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硅藻威氏海链藻铁/锰超氧化物歧化酶的特性:克隆、表达及性质

Characterization of Fe/Mn-superoxide dismutase from diatom Thallassiosira weissflogii: cloning, expression, and property.

作者信息

Ken Chuian-Fu, Hsiung Tung-Ming, Huang Zong-Xian, Juang Rong-Huay, Lin Chi-Tsai

机构信息

Institute of Bioscience and Biotechnology, National Taiwan Ocean University, 2 Pei-Ning Road, Keelung, Taiwan 202, Institute of Biotechnology, National Changhua University of Education, Changhua, Taiwan.

出版信息

J Agric Food Chem. 2005 Mar 9;53(5):1470-4. doi: 10.1021/jf048269f.

Abstract

A cDNA clone of 1114 bp encoding a putative Mn-superoxide dismutase (Mn-SOD) from diatom Thallassiosira weissflogii was cloned by the PCR technique. Nucleotide sequence analysis of this cDNA clone revealed that it was translated into 201 amino acid residues. When the sequence was compared with Mn-SODs from Vibrio mimicus and Escherichia coli, as well as two Fe-SODs from E. coli and Photobacterium leiognathi, this SOD showed higher homology to Mn-SOD. The amino acid residues required to coordinate the single manganese ion were conserved in all reported Mn-SOD sequences. This cDNA was introduced in an expression vector, pET-20b(+), and transformed into E. coli BL21(DE3)pLysS. The expressed SOD protein was then purified by a His-tag column. The recombinant enzyme was heated at 55 degrees C with a time-dependent assay; the time interval for 50% inactivation was 23 min, and its thermal inactivation rate constant K(d) was 3.03 x 10(-)(2) min(-)(1). The enzyme was inactivated either in acidic pH (below 4.0) or in the presence of imidazole (above 1.6 M) and had only a moderate effect under SDS (above 4%), whereas it was not affected under an alkaline pH (above 9.0). The atomic absorption spectrometric assay showed that 0.6 atom of iron/manganese (3:1) was present in each subunit of SOD. Reconstitution study was suggested that diatom SOD was cambialistic (Fe/Mn)-SOD. The finding of this SOD cDNA could be used for a reference in comparing the differences among marine phytoplankton species and as a probe to detect the transcription level of this enzyme, which can be applied in cosmetics for skin protection or defending unesthetic effects caused by oxygen-containing free radicals.

摘要

利用PCR技术从硅藻三角褐指藻(Thallassiosira weissflogii)中克隆出一个1114 bp的cDNA克隆,其编码一种假定的锰超氧化物歧化酶(Mn-SOD)。对该cDNA克隆进行核苷酸序列分析表明,它可被翻译为201个氨基酸残基。将该序列与模仿弧菌(Vibrio mimicus)和大肠杆菌(Escherichia coli)的Mn-SOD以及大肠杆菌和发光杆菌(Photobacterium leiognathi)的两种Fe-SOD进行比较时,这种SOD与Mn-SOD具有更高的同源性。在所有已报道的Mn-SOD序列中,配位单个锰离子所需的氨基酸残基是保守的。将此cDNA引入表达载体pET-20b(+),并转化到大肠杆菌BL21(DE3)pLysS中。然后通过His标签柱纯化表达的SOD蛋白。对重组酶进行55℃的时间依赖性加热测定;50%失活的时间间隔为23分钟,其热失活速率常数K(d)为3.03×10(-2) min(-1)。该酶在酸性pH(低于4.0)或咪唑存在(高于1.6 M)时失活,在SDS存在(高于4%)时只有中等程度的影响,而在碱性pH(高于9.0)下不受影响。原子吸收光谱测定表明,SOD的每个亚基中存在0.6个铁/锰原子(3:1)。重组研究表明硅藻SOD是兼性(铁/锰)-SOD。该SOD cDNA的发现可用于比较海洋浮游植物物种之间的差异,并作为检测该酶转录水平的探针,可应用于化妆品中用于皮肤保护或抵御含氧自由基引起的不良影响。

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