红笛鲷弧菌病血清流行病学研究方法的建立

以红笛鲷Lutjanus sanguineus弧菌病的主要病原菌——溶藻弧菌Vibrio alginolyticus为抗原制备兔抗血清,以辣根过氧化酶标记的羊抗兔血清为酶标二抗,建立了酶联免疫吸附试验检测技术。通过棋盘滴定法测定,得出溶藻弧菌菌悬液的最佳工作浓度为5×108mL-1,兔抗溶藻弧菌血清的最佳稀释度为1∶16000,酶标羊抗兔抗体的最佳稀释度为1∶2000。应用本实验建立的间接双抗体夹心法对红笛鲷进行现场检测,患病红笛鲷特异性抗体的检出率为70%,外观健康红笛鲷的检出率为20%。结果表明,本实验所建立的酶联免疫吸附试验(ELISA)检测法可以用于红笛鲷弧菌病的血清流行病学研究,而且可以检测出隐性感染状态下的红笛鲷。     

黄鳍鲷细菌性溃疡病致病菌研究

研究了黄鳍鲷细菌性溃疡病的病原。从患病濒死的黄鳍鲷体内分离到两株细菌,经人工感染试验确定为致病菌,通过测定其形态及生理生化特性得出：致病菌为革兰氏阴性杆菌,极生单鞭毛,发酵葡萄糖产酸不产气,氧化酶阳性、过氧化氢酶阴性,发酵乳糖,甘露醇发酵阳性,明胶酶阳性,在70g／LNaCl培养基中生长良好,对O／129不敏感;由于两株菌对山梨醇、水扬苷、七叶苷及麦芽糖等氧化发酵的结果不一致,分别被鉴定为嗜水气单胞菌不产气亚种（Aeromonashydropilaanaerogenes）和温和气单胞菌（A．sobria）变异亚种。药敏试验显示,两个菌株对氯霉素高度敏感而对氟哌酸中度敏感。两株菌对黄鳍鲷的半致死剂量（按每g鱼计算）分别为2．3×106个菌体和2．6×105个菌体。     

黄鳍鲷细菌性溃疡病致病菌研究

研究了黄鳍鲷细菌性溃疡病的病原。从患病濒死的黄鳍鲷体内分离到两株细菌,经人工感染试验确定为致病菌,通过测定其形态及生理生化特性得出：致病菌为革兰氏阴性杆菌,极生单鞭毛,发酵葡萄糖产酸不产气,氧化酶阳性,过氧化氢酶阴性,发酵糖,甘露限酵阳性,明胶酶阳性,在７０ｇ／ＬＮａＣｌ培养基上中生长良好,对Ｏ／１２９不敏感;由于两株菌对山梨醇、水扬苷、七叶苷及麦芽糖等氧化发酵的结果不一致,分别被鉴定为嗜水气单胞     

南海海域4种笛鲷的微卫星DNA分析

采用聚丙烯酰胺凝胶电泳技术,从20对西大西洋笛鲷(Lutjanus campechanus)的微卫星引物中筛选适用于红鳍笛鲷(L.erythopterus)、勒氏笛鲷(L.russellii)、紫红笛鲷(L.argentimaculatus)和约氏笛鲷(L.johnii)基因组分析的微卫星引物,分析4种笛鲷的遗传多样性及系统发生。经反应条件的优化,从20对引物中筛选出17对可稳定扩增出特异片段的引物。通过测序证实扩增产物含微卫星位点后,以该17对引物对4个种的群体进行遗传多样性分析。其中16对可在约氏笛鲷、勒氏笛鲷、紫红笛鲷基因组中扩增出重复性好的特异性条带,分别有65%、65%、60%呈现出种内多态;15对可在红鳍笛鲷中扩增出重复性好的特异性条带,并且全部呈现出种内多态。四种笛鲷中,红鳍笛鲷的多态性最高,高度多态基因座占检测座位的66.67%;勒氏笛鲷的多态性最低,低度多态基因座占43.75%。获得3个种间特异性分子标记。用DS和DA两种方法计算4种笛鲷的遗传距离,构建了系统发生树。     

南海海域4种笛鲷的微卫星DNA分析

摘要：采用聚丙烯酰胺凝胶电泳技术，从20对西大西洋笛鲷（Lutjanus campechamus）的微卫星引物中筛选适用于红鳍笛鲷（L．erythopterus）、勒氏笛鲷（L.russellii）、紫红笛鲷（L.argentimaculatus）和约氏笛鲷（L.johnii）基因组分析的微卫星引物，分析4种笛鲷的遗传多样性及系统发生。经反应条件的优化，从20对引物中筛选出17对可稳定扩增出特异片段的引物。通过测序证实扩增产物含微卫星位点后，以该17对引物对4个种的群体进行遗传多样性分析。其中16对可在约氏笛鲷、勒氏笛鲷、紫红笛鲷基因组中扩增出重复性好的特异性条带，分别有65％、65％、60％呈现出种内多态：15对可在红鳍笛鲷中扩增出重复性好的特异性条带，并且全部呈现出种内多态。四种笛鲷中，红鳍笛鲷的多态性最高，高度多态基因座占检测座位的66．67％；勒氏笛鲷的多态性最低，低度多态基因座占43．75％。获得3个种间特异性分子标记。用风和DA两种方法计算4种笛鲷的遗传距离，构建了系统发生树。     

三种笛鲷属鱼类的随机扩增多态性DNA初步研究

RAPD技术是由 Williams[1]和 Welsh[2 ]领导的两个科研小组于 1 990年几乎同时独立创立的一种 DNA多态性分析技术 ,它的原理是利用一系列随机排列的寡核苷酸单链引物 ,以研究对象的基因组 DNA为模板进行 PCR扩增 ,通过扩增产物 DNA片段的多态性来检测基因组 DNA的多态性。该技术已被广泛地应用于种质鉴定、遗传多样性、亲缘关系及系统分类研究 [3～ 6]。但对海水鱼类RAPD研究报道较少。红鳍笛鲷 (L utjanus erythopterus Bloch)、紫红笛鲷 (L utjanus argentimaculatus Forskal)和勒氏笛鲷 (L utjanus russelli Bleeker)具有…     

红笛鲷IRAK-1基因克隆及哈维弧菌感染后的组织表达

用同源克隆和RACE的方法克隆红笛鲷(Lutjanus sanguineus)白细胞介素1受体相关激酶1(Interleukin-1receptor-associated kinase 1,IRAK-1)基因的cDNA全序列,并用荧光定量PCR分析其在健康鱼及哈维弧菌感染后红笛鲷的组织表达。结果表明,该序列全长3 207 bp(登录号KF728204),包含5′非编码区(UTR)202 bp,3′UTR752 bp,开放阅读框(ORF)2 253 bp,编码750个氨基酸。根据推导的氨基酸序列预测其蛋白分子质量为82.6 ku,理论等电点为6.59。IRAK-1包含1个N端死亡结构域、proST结构域、中央激酶结构域和C末端结构域。荧光定量PCR分析显示,红笛鲷IRKA-1基因在肝脏和皮肤的表达量最高,其次是心脏、鳃、肌肉和胸腺,其余组织的表达量较低。哈维弧菌侵染红笛鲷后,各组织中IRAK-1基因mRNA表达量均呈上调趋势,肝组织中变化最显著。     

红鳍笛鲷和紫红笛鲷种类和群体的矢耳石地标点法识别

【目的】探讨矢耳石地标法在笛鲷种内及种间中的判别作用。【方法】利用2017年购自广西北海、海南文昌、广东阳江的87尾红鳍笛鲷(Lutjanus erythropterus)和76尾紫红笛鲷(Lutjanus argentimaculatus)成鱼的矢耳石样本,基于地标点法分析耳石的形态差异,运用判别分析检验耳石形态差异在2种笛鲷的种间和同种不同群体间的判别功效。【结果】位于听沟前中部交叉点的两个地标点10、11贡献较大,解释了耳石形态变异的64.88%～65.85%,表明两种笛鲷耳石形态的种间差异和种内群体差异主要集中于听沟前中部。基于耳石形态的地标点方法对2种笛鲷的种间判别成功率为97.4%和100.0%;红鳍笛鲷和紫红笛鲷的种内不同群体判别成功率分别为85.7%、83.3%、80.0%和94.1%、78.1%、81.5%。【结论】矢耳石地标点法可作为2种笛鲷种间和种内判别的有效工具。     

注射氟苯尼考对红笛鲷免疫指标的影响

以0、5、10、20 mg.kg-1的氟苯尼考腹腔注射红笛鲷,研究氟苯尼考在国家规定的使用范围内对红笛鲷血清部分免疫指标的影响。结果显示:5 mg.kg-1组氟苯尼考对所测的各项指标无影响或影响不显著;10 mg.kg-1组中氟苯尼考对红笛鲷血清SOD活力、AKP活力有显著性提高(P<0.05),对溶菌酶的含量、IgM的含量无显著性影响;20 mg.kg-1组中红笛鲷血清碱性磷酸酶AKP、超氧化物歧化酶SOD活力、溶菌酶、抗体IgM均受到显著性抑制(P<0.05),但影响持续时间不同,这表明高浓度氟苯尼考显著抑制红笛鲷各项免疫指标,从而影响到鱼体自身的免疫功能。     

噬菌弧菌N1对淡水和海水养殖水体细菌群落影响PCR-DGGE分析

【目的】研究噬菌弧菌Bacteriovorax sp. N1在一个投放周期内对淡水和海水养殖环境中细菌、弧菌总数及细菌群落结构的影响。【方法】自市售微生态制剂分离蛭弧菌N1并进行分子鉴定,测定其裂解效果,制备高浓度N1菌液分别投放至淡水红鲤鱼(red carp)和海水仿刺参(Apostichopus japonicus)养殖水体,采用细菌平板计数法及PCR-变性梯度凝胶电泳(PCR-DGGE)技术分析48 h内水体环境中细菌、弧菌总数及细菌群落结构变化。【结果】经鉴定蛭弧菌N1为噬菌弧菌,其对大肠杆菌(Escherichia coli)、溶藻弧菌(Vibrio alginolyticus)、黄海希瓦氏菌(Shewanella smarisflavi)、灿烂弧菌(Vibrio splendidus)、哈氏弧菌(Vibrio harveyi)和金黄色葡萄球菌(Staphylococcus aureus)均有裂解效果。将噬菌弧菌N1投放进淡水和海水养殖环境的12～24 h,其能显著降低两种环境中弧菌含量(P 0.05)。DGGE分析显示添加噬菌弧菌N1后淡水组优势菌群弧菌属(Vibrio,a1)和不可培养杆菌属(Uncultured bacterium, a5)在12 h以后含量有明显的减少,假单胞菌属(Pseudomonas, a3)和红杆菌科Shimia属(Shimia, a6)菌含量增加。海水组优势菌群不可培养杆菌属(c2)菌在12 h时变成非优势菌群,而白杆菌属(Albirhodobacter,c1)增加成为优势菌群。噬菌弧菌N1在水中含量在24 h时降至最低。【结论】噬菌弧菌N1对海水和淡水环境中的弧菌属和不可培养杆菌属菌群有明显的裂解作用导致其含量下降,但也使假单胞菌属(Pseudomonas),红杆菌科Shimia属和白杆菌属(Albirhodobacter)菌群含量增加,但生物效应不明。为维持噬菌弧菌N1对弧菌的控制,需要24 h左右重新补充投放。     

Screening on DHA-producing Antarctic bacteria N- 6 and its cultural conditions

1 IntroductionPolyunsaturated fatty acids (PUFAs) have remained as a natural product due to thesynthetic difficulty of reproducing the methylene interrupted double bond sequence by in-dustrial chemistry. Their significance to animals and humans lies in th…     

A VIBRIO ANGUILIARUM STRAIN ASSOCIATED WITH SKIN ULCER ON CULTURED FLOUNDER, PARALICHTHYS OLIVACEUS

The characteristics of a bacterium strain M3, isolated from cultured flounderParalichthys olivaceus with remarkable external sign of skin ulcer during an epizootic outbreak, indicated that the bacterium belonged to the speciesVibrio anguillarum. Challenge by I.M. (intramuscular injection), bath, and oral administration with M3 showed that it was highly pathogenic forParalichthys olivacues. The LD₅₀ dose was 5.144×10³ CFU/ per fish infection by I.M. injection. Recovered inoculated bacteria from the surviving fish revealed that the asymptomatic carriers could be a latent contagious source. Study of the effect of bacterial culture CFS (cell-free-supernatant) showed that the exotoxins produced by M3 play an important role in its pathogenicity for flounder. The resistance of M3 to 36 out of 41 antibiotics indicated that the bacterial disease outbreak was mainly attributable to the frequent and excessive use of antimicrobial agents; and that vaccination would be an effective precaution against bacterial disease. Contribution No. 4107 from Institute of Oceanology, Chinese Academy of Science. Contribution No. 270 from Experimental marine Biology Laboratory, CAS. Funded by projects under the Major State Basic Research Development Program, Grant G1999012003.     

Optimization of culture conditions and medium composition for the marine algicidal bacterium Alteromonas sp. DH46 by uniform design

Harmful algal blooms (HABs) have led to extensive ecological and environmental issues and huge economic losses. Various HAB control techniques have been developed, and biological methods have been paid more attention. Algicidal bacteria is a general designation for bacteria which inhibit algal growth in a direct or indirect manner, and kill or damage the algal cells. A metabolite which is strongly toxic to the dinoflagellate Alexandrium tamarense was produced by strain DH46 of the alga-lysing bacterium Alteromonas sp. The culture conditions were optimized using a single-factor test method. Factors including carbon source, nitrogen source, temperature, initial pH value, rotational speed and salinity were studied. The results showed that the cultivation of the bacteria at 28°C and 180 r min^?1 with initial pH 7 and 30 salt contcentration favored both the cell growth and the lysing effect of strain DH46. The optimal medium composition for strain DH46 was determined by means of uniform design experimentation, and the most important components influencing the cell density were tryptone, yeast extract, soluble starch, NaNO₃ and MgSO₄. When the following culture medium was used (tryptone 14.0g, yeast extract 1.63g, soluble starch 5.0 g, NaNO₃ 1.6 g, MgSO₄ 2.3 g in 1L), the largest bacterial dry weight (7.36 g L^?1) was obtained, which was an enhancement of 107% compared to the initial medium; and the algal lysis rate was as high as 98.4% which increased nearly 10% after optimization.     

Biodegradation of Enteromorpha Polysaccharides by Intestinal Micro-Community from Siganus oramin

Micro-communities are supposed to have more potential functions of biodegradation of polysaccharides than single strain; however, the intestinal micro-communities involved in the biodegradation of Enteromorpha polysaccharides(EP) were seldom reported. In order to obtain the EP-degrading micro-community, the intestines of Siganus oramin was obtained to isolate the micro-communities, which were enriched by 0.3% of EP as the sole carbon source. A stable micro-community with EP degradative capability was achieved after seven generations of subculture, named H1. Results showed that H1 was able to degrade 75% of EP within 24 hours, and the activity of EP lyases reached 500 U m L~(-1) in 32 hours. With denaturing gradient gel electrophoresis(DGGE) and 16 S r RNA gene clone library analysis, ten bacteria closely related to Marinomonas pontica, Microbacterium sp., Leucobacter chironomi, Cyclobacterium sp., Algoriphagus winogradskyi, Pseudoalteromonas sp. and Vibrio sp. were determined. Furthermore, compared with the DGGE bands sequence and the clone library analysis, the dominant bacteria of the EP-biodegrading micro-community were Pseudoalteromonas sp. and Vibrio sp., with the respective proportion of 38% and 46%, and they should play an important role in EP degradation together with other degrading bacteria in the micro-community H1.     

波吉卵囊藻对弧菌生长的影响

研究波吉卵囊藻及藻―菌体系对创伤弧菌(Vibrio vulnificus)、副溶血弧菌(Vibrio parahaemolyticus)和溶藻弧菌(Vibrio alginolyticus)生长的影响,结果显示:无菌波吉卵囊藻对创伤弧菌、副溶血弧菌的生长均有显著促进作用(P<0.05),对溶藻弧菌的生长无显著影响(P>0.05);波吉卵囊藻―沼泽红假单胞菌体系对溶藻弧菌有明显抑制作用(P<0.05);无菌波吉卵囊藻―枯草芽孢杆菌体系对溶藻弧菌的生长有显著促进作用(P<0.05),对创伤弧菌、副溶血弧菌的生长无显著影响(P>0.05);带菌波吉卵囊藻对三株弧菌均有明显抑制作用(P<0.05);带菌波吉卵囊藻共栖细菌对三株弧菌均无明显抑制作用(P>0.05);在无菌波吉卵囊藻中回加带菌藻共栖细菌,分析实验10～18d的数据发现的数据发现藻―菌体系对创伤弧菌、副溶血弧菌的生长有显著影响(P<0.05),藻―菌体系逐渐恢复对三株弧菌的抑制作用。     

溶藻弧菌双组分调控系统PhoR/PhoB的基因克隆及生物信息学分析

双组分调控系统（Two-component Regulatory System）在致病菌的生长及毒力调控中起重要作用.克隆溶藻弧菌（Vibrio alginolyticus）HY9901 株组氨酸激酶PhoR 和反应调控因子PhoB 的全长基因,并对其进行生物信息学分析.序列分析结果显示,phoR（GenBank 登录号：KJ958404）全长1 299 bp,共编码432 个氨基酸;phoB（GenBank 登录号：KJ863646）全长690 bp,编码229 个氨基酸.构建PhoR/PhoB 的系统进化树,结果显示,溶藻弧菌PhoR/PhoB 与副溶血弧菌（Vibrio parahaemolyticus）、哈氏弧菌（Vibrio harveyi）有较近亲缘关系.利用SWISS-MODEL 软件,对PhoR/PhoB 中两个相对保守的功能域HATPase_c 和REC 进行同源建模,发现HATPase_c具有1 个ATP 结合位点,REC 具有4 个天冬氨酸活性位点.     

海洋短小芽孢杆菌ZH1-6菌株的鉴定及生物学特性

从新鲜近江牡蛎中分离到一株拮抗细菌,命名为ZH1-6,该菌对金黄色葡萄球菌、乙型副伤寒沙门氏菌及大肠杆菌等多种病原菌有较强的抑制作用。通过形态学观察、常规生理生化指标测定、16SrDNA序列测定和同源性分析,鉴定该菌株为短小芽孢杆菌。研究表明:ZH1-6能利用多种碳、氮源,其生长温度范围为10-50℃,生长pH范围为pH3-10,最适初始pH为6.0。     

Isolation and characteristics of one marine psychrotrophic cellulase-generating bacterium Ar/w/b/75°/10/5 from Chuckchi Sea,Arctic

Microorganisms living in polar zones play an important part as the potential source of organic activity materials with low temperature characteristics in the bio-technological applications. A psychrotrophic bacterium (strain Ar/w/b/75°/10/5) , producing cellulose at low temperatures during late-exponential and early-stationary phases of cell growth, was isolated from sea ice-covered surface water in Chuckchi Sea, Arctic. This bacterium, with rod cells, was Gram-negative, slightly halophilic. Colony growing on agar plate was in black. Optimum growth temperature was 15℃. No cell growth was observed at 351 or above. Optimum salt concentration for cell growth was between 2 and 3 % of sodium chloride in media. Maximal cellulase activity was detected at a temperature of 35℃ and pH8. Cellulase was irreversibly inactivated when incubated at 55℃ within 30 min. Enzyme can be kept stable at the temperature no higher than 25℃. Of special interest was that this bacterium produced various extracellular enzymes i     

Isolation and characterization of a marine bacterium producing protease from Chukchi Sea, Arctic

A Gram negative bacterium Ar/W/b/75°25＇N/1 producing extracellular alkaline protease was isolated from surface water of latitude 75°25＇N, and longitude 162°25＇W in Chukchi sea, Arctic. The strain can grow at the temperature range from 7℃ to 30℃, and grow better at 30(℃. It can not grow at 40℃. Keeping certain salinity concentration in medium is necessary for cell growth. It grows well in medium containing salinity concentration from 0. 5 % to 10 % sodium chloride. Glucose, sucrose and soluble starch can be utilized by the strain, among which glucose is the optimal carbon source. Peptone is the optimal organic nitrogen source for cell growth and protease producing, and ammonium nitrate is the optimal inorganic nitrogen source.About 75.7% of total protease of the strain are extracellular enzyme. Optimal temperature for proteolytic activity is at 40℃. Protease of the strain keeps stable below 40℃, and shows high proteolytic activity within the pH range from 7 to 11.     

Analysis of cultivable aerobic bacterial community composition and screening for facultative sulfate-reducing bacteria in marine corrosive steel

Anaerobic, aerobic, and facultative bacteria are all present in corrosive environments. However,as previous studies to address corrosion in the marine environment have largely focused on anaerobic bacteria, limited attention has been paid to the composition and function of aerobic and facultative bacteria in this process. For analysis in this study, ten samples were collected from rust layers on steel plates that had been immersed in seawater for dif ferent periods(i.e., six months and eight years) at Sanya and Xiamen,China. The cultivable aerobic bacterial community structure as well as the number of sulfate-reducing bacteria(SRB) were analyzed in both cases, while the proportion of facultative SRB among the isolated aerobic bacteria in each sample was also evaluated using a novel approach. Bacterial abundance results show that the proportions are related to sea location and immersion time; abundances of culturable aerobic bacteria(CAB) and SRB from Sanya were greater in most corrosion samples than those from Xiamen,and abundances of both bacterial groups were greater in samples immersed for six months than for eight years. A total of 213 isolates were obtained from all samples in terms of CAB community composition,and a phylogenetic analysis revealed that the taxa comprised four phyla and 31 genera. Bacterial species composition is related to marine location; the results show that Firmicutes and Proteobacteria were the dominant phyla, accounting for 98.13% of the total, while Bacillus and Vibrio were the dominant genera,accounting for 53.06% of the total. An additional six facultative SRB strains were also screened from the isolates obtained and were found to encompass the genus Vibrio(four strains), Staphylococcus(one strain),and Photobacterium(one strain). It is noteworthy that mentions of Photobacterium species have so far been absent from the literature, both in terms of its membership of the SRB group and its relationship to corrosion.