
Hindawi Publishing Corporation
Evidence-Based Complementary and Alternative Medicine
Volume 2011, Article ID 128349, 5 pages
doi:10.1093/ecam/nen077

Original Article

Byrsonima fagifolia Niedenzu Apolar Compounds with
Antitubercular Activity

C. T. Higuchi,1 M. Sannomiya,2 F. R. Pavan,1 S. R. A. Leite,2 D. N. Sato,3

S. G. Franzblau,4 L. V. S. Sacramento,1 W. Vilegas,2 and C. Q. F. Leite1

1 Unesp, Universidade Estadual Paulista, Faculdade de Ciências Farmacêuticas, Rodovia Araraquara-Jaú km 01,
CEP 14801-902, Araraquara – SP, Brazil

2 Unesp, Universidade Estadual Paulista, Instituto de Quı́mica, Rua Francisco Degni s/n. Bairro Quitandinha,
C.P.335. CEP 14800-900, Araraquara – SP, Brazil

3 Instituto Adolfo Lutz, Laboratório de Micobacteriologia, Rua Minas, 887, CEP 14085-410, Ribeirão Preto, SP, Brazil
4 Institute for Tuberculosis Research, College of Pharmacy, University of Illinois at Chicago, USA

Correspondence should be addressed to C. Q. F. Leite, leitecqf@fcfar.unesp.br

Received 28 June 2008; Accepted 14 November 2008

Copyright © 2011 C. T. Higuchi et al. This is an open access article distributed under the Creative Commons Attribution License,
which permits unrestricted use, distribution, and reproduction in any medium, provided the original work is properly cited.

Bioassay-guided fractionation of the chloroform extract of Byrsonima fagifolia leaves led to the isolation of active antitubercular
compounds alkane dotriacontane (Minimal Inhibitory Concentration—MIC, 62.5 μg mL−1), triterpenoids as bassic acid (MIC
= 2.5 μg mL−1), α-amyrin acetate (MIC = 62.5 μg mL−1), a mixture of lupeol, α- and β-amyrin (MIC = 31.5 μg mL−1) and a
mixture of lupeol, and acetates of α- and β-amyrin (MIC = 31.5 μg mL−1). The antimycobacterial activity was determined by the
Microplate Alamar Blue Assay (MABA) and the structures of promising compounds were determined by spectroscopic analysis.
This investigation constitutes the first report of a chemical and antitubercular study of apolar compounds from B. fagifolia
Niedenzu (IK).

1. Introduction

Mycobacterium tuberculosis, the agent of tuberculosis, is
responsible for high mortality worldwide, killing roughly 1.7
million people annually [1]. The situation with multidrug
resistant (MDR) tuberculosis (TB) today worries the health
authorities of the whole world, mainly in the developing
countries, where the situation is more severe. The appearance
of resistant strains to the medicines now in use makes
urgent the search for new synthetic or natural tuberculostatic
drugs. There are several reasons that justify the need to
search for new drugs for TB, for example, improvement of
current treatment by shortening its duration, to get effici-
ent treatment for MDR TB and to eradicate the latent
infection. So, the development of new drugs for shortening
the duration of the treatment and to fight against multidrug
resistant tuberculosis strains is urgent [2].

An approach to the search for new drugs is to look in
nature, mainly for the extremely rich and varied flora of the
tropical areas. In this search, information obtained from folk
knowledge and traditional medicine of different cultures can

be valuable. This trend in associating popular or alternative
medicine with pharmaceutical research has been growing for
some years [3].

Byrsonima fagifolia Niedenzu (IK) is a member of the
Malpighiaceae family and is a native species from the
Brazilian Cerrado (savannah-like vegetation). The Cerrado is
considered the most extensive woodland-savannah in South
America and contains over 5000 species of higher plants [4],
some of then with antimicrobial activities [5]. B. fagifolia is
popularly known as murici-cascudo or murici-vermelho [6].
In Brazilian folk medicine, the leaves of B. fagifolia are used
as an antiemetic, diuretic, febrifuge and to treat peptic ulcers
[6]. Previously, we also have reported the antiulcer activity of
B. crassa extracts [7] and the antidiarrhoeal activity observed
with the methanol extract of B. cinera [8]. Despite the popu-
lar use of B. fagifolia as a medicinal plant, there are no data on
the antitubercular activity of its leaves extract or compounds.

Plants extracts are attractive sources of new drugs, and
bioassay-guided fractionation is the state-of-art process to
identify the active compounds contained in crude natural
products. The aim of this study is to evaluate by Microplate


2 Evidence-Based Complementary and Alternative Medicine

Alamar Blue Assay (MABA), the potential antitubercular
activity of B. fagifolia leaves extracts, enriched fractions and
pure compounds, identified by phytochemical analysis.

2. Methods

2.1. Plant Material. The fresh leaves of B. fagifolia Niedenzu
(IK) were collected at Estrada do Brejinho de Nazaré,
Tocantins State, Brazil (11◦01′S, 48◦34′W, elevation 240 m)
and the species was identified by Dr Eduardo Ribeiro dos
Santos of Tocantins University. A voucher specimen was
deposited in the herbarium of the same university under the
number 6398.

2.2. Extraction and Isolation. The air-dried and powdered
leaves (2.0 kg) of B. fagifolia were extracted exhaustively with
chloroform, methanol and 80% methanol (methanol/water
80/20 v/v), successively at room temperature (48 h for each
solvent). Solvents were evaporated at 60◦C under reduced
pressure to yield the chloroform (92.7 g), methanol (303.8 g)
and 80% methanol (201.2 g) extracts. The yields (w/w) for
the extracts from the dried powders of B. fagifolia leaves were
4.63, 15.19 and 10.06%, respectively.

A portion of the chloroform extract (10.0 g) was chro-
matographed on a Merck silica gel column (15 cm × 6.0 i.d)
in order to separate the compounds according to their
polarity.

The column was eluated sequentially with hexane, then
dichloromethane and finally methanol. Evaporation of the
solvents yielded the dry eluates from hexane (0.76 g), dichlo-
romethane (3.9 g) and methanol (2.2 g).

The fraction eluated by hexane (0.76 g) was rechromato-
graphied on a silica gel 60 column (13.0 × 2.0 cm i.d.) and
eluated with pure n-hexane. Analogously, the other two frac-
tions (eluated with methanol and dichloromethane) were
fractionated on a similar column (13.0 × 3.0 cm i.d.) using
pure chloroform as mobile phase, and gradually in-creasing
the polarity with methanol (for the first fraction) or dichlo-
romethane (for the second one).

2.3. Gas Chromatography Analysis. Gas chromatography
(GC) analysis for hydrocarbon identification was performed
using a Varian 3380 gas chromatograph equipped with a
fused silica CBP-5 capillary column (25 m × 0.33 mm i.d.;
film thickness 0.5 m) and a flame ionization detector (FID).
Hydrogen was used as the carrier gas (60 kPa), and the
injection split ratio was 1 : 30. The injection temperature
was 250◦C; the column temperature was held at 50◦C for
1 min, and then increased to 300◦C at 10◦C min−1, and this
temperature was held for 10 min; the detector temperature
was 280◦C. Samples of 1 μlLwere injected using a 10 μL
Hamilton syringe. The fraction eluated by hexane from the
silica gel column of the B. fagifolia extract in chloroform
was then analyzed by GC, and the chromatograms compared
with standard hydrocarbons (straight chain alkanes kit, C9 to
C32, from Aldrich), obtaining the retention times.

2.4. Structural Identification of the Triterpenes. Structural
identification of the triterpenes was performed by 13C Nu-

clear Magnetic Resonance (NMR) spectroscopy. The NMR
spectra in deuterated chloroform (CDCl3) were obtained
using a Varian INOVA 500 spectrometer, operating at
500 MHz for 1H and 150 MHz for 13C. Chemical shifts were
given in δ (p.p.m.) using tetramethylsilane (TMS) as the
internal standard. The NMR spectra data obtained were
compared with those reported in the literature [9]. The
identification of the isomeric amyrins and its acetates (α
and β) is perfectly possible by the 13C NMR spectrum, even
if they are mixed, once some similar bands of the isomeric
ones have very different chemical shifts. Similarly, other
triterpenes may be identified in mixtures, without previous
separation [10].

2.5. Antitubercular Activity Assay. The antitubercular activity
of chloroform, methanol and 80% methanol extracts of B.
fagifolia leaves, the enriched fractions and pure compounds
were determined using the MABA [11] as the analytical
method. Stock solutions of the tested compounds were
prepared in dimethyl sulfoxide [11] and were diluted in
Middlebrook 7H9 (Difco) broth supplemented with oleic
acid, albumin, dextrose and catalase (OADC enrichment—
BBL/Becton-Dikinson, Sparks, MD, USA) to obtain final
sample concentrations ranges of 0.15–1600 μg mL−1. Iso-
niazid was solubilized with distilled water according to
the manufacturers’ recommendations (Difco laboratories,
Detroit, MI, USA) and used as a positive control drug. M.
tuberculosis H37Rv ATCC 27294 was grown for 7–10 days
in Middlebrook 7H9 supplemented with OADC added of
0.05% Tween 80 to avoid clumps. Suspensions were prepared
and their turbidities matched to a McFarland no. 1 (turbidity
standard). After further dilution of 1 : 25 in Middlebrook
7H9 supplemented with OADC, the inoculum was added
to each well of the 96 well microtiter plate (Falcon 3072;
Becton–Dickinson, Lincoln Park, NJ, USA) together with
the compounds. Samples were set up in triplicate. Cultures
were in incubated for 7 days at 37◦C, and after additioned
Alamar Blue for the reading. The minimum inhibitory
concentration (MIC) was defined as the lowest concentration
resulting in 90% inhibition of growth of M. tuberculosis [11]
measuring the fluorescence (excitation/emission of 530/590
filters, resp.) in a SPECTRAfluor Plus (Tecan) [12]. For
standard test, the MIC value of isoniazid was determined
each time. The acceptable MIC of Isoniazid ranged from
0.015 to 0.05 μg mL−1.

3. Results

The fractions originating from the initial chromatography of
the extract in chloroform of B. fagifolia leaves were submitted
for subsequent column chromatographic separations, as
described in Experimental section, yielded the following
compounds:

The fraction eluated with hexane (0.76 g) yielded 530 mg
of the n-alkane dotriacontane and 15.4 mg of the triter-
pene α-amyrin acetate. The triterpene bassic acid (234 mg)
was obtained from 2.0 g of the methanol eluate and the
dichloromethane fraction (2.0 g) resulted in a mixture of
the triterpenes lupeol, α- and β-amyrin (223 mg), as well as


Evidence-Based Complementary and Alternative Medicine 3

H

HHO

HO

HO

COOH

Bassic acid

H

H

H

HO

Lupeol

H

H

H

R

R = OH, β-amyrin

R = AcO, β-amyrin acetate

H H

HR

R = OH, α-amyrin

R = AcO, α-amyrin acetate

H3C
CH3

Dotriacontane

Figure 1: Compounds identified from the chloroform extract of Byrsonima fagifolia.

the corresponding acetates (124 mg). The structures of the
compounds are shown in Figure 1. The alkane dotriacontane
was identified by GC and all triterpenes were identified by
their 13C NMR spectra.

The chloroform, methanol and 80% methanol extracts
of leaves yielded MIC values of 62.5, 250 and 500 μg mL−1,
respectively (Table 1). MIC of 31.25 μg mL−1 was observed in
both mixtures obtained from the dichloromethane fraction
of the chloroform extract (one with lupeol, α- and β-amyrin
and the other with lupeol and acetates of α- and β-amyrin).
The pure compounds α-amyrin acetate and dotriacontane,
both showed MIC of 62.5 μg mL−1, and the bassic acid
presented a very promising MIC value of 2.5 μg mL−1. The
MIC of Isoniazid, used as a positive control drug, was
0.03 μg mL−1.

4. Discussion

According to Copp [13], terpenes dominate the number of
natural products reported with antimycobacterial activity.
Several terpenes (diterpenes, sesquiterpenes, sesterpenes and
triterpenes) have demonstrated this biological activity [14].

Tosun et al. [15] considered inactive those plants extracts
that could not prevent growth of M. tuberculosis up to a
concentration of 200 μg mL−1 and according to Gu et al.
[16] the MIC value of ≤128 μg mL−1 is defined as active. In

Table 1: Determination of MIC values of extracts, fractions and
compounds from leaves of B. fagifolia against M. tuberculosis ATCC
27294, using MABA.

Samples MIC (μg/mL)

Extracts

80% MeOH 500

MeOH 250

CHCl3 62.5

Enriched fraction/compounds

Mixture of lupeol, α- and β-amyrin 31.25

Mixture of lupeol, acetates of α- and β-amyrin 31.25

α-Amyrin acetate 62.5

Dotriacontane 62.5

Bassic acid 2.5

Reference drug

Isoniazid 0.03

MeOH, Methanol extract; CHCl3, Chloroform extract.

the present study, the mixture of lupeol, α- and β-amyrin
displayed lower MIC (31.25 μg mL−1) than those previously
reported with pure lupeol [17] and α- and β-amyrin [18]
isolated from Chuquiraga ulcina H. et A. and from Asteraceae
Martinov flowers (64 μg mL−1). Their synergistic activity
in the mixture might explain these results. In theory,


4 Evidence-Based Complementary and Alternative Medicine

fractionation allows for the isolation of pure compounds
with higher activity than the mixture, but it is common
the original extract or the mixture to have better activity.
Houghton et al. [19] published an excellent review about this
matter. The mixture containing lupeol and α- and β-amyrin
acetates showed the same MIC value of 31.25 μg mL−1,
suggesting that the acetylation of α- and β-amyrin does
not influence their activity. A MIC of 62.5 μg mL−1, for the
pure acetate of α-amyrin, double the value for the mixture,
reinforces the synergistic effect among the components of
the mixture against M. tuberculosis.

In previous study performed in Brazil, the new triterpene
lupenone was isolated from B. microphyla A. Juss. [20] an
other species of Byrsonima. Lupenone was not found in B.
fagifolia but its activity against M. tuberculosis was tested by
our group being found MIC of 125 μg mL−1 (Nasser ALM
et al., unpublished data).

The triterpene bassic acid showed strong antitubercular
activity with MIC values of 2.5 μg mL−1. This value is
comparable with that found by Woldemichael et al. [21]
for diterpenes isolated from Calceolaria pinnifolia Cav. and
sterols from Ruprechitia triflora Griseb. with MICs of 2–
4 μg mL−1. Although this MIC value is larger than the ref-
erence drug Isoniazid (MIC = 0.03 μg mL−1), the inhibitory
concentration value of 2.5 μg mL−1 is comparable to MICs
of the other first-line tuberculosis drugs, such as ethambutol
(1–5 μg mL−1) and streptomycin (2–8μg mL−1), and better
than pyrazinamide (20–100μg mL−1) [22].

The biological activity against Leishmania [23] and the
hypoglycemic activity [24] were already described for bassic
acid but never for M. tuberculosis.

Dotriacontane is an alkane with 32 carbons, and its anti-
tubercular activity (62.5 μg mL−1) was also never described
before, but the antimycobacterial activity of other alkanes
is documented in an extensive review covering 12 years
of natural products literature [16]. Two alkenes derived
from the microbial products, cerulenin and thiolactomycin,
inhibit the function of β-ketoacyl-acyl carrier protein (ACP)
synthases, which are key regulators of type II fatty acid
biosynthesis [25]. As mycolic acids are prevalent in the outer
lipid layer of mycobacteria, inhibitors of fatty acid biosyn-
thesis represent existing and potential antimycobacterial
agents.

In conclusion, the bioassay-directed fractionation of the
chloroform extract of B. fagifolia leaves yielded the pure
triterpene bassic acid with potent anti-TB activity. Promising
activities were also verified for the mixture of lupeol, α-
amyrin and β-amyrin or their acetates, and for dotria-
contane.

Acknowledgments

The authors thank the Fundação de Amparo à Pesquisa
do Estado de São Paulo (FAPESP) for a grant to Miriam
Sannomiya and Fernando Rogério Pavan, and for funding
of the project Biota-Fapesp 02/05503-6. They also thank
CNPq for a grant to W. Vilegas. They thank Henri Berghs
for assistance with revision of the manuscript.

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