苯并(a)芘诱导对双齿围沙蚕腺苷酸环化酶(AC)基因及酶活性表达的影响

为探讨双齿围沙蚕Perinereis aibuhitensis对外源污染物的毒性响应,分析了不同苯并(a)芘[B(a)P]浓度(0.5、5、10、15μg/L)胁迫下双齿围沙蚕(体质量为1.5~2.5 g)腺苷酸环化酶(adenylate cyclase,AC)的基因表达和酶活性变化特征,利用RACE方法获得了沙蚕AC基因cDNA全长,并利用实时荧光定量PCR技术分析了苯并(a)芘诱导下沙蚕AC基因的变化。结果表明:双齿围沙蚕AC基因cDNA全长为4900 bp,包括5′非翻译区127 bp,3′非翻译区1536 bp,开放阅读框3237 bp,编码1078个氨基酸;该序列包含两个保守环化酶催化结构域,与其他动物氨基酸序列一致性为34%~47%;不同浓度的苯并(a)芘诱导会引起沙蚕AC基因表达量上升,0.5、10μg/L苯并(a)芘浓度组AC表达量在诱导第7天时达到最大,而5、50μg/L苯并(a)芘浓度组在诱导第14天时达到最大;利用ELISA试剂盒分析苯并(a)芘诱导下双齿围沙蚕AC酶活性变化,结果显示,在第4天时0.5、5、50μg/L浓度组AC酶活性上升到最高,之后随时间的延长酶活性降低,而10μg/L浓度组AC酶活性略低于空白对照组且在第7天时达到最高值。研究表明,苯并(a)芘会在一定程度上诱导沙蚕AC的基因表达及酶活性变化。

The expression characteristics of vitellogenin(VTG) in response to B(a)p exposure in polychaete Perinereis aibuhitensis

In order to investigate the endocrine toxicity of B(a)p to marine polychaete P erinereis aibuhitensis, vitellogenin(VTG) cDNA from the P. aibuhitensis was isolated, recombinated and expressed for the first time. The full length P. aibuhitensis vitellogenin gene(PaVTG) was 5 325 bp, and encoded 1 692 amino acids. It contained the vitellogenin_N domain of unknown function(DUF1943), a von Willebrand factor type D domain, as well as a conserved KALGNAG motif. The expression of VTG gene and protein were mainly up-regulated after exposed to B(a)p at transcriptional and translational levels. PaVTG gene expression did not change significantly at day 4. At day 7 PaVTG expression was up-regulated in 0.5 μg/L and 5 μg/L B(a)p group. At day 14 PaVTG was significantly up-regulated in 0.5–10 μg/L B(a)p. The protein expression of PaVTG in 0.5 μg/L and 10 μg/L B(a)p group was up-regulated with time prolonging, but the expression in 5 μg/L and 50 μg/L B(a)p group exhibited first increased and then decreased trend. With the increasing of B(a)p concentration PaVTG mRNA and protein expression both firstly increased then decreased. In contrast to B(a)p exposure, estradiol did not induce PaVTG gene and protein expression, until late times of exposure(14 d). Overall, the results in this study indicate that PaVTG could be used as a potential indicator of the effects environmental estrogenic compounds.

辛硫磷胁迫对异育银鲫细胞基因表达的影响

辛硫磷(Phoxim)是一种高效、低毒、低残留的广谱有机磷农药,因其对水生动物寄生虫有较好的防控效果,在水产养殖中被大量使用;但辛硫磷对水生动物生理水平、基因水平的影响研究尚属空白。本研究围绕辛硫磷使用中的潜在安全性开展基因水平的风险评估研究。采用高通量测序平台Illumina HiSeqTM2500,对经0.5 mg/L的辛硫磷(DMSO溶解)处理的异育银鲫尾鳍细胞(GiCF)样品进行测序分析。研究结果显示:细胞活性检测试验(CCK)证明0.5 mg/L的辛硫磷对细胞活性无显著影响;与对照组(0.25%DMSO处理)表达的基因相比,辛硫磷处理组细胞中分别有550个和422个基因显著上调和下调。根据GO功能分类,差异表达基因可分为生物过程、细胞组分、分子功能等三大类别中的55个分支。KEGG信号通路显著性富集分析结果表明:差异表达基因共涉及260条生物学代谢途径,包括赖氨酸降解、谷胱甘肽代谢、PI3K/AKT等通路;其中和药物代谢相关的信号通路有药物代谢—细胞色素P450、药物代谢—其他酶类和酪氨酸激酶抑制剂耐药。为了验证转录组结果的准确性,运用荧光定量RT-PCR技术对随机挑选的9个上调或下调的宿主基因进行了辛硫磷胁迫下的表达水平分析,其变化与转录组测序结果基本一致。本研究结果表明0.5 mg/L浓度的辛硫磷对GiCF无显著毒性,但是能对其基因表达谱产生系统性影响。该结果也表明GiCF细胞可以作为农药的细胞毒性研究材料。本研究为深入揭示辛硫磷对Gi CF细胞基因水平的影响及潜在生理毒性提供了依据,相关转录组数据可以为辛硫磷在水产养殖中的分子毒理学评价提供参考。