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1.
从患腹水病大菱鲆和褐牙鲆成鱼体内分离到两株致病作用强的病原菌FS1和FS2,经人工感染实验表明菌株FS1和菌株FS2为腹水症的致病菌。采用常规的生理生化鉴定方法及梅里埃全自动微生物分析系统(VITEK32),结合分子生物学方法进行病原菌的鉴定。结果表明,菌株FS1和菌株FS2分别为迟缓爱德华氏菌(Edwardsiellatarda)和溶藻弧菌(Vibrioalginolyticus)。菌株FS116SrRNA基因序列与迟缓爱德华氏菌的同源性达99%;菌株FS2的16SrRNA基因序列与溶藻弧菌、哈维氏弧菌、副溶血弧菌等的同源性均达99%。为最终确定菌株FS2的分类地位,测定了其HSP60基因序列,进行网上同源性比对。分析结果表明,菌株FS2与溶藻弧菌的同源性达99%,而与其他弧菌HSP60基因的同源性均低于91%。这两种致病菌混合感染或分别感染均可造成养殖鲆鱼腹水病。  相似文献   

2.
为获得琼胶酶活性高产菌株,对采集的海水样品进行了产酶微生物的分离、筛选和鉴定。经过平板培养预筛和两次摇瓶培养筛选,从浙江省舟山市普陀区近海海水样品中分离到一株琼胶酶产生菌G-5,该菌株液体培养产酶活力可达到413.8 U/mL。G-5菌株的菌落呈乳白色、半透明、表面湿润;菌体革兰氏染色阴性,大小0.58~0.69μm×1.50~2.26μm;光学显微镜下呈短杆状,略有弧形。G-5菌株的16S rDNA序列与NCBI数据库中15个弧菌属(Vibrio)菌株的16S rDNA有98%的同源性,可以确定G-5菌株是一株弧菌(Vibrio sp.)。  相似文献   

3.
为获得琼胶酶活性高产菌株,对采集的海水样品进行了产酶微生物的分离、筛选和鉴定。经过平板培养预筛和两次摇瓶培养筛选,从浙江省舟山市普陀区近海海水样品中分离到一株琼胶酶产生菌G-5,该菌株液体培养产酶活力可达到413.8 U/mL。G-5菌株的菌落呈乳白色、半透明、表面湿润;菌体革兰氏染色阴性,大小0.58~0.69 μm1.50~2.26 μm;光学显微镜下呈短杆状,略有弧形。G-5菌株的16S rDNA序列与NCBI数据库中15个弧菌属(Vibrio)菌株的16S rDNA有98%的同源性,可以确定G-5菌株是一株弧菌(Vibrio sp.)。  相似文献   

4.
采用点种法并以副溶血弧菌(Vp1.2164)和溶藻弧菌(Va-Y)为弧菌指示菌,对从健康的大黄鱼肠道内分离的115株细菌进行体外拮抗试验。并对筛选出的拮抗菌进行抗菌谱测定,最后利用VITEK-32细菌快速鉴定系统和16SrRNA基因序列对拮抗菌进行鉴定。结果表明,从中筛选到3株有较强拮抗作用的菌株,编号分别为X1402-1、X1108和X3914,且菌株X1402-1的抗菌作用最强,抗菌谱最广,21株病原指示菌中,对16株均能产生较强的抑制作用,其中对Vp-1.2164的抑菌直径最大,达到28.5mm,对Va-Y的抑菌直径为8.7mm;其次为菌株X1108和X3914,对两种指示弧菌的抑菌直径分别为:12.0mm、9.0mm和0mm、7.2mm。经VITEK-32细菌快速鉴定系统鉴定,3株拮抗菌分别与铜绿假单胞菌,恶臭假单胞菌,地衣芽孢杆菌的相似性均为99%。通过16SrRNA基因序列分析表明,3株拮抗菌分别与类产碱假单胞菌Pseudomonas pseudoalcaligenes(EU419918)、恶臭假单胞菌Pseudomon asputida(FJ440105)和地衣芽孢杆菌Bacillus licheniformis(DQ988136)的16SrRNA基因同源性最高,分别为100.0%、97.5%、99.0%。综合分析试验结果,X1402-1、X1108和X3914分别被确定为类产碱假单胞菌、恶臭假单胞菌和地衣芽孢杆菌。  相似文献   

5.
分子鉴定方法研究大亚湾水体弧菌种类变化   总被引:2,自引:0,他引:2  
借助分子鉴定方法监测大亚湾水体中弧菌Vibrio种类季节性动态的变化规律.通过增菌培养、菌株分离,在224份海水中共分离出弧菌368株,并用分子生物学辅助生化鉴定方法鉴定弧菌菌株.结果表明,在大亚湾海域水体中鉴定的弧菌种类有溶藻弧菌Vibrio alginolyticus、副溶血弧菌V.parahaemolyticus、哈氏弧菌V.harveyi和创伤弧菌V.vuinificus,没有检测到霍乱弧菌V.cholerae、拟态弧菌V.mimicus、河流弧菌V.fluvialis和霍利斯弧菌V.hollisae.溶藻弧菌和副溶血弧菌为优势菌群,分别占弧菌总数的27.99%和21.74%.  相似文献   

6.
研究海洋微生物特征,从青岛近岸养殖密集区、工业区、洁净区分离了428株海洋异养细菌,采用BIOLOG技术对其进行了鉴定和聚类,从中选出13株具有代表性的菌株,克隆其16SrDNA片段,进行分子鉴定。结果表明,它们分别属于弧菌属(Vibrio)、不动杆菌属(Acinetobacter)、假交替单胞菌属(Pseudoalteromonas)、假单胞菌属(Pseudomonas)、海单胞菌属(Oceanimonas)、噬纤维菌属(Cellulophaga)、赤细菌属(Erythrobacter)和Rhodovirga。在3种特征环境中,海洋异养细菌的分布具有一定的规律性:其中洁净区的特征类群属于弧菌属(Vibrio),工业区的特征类群属于弧菌属(Vibrio)和不动杆菌属(Acinetobacter),养殖密集区的特征类群属于弧菌属(Vibrio)、假交替单胞菌属(Pseudoalteromonas)、假单胞菌属(Pseu-domonas)、海单胞菌属(Oceanimonas)、赤细菌属(Erythrobacter)、噬纤维菌属(Cellulophaga)和噬冷菌属(Algoriphagus)。  相似文献   

7.
发光细菌一新种──青海弧菌   总被引:36,自引:0,他引:36  
于1985年8月从青海湖产的青海裸鲁体表分离到70株发光细菌,通过表型特性分析,超氧化物岐化酶的凝胶双向扩散试验,以及G+C摩尔百分比测定进行鉴定分类。结果表明,70株发光细菌在表型特性,免疫学特性等方面彼此高度相似,但与已知的各种发光细菌有显著差异。鉴定为弧菌属的一个新种,定名为青海弧菌Vibrioqinghaiensissp.nov.。典型菌株保存于华东师范大学生物系。  相似文献   

8.
从广东汕尾地区工厂化养殖的患病和死亡的杂色鲍(Haliotis diversicolor)及养殖海水中分离到3株优势菌,经回归感染试验,证实所分离的细菌为杂色鲍的致病菌。经形态、生理、生化等多项指标鉴定,该菌株为副溶血弧菌(Vibrio parahaemolyticus),并经ATB微生物自动鉴定系统证实鉴定结果。在中国大陆,由副溶血弧菌使杂色鲍致病并大量死亡的事件,本文属首次报道。  相似文献   

9.
研究了2个育苗场不同发育期的中国对虾(Penaeus chinensis)幼体的异养菌和弧菌种群变化的动态过程。以典型特征法、BIOLOGGN法和数值分类法对菌株进行鉴定。结果表明,对虾幼体样品中所分离的细菌,大多是革兰氏阴性杆菌。鉴定为假单胞菌属(Pseudomonas)、气单胞菌属(Aeromonas)和弧菌属(Vibrio)。弧菌属主要为溶藻弧菌(Vibrioal-ginozyticus)和哈维氏弧菌(Vibrio harveyi)。在对虾幼体发育早期,假单胞菌(Pseudomonas)和气单胞菌(Aeromonas)占优势,随着对虾幼体的发育,弧菌(Vibrio)渐成为优势,其中溶藻弧菌(Vibrio alginolyticus)和哈维氏弧菌(Vibrio harveyi)优势明显。二者的消长与苗期病害的发生相关,溶藻弧菌总是在虾幼体健康时出现或成为优势,而哈维氏弧菌成为优势时,苗期病害容易发生。  相似文献   

10.
以龙须菜为唯一的营养源对深海沉积物进行富集和筛选,获得一个可降解龙须菜(Gracilaria lemaneiformis)、紫菜(Porphyra umbilicalis)和海带(Laminaria japonica)产生还原性寡糖的菌群.通过16S rRNA序列及16S rRNA-RFLP分析对该菌群中的细菌多样性进行了研究.结果表明,降解菌群中的细菌组成主要为弧菌属(Vibrio,8株)、火色杆菌属(Flammeovirga,7株)和希瓦氏菌属(Shewanella,5株),其中希瓦氏菌属和火色杆菌属的细菌在菌群中的丰度较高.采用龙须菜为唯一营养源的筛选培养基对菌群中的细菌进行分离,获得4株具有琼胶酶活力的细菌,包括2株火色杆菌属和2株希瓦氏菌属细菌.培养和未培养的结果均表明火色杆菌和希瓦氏菌这2个属为所研究的深海沉积物主要的龙须菜降解菌.对原始降解菌群和所分离的关键菌株进行了龙须菜酶解产糖能力的比较,结果发现菌群中的弧菌属菌株虽然自身没有酶解龙须菜的能力,但可能可以协助关键菌株,提高菌群对龙须菜的降解效率.因此本研究中所获得的菌群和菌株有望在琼胶寡糖的绿色生产中得到广泛应用.  相似文献   

11.
青岛近海琼胶降解细菌的筛选和多样性分析   总被引:5,自引:0,他引:5  
对青岛近海海水中琼胶降解细菌进行系统的分离,筛选得到87株海洋琼胶降解细菌。从中选出15株有代表性的菌株,克隆其16SrDNA序列,进行分子鉴定。结果表明,这些细菌主要分布在Cellulophaga,Cytophaga,Microbulbifer,Glaciecola,Pseudoalteromonas,Pseudomonas,Alteromonas和Agarivorans共8个属中。其中QM5,QM21,QM36鉴定为Cellulophaga lytica,QM15和QM28鉴定为Glaciecola mesophila,QM11,QM35,QM47,QM65分别鉴定为Cytophaga fuci-cola,Pseudoalteromonas atlantica,Pseudoalteromonas haloplanktis,Alteromonas addita。其余5株菌能够鉴定到属的水平。其中1株细菌QM42还不能确立分类地位。  相似文献   

12.
采用TCBS选择性培养基从厦门某鲍鱼养殖场的养殖水体中分离到19株细菌.经16S rDNA序列分析,所有菌株均属于弧菌属(Vibrio),且与最近似的弧菌模式种的同源性都在98.99%以上.由于弧菌种间16S rDNA序列相似度极高,无法仅靠16S rDNA序列比对来鉴定这些菌株到种的水平.16S rDNA序列的系统发育分析也显示,大多数菌株与弧菌模式种无法归为一簇,表明16S rDNA基因在弧菌种的分类鉴定上分辨率不高.进一步采用基于4种看家基因(rpo A、pyr H、gap A和top A)的多位点序列分析技术(MLSA)对分离到的弧菌菌株进行分类鉴定,结果显示19株海洋弧菌归于溶藻弧菌(Vibrio alginalyticus)与魔鬼弧菌(Vibrio diabolicus)2个种,表明这两种弧菌是该鲍鱼养殖场水体环境中的优势弧菌种,在鲍鱼养殖弧菌病害防治方面需要重点关注.此外,看家基因与16S rDNA基因的多态性分析表明,4种看家基因的多态位点比率均高于16S rDNA.4种看家基因串联后的多态位点比率高达41.1%,远高于16S r DNA基因的13.4%,表明看家基因相较于16S rDNA基因有着更高的分辨率,更适合于海洋弧菌的分类鉴定.  相似文献   

13.
大黄鱼病原弧菌拮抗放线菌的筛选与人工诱变   总被引:4,自引:0,他引:4  
从厦门集美海滩底泥分离得到38株放线菌,用琼脂块法测定它们对大黄鱼病原弧菌-溶藻弧菌和副溶血弧菌的拮抗效果,选择两株拮抗效果较好的放线菌进行诱变,测定诱变后各菌株的抗菌效果,并选择抗菌效果较好的菌株进行第二次诱变,如此反复诱变3次,共得到97株放线菌,结果表明;38株放线菌中的22株对两株病原菌有一定的拮抗作用;用紫外线照射可以获得少量对两株病原菌拮抗作用加强的菌株。  相似文献   

14.
海湾扇贝(Argopecten irradians)附着基异养细菌区系初探   总被引:1,自引:0,他引:1  
从海湾扇贝附着基上分离出61株异养细菌,对其进行80项生理生化特征测定,以数值分类法进行分析。鉴定结果表明,海湾扇贝附着基上异养菌属于假单胞菌(Pseudomonas)、气单胞菌(Aeromonas)、弧菌(Vibrio)、芽孢杆菌(Bacillus)和产碱杆菌(Alcaligenes)。扇贝幼虫附着前附着的细菌主要为芽孢杆菌与假单胞菌,扇贝幼虫附着后气单胞菌成为优势,弧菌数量明显增加,与假单胞菌数量相当。  相似文献   

15.
A total of 117 agar-decomposing cultures were isolated from coastal seawater around Qingdao,China.The phenotypic and agarolytic features of an agarolytic isolate,QM38,were investigated.The strain was gram negative,strictly aerobic,curved rod and polar flagellum.On the basis of several phenotypic characters,biochemical and morphological characters and phylogenetic analysis of the gene coding for the 16S rRNA,the strain was identified as Agarivorans albus strain QM38.This strain can liquefy the agar on the solid agar plate.An excellular agarase activity was determined in liquid culture.The enzyme exhibited maximal activity at 40℃,pH 7.6.Its activity was greatly affected by different concentrations of agarose.The highest activity 32 U/ml was achieved in the culture supernatant.The hydrolytic product was analyzed by fluorophore-assisted carbohydrate electrophoresis (FACE).After complete hydrolysis of agarose,a series of agaro-oligosaccharides were produced.The main products of the enzymes were oligosaccharides in the degree of polymerization (DP) of 2,4,6 and 8.Three genes agaD01,agaD02 and agaD03,encoding β-agarases,had been cloned from genomic DNA of Agarivorans albus strain QM38.The open reading frame of agaD01,consisted of 2 988 bp,and shared 95.5%-98.9% identity to the β-agarase genes of some strains of Vibrio and Agarivorans.Gene agaD02 comprised 2 868 bp and encoded a 955-amino-acid protein.It showed 97.4% and 98.7% identity to the β-agarase genes of strain Vibrio sp.PO-303 and strain Vibrio sp.JT0107,respectively.Only partial sequence of agaD03 gene has been cloned.It showed 96.5% identity to β-agarase gene (agaB) of Pseudoalteromonas sp.CY24,and shared 96.8% identity to β-agarase-c gene of Vibrio sp.PO-303.  相似文献   

16.
东山九孔鲍细菌性疾病研究   总被引:28,自引:0,他引:28  
张朝霞  王军  张蕉南  苏永全  黄英  鄢庆枇 《台湾海峡》2001,20(2):193-199,T001
本文分离纯化了1999年春东山县患病九孔鲍的2株主要病原菌,进行了回归感染、药敏试验、病变组织的超薄切片观察。结果表明此次暴发性流行鲍病的致病菌主要是溶藻弧菌和副溶血弧菌。在所进行的48种药物的药敏试验中,2株菌仅对氯霉素和复方新诺明等8种药物共同敏感,药物联合抗菌试验还表明复方新诺明与磺胺甲基异恶唑等有协同作用,氯霉素与复方新诺明等有加成作用。  相似文献   

17.
一种新的中国对虾弧菌病原菌──产气弧菌   总被引:11,自引:0,他引:11  
于1993年8月,从山东省昌邑县下营镇患败血病的中国对虾血淋巴内分离到多株细菌,其中2株人工感染证实为病原菌;经50多项形态,生理,生化特性测试鉴定为产气弧菌Vibiogazogenes。其主要特性为:革兰氏阴性,弧状,极生单鞭毛,产生红色素,氧化酶呈阳性,精氨酸双水解酶,赖氨酸脱羧酶,鸟氨酸脱羧酶均为阴性,淀粉酶,明胶酶为阳性,硝酸盐还原阴性,利用木糖,水杨苷,山梨醇发酵葡萄糖产气,利用柠檬酸盐  相似文献   

18.
A study was undertaken to investigate the heterotrophic bacterial flora associated with the sea anemones. Samples of the sea anemones Anthopleura midori were collected from the coast of Weihai and bacteria were isolated from these samples. Additionally, high numbers of viable bacteria were obtained from the celom wall and surface of anemone, the community of cultivable bacteria was very diverse. As a result of this isolation, 60 strains were obtained, 56 of them were selected for identification and characterization by 16S rRNA gene sequence analysis and limited phenotypic testing. Among these isolates, 16 strains were phylogenetically related to members of the genus Pseudoalteromonas and neighboring taxa. Other isolates included members of the genera Colwellia, Vibrio, Acinetobacter, Pseudomonas, Endozoicomonas, Roseovarius, Paracoccus, Loktanella, Leisingera, Sulfitobacter, Bacillus, Staphylococcus, Plantibacter, Microbacterium, Micrococcus, Joostella, Psychroserpens, Cellulophaga, Krokinobacter, Polaribacter and Psychrobacter. Seven potential novel species were found. Among 60 strains, 17 of them can produce proteolytic exoenzyme, 20 can produce lipolytic exoenzyme. Strain NQ8 has strong antagonistic effects on some Vibrio strains. This study demonstrates that the culturable fraction of bacteria from the sea anemones Anthopleura midori is diverse and appears to possess much potential as a source for the discovery of novel bioactive materials.  相似文献   

19.
Trimethylamine N-oxide(TMAO) is widely dispersed in marine environments and plays an important role in the biogeochemical cycle of nitrogen. Diverse marine bacteria utilize TMAO as carbon and nitrogen sources or as electron acceptor in anaerobic respiration. Alteration of respiratory component according to the pressure is a common trait of deep-sea bacteria. Deep-sea bacteria from dif ferent genera harbor high hydrostatic pressure(HHP) inducible TMAO reductases that are assumed to be constitutively expressed in the deep-sea piezosphere and facilitating quick reaction to TMAO released from ?sh which is a potential nutrient for bacterial growth. However, whether deep-sea bacteria universally employ this strategy remains unknown. In this study, 237 bacterial strains affliated to 23 genera of Proteobacteria,Bacteroidetes, Firmicutes and Actinobacteria were isolated from seawater, sediment or amphipods collected at dif ferent depths. The pressure tolerance and the utilization of TMAO were examined in 74 strains. The results demonstrated no apparent correlation between the depth where the bacteria inhabit and their pressure tolerance, regarding to our samples. Several deep-sea strains from the genera of Alteromonas, Halomonas,Marinobacter, Photobacterium, and Vibrio showed capacity of TMAO utilization, but none of the isolated Acinebacter, Bacillus, Brevundimonas, Muricauda, Novosphingobium, Rheinheimera, Sphingobium and Stenotrophomonas did, indicating the utilization of TMAO is a species-speci?c feature. Furthermore, we noticed that the ability of TMAO utilization varied among strains of the same species. TMAO has greater impact on the growth of deep-sea isolates of Vibrio neocaledonicus than shallow-water isolates. Taken together, the results describe for the ?rst time the TMAO utilization in deep-sea bacterial strains, and expand our understanding of the physiological characteristic of marine bacteria.  相似文献   

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