鳗弧菌(Vibrio anguillarum)侵染对青蛤(Cyclina sinensis)髓样分化因子88基因表达的影响     

高晶  任毅鹏  潘宝平  闫春财 《海洋与湖沼》2015,46(2):440-445

经转录组测序后筛选并克隆得到青蛤(Cyclina sinensis)髓样分化因子88(myeloid differenttiation factor 88,My D88)的c DNA序列。在鳗弧菌(Vibrio anguillarum)胁迫下,采用荧光定量PCR法分析了My D88基因在青蛤体内的表达过程。结果显示,青蛤My D88基因的开放阅读框为1521bp,编码506个氨基酸,分子量约为57.14k Da,氨基酸N段存在DEATH结构域,C段存在TIR结构域(Toll/Interleukin-1 receptor domain)。My D88基因在青蛤血淋巴、肝脏、外套膜、鳃和闭壳肌等组织中普遍表达,但在血淋巴中表达量最高,与其它组织出现显著性差异(P0.05)。通过检测鳗弧菌刺激下My D88基因在青蛤血淋巴中的表达值,发现My D88基因在24h开始升高,48h达到最大值,约为对照组的10倍,实验组与对照组及空白组均出现了极显著性差异(P0.01);研究结果表明,该基因在软体动物的免疫应答反应中对革兰氏阴性菌有识别作用。  相似文献   

牙鲆(Paralichthys olivaceus)TLR21 基因在迟缓爱德华氏菌(Edwardsiella tarda)感染后的表达特征     

张洁  郑津辉  李庆亚  耿绪云  孙金生  潘宝平  孙世南  高虹 《海洋与湖沼》2015,46(6):1502-1508

应用荧光定量PCR技术, 检测了TLR21 基因在牙鲆(Paralichthys olivaceus)感染迟缓爱德华 氏菌(Edwardsiella tarda)后, 在0 h、1 h、3 h、6 h、12 h、1 d、3 d、6 d 后, 在心脏、肝脏、脾脏、 头肾、鳃、小肠、肌肉和血的时空表达特征, 并探讨了它们与牙鲆先天免疫反应的关系。结果表明, 大 多组织在感染病原6 h 后TLR21 基因表达明显上调, 尤其是头肾和小肠。头肾6 h 的表达量达到了 对照组的59.3 倍, 小肠6 h 的表达量为对照组的38.6 倍。迟缓爱德华氏菌感染引起牙鲆体内各组织 中TLR21 的上调表达和变化, 为研究牙鲆对迟缓爱德华氏菌的防御机制提供了理论依据。  相似文献   

长牡蛎(Crassostrea gigas)微卫星多重PCR 体系构建及其在家系鉴定中的应用     

纪仁平  李焕军  冯艳微  张荣良  王卫军  杨建敏 《海洋与湖沼》2015,46(6):1542-1548

筛选多态性高、特异性好、片段大小适中的10 个长牡蛎微卫星位点进行优化组合, 根据扩 增片段大小及同一荧光不重叠原则构建了两组五重PCR 体系。运用CERVUS 3.0 软件对0527 组27 个长牡蛎全同胞家系的643 个子代和0612 组27 个全同胞家系382 个子代分别进行亲权鉴定。结果 发现, 用两组微卫星五重PCR 鉴别时, 在0527 组和0612 组的鉴定成功率均为100%; 只用第一组微 卫星五重PCR, 可以将0527 组96%的子代和0612 组96%的子代鉴定到亲本; 只用第二组微卫星五 重PCR, 可以将0527 组97%的子代和0612 组95%的子代鉴定到亲本。本研究中筛选出的两组微卫 星五重PCR 体系在两组家系中的鉴定效率均较高, 可以快速有效地将子代个体鉴定至所属父母本, 在长牡蛎家系鉴定中具有很好的应用价值。  相似文献   

Depuration dynamics of oysters (Crassostrea gigas) artificially contaminated by Salmonella enterica serovar Typhimurium     

de Abreu Corrêa A  Albarnaz JD  Moresco V  Poli CR  Teixeira AL  Oliveira Simões CM  Monte Barardi CR 《Marine environmental research》2007,63(5):479-489

The State of Santa Catarina produces the greatest quantity of edible mollusks in Brazil. To guarantee sanitary qualify, mollusk cultures should be monitored for contamination by pathogenic microorganisms. A self-purification or "depuration" system that eliminates Salmonella enterica serovar Typhimurium contamination from oysters has been developed and evaluated. The depuration process occurred within a closed system, in which 1000 L of water was recirculated for 24 h. The water was sterilized with ultraviolet (UV) light, chlorine, or both together. Oysters (Crassostrea gigas) artificially contaminated with S. typhimurium were harvested every 6 h. Samples of oyster tissue were excised and both the presence and numbers of bacteria were determined. Combined UV light and chlorine treatments resulted in total elimination of bacteria within 12 h. Polymerase chain reaction detected bacteria in water exposed to the three treatments. This pioneering study is the first of its kind in Brazil and represents a major contribution to commercial mollusk culture in this country.  相似文献   

福建沿海巨蛎属牡蛎的主要种类及其分布   总被引：4，自引：0，他引：4  

杜玄  郭希明  钱鲁闽 《台湾海峡》2009,28(3):399-404

本实验采用了多重种类特异性PCR（multiplex species—specific PCR）技术，研究了巨蛎属（Crassostrea）牡蛎主要种类在福建沿海的分布．从沿海11个采样地点共采集了657个野生牡蛎样本，随机抽取了327个牡蛎样本进行基因组DNA的提取和线粒体COI基因的鉴定，结果发现200个个体为葡萄牙牡蛎（Crassostrea angulata），101个个体为近江牡蛎（Crassostrea ariakensis），20个个体为熊本牡蛎（Crassostrea sikamea），6个个体为香港巨牡蛎（Crassostrea hongkongensis）．此次实验中未发现长牡蛎（Crassostrea gigas）．结果表明，福建沿海有葡萄牙牡蛎、近江牡蛎、熊本牡蛎和香港巨牡蛎4种巨蛎属牡蛎分布．  相似文献   

Differential gene expression in the brain of Sebastiscus marmoratus in response to exposure to polychlorinated biphenyls (PCBs)     

Li B  Wang C  Ye K  Yu A  Chen Y  Zuo Z 《Marine environmental research》2008,66(5):548-552

Effects of exposure to polychlorinated biphenyls (PCBs) on Sebastiscus marmoratus were investigated using a suppression subtractive hybridization method. A total of 108 gene sequences were identified as having the potential for being differentially expressed, and 45 could be identified with homologous database sequences. Functions with which they were associated included long-term potentiation and neurotransmitter release, neuroendocrine, mitosis and cell proliferation, energy-related metabolism, general metabolism, signal protein, hemopoiesis system, immune system, and structure. The expression of 17 of these genes was analyzed in the brain using real time fluorescent quantitative PCR. The present study provided a basis for studying the response of fish to PCB exposure and allowed the characterization of new potential neurotoxicol biomarkers of PCB contamination in seawater.  相似文献   

东海原甲藻线粒体细胞色素b(Cytb)基因的定量检测   总被引：3，自引：0，他引：3  

赵丽媛  于志刚  甄毓  米铁柱 《中国海洋大学学报(自然科学版)》2009,39(3)

建立了检测东海原甲藻线粒体细胞色素b(Cytb)基因mRNA含量的实时荧光定量PCR方法.以甲藻Cytb基因的简并引物扩增得到984 bp长的东海原甲藻Cytb基因片段,经克隆、测序,制备并纯化质粒.以光度法测定质粒浓度并作为标准品.对上述基因片段,利用PRIMER EXPRESS 3.0 设计引物,以梯度稀释的质粒标准品进行定量PCR反应,以SYBR Green I为荧光染料,制作标准曲线,得到基因拷贝数X与Ct值的关系为:Ct=-3.50 lg X+39.35(相关系数r为0.999).通过对不同生长时期的东海原甲藻样品的Cytb基因mRNA含量检测,发现该基因的表达量较稳定,平均值为(45.4±4.7)拷贝/细胞,受生长状态影响不大,可作为实时荧光定量PCR的内参基因.  相似文献   

Multiplex PCR allows simultaneous detection of pathogens in ships' ballast water     

Aridgides LJ  Doblin MA  Berke T  Dobbs FC  Matson DO  Drake LA 《Marine pollution bulletin》2004,48(11-12):1096-1101

There is enormous potential for global transfer of microorganisms, including pathogens, in ships' ballast water. We contend that a major advancement in the study of ballast-water microorganisms in particular, and of aquatic pathogens in general, will be expedited sample analysis, such as provided by the elegant technology of DNA microarrays. In order to use DNA microarrays, however, one must establish the appropriate conditions to bind target sequences in samples to multiple probes on the microarrays. We conducted proof-of-concept experiments to optimize simultaneous detection of multiple microorganisms using polymerase chain reaction (PCR) and Southern hybridization. We chose three target organisms, all potentially found in ballast water: a calicivirus, the bacterium Vibrio cholerae, and the photosynthetic protist Aureococcus anophagefferens. Here, we show simultaneous detection of multiple pathogens is possible, a result supporting the promising future use of microarrays for simultaneous detection of pathogens in ballast water.  相似文献   

Analysis of the 16S-23S rDNA intergenic spacers (IGSs) of marine vibrios for species-specific signature DNA sequences   总被引：7，自引：0，他引：7  

Lee SK  Wang HZ  Law SH  Wu RS  Kong RY 《Marine pollution bulletin》2002,44(5):412-420

Vibrios are widespread in the marine environment and a few pathogenic species are known to be commonly associated with outbreaks of diarrheal diseases in humans due to the consumption of raw or improperly cooked seafood. However, there are also many Vibrio species which are potentially pathogenic to vertebrate and invertebrate aquatic animals, and of which little is known. In an attempt to develop rapid PCR detection methods for these latter class of vibrios, we have examined the 16S-23S intergenic spacers (IGSs) of 10 lesser-known Vibrio species and successfully developed species-specific primers for eight of them--Vibrio costicola, V. diazotrophicus, V. fluvialis, V. nigripulchritudo, V. proteolyticus, V. salmonicida, V. splendidus and V. tubiashii. The IGS amplicons were amplified using primers complementary to conserved regions of the 16S and 23S rRNA genes, and cloned into plasmid vectors and sequenced. Analysis of the IGS sequences showed that 37 ribosomal RNA (rrn) operons representing seven different IGS types have been cloned from the 10 vibrios. The three IGS types--IGS(0), IGS(IA) and IGS(Glu)--were the most prevalent forms detected. Multiple alignment of representative sequences of these three IGS types from different Vibrio species revealed several domains of high sequence variability, which were used to design species-specific primers for PCR. The specificity of the primers were evaluated using total DNA prepared from different Vibrio species and bacterial genera. The results showed that the PCR method can be used to reliably detect eight of the 10 Vibrio species in marine waters in this study.  相似文献   

A Method To Detect Viable Helicobacter pylori Bacteria in Groundwater     

Debbie Flanigan  Mark Rodgers 《洁净——土壤、空气、水》2003,31(1):45-48

The inability to detect the presence of viable Helicobacter pylori bacteria in environmental waters has hindered the public health community in assessing the role water may play in the transmission of this pathogen. This work describes a cultural enrichment method coupled with an H. pylori‐specific PCR to identify these bacteria in water. While far from perfected at the present time, this represents an exciting new approach to studying the significance of water as a transmission mechanism for H. pylori. Evidence is presented that indicates culturable H. pylori bacteria were found using this enrichment/PCR method in a local groundwater source.  相似文献