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Homology Modeling and Probable Active Site Cavity Prediction of Uncharacterized Arsenate Reductase in Bacterial spp.

Authors
Rahman, Md ShahedurHossain, Md SaddamSaha, Subbroto KumarRahman, SoikatSonne, ChristianKim, Ki-Hyun
Issue Date
Jan-2021
Publisher
SPRINGER
Keywords
arsC gene; Bioremediation; Predicted model; Bioinformatics; Active site
Citation
APPLIED BIOCHEMISTRY AND BIOTECHNOLOGY, v.193, no.1, pp.1 - 18
Indexed
SCIE
SCOPUS
Journal Title
APPLIED BIOCHEMISTRY AND BIOTECHNOLOGY
Volume
193
Number
1
Start Page
1
End Page
18
URI
https://scholarworks.bwise.kr/hanyang/handle/2021.sw.hanyang/8074
DOI
10.1007/s12010-020-03392-w
ISSN
0273-2289
Abstract
The arsC gene-encoded arsenate reductase is a vital catalytic enzyme for remediation of environmental arsenic (As). Microorganisms containing the arsC gene can convert pentavalent arsenate (As[V]) to trivalent arsenite (As[III]) to be either retained in the bacterial cell or released into the air. The molecular mechanism governing this process is unknown. Here we present an in silico model of the enzyme to describe their probable active site cavities using SCFBio servers. We retrieved the amino acid sequence of bacterial arsenate reductase enzymes in FASTA format from the NCBI database. Enzyme structure was predicted using the I-TASSER server and visualized using PyMOL tools. The ProSA and the PROCHECK servers were used to evaluate the overall significance of the predicted model. Accordingly, arsenate reductase fromStreptococcus pyogenes,Oligotropha carboxidovoransOM5,Rhodopirellula balticaSH 1, andSerratia ureilyticahad the highest quality scores with statistical significance. The plausible cavities of the active site were identified in our examined arsenate reductase enzymes which were abundant in glutamate and lysine residues with 6 to 16 amino acids. This in silico experiment may contribute greatly to the remediation of arsenic pollution through the utilization of microbial species.
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