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首页> 外文期刊>Comparative biochemistry and physiology, Part B. Biochemistry & molecular biology >Sequence analysis and tissue expression pattern of Sparus aurata chymotrypsinogens and trypsinogen
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Sequence analysis and tissue expression pattern of Sparus aurata chymotrypsinogens and trypsinogen

机译:Sparus aurata糜蛋白酶和胰蛋白酶原的序列分析和组织表达模式

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Two apparently full-length cDNA clones encoding chymotrypsinogens I and II (CHTRI, 1022 bp; CHTRII, 909 bp) and one eDNA clone encoding trypsinogen II (TRPII, 848 bp) were isolated from a cDNA library prepared from gilthead sea bream (Sparus aurata) liver. The deduced amino acid sequences of the isolated cDNAs contain highly conserved residues essential for serine protease catalytic activity and conformational maintenance. The deduced amino acid sequences of CHTRI and CHTRII are 261 as and 277 as long, respectively, and share only 61% identity. Sea bream CHTRII appears to be the longest of all known teleostean chymotrypsinogen forms and contains a high number of methionine residues. Compared with CHTRI, CHTRII is more hydrophobic and has a lower isoelectric point. On the other hand, deduced amino acid sequence of TRPII is 241 as long and has a signal peptide of thirteen amino acid residues and an activation peptide of seven amino acids long. In contrast to CHTRI and CHTRII, TRPII has a low isoelectric point (4.95), which makes it anionic at neutral pH. Northern blot analysis revealed that liver is the major transcription site for all zymogens. As expected, all zymogen transcripts were detected in parts of the digestive tract (stomach, pyloric cacca, anterior and posterior intestine) and pyloric caeca presented the most intense expression. In all tissues and amongst all zymogens, TRPII constitutive expression was the highest. (c) 2007 Elsevier Inc. All rights reserved.
机译:从由头鲷(Sparus aurata)制备的cDNA文库中分离出两个编码胰凝乳蛋白酶原I和II(CHTRI,1022 bp; CHTRII,909 bp)的显然全长cDNA克隆和一个编码胰蛋白酶原II(TRPII,848 bp)的eDNA克隆。 ) 肝。分离的cDNA的推导的氨基酸序列包含高度保守的残基,这些残基对于丝氨酸蛋白酶催化活性和构象维持是必不可少的。推导的CHTRI和CHTRII的氨基酸序列分别长为261 as和277 as,并且仅具有61%的同一性。鲷CHTRII似乎是所有已知的硬骨胰凝乳蛋白酶原形式中最长的一种,并且含有大量的蛋氨酸残基。与CHTRI相比,CHTRII疏水性更高,等电点更低。另一方面,推导的TRPII的氨基酸序列长为241,具有13个氨基酸残基的信号肽和7个氨基酸长的激活肽。与CHTRI和CHTRII相比,TRPII具有较低的等电点(4.95),这使其在中性pH下为阴离子。 Northern印迹分析表明,肝脏是所有酶原的主要转录位点。如预期的那样,在消化道的某些部分(胃,幽门腺,前肠和后肠)检测到所有的酶原转录物,而幽门盲肠的表达最为强烈。在所有组织中和所有酶原中,TRPII组成型表达最高。 (c)2007 Elsevier Inc.保留所有权利。

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