Isolation and characterization of mercuric reductase by newly isolated halophilic bacterium, Bacillus firmus MN8

Isolation and characterization of mercuric reductase by newly isolated halophilic bacterium, Bacillus firmus MN8

The current study was aimed at isolating and identifying the halophilic and halotolerant bacteria which can produce mercuric reductase in Gavkhuni wetland in Iran. Moreover, tracking and sequencing merA gene and kinetic properties of mercuric reductase in the selected strain were performed in this s...

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Main Authors: M. Noroozi, M.A. Amoozegar, A.A. Pourbabaei, N.S. Naghavi, Z. Nourmohammadi
Format: Article
Language:English
Published: GJESM Publisher 2017-12-01
Series:Global Journal of Environmental Science and Management
Subjects:
Halophilic bacteria
merA gene
Mercuric reductase enzyme
Mercury
Polymerase chain reaction (PCR)
Online Access:http://www.gjesm.net/article_26733_e6562214d0ea5eb3b5c58a6c94575151.pdf
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spelling doaj-d18a7d2af50f404f90bc38bf2a43d79f2021-02-02T07:58:56ZengGJESM PublisherGlobal Journal of Environmental Science and Management2383-35722383-38662017-12-013442743610.22034/gjesm.2017.03.04.00826733Isolation and characterization of mercuric reductase by newly isolated halophilic bacterium, Bacillus firmus MN8M. Noroozi0M.A. Amoozegar1A.A. Pourbabaei2N.S. Naghavi3Z. Nourmohammadi4Department of Biology, Science and Research Branch, Islamic Azad University, Tehran, IranDepartment of Microbiology, Faculty of Biology, College of Science, University of Tehran, Tehran, IranSoil Science Department, Faculty of Agricultural Engineering and Technology, University College of Agriculture and Natural Resources, University of Tehran, Tehran, IranDepartment of Microbiology, Falavarjan Branch, Islamic Azad University, Isfahan, IranDepartment of Biology, Science and Research Branch, Islamic Azad University, Tehran, IranThe current study was aimed at isolating and identifying the halophilic and halotolerant bacteria which can produce mercuric reductase in Gavkhuni wetland in Iran. Moreover, tracking and sequencing merA gene and kinetic properties of mercuric reductase in the selected strain were performed in this study. Soil samples were taken from Gavkhuni wetland and cultured in nutrient agar medium with 5% NaCl. To examine the tolerance of purified colonies to mercury, agar dilution method was administered. Similarly, the phylogenetic analysis based on 16SrRNA gene sequencing was conducted. To investigate enzyme activity of kinetic parameters, a spectrophotometer was used to measure the NADPH oxidation decrease at 340 n.m. The results showed that among the 21 halophilic and halotolerant strains isolated from Gavkhuni wetland, 4 were resistant to mercuric chloride. A strain designated MN8 was selected for further studies because it showed the highest resistance to mercury. According to phylogenetic sequencing of 16S rRNA gene and phenotypic characteristics, the strain was categorized in the Bacillus genus and nearly related to Bacillus firmus. This strain had merA gene. The mercuric reductase showed Vmax and Km values of 0.106 U/mg and 24.051 µM, respectively. Evaluation of different concentrations of NaCl at 37°C and pH=7.5 in mercuric reductase enzyme activity indicated that the enzyme shows 50% activity in concentration of 1.5 M. Optimum pH and temperature of  enzyme activity were 7.5 and 35 °C, respectively. The results suggested that MN8 strain could be a proper candidate for bioremediation of mercury-contaminated environments such as industrial wastewaters.http://www.gjesm.net/article_26733_e6562214d0ea5eb3b5c58a6c94575151.pdfHalophilic bacteriamerA geneMercuric reductase enzymeMercuryPolymerase chain reaction (PCR)
collection DOAJ
language English
format Article
sources DOAJ
author M. Noroozi
M.A. Amoozegar
A.A. Pourbabaei
N.S. Naghavi
Z. Nourmohammadi
spellingShingle M. Noroozi
M.A. Amoozegar
A.A. Pourbabaei
N.S. Naghavi
Z. Nourmohammadi
Isolation and characterization of mercuric reductase by newly isolated halophilic bacterium, Bacillus firmus MN8
Global Journal of Environmental Science and Management
Halophilic bacteria
merA gene
Mercuric reductase enzyme
Mercury
Polymerase chain reaction (PCR)
author_facet M. Noroozi
M.A. Amoozegar
A.A. Pourbabaei
N.S. Naghavi
Z. Nourmohammadi
author_sort M. Noroozi
title Isolation and characterization of mercuric reductase by newly isolated halophilic bacterium, Bacillus firmus MN8
title_short Isolation and characterization of mercuric reductase by newly isolated halophilic bacterium, Bacillus firmus MN8
title_full Isolation and characterization of mercuric reductase by newly isolated halophilic bacterium, Bacillus firmus MN8
title_fullStr Isolation and characterization of mercuric reductase by newly isolated halophilic bacterium, Bacillus firmus MN8
title_full_unstemmed Isolation and characterization of mercuric reductase by newly isolated halophilic bacterium, Bacillus firmus MN8
title_sort isolation and characterization of mercuric reductase by newly isolated halophilic bacterium, bacillus firmus mn8
publisher GJESM Publisher
series Global Journal of Environmental Science and Management
issn 2383-3572
2383-3866
publishDate 2017-12-01
description The current study was aimed at isolating and identifying the halophilic and halotolerant bacteria which can produce mercuric reductase in Gavkhuni wetland in Iran. Moreover, tracking and sequencing merA gene and kinetic properties of mercuric reductase in the selected strain were performed in this study. Soil samples were taken from Gavkhuni wetland and cultured in nutrient agar medium with 5% NaCl. To examine the tolerance of purified colonies to mercury, agar dilution method was administered. Similarly, the phylogenetic analysis based on 16SrRNA gene sequencing was conducted. To investigate enzyme activity of kinetic parameters, a spectrophotometer was used to measure the NADPH oxidation decrease at 340 n.m. The results showed that among the 21 halophilic and halotolerant strains isolated from Gavkhuni wetland, 4 were resistant to mercuric chloride. A strain designated MN8 was selected for further studies because it showed the highest resistance to mercury. According to phylogenetic sequencing of 16S rRNA gene and phenotypic characteristics, the strain was categorized in the Bacillus genus and nearly related to Bacillus firmus. This strain had merA gene. The mercuric reductase showed Vmax and Km values of 0.106 U/mg and 24.051 µM, respectively. Evaluation of different concentrations of NaCl at 37°C and pH=7.5 in mercuric reductase enzyme activity indicated that the enzyme shows 50% activity in concentration of 1.5 M. Optimum pH and temperature of  enzyme activity were 7.5 and 35 °C, respectively. The results suggested that MN8 strain could be a proper candidate for bioremediation of mercury-contaminated environments such as industrial wastewaters.
topic Halophilic bacteria
merA gene
Mercuric reductase enzyme
Mercury
Polymerase chain reaction (PCR)
url http://www.gjesm.net/article_26733_e6562214d0ea5eb3b5c58a6c94575151.pdf
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AT aapourbabaei isolationandcharacterizationofmercuricreductasebynewlyisolatedhalophilicbacteriumbacillusfirmusmn8
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AT znourmohammadi isolationandcharacterizationofmercuricreductasebynewlyisolatedhalophilicbacteriumbacillusfirmusmn8
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