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首页> 外文期刊>The Journal of Experimental Biology >Cytoplasmic carbonic anhydrase isozymes in rainbow trout Oncorhynchus mykiss: comparative physiology and molecular evolution
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Cytoplasmic carbonic anhydrase isozymes in rainbow trout Oncorhynchus mykiss: comparative physiology and molecular evolution

机译:虹鳟Onkihynchus mykiss的细胞质碳酸酐酶同工酶:比较生理学和分子进化

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It is well established that the gills of teleost fish contain substantial levels of cytoplasmic carbonic anhydrase (CA), but it is unclear which CA isozyme(s) might be responsible for this activity. The objective of the current study was to determine if branchial CA activity in rainbow trout was the result of a general cytoplasmic CA isozyme, with kinetic properties, tissue distribution and physiological functions distinct from those of the red blood cell (rbc)specific CA isozyme. Isolation and sequencing of a second trout cytoplasmic CA yielded a 780 bp coding region that was 76% identical with the trout rbc CA (TCAb), although the active sites differed by only 1 amino acid. Interestingly, phylogenetic analyses did not group these two isozymes closely together, suggesting that more fish species may have multiple cytoplasmic CA isozymes. In contrast to TCAb, the second cytoplasmic CA isozyme had a wide tissue distribution with high expression in the gills and brain, and lower expression in many tissues, including the red blood cells. Thus, unlike TCAb, the second isozyme lacks tissue specificity and may be expressed in the cytoplasm of all cells. For this reason, it is referred to hereafter as TCAc (trout cytoplasmic CA). The inhibitor properties of both cytoplasmic isozymes were similar (K-i acetazolamide 1.21 +/- 0.18 nmol l(-1) and 1.34 +/- 0.10 nmol l(-1) for TCAc and TCAb, respectively). However, the turnover of TCAb was over three times greater than that of TCAc (30.3 +/- 5.83 vs 8.90 +/- 1.95 e(4) s(-1), respectively), indicating that the rbc-specific CA isoform was significantly faster than the general cytoplasmic isoform. Induction of anaemia revealed differential expression of the two isozymes in the red blood cell; whereas TCAc mRNA expression was unaffected, TCAb mRNA expression was significantly increased by 30- to 60-fold in anaemic trout.
机译:众所周知,硬骨鱼类的ill中含有大量的细胞质碳酸酐酶(CA),但目前尚不清楚哪种CA同工酶可能引起这种活动。本研究的目的是确定虹鳟鱼中的分支CA活性是否是一般细胞质CA同工酶的结果,其动力学特性,组织分布和生理功能不同于红细胞(rbc)特异性CA同工酶。第二个鳟鱼胞质CA的分离和测序产生了一个780 bp的编码区,与鳟鱼rbc CA(TCAb)的同源性为76%,尽管活性位点仅相差1个氨基酸。有趣的是,系统发育分析并未将这两种同工酶紧密地分组在一起,这表明更多的鱼类可能具有多种胞质CA同工酶。与TCAb相比,第二种胞质CA同工酶具有广泛的组织分布,在the和脑中高表达,而在包括红血球在内的许多组织中低表达。因此,与TCAb不同,第二同工酶缺乏组织特异性并且可以在所有细胞的细胞质中表达。因此,以下将其称为TCAc(鳟鱼胞质CA)。两种胞质同工酶的抑制剂性质相似(分别为TCAc和TCAb的K-1乙酰唑酰胺1.21 +/- 0.18 nmol l(-1)和1.34 +/- 0.10 nmol l(-1)。但是,TCAb的周转率是TCAc的周转率的三倍以上(分别为30.3 +/- 5.83对8.90 +/- 1.95 e(4)s(-1)),表明rbc特异性CA同种型显着比一般的细胞质亚型更快。贫血的诱导揭示了红细胞中两种同工酶的差异表达。而TCAc mRNA表达不受影响,贫血鳟鱼中TCAb mRNA表达显着增加30到60倍。

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