundary plate. The cysts were then incubated
(in thermostat cabinet AQUA LYTIC® , Camberley, Surrey, United Kingdom) for 48 h at
24 ◦ C. The compartment with the eggs was covered to maintain a dark ambiance. The other
compartment was illuminated to attract the phototropic newly hatched nauplii through
perforations on the boundary plate. The brine shrimps that had moved to the illuminated
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compartment were collected and used in the lethality assay. Ten to fifteen nauplii were
transferred into 24-well plates containing artificial seawater, and 100 µL of each sample
was added to the wells (final volume per well: 1 mL). After 24 h exposure to the samples
(24 ◦ C), the number of dead nauplii (mortality rate (%)) was determined (Equation (2)). In
addition, LC50 (Lethal Concentration, 50%) values (µg/mL) were calculated for the most
toxic extracts. DMSO was used as the solvent and was kept at 10% (v/v) in all samples
tested. Potassium dichromate was used as the positive control. All samples were tested in
triplicates-at a concentration of 10 ppm for each sample.
()Lethal concentration (%) =
Total A. salina − Alive A. salina
× 100
Total A. salina
(2)
3.6. Cytotoxicity Screening Assays
3.6.1. Cells and Cell Culture
Human colon (HCT116), breast adenocarcinoma (MCF-7), lung carcinoma (H460),
and triple-negative breast cancer, MDA-MB-231S, cell lines were purchased from ATCC
(Rockville, MD, USA). Cell lines were routinely cultured in 293 RPMI-1640 with ultraglutamine or DMEM (MDA-MB-231 cells) medium from Lonza (VWR, 294 Carnaxide,
Portugal) supplemented with 10% fetal bovine serum from Gibco (Alfagene, Carcavelos,
Portugal) and maintained in a humidified atmosphere at 37 ◦ C with 5% CO2 .
3.6.2. Sulphorhodamine Assay
The cytotoxicity of five of the most toxic extracts on the brine shrimp lethality bioassay
was carried out using the sulforhodamine B (SRB) assay as previously described [17,44,45].
Briefly, the extracts were tested in different cancer cell lines: colon colorectal carcinoma
(HCT116), human breast adenocarcinoma (MCF-7), and lung cancer carcinoma (H460).
Cells were plated in 96-well plates at a final density of 5.0 × 103 cells/well and incubated
for 24 h. Cells were then exposed to serial dilutions of each extract (from 1.56 to 50 µg/mL).
The effect of the extracts was analyzed following 48 h incubation, using the sulforhodamine
B (SRB) assay. Briefly, following fixation with 10% trichloroacetic acid from Scharlau (Sigma–
Aldrich, Sintra, Portugal), plates were stained with 0.4% SRB from Sigma–Aldrich (Sintra,
Portugal) and washed with 1% acetic acid. The bound dye was then solubilized with
10 mM Tris Base and the absorbance was measured at 510 nm in a microplate reader (Biotek
Instruments Inc., Synergy, MX, USA). The solvent of the extracts (DMSO) corresponding to
the maximum concentration used in these assays (0.25%) was included as a control. The
concentration of extract that causes a 50% reduction in the net protein increase in cells
(IC50 ) was determined for all tested extracts. Data are mean ± SEM of 4–5 independent
experiments.
3.6.3. MTT Assay
MDA-MB231S cell line was grown in DMEM L050-500 culture medium Biowest
supplemented with 10% fetal bovine serum, L-glutamine, and penicillin-streptomycin at
37 ◦ C and 5% CO2 . For the MTT assay, 1000 cells/well were placed in a 96-well plate and
the compound to be tested was added 24 h after sowing.
The extract and compound were prepared as stock solutions in DMSO (Scrharlau;
SU01531000) at a concentration of 20 mg/mL in the case of the extract (which allowed us
to use a reduced DMSO percentage at higher concentrations) and 10 mM in the case of
the compound. They were stored at 4 ◦ C. The extract and compound were prepared at
different concentrations. For the extract, the following dilutions were made: 80 µg/mL,
40 µg/mL, 20 µg/mL, 10 µg/mL, and 2 µg/mL in culture medium. For the compound,
the following dilutions were prepared: 10 µM, 3 µM, 1 µM, 0.3 µM, and 0.1 µM. Each
concentration was assayed in triplicate in a 96-well plate.
After 48 h of treatment with the compound or extract, the cells were incubated for 2 h
with MTT. After this time, the culture medium was removed, and the formazan crystals
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were dissolved by adding 200 µL of DMSO. The absorbance of each well was measured at
595 nm.
3.7. Statistical Analysis
The results were expressed as the mean value ± SD. Comparisons were performed
within groups by the analysis of variance, using the ANOVA with Dunnett’s post-test.
Significant differences between control and experimental groups were assessed using
GraphPad Prism version 5.00 for Windows, GraphPad Software, San Diego, CA, USA,
www.graphpad.com, accessed on 5 February 2021. A probability level p < 0.05 was
considered to indicate statistical significance.
4. Conclusions
Natural products are known to be an important source of new anticancer agents. This
study investigated the diverse biological activity of sixteen Plectranthus extracts. Among
the studied extracts, P. hadiensis leaves and P. mutabilis had the highest percentage extraction
yield, antimicrobial and antioxidant activities. P. hadiensis and P. ciliatus were the most
cytotoxic extract against HCT116, MCF-7, and H460 cancer cell lines. 7α-acetoxy-6βhydroxyroyleanone was isolated from the most cytotoxic extract (P. hadiensis) and was
found to be 12 times more bioactive than the extract in the MDA-MB-231S cell line (triplenegative breast cancer). Therefore, it is noteworthy that 7α-acetoxy-6β-hydroxyroyleanone
present in the most cytotoxic extract has interesting antitumoral activities in different cancer
cell lines and might thus be responsible for the biological activity of this extract. However
further phytochemical studies should be done to find out more compounds that could
contribute to the cytotoxicity of P. hadiensis.
Supplementary Materials: The following are available online at https://www.mdpi.com/article/10
.3390/ph14050402/s1, Figure S1: 1H-NMR data information for 7α-acetoxy-6β-hydroxyroyleanone,
Figure S2: HPLC chromatograms (270 nm) of P. hadiensis leaves showing the major compound,
7α-acetoxy-6β-hydroxyroyleanone, Figure S3: UV spectrum of 7α-acetoxy-6β-hydroxyroyleanone,
Figure S4: Concentration-response curves (IC50 µM) for 7α-acetoxy-6β-hydroxyroyleanone; Table S1:
NMR spectroscopy data characterization, 1 H NMR (300 MHz, CDCl3 ), 13 C (75 MHz, CDCl3 .
Author Contributions: Conceptualization, P.R.; methodology, E.N., L.S., C.T., S.T.-T. and N.A.C.;
validation, L.S., A.M.D.-L. and P.R.; investigation, E.N., L.S., C.T., S.T.-T. and N.A.C.; writing—
original draft preparation, E.N.; writing—review and editing, E.M.D.-M., L.S, A.M.D.-L., P.R. and
N.D.; supervision, N.D. and P.R. All authors have read and agreed to the published version of
the manuscript.
Funding: This research was funded by Fundação para a Ciência e Tecnologia (FCT) projects
UIDB/04567/2020, UIDP/04567/2020, CBIOS/COFAC/FIPID/1/2019 and COFAC/ILIND/CBIOS/
1/2020. The authors gratefully acknowledge Fundação para a Ciência e Tecnologia (FCT) for the financial support under the reference CBIOS/COFAC/FIPID/1/2019, UIDB/50006/2020, UID/MULTI/
04378/2013 and the project (3599-PPCDT) PTDC/DTP-FTO/1981/2014–POCI-01-0145-FEDER-016581
and the predoctoral FPU 2019 fellowship from the University of Alcalá awarded to E.M.D-M.
Data Availability Statement: Not applicable.
Acknowledgments: This work was supported by PADDIC 2019 (ALIES-COFAC) as part of the PhD
Program in Health Sciences from Universidad de Alcalá and Universidade Lusófona de Humanidades
e Tecnologias.
Conflicts of Interest: The authors declare no conflict of interest. The funders had no role in the design
of the study; in the collection, analyses, or interpretation of data; in the writing of the manuscript, or
in the decision to publish the results.
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