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首页> 外文期刊>Comparative biochemistry and physiology, Part B. Biochemistry & molecular biology >Cloning and characterization of two glutathione peroxidase cDNAs from southern bluefin tuna (Thunnus maccoyii)
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Cloning and characterization of two glutathione peroxidase cDNAs from southern bluefin tuna (Thunnus maccoyii)

机译:南部蓝鳍金枪鱼(Thunnus maccoyii)的两个谷胱甘肽过氧化物酶cDNA的克隆和鉴定

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摘要

Glutathione peroxidases (GPXs; EC 1.11.19) are key enzymes in the antioxidant defence systems of living organisms, including fish. Here we report the cloning of two GPX cDNAs from southern bluefin tuna (SBT, Thunnus maccoyii). One encodes a GPX1 or classical GPX and the other encodes a GPX4 or phospholipid hydroperoxide GPX. The 898 base-pair (bp) SBT GPX1 cDNA (GenBank accession no. EF452497) includes the complete protein coding region plus 35. bp of the 5'-untranslated region (5'-UTR) and 296. bp of the 3'-untranslated region (3'-UTR). The 974. bp SBT GPX4 cDNA (GenBank accession no. EF452498) includes the complete protein coding region plus 101. bp of the 5'-UTR and 306. bp of the 3'-UTR. Both cDNAs contain a selenocysteine (Sec) codon in the protein coding region and a selenocysteine insertion sequence (SECIS) element in the 3'-UTR. The SBT GPX4 cDNA may encode a mitochondrial targeting sequence. A deduced amino acid sequence comparison revealed that the SBT GPX1 sequence was 67% identical to a human GPX1 sequence (GenBank accession no. X13709) and 69-83% identical to other fish GPX1 sequences. Similarly, the SBT GPX4 sequence was 63% identical to a human GPX4 sequence (GenBank accession no. BC046163) and 72-93% identical to other fish GPX4 sequences. GPX1 and GPX4 gene expressions and total GPX enzyme activity were investigated in SBT liver, muscle, kidney, spleen, heart, stomach, gill and pyloric caeca. Expression of the two genes varied from one tissue to the next and roughly paralleled the inter-tissue variation in GPX enzyme activity. The results are discussed in relation to possible roles for GPX1 and GPX4 genes in antioxidant defense in SBT.
机译:谷胱甘肽过氧化物酶(GPXs; EC 1.11.19)是包括鱼类在内的生物体的抗氧化防御系统中的关键酶。在这里,我们报道了从南部蓝鳍金枪鱼(SBT,金枪鱼Maccoyii)克隆了两个GPX cDNA。一个编码GPX1或经典GPX,另一个编码GPX4或磷脂氢过氧化物GPX。 898个碱基对(bp)SBT GPX1 cDNA(基因库登录号EF452497)包括完整的蛋白质编码区,以及5'-非翻译区(5'-UTR)的35.bp和3'-的296.bp。非翻译区(3'-UTR)。 974.bp的SBT GPX4 cDNA(GenBank登录号EF452498)包括完整的蛋白质编码区,加上5'-UTR的101.bp和3'-UTR的306.bp。两种cDNA均在蛋白质编码区中包含一个硒代半胱氨酸(Sec)密码子,并在3'-UTR中包含硒代半胱氨酸插入序列(SECIS)元件。 SBT GPX4 cDNA可编码线粒体靶向序列。推导的氨基酸序列比较显示,SBT GPX1序列与人GPX1序列(GenBank登录号X13709)具有67%相同,与其他鱼类GPX1序列具有69-83%相同。类似地,SBT GPX4序列与人GPX4序列(GenBank登录号BC046163)具有63%的同一性,与其他鱼类GPX4序列具有72-93%的同一性。研究了SBT肝脏,肌肉,肾脏,脾脏,心脏,胃,ill和幽门盲肠中GPX1和GPX4基因的表达以及总GPX酶的活性。这两个基因的表达在一个组织之间变化,并且大致平行于GPX酶活性的组织间变化。讨论了有关GPX1和GPX4基因在SBT中抗氧化剂防御中的可能作用的结果。

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