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143 
Bioscience Journal  Original Article 

Biosci. J., Uberlândia, v. 36, Supplement 1, p. 143-155, Nov./Dec. 2020 
https://doi.org/10.14393/BJ-v36n0a2020-48215 

ESSENTIAL OILS IN THE MANAGEMENT OF SOFT ROT OF KALE IN THE 
BRAZILIAN SEMIARID REGION 

 
ÓLEOS ESSENCIAIS NO MANEJO DA PODRIDÃO MOLE EM COUVE NO 

SEMIÁRIDO BRASILEIRO 
 

Marcia Ferreira QUEIROZ1; Meridiana Araujo Gonçalves LIMA2; 
Josineide Edinalva PEREIRA1; Karol Alves BARROSO1;Cristiane Domingos DA PAZ2; 

Angélica Maria LUCCHESE3;Ana Rosa PEIXOTO2 
1. Posgraduate Program in Agronomy: Irrigated Horticultute, State University of Bahia, Juazeiro, BA, Brazil. 

marciaqueiroz.mfq@gmail.com; 2. Department of Technology and Social Sciences, State University of Bahia, Juazeiro, BA, Brazil;  
3. Departament of Exact Sciences, State University of Feira de Santana, Feira de Santana, BA, Brazil. 

 
ABSTRACT: The aim of this study was to analyze the effect of essential oils on the control of soft rot 

of kale. Clove essential oil at 0.25%, lemongrass and palmarosa essential oils at 0.5%, melaleuca and orange 
essential oils at 0.75%, bergamot, rosemary, sage and ginger essential oils at 1% were evaluated for the in vitro 
inhibition of Pectobacterium carotovorum subsp. brasiliensis (Pcb) and control of soft rot of kale, sprayed 72 
hours before or seven hours after inoculation. Clove, citronella, bergamot, rosemary, palmarosa, sage, 
melaleuca, and lemongrass oils completely inhibited the growth of Pcb. Lemongrass oil (0.5%) caused 0% of 
disease incidence (INC), providing 100% of disease control in both periods of inoculation. Clove oil (0.25%) 
showed a lower INC (25%) when applied after inoculation, providing a control percentage of 71.42%. The 
lemongrass and clove essential oils were analyzed by GC/FID (Gas Chromatography – Flame Ionization 
Detector) and by GC/MS (Gas Chromatography /Mass Spectrometer). The major components were eugenol 
(91,9%) for clove oil and citral, isometric mixture of neral (34,1%) and geranial (42,9%) for lemongrass oil. 
The Minimum inhibitory concentration (MIC) of lemongrass, clove oils and their major components (citral and 
eugenol, respectively) was determined by using a broth macrodilution technique, as well as they were evaluated 
at different concentrations on the control of soft rot of kale, sprayed according descriptions above. The MIC 
was 0.03125% for citral, and 0.0625 and 0.125% for lemongrass and clove oils, respectively. Eugenol didn't 
show MIC. Lemongrass oil at 0.125% (post-inoculation) and citral at 0.125% (pre and post-inoculation) 
provided the highest percentages of disease control (33.33, 50, and 100%, respectively). Clove oil at 0.125% 
(post-inoculation) showed better effectiveness than eugenol (0.25%), providing a percentage of disease control 
of 16.67%. Lemongrass and clove essential oils were the most effective in control of soft rot of kale, suggesting 
that these oils have a potential to be used as antibacterial agents. 

 
KEYWORDS: Alternative control. Brassica oleraceae var. acephala. Citral. Clove. Eugenol. 

Lemongrass. P. carotovorum subsp. brasiliensis. 
 

INTRODUCTION 
 
Kale (Brassica oleracea L. var. acephala 

DC) is cultivated throughout the year in Brazil, and 
it remains productive for several months, which 
makes it an attractive source of income, mostly for 
family farmers who cultivate it in small areas during 
the year (SILVA et al., 2012b). One of the factors 
that might compromise crop yield is 
phytobacterioses, e.g. soft rot caused by pectinolytic 
bacteria of the genus Pectobacterium (FILGUEIRA, 
2008; MARINGONI; SILVA JR, 2016).  

The species P. carotovorum is considered 
one of the top ten phytopathogenic bacteria in 
scientific and economic importance worldwide 
(MANSFIELD et al., 2012). Soft rot of kale is 

commonly caused by P. carotovorum 
(MARINGONI; SILVA JR, 2016). However, the 
genus Pectobacterium is comprised of a diversity of 
species and subspecies (DUARTE et al., 2004; 
GARDAN et al., 2003; HAUBEN et al., 1998; 
NABHAN et al., 2013; SAMSON et al., 2005), 
most of which have no specificity and might infect a 
wide range of hosts, and one crop might be infected 
by several species or subspecies of this genus 
(MARIANO et al., 2005). In 2004, a new, highly 
aggressive subspecies, designated as P. 
carotovorum subsp. brasiliensis Duarte et al. (2004) 
(Pcb), was characterized in potato crops in Brazil 
(DUARTE et al. 2004). Since then, this subspecies 
has been reported in several countries and botanic 
families, including Brassicaceae, e.g. chinese 

Received: 15/04/19 
Accepted: 01/12/20 



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Essential oils...  QUEIROZ, M. F. et al. 

Biosci. J., Uberlândia, v. 36, Supplement 1, p. 143-155, Nov./Dec. 2020 
https://doi.org/10.14393/BJ-v36n0a2020-48215 

cabbage (Brassica pikinensis L) (LEE et al. 2014). 
In Brazil, the first report of Pcb causing severe soft 
rot symptoms in kale was published in 2017 
(QUEIROZ et al., 2017). 

Soft rot disease is difficult to control due to 
the heterogeneity of species of the genus 
Pectobacterium, which have a wide host range and 
geographical distribution (LEE et al. 2014), are 
capable of surviving in crop remains, in the soil, and 
in the rhizosphere of cultivated or invasive plants 
(CHARKOWSKI, 2015; MARINGONI; SILVA JR, 
2016), and is transmitted through different means 
(HADAS et al. 2001; MARINGONI; SILVA JR, 
2016). Nevertheless, there are some integrated 
control measures involving: planting on well-
drained soils, insect control, elimination of diseased 
plants, crop rotation (MARIANO et al., 2001;  
MARINGONI; SILVA JR, 2016), biological control 
(SILVA et al., 2014b), use of resistance inducers 
(acibenzolar-S-methyl) (BENELLI; DENARDIN; 
FORCELINI, 2004), use of calcium phosphite, 
potassium phosphite (SILVA et al., 2014b), plant 
extracts (SILVA et al., 2012a), and chemical control 
using antibiotics and copper-based fungicides 
(CHARKOWSKI, 2015; INOUE-NAGATA et al., 
2016). However, there is no registered product in 
Brazil for the control of soft rot in brassicas 
(AGROFIT, 2018). 

In the last years plant essential oils have 
been extensively studied and are a promising 
alternative for plant disease management due to 
their antimicrobial properties (DEBERDT et al., 
2018; SILVA et al., 2017). Several previous studies 
have shown that essential oils can be used in the 
management of soft rot caused by Pectobacterium 
species, such as P. carotovorum subsp. carotovorum 
(Jones) Haubenet al (Pcc) in chinese cabbage 
(GUERRA et al., 2014) and lettuce (Lactuca sativa 
L.) (SILVA et al., 2012a). Positive in vitro results of 
essential oils were also obtained for Pcc (COSTA et 
al. 2008a; 2008b; FERNÁNDEZ et al. 2014; 
JEONG et al. 2009; SOTELO-BOYÁS et al., 2015). 
In a study by Joshi et al. (2016), they demonstrate 
the potential envolviment of essential oils active 
compound in the control of Pcb and P. aroidearum 
Nabhan et al. (2013) on potato tubers, cabbage and 
calla lily leaves as hosts. 

However, no studies have been found 
involving the use of essential oils in the 
management of soft rot caused by Pcb on kale. 

Therefore, the aim of present study was to 
evaluate the in vitro and in vivo inhibitory effects of 
different concentrations of essential oils on the 
growth of Pcb and on the control of soft rot of kale.  

 

MATERIAL AND METHODS 
  
Experiments were conducted at the 

Phytopathology Laboratory and Greenhouse of the 
Department of Technology and Social Sciences of 
the Universidade do Estado da Bahia (UNEB), 
Campus III, Juazeiro, Bahia State, Brazil and 
Universidade Estadual de Feira de Santana (UEFS), 
Feira de Santana, Bahia State, Brazil. 

 
Obtaining and preparation of the inoculum 

Isolate of P. carotovorum subsp. 
brasiliensis (UNEB8) was obtained from the 
collection of cultures of the Laboratory of 
Phytopathology of UNEB, having been obtained 
from kale plants (cv. Manteiga) with severe soft rot 
symptoms and identified through biochemical, 
metabolic and molecular tests (QUEIROZ et al., 
2017). For its use in the experiments, UNEB8 
isolate was cultivated on peptone-casamino acid-
glucose medium (CPG) for 48h for the preparation 
of the suspensions. Bacterial suspension 
concentration was adjusted using a photocolorimeter 
(Analyser 500, Brazil) to 1x109 CFU mL-1.  

 
Essential Oils (EOs) and test for phytotoxicity 

The EOs used were of clove (Eugenia 
caryophyllata Thunb), citronella (Cymbopogon 
winterianus Jowitt), bergamot (Citrus bergamia 
Risso et Poiteau), rosemary (Rosmarinus officinalis 
L.), palmarosa (Cymbopogon martin [Roxb.] Wats), 
sage (Salvia sclarea L.), ginger (Zingiber officinalis 
Roscoe), melaleuca (Melaleuca alternifolia Maiden 
& Betche, Cheel), orange (Citrus aurantium L.), and 
lemongrass (Cymbopogon citratus Stapf), all 100% 
pure and produced by Phytoterapica (Phytoterapica 
– Solua Comercial Ltda., São Paulo, Brazil). Citral 
and eugenol compounds were purchased from 
Sigma-Aldrich, Brazil. 

In all the experiments, 60-day-old kale 
plants (cv. Manteiga) were used. Sowing was 
performed on polyurethane trays containing 
commercial substrate. After 18 days, seedlings were 
transplanted to vases with capacity of 1000 mL 
containing a 2:1 (v/v) mixture of clayish soil and 
sand, previously sterilized in autoclave. Irrigation 
was performed as required.  

To determine potential phytotoxicity and 
choose the concentrations to be used, the 10 EOs 
were previously tested at concentrations of 0; 0.25; 
0.50; 0.75 and 1.00%, obtained by dilution in 
sterilized distilled water (SDW) mixed with Tween 
20 (1:1). Kale plants were sprayed until leaf surface 
was completely wet. Phytotoxicity evaluation was 
performed by observing abnormal plant 



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https://doi.org/10.14393/BJ-v36n0a2020-48215 

development or color up to 48 hours after treatment 
application (GUERRA et al., 2014). Experiments 
were carried out in a completely randomized 
factorial block design 10 x 5, comprised of 10 OEs 
and five concentrations. Each treatment had five 
replicates, and each replicate was represented by a 
plant. 

 
In vitro sensitivity of Pectobacterium carotovorum 
subsp. brasiliensis to essential oils 

In vitro sensitivity of Pcb to different EOs 
was determined by colony counts per dish (PARET 
et al., 2010). One hundred milliliters of CPG 
medium were used in each treatment. The medium 
was amended with 250 μL, 500 μL, 750 μL, and 
1000 μL of oils to give final concentrations of 0.25; 
0.50; 0.75 and 1.00 % (v/v), respectively. Clove oil 
was used at 0.25%, lemongrass and palmarosa oils 
were used at 0.50%, citronella, orange, and 
melaleuca were used at 0.75%, and the others were 
used at 1.00%. The medium mixed with emulsified 
oils in Tween 20 (1:1), at their corresponding 
concentrations, was poured into Petri dishes and 
cooled in a laminar flow chamber for 20 min. After 
that, 100 μL of bacterial suspension (103 CFU mL-1) 
was spread over the medium. The Petri dishes were 
maintained at 28 °C for 48 h. Subsequently, the 
number of colonies per dish was counted and CFU 
mL-1 was calculated. The medium with addition of 1 
mL of Tween 20 represented the control treatment. 
Experiment was comprised of 11 treatments (10 
essential oils + control) with four replicates and 
three plots, and each plot was represented by a Petri 
dish. 

 
Essential oils in the control of soft rot in kale 

EOs were sprayed onto kale plants as 
previously described, in different periods: prior to 
inoculation-pre (oils applied 72 hours prior to 
inoculation), or after inoculation-post (oils applied 
seven hours after inoculation). Plants were 
inoculated at the base of the petiole, using the 
pricking method adapted from Ren, Petzoldt and 
Dickson (2001), in which the plant tissue is 
penetrated with the insertion of an entomological 
pin, followed by the deposition of 10 µL of bacterial 
suspension. After that, plants were placed in a moist 
chamber for six hours, and remained under 
greenhouse conditions (T of 29.5°C ±2). Incidence 
(INC), expressed by the percentage of diseased 
plants, was evaluated 48 h after inoculation (in the 
experiment in which oils were applied prior to 
inoculation) or 48 h after the application of essential 
oils (in the experiment in which oils were applied 
after inoculation). 

The experimental design was completely 
randomized, and each experiment was comprised of 
11 treatments, with 10 essential oils and 1 control 
(treated with SDW, inoculated with Pcb). Each 
treatment had four replicates, and each replicate was 
comprised of one plant, with three leaves 
inoculated.   

The essential oils of lemongrass and clove 
for promoting the highest percentages of soft rot 
control were selected to conduct further 
experiments. 

 
Chemical composition of lemongrass and clove 
essential oils 

Essential oils were analyzed by GC/FID 
(Gas Chromatography – Flame Ionization Detector) 
and by GC/MS (Gas Chromatography /Mass 
Spectrometer) as Silva, Uetanabaro and Lucchese 
(2013) with some modifications. Before injection, 
25 mg of essential oil were diluted in 1 mL of 
dichloromethane, and 0.5 μL was injected. The GC 
used was a Varian® CP–3380 model, equipped with 
a FID detector. The analysis was performed with a 
Chrompack CP-SIL 5 (30 m x 0.5 mm i.d. x 0.25 
μm film) capillary column. The temperatures of the 
FID and of the injector were 240 ◦C and 220 ◦C, 
respectively. The oven temperature was 
programmed at 60 ◦C with an increase of 3 ◦C/min 
until 240 ◦C, and maintained for 20 min. The carrier 
gas was helium, at a flow rate of 1 mL/min, in split 
mode (ratio of 1:50). The results are expressed in 
relative percentage of each constituent, calculated 
by normalisation of the chromatographic peak areas 
reported as mean value of three oils injections. The 
GC-MS used was a Shimadzu GC-2010 model, 
coupled to a GC/MS-QP 2010 Shimadzu mass 
detector model with a DB-5 ms (30 m × 0.25 mm 
i.d. × 0.25 µm film) capillary column, under the 
same analysis conditions as set out above. The 
temperature of the ionization source was maintained 
at 240°C, the ionization energy at 70 eV and the 
current at 0.7 kV. Retention indices of the separated 
compounds were determined on the basis of a 
homologous series of n-alkanes (C8– C24). The 
identification of the constituents was performed by 
comparison of the retention indices (Kovats indices) 
with literature data (ADAMS, 2017) and authentic 
reference compounds, as well as by MS matching 
with National Institute of Standards and Technology 
libraries (NIST21 and NIST107). 

 
 
 



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https://doi.org/10.14393/BJ-v36n0a2020-48215 

Determining minimum inhibitory concentration 
(MIC) of lemongrass and clove essential oils and 
their major components 

Lemongrass and clove EOs with their major 
components, citral and eugenol, respectively, were 
initially emulsified in 0.05 mL of Tween 20 and 
diluted in SDW to obtain the standard solution of 
initial concentration of 1% for lemongrass and 
citral, and 0.5% for clove and eugenol. MIC was 
determined by using a broth macrodilution 
technique (CLINICAL LABORATORY 
STANDARDS INSTITUTE, 2015) with 
modifications. Sterilized test tubes were used to 
perform serial dilutions, to which 400 μL of the 
CPG medium without agar were added, followed by 
600 μL of the Pcb bacterial suspension (103 CFU 
mL-1). After that, 1 mL of the standard essential oil 
or major component solution was added to obtain 
the initial concentration of 0.5% for lemongrass oil 
and citral, and 0.25% for clove oil and eugenol. 
Subsequent concentrations were obtained by serial 
dilution, transferring 1 mL of the content into the 
subsequent tube. For lemongrass oil and citral, the 
concentrations obtained were: 0.5, 0.25, 0.125, 
0.0625, and 0.03125%. For clove oil and eugenol, 
the concentrations obtained were: 0.25, 0.125, 
0.0625, 0.03125, and 0.015625%. To follow the 
growth of Pcb, essential oils and major components 
were not added. For sterilization control, on the 
other hand, only the culture medium was added to 
the tubes, which were incubated at 28 °C for 48 h. 
MIC corresponded to the last dilution in which the 
presence of bacterial precipitate was not observed.    

Experiment design was completely 
randomized, with 22 treatments represented by 
lemongrass and clove essential oils, and their major 
components, citral and eugenol, at five 
concentrations, plus Pcb medium and growth 
control, with four replicates, each one represented 
by a test tube. 

To confirm the bactericide activity of EOs 
and major components, 100 μL aliquots of dilutions 
corresponding to MIC were sowed on the CPG 
medium. Subsequently, Petri dishes were incubated 
at 28 °C for 48 h. Results were descriptively 
analyzed according to the presence or absence of 
bacterial growth. 
 
Effect of MIC of lemongrass and clove essential 
oils and their major components on the control of 
soft rot of kale 

Lemongrass and clove essential oils, with 
their major components, citral and eugenol, 
respectively, were sprayed prior to or after pathogen 

inoculation in kale plants according to the 
methodology previously described. Inoculation and 
INC evaluations were carried out according the 
descriptions above. 

Experiment design was completely 
randomized with eight treatments each, comprised 
of clove oil (0.125%); lemongrass oil (0.0625% and 
0.125%); eugenol (0.25%); citral (0.03125%, 
0.0625%, and 0.125%), and control (treated with 
ADE, inoculated with Pcb). Each treatment had four 
replicates, and each replicate was comprised of one 
plant, with three leaves inoculated. 

 
Statistical analyses  

All experiments and tests shown were 
repeated twice. Statistical analyses were performed 
with the help of STATISTIX® (version 9.0, 
Analytical Software, Tallahassee) and Assistat 
(version 7.6) programs. The significance level of 
5% was adopted in all statistical procedures. 

 
RESULTS AND DISCUSSION 

 
In the assay performed in a greenhouse to 

determine phytotoxic concentrations of EOs, 
rosemary, sage, bergamot, and ginger oils did not 
cause phytotoxicity at any of the concentrations 
tested. On the other hand, citronella, melaleuca, and 
orange oils at 1% were phytotoxic, as were 
lemongrass and palmarosa, at concentrations of 0.75 
and 1%, and clove oil, at 0.5, 0.75, and 1%. The 
symptoms of phytotoxicity are characterized by the 
presence of leaf spots, and clove oil at 
concentrations higher than 0.25% caused dry leaves 
and plant death. 

EOs employed in phytopathogen control are 
generally used at concentrations ranging from 0.1 to 
1% (ALVES et al. 2014; GUERRA et al. 2014; 
HUANG; LAKSHMAN, 2010; SILVA et al., 
2012a). The higher these concentrations, the more 
phytotoxicity they might cause, which precludes 
their use in the alternative control of plant diseases. 
Thus, we used the highest non-phytotoxic 
concentration of each essential oil in subsequent 
experiments.  

Regarding the in vitro sensitivity of Pcb to 
EOs, rosemary, bergamot, sage oils at 1%, 
citronella, melaleuca oils at 0.75%, lemongrass, 
palmarosa at 0.5%, and clove oil at 0.25% 
completely inhibited pathogen growth (P≤0.05) 
after 48 h of incubation at 28 °C. On the other hand, 
essential oils of ginger at 1% and orange at 0.75% 
did not significantly inhibit bacterial growth 
compared to the control treatment (Table 1). 

 



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https://doi.org/10.14393/BJ-v36n0a2020-48215 

Table 1. In vitro sensitivity of Pectobacterium carotovorum subsp. brasiliensis to essential oils, determined by 
colony counts per Petri dish. 

Treatments Concentrations (%) Log(UFC/mL+1) 
Rosemary      1.00 0 a1 
Bergamot 1.00 0 a 
Lemongrass 0.50 0 a 
Citronella 0.75 0 a 
Clove      0.25 0 a 
Melaleuca 0.75 0 a 
Palmarosa 0.50 0 a 
Sage 1.00 0 a 
Ginger 1.00  8.53 b 
Orange      0.75 8.47 b 
Control  - 8.62 b 
1Means followed by the same letter on the column do not differ from each other according to Tukey's test (P≤0.05). 

 
In vitro microbial activity of EOs has been 

proved by several authors, including for 
phytopathogenic bacteria. Paret et al. (2010) 
observed that palmarosa and lemongrass oils at 0.07 
and 0.14% completely inhibited the growth of 
Ralstonia solanacearum (Smith) Yabuuchi et al. 
(Rs). Amorim et al. (2011), testing the effect of 
different concentrations (1.25, 3.5, 3.75, and 5%) of 
EOs on the growth of Rs, observed that citronella 
and clove oils inhibited bacterial growth at all 
concentrations tested. Lucas et al. (2012a) observed 
the direct toxic effect of citronella, clove, 
lemongrass, eucalyptus, melaleuca, thyme (Thymus 
vulgaris L.), and cinnamon (Cinnamomum 
zeylanicum Blume) oils at 10% on Xanthomonas 
vesicatoria (ex Doidge) Vauterin et al. On the other 
hand, Silva, Martins and Alves (2014a) observed 
that citronella, lemongrass, cinnamon, and 
eucalyptus (Corymbia citriodora Hill & Johnson) 
oils at 1%, and thyme and clove oils at 10% 
effectively inhibited the growth of Pseudomonas 
syringae pv. tomato (Okabe) Young, Dye & Wilkie. 
These results reinforce the antibacterial potential of 
palmarosa, lemongrass, citronella, clove, and 
melaleuca essential oils, which was also observed in 
our study. 

Our results on potential of EOs were further 
corroborated with other studies, which confirmed 
the antibacterial potential of EOs on Pcc. Citronella 
essential oil at 1.00% and rosemary essential oil at 
4.00% showed high inhibition on six Pcb isolates 
obtained from Brassica oleraceae L. var. capitata 
DC and Lactuca sativa L. (COSTA et al. 2008a; 
2008b). Moreover, Jeong et al. (2009) proved the 
inhibitory activity of lemongrass oil on three Pcc 
isolates, with complete inhibition at 0.5%. This 
result agree with results of our investigation, in 

which lemongrass oil at 0.5% completely inhibited 
the growth of Pcb.    

Other essential oils have shown 
effectiveness on Pcc. Fernández et al. (2014) 
observed that thyme essential oil at 0.10% 
completely inhibited the growth of Pcc, whereas 
Sotelo-Boyás et al. (2015) observed inhibitory 
activity of thyme oil at 2.80% and lime (Citrus 
aurantifolia (Cristm.) Swingle) oil at 11.20% on this 
pathogen.  

The bactericide activity of rosemary, 
citronella, melaleuca, palmarosa, clove, and 
lemongrass EOs observed in this study might be 
related to their complex chemical constituents, such 
as terpens and aromatic compounds (BAKKALI et 
al. 2008). 

Components of essential oils are highly 
cytotoxic and their antimicrobial activity occurs due 
to interference in cell wall structure and cytoplasm 
membranes, increasing permeability and loss of cell 
constituents, changing a variety of enzyme systems, 
including those involved in the production of cell 
energy, synthesis of structure components, and 
inactivation or destruction of genetic material 
(BURT, 2004; BAKKALI et al. 2008). Huang and 
Lakshman (2010) suggested that the components of 
clove oil were mostly responsible for its 
antibacterial properties on Pcc, Rs, Rhizobium 
rhizobacter (Beijerinck and van Delden) Young et 
al., Xanthomonas hortorum pv. Pelargonii (Brown) 
Vauterin et al., Streptomyces spp., and Rhodococcus 
fascians (Tilford) Good fellow. 

In this study, essential oils of ginger and 
orange did not show satisfactory results. However, 
some studies have already observed the bioactivity 
of ginger oil on Rs (AMORIM et al. 2011), 
Staphylococcus aureus, and Escherichia coli 
(SILVA et al., 2009). Some Pcb bacterial cells have 



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https://doi.org/10.14393/BJ-v36n0a2020-48215 

probably remained viable and were capable of 
multiplying, even in the presence of these oils. 
Using electronic transmission microscopy, Lucas et 
al. (2012a) observed that clove, lemongrass, 
citronella, and melaleuca essential oils at 0.1% 
caused damages to the cell structure of X. 
vesicatoria, however, they were not capable of 
inhibiting bacterial growth, thus indicating that 
some cells remained viable and promoted bacterial 
multiplication. Additionally, other factors might 
influence bioactivity of essential oils, among which 
is the pathogen to be controlled and chemical 
composition of EOs. This chemical composition 
might be determined by cultivation conditions, 
climate, extraction method, harvest time, and organ 
harvested (BURT, 2004; FALEIRO et al., 2003), 

and a different chemical composition might take on 
different bioactive properties (TORRAS et al., 
2007). Guerra et al. (2014) and Silva et al. (2012a) 
did not observe a direct effect of sweet orange 
(Citrus sinensis L.) oil at a 0.5% concentration on 
Pcc. These results corroborate those obtained for 
sour orange oil at 0.75% in our study. 

Kale treated with lemongrass oil, before or 
after inoculation, showed INC of 0%, representing 
100% of disease control, significantly differing from 
the other treatments when applied prior to 
inoculation. However, when applied after 
inoculation, it did not differ from clove oil, which 
provided a control percentage of 71.42% (P≤0.05) 
(Table 2).  

 
Table 2. Effect of essential oils on reduced incidence of soft rot caused by Pectobacterium carotovorum subsp. 

brasiliensis on kale under greenhouse conditions. 
Treatments/ INC* % control4 
Concentrations (%) Pre2 Post3 Pre Post 
Lemongrass (0.5) 0.00a1 0.00a 100 100 
Clove (0.25) 50 b 25 ab 42.85 71.42 
Citronella (0.75) 75 b 62.5 bc 14.28 28.57 
Melaleuca (0.75) 75 b 62.5 bc 14.28 28.57 
Palmarosa (0.5) 75 b 50 bc 14.28 42.85 
Bergamot (1) 62.5 b 62.5 bc 28.57 28.57 
Orange (0.75) 62.5 b 87.5 c 28.57 0.00 
Ginger (1) 62.5 b 75 bc 28.57 14.28 
Rosemary (1) 62.5 b 50 bc 28.57 42.85 
Sage (1) 75 b 62.5 bc 14.28 28.57 
Control 87.5 b 87.5 c NA NA 
CV(%) 22.76 23.75 NA NA 
1Means followed by the same letter on the column do not differ from each other according to Duncan's test (P≤0,05).2 Treatment 

application prior to inoculation. 3Treatment application after inoculation. *Data transformed by the equation  to better fit the 
assumptions of the analysis of variance (ANOVA). Incidence (INC), expressed by the percentage of diseased plants; 4Compared to 
control treatment; Not applicable (NA). 

 
Essential oils are known for their direct 

antimicrobial activity and resistance inducing 
activity on plants (AMINIFARD; MOHAMMADI, 
2013; LUCAS et al., 2012a; LUCAS et al., 2012b; 
PEREIRA et al., 2008; PEREIRA et al., 2012). 
Lemongrass oil effectively reduced disease 
incidence in both application periods; this is 
probably related to its direct action and defense-
eliciting activity. A similar result was found by 
Lucas et al. (2012a) who observed that lemongrass 
oil at 0.1% applied pre- and post-inoculation 
promoted a significant reduction in bacterial spot of 
tomato. Guerra et al. (2014), also evaluating the 
potential of different essential oils on reduced soft 
rot severity in chinese cabbage caused by Pcc, 
observed that lemongrass oil at 0.5% significantly 
reduced severity compared to the control treatment, 

attributing this result to a potential resistance-
inducing activity. 

Clove, citronella, melaleuca, palmarosa, 
bergamot, rosemary, and sage oils did not show the 
expected results compared to the effective 
bioactivity showed in vitro assays. However, in 
vitro tests not always are representative as 
pathogens behave differently when they are both 
interacting with plants and exposed to 
environmental variables. In general, inhibitory 
concentrations observed in vitro must be increased 
when applied in vivo in order to maintain the same 
effectiveness (BURT, 2004). However, clove oil 
promoted a higher percentage of disease control, 
71.42%, when applied after inoculation, thus 
emphasizing its more effective direct antibacterial 
activity. Positive results using clove oil in plant 



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disease control have already been observed. Huang 
and Lakshman (2010) observed that clove oil at 
0.5% provided 100% control of tomato bacterial 
wilt. In addition, Amorim et al. (2011) observed 
25% effectiveness in banana moko control using 
clove oil at 3.75%. 

The major chemical component of clove oil 
is eugenol (COSTA et al., 2011; SCHERER et al., 

2009), whereas the major component of lemongrass 
oil is citral (isometric mixture of neral and geranial) 
(GUIMARÃES et al., 2011). Analysis of the 
chemical composition of clove essential oil showed 
high contents of eugenol (91.9%) (Table 3), and 
lemongrass oil showed high contents of neral 
(34.1%) and geranial (42, 9%) (Table 4). 

 
Table 3. Chemical composition of essential oil from clove 
Constituent AIlit

1 AIcalc
2 % ± SD3 

Eugenol 1356 1360 91,9±0,2 
β-caryophyllene 1417 1419 6,4±0,2 
α-humulene 1452 1455 1,3±0 
δ -cadinene 1522 1526 Trace 
caryophyllene oxide 1582 1587 0,4±0,1 
1AIlit= arithmetic index from literature; 

2AIcalc = calculated arithmetic index; 
3Means ±standard deviation from triplicate samples  

 
Table 4. Chemical composition of essential oil from lemongrass 

Constituent AILIT
1 AICALC

2 % ± SD3 

α-pinene 932 935 0,1±0,1 
Camphene 946 947 0,7±0,1 
6-methyl-5-hepten-2-one 981 985 1,9±0,2 
Limonene 1029 1032 0,2±0,1 
Z-β-ocimene 1032 1037 0,2±0,0 
E-β-ocimene 1044 1048 0,1±0,0 
4-nonanone - 1076 0,6±0,1 
Linalool 1095 1100 1,5±0,1 
Citronellal 1148 1150 0,4±0,0 
Borneol 1169 1171 0,2±0,0 
Isocitral 1177 1180 0,9±0,1 
α-terpineol 1186 1190 0,6±0,1 
Decanal 1201 1202 0,1±0,0 
Nerol 1227 1230 0,3±0,1 
Neral 1235 1237 34,1±0,2 
Geraniol 1249 1253 5,3±0,2 
Geranial 1264 1268 42,9±0,4 
Cyclosativene 1369 1373 0,2±0,0 
geranyl acetate 1379 1383 4,1±0,1 
β-cubebene/β-elemene4 1387/1389 1391 0,1±0,1 
β-caryophyllene 1417 1422 2,2±0,0 
α-humulene 1452 1459 0,4±0,1 
germacrene D 1484 1487 0,2±0,0 
δ-amorphene 1511 1518 1,0±0,1 
γ-cadinene 1513 1514 0,7±0,1 
caryophyllene oxide 1582 1589 0,3±0,1 
1AIlit= arithmetic index from literature; 

2AIcalc = calculated arithmetic index; 
3Means ±standard deviation from triplicate samples; 4co-

eluted compounds 
 

In vitro assays with lemongrass and clove 
essential oils and their major components showed 
differences as to their minimum Pcb growth-
inhibiting concentration (Table 5).  Lemongrass 

essential oil completely inhibited the growth of Pcb 
at 0.5, 0.25, 0.125, 0.0625%, whereas its chemical 
component citral promoted total inhibition at all 
concentrations tested. On the other hand, clove oil 



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promoted complete inhibition only at higher 
concentrations (0.25 and 0.125%) and its major 
chemical component, eugenol, did not effectively 

inhibit the growth of Pcb at any of the tested 
concentrations. 

 
Table 5. Minimum inhibiting concentrations (MIC) of lemongrass and clove essential oils and their major 

chemical components against Pectoctobacterium carotovorum subsp. brasiliensis. 

Concentrations (%) Clove oil    Eugenol  
Lemongrass 
oil 

Citral 

0.5 NA  NA1 -2 - 
0.25 - +3 - - 
0.125 - + - - 
0.0625 + + - - 
0.03125 + + + - 
0.015625 + + NA NA 
Growth control + + + + 
Medium control  -  -  -  - 
1(NA) Not applicable, 2(-) Absence of growth, 3(+) Microbial growth 
 

Similar results were obtained by Lee et al. 
(2012) where the eugenol was found as main 
component of clove oil, but the diameter of 
inhibition zone at major concentration (10 ul/disc) 
was lower than in the treatment with clove oil. 

In the current study, lemongrass oil at 
0.125% applied post-inoculation and the chemical 
compound citral at 0.125% applied prior or after 
inoculation provided the highest percentages of 
disease control (33.33, 50, and 100%, respectively). 
Plants treated with citral at 0.125% after inoculation 

showed an INC of 0%, significantly differing from 
the other treatments (P≤0,05), except for the 
treatment with citral 0.125% prior to inoculation, 
which showed INC of 37.5%. INC in treatments 
with clove oil at 0.125% and eugenol at 0.25% did 
not differ from the control treatment (P≤0.05). 
However, clove oil at 0.125% applied after 
inoculation showed better effectiveness than its 
major component, providing a percentage of disease 
control of 16.67% (Figure 1). 

 

 
Figure 1. Effect of lemongrass and clove essential oils and their major components (citral and eugenol) on soft 

rot caused by Pectobacterium carotovorum subsp. brasiliensis, in kale.  
Test (Control treatment); CL 0.125(clove oil at 0.125%); EU 0.25 (eugenol at 0.25%); LE 0.0625 (lemongrass at 0.0625%); 
LE 0.125 (lemongrass at 0.125%); CT 0.03125 (citral at 0.03125%); CT 0.0625 (citral at 0.0625%); CT 0.125 (citral at 
0.125%); Pre (treatment application prior to inoculation); Post (treatment application after inoculation). Means followed by the 
same letter do not differ according to Duncan's test (P≤0.05). 
 
The action mechanism of essential oils is 

usually associated to their major chemical 
components (BAKKALI et al., 2008), which show a 

wide activity spectrum, acting directly on pathogen 
structures (LUCAS et al., 2012a; NAZZARO et al., 



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2013), as well as activating plant defense 
biochemical pathways (PEREIRA et al., 2008). 

The antimicrobial activity of essential oils is 
not attributable to a unique mechanism but is related 
a several reactions involving the entire bacterial cell. 
More recently, Joshi et al. (2016) demonstrated that 
the phenolic volatiles carvacrol and eugenol act 
through the Quorum sensing machinery to inhibit 
specific virulence determinants in pectobacteria, 
such as biofilm formation and plant cell wall 
degrading enzymes (PCWDEs). 

Considering the results obtained, we might 
infer that citral is the component responsible for the 
bactericide activity of lemongrass oil on Pcb and 
soft rot control on kale in the assays conducted. 
Differently, eugenol did not prove to be responsible 
for clove oil effectiveness as it showed 
unsatisfactory results even at a higher concentration 
than clove oil. This suggests that the action of clove 
oil is provided by the synergic effect of its 

constituents. According to Burt (2004) and Bakkali 
et al. (2008), synergism is observed when the effect 
of combined substances is higher than their 
individual effects, once essential oils are complex 
mixtures of numerous molecules. 

 
CONCLUSION 

 
Lemongrass and clove essential oils proved 

to be a promising alternative to be employed as an 
integrated management method of soft rot of kale, 
thus reducing the use of agrochemicals, and 
consequently, contributing with reduced resistant 
microorganisms, risks to farmer's and consumers' 
health, and preserving the environment. 
 
ACKNOWLEDGMENTS 

 
The authors thank CAPES for their financial 

support for this work. 
 
 
RESUMO: O objetivo do estudo foi avaliar o efeito de óleos essenciais no controle da podridão mole 

em couve. Os óleos essenciais de cravo a 0,25%, capim-limão e palmarosa a 0,5%, citronela, melaleuca e 
laranja a 0,75%, bergamota, alecrim, sálvia e gengibre a 1% foram avaliados na inibição in vitro de 
Pectobacterium carotovorum subsp. brasiliensis (Pcb) e controle da podridão mole em couve, pulverizados 72 
horas antes ou sete horas após a inoculação. Os óleos essenciais de cravo, citronela, bergamota, alecrim, 
palmarosa, sálvia, melaleuca e capim-limão inibiram completamente o crescimento de Pcb. O óleo de capim-
limão (0,5%) promoveu 0% de incidência (INC) da doença (percentual de controle de 100%), em ambos os 
períodos de inoculação. O óleo de cravo (0,25%) proporcionou menor INC (25%) quando aplicado após 
inoculação (percentual de controle de 71,42%). Os óleos essenciais de capim-limão e cravo foram analisados 
por GC/FID (cromatografia gasosa/detector por ionização de chama) e por GC/MS (cromatografia gasosa/ 
espectometria de massas). Os componentes majoritários foram eugenol (91,9%) no óleo de cravo e citral (neral-
34,1% e geranial- 42,9%) no óleo de capim-limão. A concentração inibitória mínima (CIM) dos óleos 
essenciais de capim-limão e cravo e de seus componentes majoritários (citral e eugenol, respectivamente) foi 
determinada por meio da técnica de macrodiluição em caldo, bem como foram avaliados, em diferentes 
concentrações, no controle da podridão mole em couve, pulverizados conforme descrito acima. A concentração 
inibitória mínima (CIM) foi de 0,03125% para o citral, e de 0,0625 e 0,125% para os óleos de capim-limão e 
cravo, respectivamente. O eugenol não apresentou CIM. O óleo de capim-limão a 0,125% (pós-inoculação) e o 
citral (0,125%), em ambos os períodos de inoculação, proporcionaram os maiores percentuais de controle 
(33,33; 50 e 100%, respectivamente). O óleo de cravo a 0,125% (pós-inoculação) mostrou maior eficiência que 
o eugenol (0,25%), promovendo um percentual de controle de 16,67%. Os óleos essenciais de capim-limão e 
cravo destacaram-se na eficiência de controle da podridão mole em couve, sugerindo que esses óleos têm 
potencial para serem utilizados como agentes antibacterianos. 

 
PALAVRAS-CHAVES: Brassica oleracea var. acephala. Controle alternativo. Capim-limão. Citral. 

Cravo. Eugenol. P. carotovorum subsp. brasiliensis. 
 
 

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