Protease Production Capabilities of Micrococcus Luteus and Bacillus Species Isolated from Abattoir Environment

The study investigated the optimum conditions of temperature, pH, inoculum size and time of incubation on bacterial p rotease production. Protease producing bacterial species were isolated from abattoir soil and identified as Micrococcus luteus and Bacillus species. The optimum conditions observed for protease production was 37°C at pH 7, with 1% inoculum in the medium for 24 h of incubation in Micrococcus luteus while in Bacillus species, the optimum conditions observed was 47°C at pH 9, with 2% inoculum concentration in the medium for 96 h of incubation. Generally, temperature and pH had more effect on the protease activity of Micrococcus luteus while inoculum concentration and time of incubation had more effect on the protease activity of Bacillus species. The study gave evidence that these bacterial isolates could be potentially applied in biotechnological processes.


Introduction
Microbial protease represents about 60% of all the industrial enzy me's sales in the world due to their applications in several industrial sectors [1]. The induction of protease requires a substrate having peptide bonds including substrates like peptone, casein and other protein sources. The ammon ia, as final product of enzy matic reaction of substrate hydrolysis, represses enzyme synthesis by a well-known mechanis m of catabolite repression. This ext racellular protease has also been commercially exp loited to assist protein degradation in various industrial processes [2]. The great advantages offered by microbial en zy mes are low material costs coupled with high and faster productivity and the ease with which the en zy mes can be mod ified [3]. At present, due to high cost of substrates and mediums used, the overall cost of enzyme production is very high and therefore, development of novel processes to increase the yield of proteases with respect to their industrial requirements coupled with lowering down the production cost is highly appreciable fro m the co mmercial point of v iew [4].
Pro teas es are co mp lex mu lt i-en zy me system wh ich cataly zes the hy d ro lys is o f amid e bo nd in a p ro tein mo lecu lar hence it has been used in the field o f text ile p rocess ing fo r d egu mmin g o f s ilk and p ro cess in g o f wo o l [ 5 -6 ]. W ith th e ad v en t o f n e w f ro n t ie rs in biotechnology, the spectrum of protease application has expanded into many new fields, such as clinical, med icinal and analytical chemistry. To meet the current largely increased demand, studies on the cost-effective production of industrially important enzy mes have become the need of today.
Microorganisms are the most important sources for enzy me production. Selection of the right organism p lays a key role in high yield of desirable en zy mes. For production of enzy mes for industrial use, isolation and characterization of new pro mising strains using cheap carbon and nitrogen source is a continuous process. Habitats that contain protein are the best sources to isolate proteolytic microorganisms. Waste products of meat, poultry and fish processing industries can supply a large amount of p rotein rich materials for bioconversion to recoverable products [7].
Proteases are present in all living organisms but microb ial proteases are most explo ited group of industrial en zy mes. Based on their mode of action, they are further classified into four categories: alkaline, acid, thiol and metallo proteases. Alkaline (serine) Proteases are active over a broad pH (7)(8)(9)(10)(11)(12) and temperature (35℃-80℃) ranges, [8], they are worldwide center of attraction for researchers. Several fungi, actinomycetes and bacteria are endowed with the capacity to produce alkaline serine proteases in diverse environmental and agro-climatic conditions. However bacterial proteases are preferred as they grow rapidly , need less space, can be easily maintained and are accessible for genetic man ipulations. The important protease producing bacteria are species of Bacillus, Pseudomonas, Halomonas, Arthrobacter and Serratia. Among all bacterial specie, Bacillus Species Isolated from Abattoir Environment Bacilli play an important role in production of alkaline protease owing to their chemoorganotrophic nature, several species of Bacillus are industrially emp loyed to produce thermostable alkaline protease as they grow easily under extreme pH and temperature conditions. The enhancement of protease production by genetic manipulation has been well studied in Bacillus cereus, Bacillus subtilis, Bacillus stearothermophilus etc, by a number of researchers, which further underlines the significance of this en zy me [8].
The present study is aimed at isolation of protease producing bacterial species from abattoir environ ment and to determine the optimu m conditions for protease activity.

Sample Collection and Isolation of Proteolytic Bacteria
The soil samp les were collected fro m an abattoir environment in Owerri, Imo State, Nigeria. They were stored in ice and analy zed within one hour of collection. One gram of soil sample in a 250 ml flask was homogenized with 10 ml of sterile water; it was later made up to 100 ml with sterile water, mixed and shaken on a mechanical shaker for 45 minutes. An aliquot of the homogenized sample (0.2 ml) was spread on casein agar plates (nutrient agar supplemented with 36% casein) and incubated for 48 hours at 37℃. The isolates were identified based on their morphological and biochemical characteristics [9](Ho lt et al., 1994).

Screening of Proteolytic Bacteri a
The screening method described by Amara et al. [10](2009) was adopted. Briefly, to 100 ml of sterile water contained in a 250 ml flask was added 3 g of skim milk and autoclaved for 15 min. after sterilizat ion, the suspension was decanted and the soluble solution was added to sterile water agar (16 g agar/l). The mixture was gently stirred until co mp letely homogenized and then distributed in petri d ishes. After med ia solidificat ion, the bacterial cultures were inoculated on the plated and incubated at 50℃ for Bacillus species and 37 ℃ for Micrococcus luteus. Clear zones around the bacterial colonies indicate the presence of proteolytic activity which can be confirmed using coomassie blue staining method.

Coomassie Staining Method
This was performed using the method of Weber and Osborn [11] (1969). Coo massie blue was dissolved in a solution of methanol-acetic acid-water (5:1:4[v/v/v]) to achieve 0.25% (w/v). Ten milliliter of the staining solution was added to each of the p lates and incubated at room temperature for 15 min. After the incubation the staining solution was removed fro m the plate and the plate gently washed with distilled water. Thereafter, the plates were de-stained with a solution containing 66 ml methanol, 20 ml acetic acid and 114 ml of distilled water till there was a clear contrast between the plate's background and the degradation zones around the bacterial colonies.

Protease Acti vity Assay
The protease activity was determined according to the method of Anson [12](1938) with some modifications. The isolates were grown in a mediu m containing 10 g of g lucose, 5 g of casein, 5 g of yeast extract, 2 g of KH 2 PO 4 and 10 g of Na 2 CO 3 in 100 ml o f sterile water. After sterilization, the med iu m was inoculated at 37℃ for 48 h. After incubation the culture filtrates were collected by centrifugation at 1000 x g for 12 minutes at 4 0 C. The supernatant was used as crude enzy me. 0.5 ml of the crude extract was mixed with 5.0ml of Tris-Hcl buffered casein and incubated at 37 ℃ for 30minutes. After incubation, 5ml of 110 mM t rich loroacetic acid (TCA) was added to stop the reaction. The mixture was centrifuged at 10,000 rp m for 5 minutes and the released amino acids were measured as tyrosine using the method of Folin and Ciocalteu [13](1929) by calculating the amount of tyrosine in the extract using a tyrosine standard curve. The enzy me activity was expressed in units (U). One unit of enzy me was defined as the amount of enzyme that releases 1 μmol of tyrosine per mm o f crude ext ract per minute.

Effect of Temperature on Protease Producti on
The effect of temperature on protease production was studied by incubating the culture media at different temperatures ranging fro m 27℃-77℃ for 24hrs. Protease activity was determined after 24hrs of incubation.

Effect of pH on Protease Producti on
The effect pH on protease production was determined by culturing the bacterium in the protease production media with different pH ranges (pH5 to 11). The en zy me assay was carried out after 24rs of incubation at 37℃.

Effect of Inoculum Concentration on Protease Produc tion
Effect of Inoculu m concentration on protease production was determined by inoculating the production mediu m with different concentrations (2-7%) of overnight grown bacterial culture. The inoculated mediu m was incubated at 37℃ for 24hrs after which the culture mediu m was centrifuged at 5000 rp m at 4 ℃ fo r 15mins. The protease activity was determined as stated above.

Statistical Anal ysis
Data obtained from this study were analyzed using a two-way analysis of variance (A NOVA ) and values for P≤0.05 were considered statistically significant.

Result
Temperature had effect on the production of protease in both organisms. There was an increase in protease production with increase in temperature up to the temperature o f 37 ℃ in Micrococcus luteus. After this temperature, the protease production started reducing gradually with increase in temperature t ill the end the work with the lowest protease production obtained at the temperature of 77℃, (fig. 1). The same observation was made in Bacillus species but the maximu m protease production was obtained at the temperature of 47℃ (1.249 U/ ml/ min). Temperature had more effect on the protease activity of M icrococcus luteus than on Bacillus species although there is no significant difference on the temperature activities of the two organis ms (P≤0.05).
The result showed that both organisms were affected by increase in p H. In both organisms, protease production increased with increase in p H, (fig. 2). Their maximu m protease productions were at pH 7 and 9, respectively for Micrococcus luteus and Bacillus species (1.23586 U/ ml/ min and 1.19804 U/ ml/ min, respectively). The lowest protease activities in both organisms were at pH 11. Statistical analysis showed no significant difference on the effect of pH on the protease activities of both organisms, (P≤0.05).

Micrococcus luteus Bacillus sp
Increase in inoculu m concentration increased the protease activity in both organisms. In Micrococcus luteus the highest protease production was observed at 1% inoculum concentration (1.17282U/ ml/ min). The maximu m inoculum concentration for protease activity in Bacillus species was 2% ( fig. 3). Increasing the concentration beyond these concentrations resulted in decrease in the protease production. There was a very high significant difference in the effect of inoculum concentration on protease activities of both organisms at P≤0.05. Micrococcus luteus had significantly higher p rotease activities than Bacillus species.
The result of the effect of time of incubation on protease production showed that there was an equal protease production in both organisms at the 24 th and 48 th hours of incubation (1.21065 U/ ml/ min). There was drastic decrease in protease production with increase in the time of incubation in both organisms beyond 48 hours of incubation ( fig. 4). The highest protease activities in both organisms were observed at 24 hours and 48 hours of incubation. In Micrococcus luteus, there was no further decrease in protease production beyond 96 hours of incubation while there was a sharp decrease in protease production 72 hours of incubation till 168 hours of incubation. Incubation time had significantly mo re negative effect on protease production of Bacillus species than Micrococcus luteus, (P≤0.05).

Discussion
The study investigated the optimu m conditions for protease production in Micrococcus luteus and Bacillus species. These parameters investigated included the effect of temperature, pH, inoculu m concentration and time of incubation on the production of protease. It was discovered that the parameters investigated had varying effects on the protease activities of the isolates. On temperature effect, it was discovered that there was an increase in protease production with increase in temperature up to the maximu m protease activities at the temperature of 37℃ and 47℃ for Micrococcus luteus and Bacillus species, respectively. Kalaiarasi and Sunitha [14] also reported a similar trend in Pseudomosa fluorescens where they observed that the organism could produce protease in the range of 27-57℃ with p roduction maximu m at 37℃. Ho wever, increase in temperature beyond 37℃ and 47℃ for Micrococcus luteus and Bacillus species, respectively led to decline in protease production proving that temperature plays a majo r ro le in enzy me production.
The pH of the culture strongly affects many enzy matic processes and transport of compounds across the cell memb rane. The protease activities of the isolates were also affected by the pH of the mediu m. Increase in pH resulted in corresponding increase in protease production up to the maximu m protease production at pH 7 and 9, respectively for Micrococcus luteus and Bacillus species (1.23586 U/ ml/ min and 1.19804 U/ ml/ min, respectively). The result showed that there was a stimu lation of the enzyme production at neutral pH for Micrococcus luteus and alkaline pH for Bacillus species. The result obtained is in consonance with the work of Ku mar et al. [15] who reported the protease production was at maximu m at p H 7 and 9 for Bacillus sp. and Pseudomonas sp. respectively although vary in the organisms involved. This same result was also obtained by Amara et al. [10] and Sathees Kumar et al. [16] who observed an optimu m protease activity of 34 Unit/ ml and 215.56 U/ ml for Geobacillus sp and Pseudomonas aeruginosa, respectively at pH 9 and the work of Sally [17] who, using Azocoll as a protease substrate, observed highest specific protease activity of Burkholderia strain 2.2 N at pH 7.5. Production of protease at alkaline pH has been reported by so many authors. The bacterial isolate, Bacillus amovivorus, was found by Sharmin et al. [18] to exhib it maximu m protease production at mediu m pH 8.5 but the highest biomass yield was recorded at med iu m pH 7.0. Aftab et al. [19] also reported that alkaline protease production by Bacillus brevis was found in alkaline mediu m at p H 10.5 Previously, Freshteh et al. [20] also reported production of alkaline protease by Bacillus strain L2 at pH 10.5. Maximu m protease production from the genus Bacillus was observed by Mahendran et al. [21] at pH 8.0 while at pH 10, the protease production was about 60%.
Initial inoculu m concentration influenced the production of protease in both organisms. It was observed that increase in inoculu m concentration increased the protease activity in both organisms up to the maximu m of 1.17282 U/ ml/ min at 1% inoculu m concentration for Micrococcus luteus and 1.16021 U/ ml/ min at 2% Bacillus species. Increasing the inoculum concentration beyond these percentages resulted in decrease in the protease activity in both organisms. These results were partly in accordance with Elibol et al. [22] who reported that 2.5% inoculu m level g ives higher protease production.
Time of incubation also had effect on the protease production of the two bacterial isolates. The result of the effect of time of incubation on protease production showed that there was a drastic decrease in protease production with increase in the time o f incubation in both organisms. The highest protease activity observed in both organisms was at 24 and 48 hours of incubation in both organisms. This finding is in partial agreement with the work of Ku mar et al. [15] who reported that Pseudomonas sp. S22 showed a peak for protease production at 24 h of incubation and again at 108 h of incubation. However, the present result is in total agreement with the work of Kalaiarasi and Sunitha [14] who observed the same peak protease production at 24 h of incubation.

Conclusions
The data gathered in this study has provided evidence for the protease producing ability of abattoir-soil-isolated Micrococcus luteus and Bacillus species. The influence of environmental factors on the protease production of the isolates was also evident in this study. This study has given a hint that the microbial wealth of protease producing bacteria isolated fro m abattoir environ ment can be harnessed for biotechnological processes. The appreciable high en zy me activity at alkaline pH suggested that Bacillus species is a potential producer of alkaline proteases which can find application in detergent and text ile industries.