Impact of host factors on susceptibility to antifungal agents


doi: https://dx.doi.org/10.5599/admet.1164   153 

ADMET & DMPK 10(2) (2022) 153-162; doi: https://doi.org/10.5599/admet.1164  

 
Open Access : ISSN : 1848-7718  

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

Original scientific paper 

Impact of host factors on susceptibility to antifungal agents 

Balbina Plotkin
1
*, Monika Konaklieva

2 
 

1
Department of Microbiology and Immunology, College of Graduate Studies, Midwestern University, Downers Grove, IL 

60515 
2
Department of Chemistry, American University, College of Arts and Sciences, 4400 Massachusetts Ave, NW, 

Washington, DC 20016  

*Corresponding Author:  E-mail: bplotk@midwestern.edu; Tel.: +1-630-515-6163; Fax: +1-630-515-7249 

Received: November 08, 2021; Accepted: December 30, 2021; Published: January 07, 2022  

 

Abstract 

An obstacle to drug development, particularly in this era of multiple drug resistance, is the under-
appreciation for the role the host environment plays in microbial response to drugs. With the rise in fungal 
infection and drug resistance, particularly in individuals with co-morbidities, the influence serum and its 
components have on antimicrobial susceptibility requires assessment. This study examined the impact of 
physiologically relevant glucose and insulin levels in the presence and absence of 50 % human plasma on 
MICs for clinical isolates of Candida lusitaniae, Candida parapsilosis, Candida albicans, Candida tropicalis, 
Candida glabrata, Candida krusei and Cryptococcus neoformans. The addition of insulin or glucose at 
physiologic levels in RPMI medium alone altered the MIC in either a positive or negative fashion, 
depending on the organisms and drug tested, with C. glabrata most significantly altered with a 40, >32- 
and 46-fold increase in MIC for amphotericin B, itraconazole and miconazole, respectively. The addition of 
candida-antibody negative plasma also affected MIC, with the addition of glucose and insulin having a 
tandem effect on MIC. These findings indicate that phenotypic resistance of Candida and Cryptococcus can 
vary depending on the presence of insulin with glucose and plasma. This modulation of resistance may 
help explain treatment failures in the diabetic population and facilitate the development of stable drug-
resistant strains. Furthermore, these findings indicate the need for a precision approach in the choice of 
drug treatment and drug development. 

©2022 by the authors. This article is an open-access article distributed under the terms and conditions of the Creative Commons 
Attribution license (http://creativecommons.org/licenses/by/4.0/). 

Keywords 

Insulin; glucose; human serum; Candida; Cryptococcus. 

 

Introduction 

Phenotypic response to environmental shifts is essential for microbial survival and is of particular 

importance with respect to changes that occur in vivo, which affect response to antimicrobial agents. The 

potential changes in response to drugs upon growth within the host could both be responsible for 

treatment failures and provide the potential for novel drug development. Thus, it is essential to define 

these phenotypic responses to host factors, and metabolic conditions, to predict effective drug design and 

utility.  

A common metabolic condition associated with increased risks for infections is type II diabetes. People 

https://dx.doi.org/10.5599/admet.1164
https://doi.org/10.5599/admet.1164
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mailto:bplotk@midwestern.edu
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Plotkin and Konaklieva  ADMET & DMPK 10(2) (2022) 153-162 

154  

with type II diabetes can exhibit hyperglycemia, hyperinsulinemia, and/or combined hyperglycemia-

hyperinsulinemia, as a result of insulin intolerance [1,2]. A metabolic immunosuppressive condition, type II 

diabetes, places individuals at increased risk for fungal diseases [3-6]. Thus, during the infectious process, a 

pathogen can be exposed to elevated levels of insulin and/or glucose as compared to the metabolically 

normal host.  

A critical disconnect regarding predicted sensitivity via in vitro testing and efficacy is the lack of 

congruency with the metabolic disorders most commonly at risk for fungal infections, e.g., type II diabetes, 

since antimicrobial activity testing is predicated on the host being in a normal metabolic state. Most 

studies examining serum effects are focused on the impact normal serum/plasma has on antimicrobial 

activity, or on the effect of high glucose (2 mg/dl) concentrations, which are reported to affect the ability 

of antifungal agents to bind to their targets [7-9]. To date, studies of glucose-fungal-antifungal agent 

interactions fail to take into consideration the concomitant presence of insulin with glucose. This becomes 

important since organisms across the taxonomic kingdoms are reported to produce and/or react to insulin 

[10-16]. In Candida albicans, insulin has been associated with increased expression of virulence-associated 

morphological transition, from blastospore to hyphal production [17]. The mechanism via which insulin 

promotes yeast to hyphal transition is by enhancing uptake of proline by C. albicans. Conversely, glucose 

concentrations can affect morphogenic expression [18,19]. In the present study, the effect on in vitro 

antifungal activity in the presence and absence of human plasma by insulin and/or glucose, at levels 

analogous to those reported in type II diabetes, was determined.  

Experimental  

Fungal species and culture  

Candida lusitaniae, Candida parapsilosis, Candida albicans, Candida tropicalis, Cryptococcus 

neoformans, Candida glabrata, and Candida krusei clinical isolates (a generous gift from the lab of Paul 

Schreckenberger, Loyola University Medical School) were maintained at -70 °C and passed at least twice on 

Sabouraud dextrose agar (SDA) prior to testing.  

Drug testing 

Antifungal activity determinations were done using the standard CLSI (NCCLS M27-T) microbroth 

dilution method with modifications [20,21]. Susceptibility to amphotericin B (Sigma-Aldrich), fluconazole 

(Pfizer), itraconazole (Janssen Pharmaceuticals), and miconazole (Sigma-Aldrich) was determined using 

antifungal agents constituted and serially diluted. Microtiter plates containing the serial dilutions of the 

antifungal agents were made as recommended and stored frozen (-70 °C; < 7 days) or refrigerated 

(itraconazole; < 3 days). Antifungal activity in the presence or absence of normal human plasma (type A, Rh 

+), was performed using 2X RPMI medium (50 % v/v). Plasma was screened for specific fungal antibodies, 

as described below, by indirect immunofluorescent microscopy (FITC-Protein A) to detect the presence of 

yeast-bound antibodies. Minimum lethal concentrations (MLC) were determined by plating 10 µl of all 

wells showing no growth onto SDA.  

To simulate glucose and insulin levels reported for type II diabetes, glucose (285 mg/dl) and/or insulin 

(200 µU/ml), final concentrations were tested in RPMI with and without 50 % plasma medium. Endogenous 

glucose levels were determined using a kit according to the manufacturer’s instructions (Sigma-Aldrich). 

The reported mid-range value for normal human insulin levels (18 µU/ml) was used as the basis for 

calculating the amount of insulin to add. Glucose and/or insulin in RPMI medium had no effect (data not 



ADMET & DMPK 10(2) (2022) 153-162 Host factors on susceptibility to antifungal agents 

doi: https://dx.doi.org/10.5599/admet.1164   155 

shown) on fungal growth kinetics as determined by both turbidimetric measurements (absorbance 560 

nm) and a direct microscopic count of yeast and hyphal forms. The growth rates and the relative 

production of yeast and hyphal forms during growth in RPMI medium with and without glucose and/or 

insulin were measured to determine if changes in the MIC and MLC of the antifungal agents tested in the 

presence of glucose and/or insulin could be correlated to alterations in fungal growth. No significant 

differences in generation time or proportion of yeast and hyphal forms were measured. The differences in 

the rate of growth between organisms also appear to be unrelated to the alterations in MIC and MLC 

measured in the presence of glucose and/or insulin and to the relative susceptibility of the organisms. The 

antifungal agents were not exposed to the media supplements (glucose and insulin) until organisms were 

added to the agent. Sterility controls and growth controls for all test conditions were run simultaneously 

with the tests.  

To determine antifungal activity in the presence of normal human plasma (type A, Rh +), a modified 

protocol was developed. Plasma was screened for specific fungal antibodies by indirect immunofluorescent 

microscopy using FITC-Protein A to detect the presence of bound antibodies. Equal volumes of normal 

human plasma were added to 2X NCCLS RPMI medium to yield a medium that contained 1X RPMI with 50 

% v/v of plasma. For glucose in a medium containing 50 % plasma (plasma medium), glucose and/or insulin 

were added to ensure equivalent amounts were used for the medium alone. Antifungal agents were 

prepared, as described above, in this plasma medium. Antifungal activity in the presence and absence of 

plasma was determined on the same day using the same drug lot and microbial suspension. Minimum 

inhibitory concentrations (MIC) were determined by visual inspection of the wells at 24, 36 and 72 hrs after 

initiation of the incubation period. Minimum lethal concentrations (MLC) were determined by plating 10 μl 

of all wells showing no growth onto Sabouraud dextrose agar (Difco) at 36 hrs post-initiation of the 

incubation period.  

Results and discussion 

Amphotericin B 

The overall effect of insulin and glucose alone or together were drug and fungal species-specific (Table 

1). Amphotericin B (AmB) activity was relatively unaffected by insulin and glucose combined with the 

exception of C. glabrata (40-fold greater MIC than RPMI alone; Table 1). For AmB, the presence of plasma 

with and without glucose and/or insulin decreased the MIC < 4 fold of that measured for medium alone for all 

organisms, with the exception of C. glabrata and C. neoformans. For amphotericin B in plasma supplemented 

with glucose, its MIC increased from four to a maximum of 32-fold for C. krusei compared to medium with 

plasma alone (Table 2). Like with itraconazole, with amphotericin B, there was a difference between the MIC 

and MLC. The MLC of C. albicans was 32-fold higher than the MIC in the presence of plasma without 

supplements. The plasma effect on the candidal MLC was overcome by the addition of glucose and/or insulin. 

The MLC was within 2-fold of the amphotericin B MIC for all other isolates. Comparison of medium with plasma 

to medium alone (Table 3) indicated that the addition of 50 % normal human plasma to medium decreased 

the MIC of amphotericin B > 16-fold for all isolates, except C. lusitaniae and C. krusei, which were unaffected.  

5-Fluorocytosine 

The MIC of 5-fluorocytosine in media supplemented with glucose alone either was unaffected (C. 

lusitaniae, C. neoformans, and C. krusei), or decreased (Table 1). The effect of insulin on the MIC in media 

was also isolate-dependent. Insulin alone had the greatest negative impact on 5-fluorocytosine activity for 

C. tropicalis (~25-fold), with C. parasilosis and C. glabrata exhibiting a ~6-fold increase in MIC. In general, 

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the MIC of all isolates in medium supplemented with glucose and insulin was decreased compared to 

medium alone, although the degree of decrease was isolate-dependent. The presence of plasma (50 % v/v 

RPMI medium) resulted in an increase in 5-fluorocytosine MIC maximally for C. parasilosis, (32-fold) and C. 

tropicalis (16-fold), as compared to RPMI medium alone for all isolates, with the exception of C. glabrata, 

whose MIC was markedly decreased (Table 2). The MLC in media, and in the presence of plasma with or 

without supplements correlated within two-fold of the MIC, with the exception of C. glabrata, which in the 

presence of plasma was four-fold higher than that measured for media alone. The addition of insulin to 

both medium alone, and with plasma, resulted in an increase in the MIC to a maximum increase measured 

for C. glabrata when exposed to 5-fluorocytosine (40-fold increase; 25 μg/ml in media with plasma and 

insulin vs. 0.625 μg/ml media with insulin alone). Comparison of medium with plasma, to medium alone 

(Table 3), indicated that the addition of 50 % normal human plasma to medium decreased the MIC 25-fold 

for C. tropicalis only (0.25 μg/ml media with 50 % plasma vs. 6.25 μg/ml RPMI medium alone).  

Fluconazole 

Supplementation of RPMI medium containing plasma with insulin, resulted in a 1024-fold increase in 

MIC of C. albicans to fluconazole with the resultant reclassification from sensitive to resistant. However, 

addition of glucose to insulin restored the sensitivity of C. albicans to fluconazole. The only change in 

classification with regards to fluconazole was a shift from sensitive to sensitive-dose dependent for C. 

lusitaniae when both glucose and insulin were present. In contrast, the presence of plasma resulted in a 

shift from resistant to sensitive for C. neoformans with respect to fluconazole.  

Itraconazole 

For itraconazole, the addition of glucose and/or insulin to RPMI medium did not significantly alter the 

MIC or MLC (< 2-fold of MIC in medium alone) for all organisms with the exception of C. lusitaniae and C. 

glabrata (Table 1). The addition of glucose and/or insulin to RPMI medium resulted in a MIC for C. glabrata 

that exceeded the drug solubility level (see Table 1). The effect of glucose on the C. lusitaniae response to 

itraconazole was opposite of its effect when combined with insulin (8-fold higher MIC for glucose alone vs. 

8-fold lower MIC for glucose and insulin), indicating that there may be an interactive effect of glucose and 

insulin. The presence of plasma alone had a modest (< 4-fold) effect on the MIC for all isolates with the 

exception of C. glabrata, where the MIC was decreased nearly 103-fold as compared to that measured for 

medium alone (Table 2 and 3). The addition of glucose and/or insulin to plasma did not significantly alter 

the MIC or MLC of itraconazole for all organisms, except for C. neoformans, where supplementing plasma 

with insulin resulted in a 20-fold decrease in the MIC. Interestingly, the MLC for all conditions tested 

differed < 2-fold from the MIC for all organisms, except for C. neoformans (8-fold higher than MIC in 

plasma supplemented with glucose and insulin) and C. glabrata (128-fold higher than MIC in plasma 

supplemented with glucose). The MLC for C. neoformans in RPMI alone was less affected, exhibiting a five-

fold decrease in MLC compared to an MLC measured in plasma alone, or plasma supplemented with 

glucose. This differential effect of the presence of plasma, as compared to medium alone, may explain the 

treatment failure reported despite laboratory-confirmed sensitivity [22-27]. 

Miconazole 

The combination of glucose and insulin resulted in a significant alteration in the miconazole MIC for all 

isolates except C. parapsilosis. Resistance to miconazole was increased by the presence of insulin and 

glucose to a maximum of 46-fold and 23-fold over that of RPMI alone for C. glabrata and C. krusei, 



ADMET & DMPK 10(2) (2022) 153-162 Host factors on susceptibility to antifungal agents 

doi: https://dx.doi.org/10.5599/admet.1164   157 

respectively (Table 1). The MIC in media supplemented with glucose was decreased from four-fold to a 

maximum 16-fold measured for C. albicans in miconazole. C. neoformans was the only organism whose 

MIC was affected by the presence of insulin. Interestingly, while plasma alone significantly increased drug 

activity for all drugs tested against C. glabrata, the addition of insulin and/or glucose restored this activity 

to the levels measured for RPMI with plasma alone (Tables 2 and 3). In contrast, the presence of plasma 

negatively impacted miconazole (C. lusitaniae, > 185-fold; C. tropicalis, > 23-fold; C. krusei, > 92-fold) and 

with the addition of glucose and insulin, MIC returned to levels within 4-fold that of RPMI with plasma. The 

addition of glucose to plasma caused either a decrease in the MIC or did not alter the MIC. In all test 

situations, the MLC correlated with the MIC. 

Table 1. Effect of insulin and glucose on fungal MIC (g/ml)  

Organism Drug RPMI RPMI + Gluc
c 

Ratio 
RPMI + Gluc 

RPMI 
RPMI + Insu

d 
Ratio 

RPMI + Insu 
RPMI 

RPMI + 
Glucose & 

Insulin 

Ratio 
RPMI + Gluc & 

Insu RPMI 

C. lusitaniae AmB
a 

 

 

0.039 (S)
 b

 0.0195 (S) 0.5 0.0195 (S) 0.5 0.078 (S) 2 

 5-FC
a 

0.15625 (S) 0.15625 (S) 1 0.15625 (S) 1 0.00936 (S) 0.0599 

 Flucon
a 

4.0 (S) 8.0 (S) 2 2.0 (S) 0.5 16.0 (S-DD) 4 

 Itra
a 

0.5 (S-DD)
b 

4.0 (R)
 b

 8 0.5 (S-DD) 1 0.0625 (S) 0.125 

 Micon
a 

0.195 (S) 0.195 (S) 1 0.195 (S) 1 2.2425 (S) 11.5 

C. parapsilosis AmB 0.078 (S) 0.0195 (S) 0.25 0.039 (S) 0.5 0.078 (S) 1 

 5-FC 0.78 (S) 0.39 (S) 0.5 4.99 (I)
 b

 6.4 0.312 (S) 0.4 

 Flucon 2.0 (S) 8.0 (S) 4 2.0 (S) 1 8.0 (S) 4 

 Itra 0.25 (S-DD) 0.25 (S-DD) 1 0.25 (S-DD) 1 0.25 (S-DD) 1 

 Micon 0.39 (S) 0.78 (S) 2 0.39 (S) 1 0.546 (S) 0.71 

C. albicans AmB 0.039 (S) 0.0195 (S) 0.5 0.0195 (S) 0.5 0.039 (S) 1 

 5-FC 0.78 (S) 0.1 (S) 0.1299 0.39 (S) 0.5 0.078 (S) 0.1 

 Flucon 0.125 (S) 0.125 (S) 1 0.125 (S) 1 0.5 (S) 4 

 Itra 0.03125 (S) 0.0156 (S) (2) 0.03125 (S) 1 0.0625 (S) 2 

 Micon 0.39 (S) 0.0245 (S) 0.0629 0.78 (S) 2 0.01757 (S) 0.045 

C. tropicalis AmB 0.039 (S) 0.0195 (S) 0.5 0.039 (S) 1 0.156 (S) 4 

 5-FC 0.195 (S) 0.0975 (S) 0.5 4.99 (I) 25.6 0.156 (S) 0.8 

 Flucon >128.0 (R) >128.0 (R) >1 >128 (R) >1 >128 (R) >1 

 Itra >64.0 (R) >64.0 (R) >1 >64 (R) >1 >64 (R) >1 

 Micon 1.56 (S) 0.78 (S) 0.5 1.56 (S) 1 9.048 (R) 5.8 

C. neoformans AmB 0.039 (S) 0.0195 (S) 0.5 0.039 (S) 1 0.039 (S) 1 

 5-FC 6.25 (I)
b 

6.25 (I) 1 0.78 (S) 0.125 0.78 (S) 0.125 

 Flucon 8.0 (R) 8.0 (R) 1 8.0 (R) 1 8.0 (R) 1 

 Itra 0.5 (S-DD) 0.5 (S-DD) 1 0.5 (S-DD) 1 0.5 (S-DD) 1 

 Micon 0.9766 (S) 

 

0.1953 (S) 0.2 0.09766 (S) 0.1 4.492 (S) 4.6 

C. glabrata 

 

 

AmB 0.078 (S) 0.0195 (S) 0.25 0.039 (S) 0.5 3.12 (R) 40 

 5-FC 8.0 (I) 4.0 (I) 0.5 51.2 (R) 6.4 1.6 (I) 0.2 

 Flucon 0.09766 (S) 0.3906 (S) 4 0.195 (S) 2 0.195 (S) 2 

 Itra 2.0 (R) >64 (R) >32 >64 (R) >32 >64 (R) >32 

 Micon 0.39 (S) 0.78 (S) 2 0.39 1 17.94 (R) 46 

C. krusei AmB 0.078 (S) 0.039 (S) 0.5 0.078 (S) 1 0.078 (S) 1 

 5-FC 12.5 (I) 12.5 (I) 1 

 

12.5 (I) 1 5.0 (I) 0.4 

 Flucon 64.0 (R) 64.0 (R) 1 64.0 (R) 1 64.0 (R) 1 

 Itra 1.0 (R) 1.0 (R) 1 1.0 (R) 1 1.0 (R) 1 

 Micon 0.39 (S) 0.78 (S) 2 1.56 (S) 4 8.97 (R) 23 
a
amphotericin B (AmB), flucytosine (5-FC) fluconazole (Flucon), itraconazole (Itra) , and miconazole (Micon) 

b
S=sensitive; R=resistant; I=intermediate resistance; S-DD= sensitive based on reported disc diffusion concentration 

c
Gluc=glucose; 

d
Insu=insulin 

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Plotkin and Konaklieva  ADMET & DMPK 10(2) (2022) 153-162 

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Table 2. Effect of insulin and glucose in RPMI medium with human plasma (50 % v/v; RPMI-P) on the MIC (g/ml)  

Organism Drug RPMI-P
c 

Ratio 
RPMI-P 
RPMI 

RPMI-P & 
Glu

d 

Ratio 
RPMI-P & 

Gluc   
RPMI-P 

RPMI-P & 
Insu

e
 

Ratio 
RPMI-P & Insu 

RPMI-P 

RPMI-P, Gluc 
& Insu 

Ratio 
RPMI-P, Gluc 

& Insu RPMI-P 

C. lusitaniae 

 

 

 

 

 

 

AmB
a 

 

 

 

 

 

 

0.078 (S)
b 

2 9.75x10
-3 

(S) 0.25 0.0195 (S) 0.25 0.0195 (S) 0.25 

 5-FC
a
 

 

 

 

0.78 (S) 5 0.78 (S) 1 0.78 (S) 1 0.78 (S) 1 

 Fluco
n

a
 

1.0 (S) 0.25 1.0 (S) 1 4.0 (S) 4 4.0 (S) 1 

 Itra
a
 2.0 (R)

 b
 4 2.0 (R) 1 2.0 (R) 1 2.0 (R) 1 

 Micon
a
 

>36.075 (R) >185 >36.075 (R) >1 0.3608 (S) 0.01 >36.08 (R) >1 

C. parapsilosis AmB 0.0195 (S) 0.25 0.078 (S) 4 0.039 (S) 2 0.0195 (S) 1 

 5-FC 24.96 (I)
 b

 32 24.96 (I) 1 24.96 (I) 1 24.96 (I) 1 

 Fluco
n 

1.0 (S) 0.5 0.5 (S) 0.5 8.0 (S) 8 0.5 (S) 0.5 

 Itra 0.125 (S) 0.5 0.125 (S) 1 0.125 (S) 1 0.5 (S-DD) 2 

 Micon >39.88 (R) >92 >39.88 (R) 1 >39.88 (R) >1 >39.88 (R) >1 

C. albicans AmB 0.00975 (S) 0.25 0.0195 (S) 2 0.0195 (S) 2 0.0195 (S) 2 

 5-FC 3.12 (S) 4 3.12 (S) 1 3.12 (S) 1 3.12 (S) 1 

 Fluco
n 

0.075 (S) 0.5 0.075 (S) 1 >6.8 (S-R) 1024 0.3 (S) 4 

 Itra 0.03125 (S) 1 0.03125 (S) 1 0.03125 (S) 1 0.03125 (S) 1 

 Micon 0.39 (S) 1 0.065 (S) 0.166 0.0325 (S) 0.083 0.78 (S) 2 

C. tropicalis AmB 0.0195 (S) 0.5 0.0195 (S) 1 

 

 

0.0195 (S) 1 0.0195 (S) 1 

 5-FC 3.12 (S) 16 3.12 (S) 1 3.12 (S) 1 3.12 (S) 1 

 Fluco
n 

>128 (R) >1 >128 (R) 1 >128.0 (R) >1 >128.0 (R) 1 

 Itra >64 (R) 1 >64 (R) 1 >64.0 (R) 1 >64.0 (R) 1 

 Micon >35.88 (R) >23 >35.88 (R) 1 >35.88 (R) >1 >35.88 (R) >1 

C. neoformans AmB 0.00488 (S) 0.125 0.00975 (S) 2 0.00975 (S) 1 0.00975 (S) 2 

 5-FC 25.0 (I-R) 4 12.5 (I) 0.5 12.5 (I) 0.5 12.5 (I) 0.5 

 Fluco
n 

1.0 (S) 0.125 0.25 (S) 0.25 1.0 (S) 1 2.0 (S) 2 

 Itra 0.25 (S-
DD)

b 
0.5 0.25 (S-DD) 1 0.0125 (S) 0.05 0.25 (S-DD) 1 

 Micon 1.953 (S) 2 0.3906 (S) 0.2 0.078 (S) 0.04 7.812 (R) 4 

C. glabrata AmB 
3.71x10

-5 

(S) 
4.76x10

-4
 3.7 x 10

-5 
(S) 1 3.71x10

-5
(S) 1 3.71x10

-5 
(S) 1 

 5-FC 0.0615 (S) 7.69x10
-3

 <0.0615 (S) <1 <0.0615 (S) <1 0.246 (S) 4 

 Fluco
n 

<2.4x10
-

5
(S) 

<2.4x10
-4

 <2.4x10
-5 

(S) <1 <2.4x10
-5

(S) 1 <2.4x10
-5

(S) <1 

 Itra 0.0194 (S) 9.7x10
-3 

0.0194 (S) 1 0.0194 (S) 1 0.0194 (S) 1 

 Micon 1.08x10
-3 

(S) 
2.8x10

-3
 5.41 x 10

-4
(S) 0.5 0.0964 (S) 89 0.001083 (S) 1 

C. krusei AmB 0.156 (S) 2 0.624 (S) 4 0.156 (S) 1 0.156 (S) 1 

 5-FC >25.0 (I-R) >2 >25.0 (I-R) 1 >25.0 (I-R) >1 >25.0 (I-R) >1 

 Fluco
n 

64.0 (R) 1 64.0 (R) 1 64.0 (R) 1 64.0 (R) 1 

 Itra 4.0 (R) 4 4.0 (R) 1 4.0 (R) 1 4.0 (R) 1 

 Micon 35.88 (R) >92 8.97 (R) 0.25 574.08 (R) 16 >35.88 (R) >1 
a
amphotericin B (AmB), flucytosine (5-FC) fluconazole (Flucon), itraconazole (Itra), and miconazole (Micon) 

b
S=sensitive; R=resistant; I=intermediate resistance; S-DD= sensitive based on reported disc diffusion concentration 

c
P=plasma 

d
Gluc=glucose 

e
Insu=insulin 

Thus, the addition of plasma to the medium resulted in an overall decrease in the concentration of 

miconazole, itraconazole, 5-fluorocytosine, and amphotericin B needed to inhibit the growth of C. glabrata 

(Table 3). In contrast, plasma overall caused an increase in the concentration of miconazole, itraconazole, 

5-fluorocytosine, and amphotericin B needed to inhibit the growth of C. lusitaniae, C. tropicalis and C. 

krusei. The presence of the medium supplements insulin and/or glucose does not affect fungal MIC or MLC 

in a predictable manner regarding specific antifungal agents or organisms tested. The growth rate and 

relative production of yeast and/or hyphal forms in medium with and without glucose and/or insulin do 

not appear to be related to changes in the organism's MIC or MLC.  



ADMET & DMPK 10(2) (2022) 153-162 Host factors on susceptibility to antifungal agents 

doi: https://dx.doi.org/10.5599/admet.1164   159 

Table 3. Ratio of effects of insulin and glucose on antifungal activity of amphotericin B, flucytosine, 
fluconazole, itraconazole, and miconazole in the presence of RPMI with 50 % human plasma to homologous 
RPMI medium alone 

  
Organism 

 
Drug 

Ratio 
RPMI-Plasma 

RPMI 

Ratio 
RPMI-P

c
 & Gluc

d
 

RPMI-Gluc 

Ratio 
RPMI-P & Insu

e
 

RPMI-Insu 

Ratio 
RPMI-P, Gluc & Insu 

RPMI-Gluc & Insu 

C. lusitaniae 

 

 

 

 

 

 

AmB 

 

 

 

 

 

 

2.0 0.5 1.0 0.25 

 5-FC 

 

 

 

5.0 5.0 5.0 83.3 

 Flucon 0.25 0.125 2.0 0.25 

 Itra 4.0 0.5 4.0 32.0 

 Micon >185.0 >185.0 1.85 16.1 

C. parapsilosis AmB 0.25 4.0 1.0 0.25 

 5-FC 32.0 64.0 5.0 80.0 

 Flucon 0.5 0.0625 4.0 0.0625 

 Itra 0.5 0.48 0.5 2.0 

 Micon >92.0 >51.13 >102.3 >73 

C. albicans AmB 0.25 1.0 1.0 0.5 

 5-FC 4.0 31.2 8.0 40 

 Flucon 0.5 0.6 54.4 0.6 

 Itra 1.0 2.0 1.0 0.5 

 Micon 1.0 2.65 0.042 44.4 

C. tropicalis AmB 0.5 1.0 0.5 0.125 

 5-FC 16.0 32.0 0.625 20.0 

 Flucon >1.0 1.0 1.0 1.0 

 Itra 1.0 1.0 1.0 1.0 

 Micon >23.0 46.0 23.0 3.97 

C. neoformans AmB 0.125 0.5 0.25 0.25 

 5-FC 4.0 2.0 16.0 16.0 

 Flucon 0.125 0.03 0.125 0.25 

 Itra 0.5 0.5 0.025 0.5 

 Micon 2.0 2.0 0.7987 1.74 

C. glabrata AmB 4.76x10
-4

 1.897x10
-3 

9.5x10
--4 

1.2x10
-5 

 5-FC 7.69x10
-3

 1.5x10
-2 

1.2x10
-3 

1.54x10
-1 

 Flucon <2.4x10
-4

 6.1x10
-5 

1.23x10-4 1.23x10
-4 

 Itra 9.7x10
-3 

3x10
-4 

3x10
-4 

3x10
-4 

 Micon 2.8x10
-3

 6.9x10
-4 

2.47x10
-1

 6.0x10
-5 

C. krusei AmB 2.0 16.0 2.0 2.0 

 5-FC >2.0 2.0 2.0 5.0 

 Flucon 1.0 1.0 1.0 1.0 

 Itra 4.0 4.0 4.0 4.0 

 Micon >92.0 11.5 368.0 4.0 
a
amphotericin B (AmB), flucytosine (5-FC) fluconazole (Flucon), itraconazole (Itra), and miconazole (Micon) 

b
S=sensitive; R=resistant; I=intermediate resistance; S-DD= sensitive based on reported disc diffusion concentration 

c
P=plasma; 

d
Gluc=glucose; 

e
Insu=insulin 

Conclusions 

The testing of fungal susceptibility in the presence of plasma with and without the supplements glucose 

and/or insulin to simulate type II diabetes appears warranted in light of their sometimes adverse effect on 

the MIC of the antifungal agents. These results taken together indicate that alterations in the levels of 

serum components associated with type II diabetes, and simulated herein, cause an alteration in the in 

https://dx.doi.org/10.5599/admet.1164


Plotkin and Konaklieva  ADMET & DMPK 10(2) (2022) 153-162 

160  

vitro activity of certain antifungal agents that is also dependent on the presence of plasma. Since treatment 

failure in candidal infections has been an issue and is increasing, it is likely that a portion of treatment 

efficacy failure is due to phenotypic resistance [28,29]. While multiple in vitro studies show that glucose 

induces phenotypic resistance, the organism is always exposed to glucose in the presence of insulin in vivo 

[27,30,31]. Most commonly, these studies focused on the effect glucose has on end-point determinations 

for amphotericin B, fluconazole and itraconazole [32]. This study demonstrated that testing of individual 

serum components, e.g., insulin and glucose in vitro showed that not only does insulin or glucose affect 

susceptibility in a manner that was species and drug-specific, but that the interaction of the two 

components can negate the effect, either positive or negative, of the other additive. This impact of insulin 

and glucose is further compounded by testing in the presence of human plasma vs. RPMI medium alone. 

These unpredictable phenotypic changes in susceptibility to antifungal agents were demonstrated for 

amphotericin B and C. glabrata, which were sensitive to the drug in medium alone or supplemented with 

either glucose or insulin. However, when combined, the MIC was > 40-fold higher than medium alone or 

with either glucose or insulin. This effect was eliminated with the addition of anti-candidal antibody-

negative plasma. In summary, these findings present evidence that a precision approach is needed for the 

determination of fungal drug susceptibility, particularly for individuals with type II diabetes. 

 

Acknowledgements: The authors thank the Midwestern University Office of Research and Sponsored 
Programs and the Midwestern College of Graduate Studies for their support of this work. 

Conflict of interest: The authors declare that no conflict of interest exists. 

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