Purification and Characterization of an Extracellular Phosphatase Enzyme From Bacillus spp

  • سال انتشار: 1395
  • محل انتشار: مجله سلول و تحقیقات مولکولی، دوره: 8، شماره: 2
  • کد COI اختصاصی: JR_JCMR-8-2_008
  • زبان مقاله: انگلیسی
  • تعداد مشاهده: 429
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نویسندگان

Maryam Parhamfar

Department of Biology, Faculty of Science, Shahid Bahonar University of Kerman, Kerman, Iran

Arastoo Badoei-Dalfard

Department of Biology, Faculty of Science, Shahid Bahonar University of Kerman, Kerman, Iran

Milad Parhamfar

Department of Chemistry, Faculty of Science, Duissburg-Essen University, Essen, Germany

Shohreh Fahimi Rad

Department of Biotechnology, Campus of Agriculture and Natural Resources, University of Tehran, Karaj, Iran

چکیده

Phosphorus is one of the most important nutrients for plant growth and development. Chemical Pi fertilizer is used to provide the phosphorus for the plants, but it is mostly fixed in the soil into insoluble form and become unavailable to the plants. Phosphate-solubilizing bacteria have lots of application in agriculture as biological fertilizer.Consumption of biofertilizers instead of chemical fertilizers can lead to environmental pollution reduction and crop production enhancement using sustainable farming. In this study, a phosphatase-producing bacterium was isolated from agricultural soil in Kerman. Screening of phosphate solubilizing bacteria was performed on the PVK medium, based on clear area diameter. The best bacterium (AG41) was identified based on 16s rDNA gene. The optimum condition for production of phosphatase was also determined and it was purified and characterized. Sequence alignment and phylogenetic tree results show that AG41 is closely related to Bacillus subtilis, with 98% homology. Phosphatase activity was determined by end point method. The best carbon, nitrogen and phosphate sources forenzyme production were 1.0% glucose, 0.5% ammonium sulfate and (0.25%) sodium phytate +(0.25%) tricalciumphosphate, respectively. Bacterial phosphatase was partially purified using ammonium sulfate fractionation followedby dialysis. Results showed that the optimum temperature for the purified enzyme activity was 40oC and it was stableat temperatures below 60°C. This enzyme was stable between pH 3.0-7.0, and the optimal pH activity was found to5.0. These results indicated that this strain can be a notable candidate for using as biofertilizers

کلیدواژه ها

Screening, Biofertilizer, Phosphate-solubilizing bacteria, Phosphatase

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