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Ibn Al-Haitham Jour. for Pure & Appl. Sci. 33 (4) 2020 
 

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The impact of Glucose and Sodium Chloride on the Biofilm Formation of 
Pseudomonas aeruginosa & Staphylococcus aureus 

 

  

   

 

 

 

    

 

                                                                                                          			
Abstract 

       The aim of this research is to evaluate the effect of glucose and sodium chloride on biofilm 
formation by bacteria causing wound infection. For this purpose, 1% and 2% concentration of 
each of glucose and sodium chloride were used to test the biofilm formation potential of 
Staphylococcus aureus and Pseudomonas aeruginosa, which were the most common abundant 
bacteria that cause infection by biofilm. Each of the concentrations was kept in contact with the 
pathogenic bacteria for 24 hours. After the period of incubation, the concentration of 1% of 
glucose enhanced moderate biofilm formation capacity for (66% and 80%) on both bacteria 
respectively. The concentration of 2% glucose, on the other hand, led to a weak biofilm for 33% 
and 20% on both bacteria isolates respectively. In respect to the effect of sodium chloride, no 
isolate was able to form neither moderate nor strong biofilms. Nonetheless, all isolates 
succeeded in forming weak biofilms at 2% sodium chloride, while treatment with a 
concentration of 1% sodium chloride led to inhibited biofilm formation for 43% of isolates. 
Besides, Pseudomonas aeruginosa isolates were able to form moderate biofilms in the presence 
of 1% concentration of glucose, and weak producers in the presence of 2% glucose 
concentration. The isolates succeeded in forming strong biofilms at both 1% and 2% sodium 
chloride. 
 
 Keywords: Biofilms, Wounds Infections, Bacteria. 
 
  

Department of Medical and 
Biological, College of 

Biotechnology Al-Nahrain 
University, Baghdad, Iraq. 

adelestabraq@yahoo.com 

Ibn Al Haitham Journal for Pure and Applied Science 

Journal homepage: http://jih.uobaghdad.edu.iq/index.php/j/index 

Doi: 10.30526/33.4.2525 

Article history: Received 15 March 2020, Accepted 23 April 2020, Published in October 2020 

Department of Medical and 
Biological, College of 

Biotechnology Al-Nahrain 
University and Al- Farabi 

University College, Baghdad, 
Iraq 

Estabraq A. Mahdi  Abdulwahid B. Al-Shaibani  Nedhaal S. Zbar 

Department of Medical and 
Biological,College of 

Biotechnology Al-Nahrain 
University, Baghdad, Iraq. 



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1. Introduction  

       Bacterial biofilms are regarded as the major cause of chronic wound infections. Their high 
resistance against antibiotic treatments makes their annihilation more challenging. The majority 
of chronic wound infections are a result of biofilms that seriously slows down the process of 
wound healing [1]. Biofilm formation shows a protective style of growth that permits the 
microorganism to stay alive in various environments and capability of biofilm formation that is 
among the defense strategies of Staphylococcus aurous. Typical antibiotic treatments are 
generally impractical in eradicating bacteria that are embedded in biofilms, as the latter are 
naturally unsusceptible to the immune responses of a host [2]. Biofilm construction is a secure 
adjusting type of thriving that allows bacteria not only to survive in inhospitable conditions like 
those of a human body but also to propagate and spread their requirements, which are facilitated 
by their molecular crosstalk known as Quorum Sensing (QS) [3]. The main inconsistency of 
chronic infections is their inscrutability, which are in most instances associated with biofilm 
formation, as the National Institute of Health in the USA estimates that biofilms are linked to 
80% of all bacterial infection. The mechanisms of biofilm resistance to antimicrobial 
compounds include physical or chemical diffusion barriers to antimicrobial penetration into the 
biofilm. For example, ciprofloxacin binds to certain components of P. aeruginosa biofilm, thus, 
the biofilm acts as a barrier to antimicrobial agents [4]. Dead remnants of neutrophils in addition 
to other immune cells found to act as a biological network that promotes the development of 
biofilms, and neutrophils within biofilms to produce various inflammatory intermediaries, 
which cause tissue injury. Biofilm development is organized by the expression of 
polysaccharide intracellular adhesion molecule that facilitates cell to cell adhesion. The matrix 
of bacterial biofilm is made of different polymers such as polysaccharide, proteins, and 
extracellular DNA (eDNA) .The formation of biofilms is a procedure that goes through multiple 
stages, the first of which is a provisional attachment to the surface. Afterwards, the real 
attachment is induced by particular bacterial adhesions called microbial surface components, 
which recognize adhesive matrix molecules. Then bacteria agglutinate and form extracellular 
polymeric substances during the step of accumulation [5]. This process of biofilm construction 
relies on various factors such as the properties and the nature of the carbon source, its 
concentration, pH, ionic strength, and temperature [6]. Although researchers have attempted to 
refine the requirements needed for the construction of biofilms by Staphylococcal and 
Pseudomonas isolates, certain factors have yet to be sufficiently studied, including the ideal 
sugar and salt concentrations, and the richness of medium. Some researchers have studied the 
impact on the biofilm phenotype by using glucose supplementation along with Tryptone Soy 
Broth (TSB). While others have comprehensively elucidated sodium chloride (NaCl) 
dependence of biofilms in S. aureus, but their quantitative analysis and classification, according 
to the parameters of biofilm formation, are not clear and cannot be repeated in every research 
laboratory. Therefore, there is a desperate need for a simple and generally agreed-upon criterion 
for laboratory biofilm production by clinical isolates of S. aureus. As far as we are aware, 
investigators generally do not opt for a concentration of sugar and salt that is beyond 1% and 
do not conduct enough studies about how the features of S. aureus biofilms are affected by 
culture medium, fixation, elution, and the supplementation of various degrees of salt and sugar 
to a wider level of concentration [7]. On the aforementioned grounds, we aim in this study to 
establish a consensus method to attain the maximum possible in vitro biofilm construction using 



Ibn Al-Haitham Jour. for Pure & Appl. Sci. 33 (4) 2020 
 

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clinical isolates from wound infection bacteria consuming the supplementations with the 
suitable concentration of glucose and sodium chloride. 
 
2.Materials and Methods    
2.1. Clinical Iolates and Penotypic Ientification 
    Swabs samples were taken from ninety surgical wounds of patients attending Medical City 
Hospital in Baghdad, for the period from July to September 2018. The samples were taken by 
the attending physician of the hospital and collected using sterile sticks with cotton swabs in 
test tubes. Every specimen streaked on nutrient Agar, mannitol salt agar (MSA), blood agar and 
MacConky agar. Then, after 24 hours of incubation at 37 °C, the isolates were identified 
according to the microscopic characterization, colony morphological features, and gram 

staining. Various biochemical tests including the catalase, coagulase, oxidase and DNase test 
and others were carried out according to Bergey’s Manual [8]. 
2.2. Detection of Biofilm in Presence Different Concentration of Glucose and Sodium 

Chloride  
    Biofilm formation was determined by microtiter plate method (MTP) [9], which is regarded 
as the standard and most frequently applied method in the investigation of biofilm synthesis 
disclosure. The microtiter plate method was applied to bacteria isolates by incubating overnight 
in nutrient broth at 37 °C. Bacterial isolate suspension that was equal to the McFarland turbidity 
standard no. 0.5 was inoculated in the nutrient broth separate sterile, polystyrene, flat-bottomed 
tissue culture static condition 96-well plate. The nutrient broth was supplemented with 1% and 
2% concentrations of glucose and 1% and 2% concentrations of sodium chloride (NaCl). 
Subsequently, 200 µL of the inoculum was moved to the inspection wells of a sterile microtiter 
plate, which was related to an inoculum of approximately 5×106 cells per well. The lids covering 
each plate were supplied by the manufacturing company. Ultimately, the inoculated assay plates 
were incubated overnight at 37 °C, where the negative control wells consisted of the sterile 
nutrient broth alone, and the positive control wells had both the nutrient broth along with 
bacterial cells without glucose or sodium chloride. Each well was decanted and washed three 
times using Phosphate-Buffered Saline (PBS) to remove any non-adherent bacteria. The washed 
plates were first incubated for a minimum period of one hour at 60 °C to stain fix adherent cells. 
The purpose of this step was to lessen the variability caused by the biofilm loss during the 
staining procedure. After the fixation, 200 µL of 0.1 % Crystal Violet (CV) dissolved in distilled 
water was introduced to every well at least 15min. for staining. Afterwards, the reaction has 
been ended; Phosphate-Buffered Saline was used repeatedly 3 to 4 times to wash. Then every 
well was introduced with 200 µL of 95% ethanol for 10 minutes. The assays were all done in 
triplicates. The amount of crystal violet extracted by the ethanol in each well can be directly 
quantified spectrophotometrically by measuring the optical density (OD) at 630 using an 
appropriate ELISA reader [9]. Table (1) displays the classifications depending on the values of 
optical density (OD) that were obtained from various strains of Staphylococcus and 
Pseudomonas and were utilized for the sake of data simplification and calculation [10]. 
 
 
 
 



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Table 1: Bacterial Adherence Classification according to the Method of Microtiter plate 

Mean OD 630 nm Biofilm Construction Adherence 

OD ≤ ODc Non–adherent 

ODc < OD ≤ 2ODc Weakly adherent 

2ODc < OD ≤ 4ODc Moderately adherent 

4 ODc < OD Strongly adherent 

 
3. Results and Discussion       
3.1.1. Staphylococcus Isolation and Identification 
    Thirty isolates were isolated 90 samples of wound, which constitute 33% of the total number, 
were able to grew in mannitol salt agar, which is regarded as a selective and differential medium 
for the Staphylococcus species. The colonies looked round, smooth, raised, mucous and 
glistening, which indicates that these isolates belong to the genus Staphylococcus [11]. Certain 
isolates had the capability of fermenting mannitol, generating splendid production, and forming 
vast golden colonies surrounded by broad yellow fields, causing the medium color to alter from 
pink to yellow [8]. This golden color feature of S. aureus was accounted for by the carotenoid 
pigment (Staphyloxanthin) according to Clauditz et al. [12]. The gold pigment is an eponymous 
feature of the human pathogen S. aureus that shield the microbe from oxidation-based clearance 
[13]. After subjecting the thirty isolates to Gram staining, the microscopic examination showed 
that their cells appeared cocci mostly arranged in grape- like irregular clusters. The 30 isolates 
all gave a negative result to an oxidase test, which was carried out in order to distinguish genus 
Staphylococcus from genus Micrococcus that normally yields a positive response. In addition 
to that, the isolates all responded positively to the catalase test, which was performed to 
distinguish Streptococcus species that typically respond negatively to the test, from 
Staphylococcus species [14]. All mannitol fermenters were noticeably coagulase and DNase 
positive, and all S. aureus isolates provided positive responses to DNase and developed a beta 
hemolysis behavior on blood agar, as shown in Table (2). 

Table 2: Morphology and biochemical of the Staphylococcus aureus isolates 
Staphylococcus aureus Test 

Gram-positive Gram stain 

β-hemolysis Blood agar medium 

Yellow colony Mannitol salt agar 

Positive Catalase 

Negative Oxidase 

Positive Coagulase 

Positive Deoxyribonuclease (DNase agar) 

 



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3.1.2. Pseudomonas Isolation and Identification 
      A total number of 25 /90 isolates had the ability to grow on cetrimide agar plates and were 
suspected to belong to genus Pseudomonas cetrimide agar which differentiated P. aeruginosa 
from other species of Pseudomonas that could not grow on this medium. They were subject to 
further identification according to morphological characteristics and biochemical tests. 
Colonies of each isolate placed on nutrient agar showed different morphological characteristics 
of Pseudomonas species such as mucoidal growth, smooth shape with flat edges and elevated 
center, whitish or creamy color, fruity odor, and production of pyocyanin. On the other hand, 
colonies of Pseudomonas aeruginosa that grew on MacConky agar medium appeared pale in 
color and had irregular, oval, and large edges. On blood agar, Pseudomonas aeruginosa was 
able to perform hemolysis completely, which was a reasonable result in comparison with results 
demonstrated by Forbes et al. [15]. Microscopic analysis of Pseudomonas species revealed that 
the cells were bacilli; gram-negative; non-spore forming; and appeared single, in pairs, or short 
chains. These results were comparable to the reported morphological characteristics of 
Pseudomonas aeruginosa and agreed with Harley and Prescott [16], which certified the 
identification. Biochemical tests for Pseudomonas sp. were also made and their results 
indicated in Table (3) showed that these isolates gave a positive result for oxidase and catalase 
tests, which signified that they belonged o Pseudomonas aeruginosa. 
 

Table 3: Morphological and Biochemical Characteristics of the Pseudomonas aeruginosa Isolates 

Result Test 

Green on Cetrimide agar Colony color 

Bacilli Cell shape 

Negative Gram stain  

Positive Catalase 

Positive Oxidase 

Positive Growth on King A 

Positive Growth on King B 

Positive Growth on cetrimide 

Positive Citrate utilization 

Negative Growth at 4ºC in nutrient agar 

Positive Growth at 42ºC in nutrient agar 

 
   The numbers and percentages of the microorganisms isolated from the patients  ’wound 
infections were shown in Table (4). These results were obtained according to the identification 
criteria mentioned for the bacterial isolates. 
 
 
 
 
 
 



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Table 4: Numbers and percentages of bacteria isolated from the wound infection patients 

Percentages of isolates Number of isolates Types of isolates 

33.3 30 S. aureus 

27.7 25 P. aeruginosa 

38.8 35 Other types 

100 90  - 

 

         3.2. Effect of Glucose and Sodium Chloride on biofilm formation of the Isolates 
     This study showed a trend among the clinical isolates of P. aeruginosa and Staph.aureus to 
form a biofilm. All S. aureus isolates were able to form a weak biofilm in a nutrient broth 
without any supplementation, while in the presence of 1% glucose biofilm formation capacity 
was enhanced by 66% for S. aureus isolates, as shown in Table (5) and figure (1). It was noted 
in the results that glucose sugar, with a concentration of 1%, worked to increase the formation 
of the biofilm by 66%. While the concentration of 2% inhibited the formation of the biofilm by 
16% and reduced the ability of isolates to the formation of the moderate biofilm by 33%. 
Whereas it increased the ability to form a weak biofilm to 50% at a concentration of 1%, but 
the increase did not significantly effeteness. In respect to the effect of sodium chloride, it 
resulted by the inhibited the biofilm formation by 76% and 43% at a concentration of (1,2%). 
The results showed a decrease in the ability of the isolates formation of the weak biofilm to 23 
and 56% for both concentrations respectively. Collectively, results revealed that 1% glucose 
was significantly better than other glucose concentrations and NaCl in improving biofilm 
formation by S. aureus isolates. Glucose has been shown to induce the multicellular aggregation 
step of biofilm formation [17]. Sugimoto et al. suggested that the treatment with a high 
concentration of NaCl enabled them to detach and yield S. aureus biofilm matrices [18]. 

Table 5: Effect of Glucose and NaCl on a Biofilm Development by Staphylococcus aurous after 24 Hours of 
Incubation 

Number of S. aureus isolates (%) 

Media use Non 

Biofilm 

Weak 

biofilm 

Moderate 

biofilm 

Strong 

biofilm 

NB without enhancer 0 (0%) 30(100%) 0 (0%) 0 (0%) 

NB + 1% glucose 0 (0%) 10(33%) 20 (66%) 0 (0%) 

NB + 2% glucose 5(16%) 15(50%) 10(33%) 0 (0%) 

NB + 1% NaCl 23(76%) 7(23%) 0 (0%) 0 (0%) 

NB + 2% NaCl 13(43%) 17(56%) 0 (0%) 0 (0%) 

NB; nutrient broth 



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Figure 1: Effect of  Glucose and NaCl on the Biofilm Formation of S. aureus 

Regarding to P.aeruginosa isolates, the results in table (6) and figure (2) revealed that glucose 
sugar, with a concentration of 1%, worked to increase the formation of the biofilm by 80%, 
while the concentration of 2% inhibited the formation of the biofilm by 20% and reduced the 
ability of isolates to the formation of the moderate biofilm by 20%, while it increased the ability 
to form a weak biofilm to 60% after it was 20% at a concentration of 1%, In respect to the effect 
of sodium chloride, it resulted in the strong biofilm formation by 80% and 100% at a 
concentration of (1,2%).The relative quantities of extracellular polysaccharide intracellular 
adhesion and teichoic acids relied on the selection of medium and other growth conditions. 
Particularly the existence of sugars seemed to play an important role in the stimulation of this 
progression [19].  
 

Table 6: Effect of Glucose and Sodium Chloride on   Biofilm formation of Pseudomonas aeruginosa after 24 

Hours of Incubation 

Number of P. aeruginosa isolates (%) 

Media use Non 

biofilm 

Weak 

biofilm 

Moderate 

biofilm 

Strong 

biofilm 

NB without enhancer 0 (0%) 25(100%) 0 (0%) 0 (0%) 

NB + 1% glucose 0 (0%) 5(20%) 20(80%)  0 (0%) 

NB + 2% glucose 5(20%) 15(60%) 5(20%) 0 (0%) 

NB + 1% NaCl 0 (0%) 0 (0%) 5(20%) 20(80%) 

NB + 2% NaCl 0 (0%) 0 (0%) 0 (0%) 25(100%) 

 NB; nutrient broth 
 
 

0

0.02

0.04

0.06

0.08

0.1

0.12

0.14

0.16

0.18

0.2

2% glucose 1% glucose 2%NaCl 1%NaCl

O
p

ti
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a

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D

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s
it

y

Glucose  and NaCl concentration

Test

Control



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Figure 2: Effect of Glucose and NaCl on the Biofilm Formation of P.aeruginosa 

4. Conclusions 
    Supplementing media with 1% glucose led to enhance the biofilm forming capacity while 
sodium chloride caused inhibition and addition of glucose in concentration more than 1% 
caused inhibition in biofilm production. 

 
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