1. IntroductionAlkaline proteases a

1. Introduction
Alkaline proteases are widely used biocatalytic enzyme and well known for their emerging novel

properties and their exotic catalytic nature. Hence alkaline protease producing organisms have attracted more attention of the scientific community so as to enhance and ensure better utilization of proteins [3] and [20]. These enzymes find diverse applications in different industries such as detergent, food, feed, pharmaceutical, leather, silk and for recovery of silver from used X-ray films [1], [12] and [29]. Microorganisms represent an excellent source of protease owing to their broad biochemical diversity and susceptibility to genetic manipulation that are desirable for various applications [11]. Alkaline proteases can be defined as the proteases that are active in alkaline range of pH [13] and [15]. Microbial proteases are among the most important hydrolytic enzymes and have been studied extensively since the advent of enzymology. Looking into the depth of microbial diversity, there is always a chance of finding microorganism producing novel enzymes with better properties and suitable for commercial exploitation. The multitude of physiochemical diverse habitats has challenged nature to develop equally numerous molecular adaptations in the microbial world. The 16S rDNA method is sequence based taxonomy and in the present scenario, molecular characterization based on RAPD fingerprinting is additionally used to study the microbial diversity or variability and their ecological distribution. RAPD is a very convenient and cost effective method employed for bacterial identification and variability estimation [17]. The PCR based method of gene typing based on genomic polymorphism is a recent approach which is widely used for the assessment of inter and intraspecific genetic variation and uses a single short random oligonucleotide primer [36]. In most cases of bacterial genetics, RAPD assay generated the best DNA pattern for differentiation of bacteria. A number of studies have reported success in using RAPD assays to distinguish bacterial strains among diverse species [28], [4], [9] and [10]. A study on genetic variability among Arthrobacter strain by phylogenetic analysis of RAPD-PCR fingerprint patterns has been reported by Saxena and Singh (2013) [31].

2. Materials and methods
2.1. Sample collection

For the isolation of protease producing bacteria, soil samples were collected from agricultural fields of Central Soil Salinity Research Institute, slaughter house, fish harbour and dairy house etc. (Table 1). Soil samples were collected in sterile polybags and stored at 4 °C for further experiments. Prior to collection of sample the pH of the soil was monitored.