manuscript


doi: 10.5599/admet.5.2.388 126 

ADMET & DMPK 5(2) (2017) 126-134; doi: 10.5599/admet.5.2.388 

 
Open Access : ISSN : 1848-7718  

http://www.pub.iapchem.org/ojs/index.php/admet/index   

Original scientific paper 

Cellular energy status is indispensable for perillyl alcohol 
mediated abrogated membrane transport in Candida albicans 

Moiz A. Ansari, Zeeshan Fatima* and Saif Hameed* 

Amity Institute of Biotechnology, Amity University Haryana, Gurgaon (Manesar)-122413, India.  

*Corresponding Authors: Dr. Saif Hameed and Dr. Zeeshan Fatima, Amity Institute of Biotechnology, Amity University 
Haryana, Gurgaon (Manesar)-122413, India. Email: saifhameed@yahoo.co.in, drzeeshanfatima@gmail.com ; Tel.: +91-
124-2337015, Ext: 1116. 

Received: April 21, 2017; Revised: May 23, 2017; Published: June 22, 2017  

 

Abstract 

The prevalence of fungal infections and their resistance patterns in fungal isolates fro m large number of 
patients with impaired immunity still remains poorly monitored. In spite of significant advances being 
made in the improvement of antifungal drugs, only a limited number of antifungal drugs are currently 
available. The present study aimed to gain further mechanistic insights into the previously described 
anticandidal activity of natural monoterpenoid, perillyl alcohol (PA). We found that cellular transport 
across cell membrane was abrogated in presence of PA. This was demonstrated by dose and time 
dependent enhanced cellular leakage accompanied by inhibited sodium and potassium cellular transport. 
In addition, we found disrupted pH homeostasis which was depicted by enhanced extracellular pH. We 
further observed that mitochondrial energy status is highly integrated with the antifungal activity of PA. 
This was evident from inhibited propidium iodide (PI) uptake in presence of sodium azide and di-nitro 
phenol (DNP) which showed no fluorescence when treated with PA. Moreover, we observed that PA leads 
to disrupted mitochondrial membrane potential. Additional cell death hallmarks in response to PA such as 
nuclear fragmentation was also observed with 4',6-diamidino-2-phenylindole (DAPI) staining. Taken 
together, PA is a novel candidate that deserves further attention to be exploited as effective antifungal 
agent of pharmacological interest. 

Keywords 

Perillyl alcohol; sodium transport; potassium transport; pH homeostasis; mitochondria; ATP; DNA damage 

 

Introduction 

Candida albicans being an opportunistic human fungal pathogen resides commensally within the host. 

However, under immune-compromised conditions such as organ transplantation, chemotherapy and 

diabetes, it turns up into a deadly pathogen [1]. According to the recent finding, around 1.5 million people 

died per annum due to invasive fungal infections [2] and among all fungal pathogens Candida species leads 

the toll for the cause of the mortality related to the mycotic death throughout the world [3]. With the 

limited repertoire of current therapeutics which includes antifungal drugs from three major classes; azoles, 

polyenes and echinocandins, the utility of these drugs are restricted due to high cost and sometimes host 

toxicity. Moreover, emergence of drug resistant strains due to the phenomenon of multidrug resistance 

http://www.pub.iapchem.org/ojs/index.php/admet/index
mailto:saifhameed@yahoo.co.in
mailto:drzeeshanfatima@gmail.com


ADMET & DMPK 5(2) (2017) 126-134 Perillyl alcohol mediated abrogated membrane transport in C. albicans 

doi: 10.5599/admet.5.2.238 127 

(MDR) has compounded the problem and became major obstacle against effective therapeutics [4]. 

Therefore, the flux towards phytochemical research to circumvent the problem of MDR in need of new 

antifungals is in serious vigilance nowadays.  

We previously demonstrated that perillyl alcohol (PA) is a natural benzylic monoterpenoid (Fig. 1), 

similar to its class terpenoid [5], it also showed immense antifungal potential against human pathogen C. 

albicans as well as non-albicans species of Candida [6]. However, PA is immensely studied for its 

anticancerous activities and recently reported as suitable for brain tumor therapy [7-9]. Moreover, PA is 

FDA approved food additive that can be safely consumed without any toxic effect. The current study 

enhances the knowledge of mechanistic action of PA induced membrane disruption against C. albicans 

leading to the altered cationic concentration and demonstrates that cellular energy status is indispensable 

for functional anticandidal activity of PA. Additionally, we explored that PA leads to disrupted 

mitochondrial membrane potential and nuclear fragmentation.  

OH

CH2H3C  
Figure 1. Chemical structure of PA 

Experimental  

Materials 

Yeast extract, di-nitro phenol (DNP) and peptone were purchased from Himedia, India. D-Glucose, 

dimethyl sulfoxide (DMSO), rhodamine B, NaN3 and KCl were purchased from Thermofisher. Fluconazole 

(FLC) DAPI and PA were purchased from Sigma. 

Cellular leakage 

Analysis of loss of cellular material absorbing at 260 nm from Candida cell was performed using the 

method described elsewhere with little modifications [10]. Briefly, Candida cells were grown in YPD at 30°C 

for 48 h and cell suspension (OD600 as 1) was prepared in 10 mL PB. Furthermore, this suspension was 

treated with different concentrations (1 ×, 2 ×, and 4 × MIC) of PA and FLC for 1 h or at fixed concentration 

(1× MIC) for different time intervals (30, 60, 90 and 120 min). Untreated sample was run as negative 

control. After treatment, samples were centrifuged at 10,000 rpm for 10 min at 4 ᵒC, and the absorbances 

of supernatants were read at 260 nm using UV–vis spectrophotometer (VSI-501, India). 

Intracellular Na
+
 concentration 

Intracellular sodium ion concentration was obtained as described elsewhere with slight modification 

[11]. Briefly, cells were pre-grown at 30 ᵒC in YNB medium overnight. The cells were inoculated into 50 mL 

of YNB medium (with and without drug) to obtain OD600 as 0.05 and grown at 30 ᵒC to obtain OD600 

between 0.17–0.3; and the intracellular sodium content was measured. To estimate the intracellular Na
+
 



Ansari, Fatima and Hameed  ADMET & DMPK 5(2) (2017) 126-134 

128  

concentration, cell pellets, after harvesting and washing with water, were suspended in 18 mL of 

incubation buffer (20 mmol/L MES and 0.1 mmol/L MgCl2, pH 5.5 adjusted by solid Ca(OH)2). Cells were 

washed twice with washing buffer (20 mmol/L MgCl2) and lysed in 5 mL of extraction buffer (10 mmol/L 

MgCl2 and 0.2 mol/L HCl). Flame photometer (Systronics, India) was used to determine the sodium content 

in the extracts.  

K
+
 leakage estimation  

Estimation of extracellular K
+
 leakage from the fungal cell was performed using the method described 

elsewhere with little modifications [11]. Briefly, Candida cells were grown in 100 mL YPD at 30 °C, 120 rpm 

for 24 h. Cell pellets were harvested at 5000 rpm for 5 min and washed three times with sterile phosphate 

buffer (PB) and suspended in 10 mL of PB. 500 μL of the cell suspension was used to determine dry cell 

weight. 2 mL of cell suspension was mixed with 2 mL of PB containing desired concentration (1 ×, 2 × and 4 

× MIC) of test agents and incubated for 4 hr. After treatment samples were centrifuged at 10,000 rpm for 

10 min, and supernatant was removed and stored for the determination of extracellular K
+
 content 

released into the medium. The K
+
 concentration was estimated by Flame Photometer (Systronics, India) 

using potassium filter. 

PM-ATPase mediated proton pumping 

The proton pumping activity of C. albicans was estimated by monitoring the glucose-induced 

acidification of the external medium due to pH changes as previously reported [12]. Briefly, overnight 

cultures of C. albicans were grown in YEPD broth for 18 h at 30 °C. The cells were collected by 

centrifugation at 3000 g for 5 min at 4 °C and washed with sterile distilled water and 50 mM KCl (pH 6.5). 

The washed cells were resuspended in 40 ml of 50 mM KCl (pH 6.5) and incubated at 4°C overnight to 

deplete their carbon reserves. The carbon-starved cells were harvested by centrifugation, and 

approximately 1.0 g wet weight of the pellet was resuspended in 40 ml of 50 mM KCl (pH 6.5). To a 40 ml 

aliquot of the cell suspension, PA at MIC80 was added to obtain the required concentration and mixed 

well, and the volume was adjusted to 45 ml with 50 mM KCl. The cell suspension was incubated at room 

temperature with gentle stirring for 10 min, and then 5 ml of 20 % glucose (final concentration, 55 mM) 

was added and the pH of the external medium was monitored at regular intervals for 40 min at indicated 

time points. The experiment was performed in the presence of a comparable concentration of the solvent 

DMSO (control) to measure the extent of acidification of the external medium in the absence of PA. 

Propidium iodide uptake 

Propidium iodide, is a dye impermeable to membrane and is widely used to differentiate cells that have 

damaged plasma membranes from healthy cells [13]. To evaluate the effect of PA on the fungal plasma 

membrane, C. albicans SC5314 cells (approximately 1×103 CFUs/ml) were obtained from exponential 

phase and exposed to PA (225 µg/ml) for 3 h at 30 °C with gentle shaking. Subsequently, cells were 

harvested, incubated with propidium iodide for 15 min, and observed by Coslab fluorescence microscope.  

Mitochondrial membrane potential (mtΨm) 

Rhodamine B dye (Molecular Probes) was used to detect the change of mitochondrial membrane 

potential [14]. C. albicans (SC5314) cells were treated with PA (225 µg/ml) overnight at 30 °C. The treated 

cells were washed in PBS and then suspended in 40 nM rhodamine B for 20 min at 37 °C. The cells were 

centrifuged at 500 g for 5 min and the pellet was re-suspended in 1 mL PBS. The cells were analyzed using 

Coslab fluorescence microscope and fluorescent intensity was measured through Image J software. All 



ADMET & DMPK 5(2) (2017) 126-134 Perillyl alcohol mediated abrogated membrane transport in C. albicans 

doi: 10.5599/admet.5.2.238 129 

observations were confirmed with 3 independent cell cultures. 

DAPI staining 

Cells were stained with DAPI to detect nuclear fragmentation as discussed elsewhere [15]. The strains 

were grown in YEPD overnight in presence of PA at 30 °C. Fragmented nuclei were identified by staining 

with 0.1µg/mL DAPI for 15 min. The stained cells were collected then washed twice with 1 % BSA in PBS for 

5 min followed by a five minute rinse in 0.1 % BSA in PBS. Cells were visualized with Coslab fluorescence 

microscope. All observations were confirmed with 3 independent cell cultures. 

Results and Discussion 

Membrane disruption by PA leads to cellular leakage in C. albicans 

In our previous study we have determined that anticandidal effect of PA is mediated through 

membrane perturbation [6]. In this study we have explored the severity of this damage in terms of 

transport across cell membrane. For this, cellular leakage across membrane was estimated by the leakage 

of intracellular components. A cellular component that absorbs light of 260 nm wavelength signifies for a 

particular class of out-flowing components, mainly nucleotides which include uracil compounds revealing 

strongest absorbance [10]. In the PA treated cells similar to FLC, the absorbance of intracellular content 

was observed to be increased for PA in dose dependent manner (Figure 2a). We further confirmed the 

cellular leakage by studying time kinetics at MIC concentration of PA. We observed the elevation in 

absorbance from the cells treated with PA and FLC with respect to time till 120 min (Figure 2b). This proves 

that the PA treatment enhances the leakage of cellular contents through membrane disruption. 

 

Figure 2. Effect of PA and FLC on 260nm absorbing material in C. albicans: (a) concentration dependent, (b) 
time dependent. 

PA affects Na
+
 transport and pH homeostasis in C. albicans 

Enhanced cellular leakage in presence of PA prompted us to study the transport of ions across the 

membrane more closely. To verify that the leakage of cellular content due to PA treatment is also affecting 



Ansari, Fatima and Hameed  ADMET & DMPK 5(2) (2017) 126-134 

130  

cationic concentration, the intracellular Na
+
 concentration was evaluated. It was observed that the Na

+
 

concentration was significantly decreased in the PA treated cells which suggests that PA induced 

membrane disruption possibly affects Na
+
 transport across the membrane (Figure 3a).  

The two main transporters in yeast that are accountable for alkali-metal-cation permeability across the 

membrane are Na
+
/H

+
 antiporter and a Na

+
-ATPase. Both transporters harmonize each other to support 

detoxification. The Na
+
/H

+
 antiporter is active during low extracellular pH however Na

+
- ATPase is highly 

active at neutral and higher extracellular pH [16]. Thus we checked that if the decrease in Na
+
 

concentration is linked with some changes in extracellular pH. It was seen that the PA treatment leads to 

the significant increment in the extracellular pH in the Candida cells (Figure 3b). While convalescing 

themselves during starvation, Candida cells pump intracellular protons outside the cell through plasma 

membrane ATPase, utilizing available number of ATP after the addition of glucose to non-growing nutrient 

deficient cells. Thus, proton pumping action of the ATPase could be the reason for acidification of the 

medium. This confirms that PA treated Candida cells lost the ability to pump intracellular protons to the 

external medium may be due to inhibition in plasma membrane ATPase thereby elevating the pH of the 

external medium and diminishing the intracellular Na
+
 concentration. 

0

20

40

60

80

100

120

140

Control NaCl Control PA NaCl PA

N
a

+
in

(n
m

/m
g

 d
ry

 m
a

ss
)

*

*

0

1

2

3

4

5

6

0 10 20 30 40 50 60

p
H

Time (min)

Control

PA

a

b

* * * * * *

 

Figure 3. Effect of PA on membrane permeability in C. albicans: (a) effect of PA on intracellular Na
+
 

concentration (b) effect of PA on the glucose-dependent acidification of the medium by C. albicans cells. 
Mean of pH ± SD of three independent sets of experiments are shown in absence (control) and presence of PA 

with respect to time (minutes) and *P value <0.05 is considered to be significant. 

PA affects K
+
 transport in C. albicans 

As a known matter of fact, Na
+
 transport across cellular membrane is linked with K

+
 transport. 

Moreover, the concentration both of Na
+
 and K

+
 plays a critical role to maintain the membrane potential in 

the cells [17]. In fact dysregulation of ion homeostasis forms the basis of cell death for many terpenoids. 



ADMET & DMPK 5(2) (2017) 126-134 Perillyl alcohol mediated abrogated membrane transport in C. albicans 

doi: 10.5599/admet.5.2.238 131 

Thus we checked whether there are also some changes in K
+
 transport in presence of PA. This was evident 

from the elevated level of intracellular and diminished levels of extracellular K
+
 concentration respectively 

in PA treated cells (Figure 4). This result suggests that the Na
+
- K

+
 antiporters may be affected in presence 

of PA. From these observations, one may also speculate that enhanced membrane permeability due to PA 

could cause dissipation of ionic gradient across cell membrane leading to membrane depolarization, 

however, further work is needed to confirm. 

0

0.1

0.2

0.3

0.4

0.5

0.6

0.7

0.8

Control PA-MIC PA 2XMIC PA 4XMIC

K
+

C
o

n
c

(n
m

/m
g

 d
ry

 m
a

ss
)

Internal

External

 

Figure 4. Effect of PA on intracellular and extracellular K
+
 concentration in C. albicans 

Membrane perturbations due to PA is energy dependent 

Sodium azide and DNP is known for ATP reducing property by decreasing the amount of ATP in Candida 

cells targeting cytochrome oxidase of mitochondria and binds with the heme a3 iron and CuB in the 

reduction site of oxygen [18,19]. F1 domain is also an important component of mitochondria for its ATP 

generation ability. It is the assembly of alternatively arranged three α and three β subunits around the 

central stalk, which is made of γ, δ and ε subunits. Azide binds to the F1 catalytic domain and inhibits ATP 

hydrolysis [20]. To study whether the membrane disruptive action of PA is energy dependent, an assay was 

performed through PI uptake of sodium azide treated cells in the presence of PA (Figure 5). We observed 

that in cells that were not treated by sodium azide or DNP, PI uptake was efficient and showed 

fluorescence when treated with PA. However in the sodium azide or DNP treated cells this effect of PA was 

reverted and no cell was stained with PI. These observations not only confirmed non-intact membrane 

confirming our previous hypothesis of membrane disruption [6] but also suggests that the intracellular 

localization and the membrane damaging effect of PA is energy dependent. 

PA alters mitochondrial membrane potential (mtΨm) in C. albicans 

In our previous study we documented that PA inhibits the mitochondrial enzyme functioning [6]. 

Moreover, mtΨm is a sensitive indicator of the energy status of the mitochondria which is the result of an 

electrochemical gradient maintained through the electron transport chain and also plays key role in ATP 

synthesis which is derived from mitochondrial oxidative phosphorylation [21]. Hence, we study the effect 

of PA on mtΨm by employing Rhodamine B probe as described in material and methods. Rhodamine B 

spreads throughout the biological membranes in response to the Ψm. The change in mitochondrial 

potential (∆Ψm) directly correlates with the increase or decrease in ATP content of the cells, where higher 

the ∆Ψm more will be the cellular ATP level [14]. In the intact cells, the fluorescence of rhodamine B tends 

to decrease because of the formazan, quencher of rhodamine B which naturally accumulates in 

mitochondrial matrix, hence ∆Ψm will be more. However in mitochondria disrupted cells the ∆Ψm will be 



Ansari, Fatima and Hameed  ADMET & DMPK 5(2) (2017) 126-134 

132  

less due to no quenching in fluorescence depicted by red signals [14,22]. Our result clearly demonstrates 

that PA treated Candida cells showed more fluorescence (Figure 6) which suggests that PA alters the mtΨm 

in C. albicans. 

 

 

Figure 5. Effect of energy depletion on anticandidal activity of PA. Fluorescent microscopy of PI in presence of 
5mM NaN3 and DNP. 

 

Figure 6. Effect of PA on mtΨm: a) Fluorescent microscopy of Rhodamine B for analysis of mtΨm in presence of 
PA b) Fluorescent intensity of untreated (control) and PA treated cells and *P value <0.05 is considered to be 

significant. 

PA induces nuclear fragmentation in C. albicans 

Mitochondria dysfunctioning is one of the major causes that lead to the DNA damage [15]. Moreover, 

the leakage of intracellular content primarily nucleotides from this study and hypersensitivity towards PA 

in presence of DNA damaging agent from previous observation was enough evidence to study nuclear 

fragmentation [6]. Hence we checked the nuclear fragmentation using DAPI staining as described in 

material and methods. DAPI is a fluorescent dye that binds to the AT site between the minor groove of 

DNA. The fluorescence can be evaluated with irregular margin and condensed chromatin [15]. We found 

that the cells treated with PA showed nuclear fragmentation which could be linked with DNA damage 

(Figure 7). Since damaged DNA cannot replicate owing to prevention of mutations, cell cycle is arrested 

[23]. This observation is also commensurate with our earlier findings which showed PA induced down 



ADMET & DMPK 5(2) (2017) 126-134 Perillyl alcohol mediated abrogated membrane transport in C. albicans 

doi: 10.5599/admet.5.2.238 133 

regulation of several DNA repair genes and cell cycle arrest [6]. 

C
o

n
tr

o
l

P
A

Bright Fluorescence Merged

10µm 10µm 10µm

5µm 5µm 5µm

 

Figure 7. Effect of PA on nuclear fragmentation. Fluorescent microscopy of DAPI for detection of nuclear 
fragmentation in presence of PA. 

Conclusion 

Taken together, the antifungal potential of PA not only provides an opportunity to aid PA develop into 

pharmacologically acceptable and efficient antifungal but also helps in deciphering novel regulatory circuits 

governing drug resistance in C. albicans. This is evident by wide range of antifungal targets of PA in 

comparison to single mode of action of known antifungals such as azoles. Further studies are warranted to 

competently employ phytotherapeutics such as PA in treating Candida infections.  

Acknowledgements 

S.H. thank for the financial assistance in the form of Young Scientist award (SR/FT/LS-12/2012) from 

Science and Engineering Research Board (SERB), New Delhi. We are grateful to Joseph Heitman for 

providing Candida SC5314 reference strain as generous gift. We thank Rajendra Prasad, Dean, Faculty of 

Science, Engineering and Technology for encouragement. 

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