| 引用本文: | 路雅丽,李成华,苏秀榕,李太武,朱 琳,张 鹏,李 晔.浙江枝吻纽虫(Dendrorhynchus zhejiangensis) 热休克蛋白70基因克隆与表达特征研究.海洋与湖沼,2012,43(6):1156-1162. |
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| 摘要: |
| 采用同源克隆和cDNA 末端快速扩增技术(RACE)克隆了浙江枝吻纽虫热休克蛋白70(DzHSP70)基因全长cDNA序列, 并利用荧光定量PCR方法, 分析了该基因在重金属胁迫下的表达特征。结果表明, DzHSP70cDNA 全长2827bp, 包括294bp的5’UTR、628bp的3’UTR和编码634个氨基酸残基的1905bp 的开放阅读框。HSP70家族的3 个签名序列以及细胞质特异性调控基序EEVD等特征元件在DzHSP70中高度保守。重金属离子Fe3+、Pb2+和Cd2+均可上调该基因的表达, 其中Pb2+的毒理效应最强。研究结果表明DzHSP70可能参与了机体对于重金属的解毒过程。 |
| 关键词: 浙江枝吻纽虫, 热休克蛋白70, 实时荧光定量PCR, 表达 |
| DOI:10.11693/hyhz201206018018 |
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| 基金项目:浙江省自然科学基金资助项目, Y3100480 号; 浙江省教育厅(理), Y200907951号; 国家自然科学基金项目, 31272637 号。 |
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| CLONING AND EXPRESSION ANALYSIS OF HEAT SHOCK PROTEIN 70 FROM DENDRORHYNCHUS ZHEJIANGENSIS |
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LU Ya-Li1, LI Cheng-Hua1, SU Xiu-Rong1, LI Tai-Wu1,2, ZHU Lin1, ZHANG Peng1, LI Ye1
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1.School of Marine Sciences, Ningbo University;2.Ningbo City College of Vocational Technology
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| Abstract: |
| With the approaches of homology cloning, RACE, the full-length HSP70 cDNA of Dendrorhynchus zhejiangensis was identified and characterized (denoted as DzHSP70) in the present study. Meanwhile, fluorescent real-time PCR was used to analyze varying degrees of induction of DzHSP70 mRNA expression in D. zhejiangensis exposed to heavy metals (Fe3+, Pb2+ and Cd2+). The results indicated the cDNA of DzHSP70 was of 2827bp, consisting of a 5′UTR of 294bp, a 3′UTR of 628bp, and a complete open reading frame of 1905bp encoding a polypeptide with 566 amino acid residues. The conserved motifs for HSP70 protein family including three signature sequences and a cytoplasm characteristic motif of EEVD were totally found in the deduced amino acid of DzHSP70. Three heavy metals Fe3+, Pb2+ and Cd2+
all could be induced the expression of DzHSP70 at mRNA level, where Pb2+ displayed more toxic effect on worm than those of Fe3+ and Cd2+. All our results indicated that DzHSP70 might be involved into mediating the process of heavy metals detoxification in worm. |
| Key words: Dendrorhynchus zhejiangensis, Heat shock protein 70 (HSP70), Real-time fluorescent quantitative PCR, Expression |
