| 大黄鱼肌肉组织cDNA全长文库的构建及EST分析 |
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| 引用本文: | 黄伟,薛良义,李婷,杨斌.大黄鱼肌肉组织cDNA全长文库的构建及EST分析[J].台湾海峡,2010,29(2):189-195. |
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| 作者姓名: | 黄伟 薛良义 李婷 杨斌 |
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| 作者单位: | 1. 宁波大学生命科学与生物工程学院,浙江,宁波,315211
2. 宁波大学生命科学与生物工程学院,浙江,宁波,315211;宁波大学应用海洋生物技术教育部重点实验室,浙江,宁波,315211 |
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| 基金项目: | 国家863计划资助项目,国家自然科学基金资助项目,长江学者和创新团队发展计划项目 |
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| 摘 要: | 以大黄鱼肌肉组织为材料,利用Creator Smart cDNA Library Construction Kit构建了大黄鱼肌肉组织的全长cDNA文库.文库质量分析表明:cDNA文库容量不低于1.68×106cfu/mm3,重组率达96%,插入片断的平均长度大于1 000bp.随机挑取512个cDNA克隆进行5’端测序,其中430条ESTs的长度大于100bp;并初步拼接得到了230个单基因簇(unigene),其中包括58个重叠群(contigs),172个单拷贝ESTs(singletons),冗余度为46.51%.经检索,35个ESTs在BLASTx上无明显的同源性(E值≤1.00×10-10),为新基因.195个ESTs与已报道的基因有较高的同源性;其中与能量相关基因的ESTs丰度最高,占总数的20.00%.蛋白质合成、细胞骨架和信号传导次之,比例分别为13.48%、12.17%、10.00%,其中包括高迁移率族蛋白B1、瘦素受体、β1-热激蛋白等.这些EST数据为进一步筛选和克隆大黄鱼肌肉特异性表达基因提供了平台.
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| 关 键 词: | 海洋生物学 大黄鱼 肌肉组织 cDNA全长文库 表达序列标签(ESTs) |
Construction of a full length cDNA library from the skeletal muscle of Larimichthys crocea and its EST analysis |
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| HUANG Wei,XUE Liang-yi,LI Ting,YANG Bin.Construction of a full length cDNA library from the skeletal muscle of Larimichthys crocea and its EST analysis[J].Journal of Oceanography In Taiwan Strait,2010,29(2):189-195. |
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| Authors: | HUANG Wei XUE Liang-yi LI Ting YANG Bin |
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| Institution: | 1.College of Life Science and Biotechnology,Ningbo University,Ningbo 315211,China;2.Eduocation Ministry Key Laboratory of Applied Marine Biotechnology,Ningbo University,Ningbo 315211,China) |
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| Abstract: | A full-length cDNA library was constructed for the skeletal muscle of Larimichthys crocea using the Creator Smart cDNA Library Construction Kit.Library quality analysis showed that the library reached 1.68×106 cfu/mm3 in capacity with a recombinant efficiency as high as 96%.PCR results showed that the average size of inserts was larger than 1 000 bp.512 clones were randomly selected and sequenced.Of these 430 were expressed sequence tags(ESTs) longer than 100 bp.From these ESTs,230 non-repetitive sequences were acquired,including 58 contigs and 172 singletons after initial assembly and with a redundancy rate of 46.51%.From this retrieval 35 ESTs seemed to be novel genes(E-value≤1.00×10-10) as no clearly homologous known sequence was found in GenBank databases;195 ESTs were found to have considerable homology to reported genes,of which energy-related genes had the highest abundance,accounting for 20.00%,while protein synthesis,cytoskeleton and signal transduction genes made up 13.48%,12.17% and 10.00%,respectively.These included the high-mobility group protein B1,leptin receptor and β1-heat shock protein.The results provide a foundation for further screening and cloning of specific expression genes in the skeletal muscle of Larimichthys crocea. |
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| Keywords: | marine biology Larimichthys crocea skeletal muscle cDNA library ESTs |
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