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从红色海藻石花菜中鉴定和表征一种新型豆科样凝集素 cDNA 序列。

Identification and characterization of a novel legume-like lectin cDNA sequence from the red marine algae Gracilaria fisheri.

机构信息

Center of Excellence for Shrimp Molecular Biology and Biotechnology, Faculty of Science, Mahidol University, Bangkok, Thailand.

出版信息

J Biosci. 2011 Dec;36(5):833-43. doi: 10.1007/s12038-011-9144-8.

DOI:10.1007/s12038-011-9144-8
PMID:22116281
Abstract

A legume-type lectin (L-Lectin) gene of the red algae Gracilaria fisheri (GFL) was cloned by rapid amplification of cDNA ends (RACE). The full-length cDNA of GFL was 1714 bp and contained a 1542 bp open reading frame encoding 513 amino acids with a predicted molecular mass of 56.5 kDa. Analysis of the putative amino acid sequence with NCBI-BLAST revealed a high homology (30-68%) with legume-type lectins (L-lectin) from Griffithsia japonica, Clavispora lusitaniae, Acyrthosiphon pisum, Tetraodon nigroviridis and Xenopus tropicalis. Phylogenetic relationship analysis showed the highest sequence identity to a glycoprotein of the red algae Griffithsia japonica (68%) (GenBank number AAM93989). Conserved Domain Database analysis detected an N-terminal carbohydrate recognition domain (CRD), the characteristic of L-lectins, which contained two sugar binding sites and a metal binding site. The secondary structure prediction of GFL showed a beta-sheet structure, connected with turn and coil. The most abundant structural element of GFL was the random coil, while the alpha-helixes were distributed at the N- and C-termini, and 21 beta-sheets were distributed in the CRD. Computer analysis of three-dimensional structure showed a common feature of L-lectins of GFL, which included an overall globular shape that was composed of a beta-sandwich of two anti-parallel beta-sheets, monosaccharide binding sites, were on the top of the structure and in proximity with a metal binding site. Northern blot analysis using a DIG-labelled probe derived from a partial GFL sequence revealed a hybridization signal of (approx.) 1.7 kb consistent with the length of the full-length GFL cDNA identified by RACE. No detectable band was observed from control total RNA extracted from filamentous green algae.

摘要

红藻石花菜 legume-type 凝集素(L-Lectin)基因的克隆通过 cDNA 末端快速扩增(RACE)。GFL 的全长 cDNA 为 1714 bp,包含一个 1542 bp 的开放阅读框,编码 513 个氨基酸,预测分子量为 56.5 kDa。与 NCBI-BLAST 分析推测的氨基酸序列显示与豆科凝集素(L-lectin)具有高度同源性(30-68%),来自 Griffithsia japonica、Clavispora lusitaniae、Acyrthosiphon pisum、Tetraodon nigroviridis 和 Xenopus tropicalis。系统发育关系分析显示与红藻 Griffithsia japonica 的糖蛋白具有最高的序列同一性(68%)(GenBank 编号 AAM93989)。保守结构域数据库分析检测到一个 N 端碳水化合物识别结构域(CRD),这是 L-lectin 的特征,它包含两个糖结合位点和一个金属结合位点。GFL 的二级结构预测显示了β-折叠结构,与转角和卷曲相连。GFL 最丰富的结构元件是无规卷曲,而α-螺旋分布在 N-和 C-末端,21 个β-折叠分布在 CRD 中。三维结构的计算机分析显示了 GFL 的 L-lectin 的一个共同特征,它包括一个整体的球形结构,由两个反平行的β-折叠组成的β-三明治,单糖结合位点位于结构的顶部,靠近金属结合位点。使用源自 GFL 部分序列的 DIG 标记探针进行 Northern blot 分析显示杂交信号约为 1.7 kb,与 RACE 鉴定的全长 GFL cDNA 长度一致。从丝状绿藻中提取的对照总 RNA 中未观察到可检测的带。

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