Hydrolytic Enzyme Production by Thermophilic Bacteria Isolated from Saudi Hot Springs

2.1 Physico-chemical properties of the hot spring samples

The three hot springs chosen for this study; Al-Khubah, Al-Ardah and Al-Majardah are located in the southern region of Saudi Arabia. The water samples were collected in 500 ml glass bottles. The temperature, pH, electrical conductivity (EC) and total dissolved solid (TDS) of hot spring water samples were measured in real time during sampling using Benchtop Meters (OAKTON). The heavy metal content was analysed by Inductive Coupled Plasma-Optical Emission Spectrometry (TCP-OES) [14]. Na⁺, K⁺, Ca²⁺ and Mg²⁺ levels were determined using Energy Dispersive X-ray Fluorescence Spectrometer (ED-XRF) [15]. Phosphate concentration was determined by the stannous chloride method [16] and nitrate concentration was measured by the ultraviolet spectrophotometer screening method [17]. Chemical analysis of other components was performed in the laboratory using standard techniques [18].

2.2 Isolation of thermophilic bacteria

Two different isolation media were used to isolate the thermophilic bacteria, Thermus agar medium [19] and ATCC medium 697 [7]. Thermus agar medium contained (milligram /litre); nitrilotriacetic acid (100), CaSO₄ (60), MgSO₄ (100), KNO₃ (103), NaNO₃ (689), Na₂HPO₄ (111), MnSO₄ (2.2), ZnSO₄ (0.5), CuSO₄ (0.016), H₃BO₃ (1.0), Na₂ MoO₄ (0.025), CoCl₂ (0. 046), FeCl₃ (0.28), tryptophan (1.0), yeast extract (1000) and twenty grams of agar. The second isolation medium, ATCC medium 697, contained (%); NaCl (0.5), yeast extract (0.2), beef extract (0.4), peptone (0.5), and agar (2). All media were adjusted to pH 7.5 prior to autoclaving at 121°C for 20 min at 1 kg/cm₂. Two isolation methods were employed, 100 ml aliquot of each water sample was filtered using membrane filters (0.22 μm Millipore Corporation, Bedford), and the filters were then transferred onto the agar plates. The plates were incubated for 48 h at 55°C [20]. To enrich the thermophilic bacteria’s ability to produce α-amylase, protease and lipase enzymes, 5 grams each of sterile starch, casein and tributyrin were added separately to hot spring water samples, mixed and incubated for 2 weeks at 55°C [21]. The 100 μl of the diluted samples was transferred onto agar plates and incubated at 55°C for 48 h.

2.3 Screening of thermophilic bacterial isolates for hydrolytic enzyme production

Bacterial isolates were screened using hydrolytic plate assay tests on starch, casein and tributyrin agar plates for testing α-amylase, protease and lipase production, respectively. After incubation at 55°C for 48 h, starch hydrolysis was determined by flooding the plates with iodine solution [22]. Following treatment with hydrochloric acid on the casein agar plates, the isolates showing zones of clearance were selected as protease producing bacteria [23]. Lipid hydrolysis of the isolates was screened using tributyrin agar medium containing phenol red; a colour change from pink to yellow around the colonies indicating lipase production [24]. For qualitative screening of enzymes, enzyme index was measured [25]. The promising isolates showing a high potency index were then selected for further study.

2.4 Identification of the promising isolates

Bacterial genomic DNA of promising isolates was extracted from 5 ml bacterial cultures grown overnight in nutrient broth using a modified QIAamp DNA Mini Kit (Qiagen Inc., Valencia, CA) [26]. The extracted DNA from each bacterial isolate was used as a template for amplification of the 16S rRNA gene using the universal primers 5’ CCA GCA GCC GCG GTA ATA CG 3’ and 5 ‘ATC GG(C/T) TAC CTT GTT ACG ACT TC 3’. PCR reactions were carried out in a 50 μl volume containing 10 mM of Tris-HCl (pH 8.3), 50 mM of KCl, 2.5 mM of MgCl₂, each dNTP at a concentration of 0.2 mM, 1.25 IU of Taq polymerase, each primer at a concentration of 0.2 μM, and 1 μl of the DNA template. The volume was made up to 50 μl with water. PCR was performed according to the following programme: 10 min denaturation at 94°C, followed by 35 cycles of 1 min denaturation at 94°C, 1 min annealing at 55°C, 2 min extension at 72°C, and a final extension step of 10 min at 72°C. Then, 5 μl of the amplified mixture was analysed using 1.5% agarose gel dissolved in 0.5X of TBE buffer and containing ethidium bromide. The gel was run on an electrophoresis unit for 30 min at 150 V, for gene product migration and separation. The migrated bands were observed under UV light and photographed using a gel documentation system. To verify the presence of appropriate sized amplicons, the PCR product for each isolate was compared with a 1 kb DNA ladder. A product of the correct size was purified with a Taka R Agarose Gel DNA purification Kit Ver. 2.0 and sequenced in both directions using an ABI 3730 automated sequencer (Macrogen, Korea). The sequences of the selected isolates were aligned and compared with the deposited sequences in GenBank (http://blast.ncbi.nlm.nih.gov/Blast.cgi). To determine the taxonomic position of the isolates, a phylogenetic tree was constructed with MEGA version 5.0 program using a neighbour-joining algorithm. The Jukes-Cantor distance estimation method with bootstrap analyses for 1000 replicates was also performed. The nucleotide sequences of the amplified 16S rRNA genes of the selected strains reported in this study have been deposited in the GenBank nucleotide sequence databases under different accession numbers.

2.5 Production of Hydrolytic enzymes

Kitchen waste (KW) used as the carbon source for hydrolytic enzymes production was collected from King Khalid University restaurants and stored at 4°C, following drying, crushing and grinding, it was analysed for protein, fat and carbohydrate contents [27]. The selected isolates were further screened for the production of hydrolytic enzymes (α-amylase, protease and lipase) by submerged fermentation. The inoculum was prepared by growing a bacterial culture in nutrient broth medium at 55°C/150 rpm for 24 h. Erlenmeyer flasks (250 ml) containing 50 ml of ATCC medium 697 supplemented with 1% KW as the sole carbon source. The medium was inoculated with 1% inoculum (approximately 2x10⁶ CFU ml^-1) and incubated at 55°C in a shaking incubator at 150 rpm for 96 h. Samples were harvested at 12 h intervals, and growth was determined through the measurement of optical density (OD₆₀₀ nm). The cells were removed by centrifugation at 6000 rpm for 20 min, and the obtained supernatant was then used for enzymes assay [28]. The factors affecting enzymes production such as incubation period (12- 96h), pH (6-9), temperature (45-70°C) and kitchen waste concentration (1-9%) were investigated.

2.6 Enzyme assays

2.7 Statistical analysis

Analysis of variance using one-way ANOVA was carried out. Significance was determined as P ≤ 0.05 using Minitab for Windows software package version 15. The error bars represent standard error of the mean for n=3.

Ethical approval: The conducted research is not related to either human or animals use.

3.1 Physico-chemical properties of water samples

The physical and chemical properties of water samples obtained from hot springs were examined to evaluate their effect on the isolation of thermophilic bacteria (Table 1). The results showed that Jazan hot springs have a temperature gradient ranging from 60 to 70°C, while Al-Majardah hot spring has a temperature of 55°C. All of these springs had a neutral or slightly alkaline pH; the lowest value was 7.2 in the Al-Ardah site and the highest was 8.2 in the Al-Majardah site. Conductivity and TDS also varied, the highest ratio of which was observed for Al-Majardah hot spring reaching 5100 μS cm^-1 and 3147 mg l⁻¹, respectively. The results of heavy metals analysis indicated that all samples were free of toxic elements, where Cd, Cr, Fe, Co and Ni were not detected, while Cu, Pb, Zn, and Mn were detected but in very low concentrations. The remaining elements and compounds including Na, Ca, K, nitrate, ammonium, phosphate, and sulphate were variable among the hot springs (Table 1). The sodium, calcium and potassium concentrations in the Al-Majardah spring (14.64%, 12.14% and 32.95%, respectively) were high compared to those in the Al-Khubah and Al-Ardah hot springs. The concentrations of NH₄⁺, NO₃⁻, SO₄²⁻, and PO₄³⁻ nutrients in Jazan springs were lower than those of the Al-Majardah spring.

3.2 Isolation and Screening of hydrolytic-enzymes-producing bacteria from hot spring

A total of eighty-four thermophilic bacterial isolates were isolated from all hot spring sites using two isolation media. The highest numbers of thermophilic bacteria were isolated from the Al-Majardah (33 isolates) and Al-Khubah (30 isolates) hot springs, while fewer isolates were collected from the Al-Ardah hot spring (21 isolates). The occurrence of isolates in different localities may be a result of the prevailing environmental conditions and the chemical properties of the water (Table 1).

All bacterial isolates were screened to evaluate their ability to produce hydrolytic enzymes, α-amylase, protease and lipase using ATCC medium 697 [7]. Preliminary tests on media enriched with the substrate for each enzyme showed that 77 isolates exhibited enzymatic activity for one or more enzymes. Amongst the 84 thermophilic bacterial isolates, 33.33%, 29.76% and 28.57% of the strains possessed high amylolytic, proteolytic and lipolytic activities, respectively. The enzyme index differed, suggesting that some strains displayed higher activity than others. The highest α-amylase activity was produced by isolate KKU-KS5 (3.6 mm) from the Al-Khubah hot spring while, the highest protease and lipase activity were produced by isolates KKU-MS4 (4.33 mm) and KKU-MS14 (6.0 mm) from the Al-Majardah hot spring site (Figure 1). A detailed study of the promising bacterial isolates was then conducted to optimize enzymes production.

Figure 1

Hydrolysis of (A): Starch, (B): Casein and (C): Tributyrin by selected isolates using ATCC medium 697.

3.3 Bacterial identification using 16S rRNA gene sequencing and phylogenetic analysis

Three promising isolates: KKU-KS5, KKU-MS4 and KKU-MS14 were selected for identification according to their production of α-amylase, protease and lipase, respectively. The molecular genetics of the isolates was determined, to ensure accurate identification and establish the correct phylogenetic position. The primers used amplified almost 996 pb of the 16S rRNA target gene. After sequencing, the 16S rRNA gene sequences obtained for the three selected isolates were compared with the deposited sequences in GenBank for each isolate using the BLAST search of the National Center for Biotechnology Information (NCBI) databases. Alignment of the 16S rRNA gene sequences of these isolates, along with sequences obtained using a BLAST search, revealed 99% similarity to different bacterial species. The strains were virtually identical to genus Bacillus and 3 different species. These were Bacillus aerius (KKU-KS5), Bacillus licheniformis (KKU-MS4), and Bacillus sonorensis (KKU-MS14) with 99% similarity each. The three genes were deposited in GenBank, and the obtained accession numbers were recorded as KY982904, KY982906 and KY982908. In addition, Figure 2 illustrates and confirms the phylogenetic relationship among the bacterial isolates and similar strains deposited in GenBank.

Figure 2

Phylogenetic relationship among the three bacterial isolates and other bacterial strains deposited in GenBank.

3.4 Hydrolytic enzymes production

Kitchen waste (KW) collected from university kitchens was used as the sole carbon source for enzymes production. The total amount of carbohydrate, protein and lipid in KW was 76.1%, with the highest proportion being that of carbohydrate (46.2%). The total amounts of protein and fat were 18.7% and 11.2%, respectively. The production of α-amylase, protease and lipase by selected promising bacterial strains, Bacillus aerius (KKU-KS5), Bacillus licheniformis (KKU-MS4) and Bacillus sonorensis (KKU-MS14) using KW as a carbon source was investigated. The factors affecting enzyme production, including incubation period, pH, temperature and kitchen waste concentration were investigated.

3.4.1 Effect of incubation time

The fermentation process was carried out for up to 96 h with measurement of bacterial growth and enzyme activity at 12 h intervals. The results revealed that significant (P ≤ 0.05) enzyme production was initiated after the first interval, but maximum production was obtained after 72 h yielded 43.53 Uml^-1 of α-amylase, 135.2 Uml^-1 of protease and 121.26 Uml^-1 of lipase (Figure 3). Further incubation after this optimum period did not increase the enzymes activity, and a steep decrease down to 38.13%, 51.84% and 49.50%, respectively was observed after 96 h of incubation. Maximum enzyme production was obtained at the beginning of the stationary phase of bacterial growth, which suggests that enzyme production and bacterial growth correlate.

Figure 3

Effect of incubation time on bacterial growth and enzymes production.

3.4.2 Effect of initial pH

The effect of initial pH value on the production of enzymes was investigated. The results showed that enzymes production was dependent on pH value (Figure 4). Maximum α-amylase and lipase production were achieved significantly at pH 7.5 (P ≤ 0.05), while optimum protease production was obtained at pH 8.5. Enzymes production beyond these optimum pH values was markedly decreased. Enzymes production declined significantly (P ≤ 0.05) at acidic pH levels, decreasing at pH 6.0 down to 70.93%, 76.18% and 78.28% for α-amylase, protease and lipase, respectively. This suggests that these enzymes are more active in an alkaline pH.

Figure 4

Effect of initial pH on enzymes production.

3.4.3 Effect of incubation temperature

To study the effect of temperature on enzyme production, a fermentation process was carried out in the temperature range of 45 to 70°C (Figure 5). The results indicate a significant (P ≤ 0.05) relationship between enzyme production and incubation temperature up to 55-60°C. However, an increase in the temperature beyond 60°C leads to a decline in enzyme production. The activity of α-amylase and protease was optimal at 60°C with no significant reduction (P > 0.05) of α-amylase production at 65°C. Maximum lipase production was recorded at 55°C. Further increases in the incubation temperature beyond 55°C led to a rapid decline in lipase activity.

Figure 5

Effect of incubation temperature on enzymes production.

3.4.4 Effect of kitchen waste concentration

Different concentrations of the kitchen waste used as the sole carbon source were examined to establish the level for maximal enzyme production (Figure 6). Enzyme production increased gradually in proportion to the concentration of KW, it was significantly (P ≤ 0.05) rising to 5.0% (w/v) for lipase and 7.0% (w/v) for both α-amylase and protease. Enzyme production was reached 81.43 Uml^-1 for α-amylase, 281.36 Uml^-1 for protease and 167.3 Uml^-1 for lipase. It is interesting to note that optimal enzyme activity achieved dramatically decreased with a high concentration of KW. An increase in kitchen waste concentration to 9% led to a rapid decline in enzyme production of 31.27%, 17.77% and 33.45% for α-amylase, protease and lipase, respectively.

Figure 6

Effect of kitchen waste concentration % (w/v) on enzymes production.