条石鲷(Oplegnathus fasciatus)源美人鱼发光杆菌杀鱼亚种(Photobacterium damselae subsp. piscicida)的分离鉴定

2013年浙江省舟山市某网箱养殖条石鲷(Oplegnathus fasciatus)暴发了一种严重的疾病,病鱼主要症状为脾、肾出现1-2 mm的白色类结节.从患病鱼内脏处分离得到1株优势菌OF-1,经人工感染实验证实为此次引起条石鲷死亡的致病菌,半数致死量为5.93×104 CFU/g.形态学观察结果显示,菌株OF-1为革兰氏阴性、短杆状,在TCBS培养基上不生长.API 20E细菌鉴定系统、16S rRNA系统发育树分析结果证实,该菌株为美人鱼发光杆菌杀鱼亚种(Photobacterium damselae subsp.piscicida).该菌对庆大霉素、青霉素、氟哌酸、氧氟沙星、氨苄青霉素等药物高度敏感,对红霉素、链霉素、卡那霉素、苯唑青霉素等药物具有抗性.     

Insecticidal Activity and HPLC Correlation of Thuringiensin from Fermentation and Two-phase Aqueous Separation Processes

Thuringiensin produced by Bacillus thuringiensis subsp. darmstadiensis was further subjected to a two-phase aqueous separation system. A modified HPLC method and a test for quantitative pathogenicity using the house fly Musca domestica were used for analysis of thuringiensin. Within a realistic range of dosages, more effect was observed in the pupal stage than in the larval stage. The percentage effective control rate (ECR) was calculated by (100-percentage emergence); malformed and non-reproductive adults were considered as emerged. Pupal mortality, pupal weight, and ECR after feeding the three-day-old larvae were the measured response criteria for bioassay. The EC₅₀ of thuringiensin for pupae mortality was 1·64 μg ml^-1 diet, and 0·83 μg ml^-1 for mortality of adults. Insecticidal activity of the broth increased with fermentation time-course from 9th to 21st hour. The bioassay curve constructed with three-hour sampling interval during the fermentation course had good correlation to thuringiensin content as determined by the HPLC method. In the two-phase aqueous separation system, a maximum of 96·7% ECR was achieved with the bottom salt layer, compared to a value of 46·7% with the upper PEG layer. These results suggest that thuringiensin, prepared through a fermentation and recovery process, is suitable for pest control. © 1997 SCI.     

Fish photobacteriosis—The importance of rapid and accurate identification of Photobacterium damselae subsp. piscicida

MALDI‐TOF MS was tested for the identification of Photobacterium damselae subsp. piscicida on isolates grown on two media, cultured at three incubation times and applied on the target plate by the direct sample spotting (DS), by the on‐target extraction (OTE) and by the full extraction (FE) method, in triplicates. The identification of samples grown on blood agar (BA) outperformed identification on tryptic soya agar (TSA) by 0.64% for DS and OTE. The OTE gave the highest scores in both culture media, all incubation times and replicates. Reliable 24‐hr species identification was 61.54%, 84.61% and 53.85% for samples grown on TSA and identified by DS, OTE and FE, respectively. For isolates grown on BA, they were 76.92%, 96.15% and 30.77%, respectively. When identified by OTE, the 48‐hr identification was 93.58%, but for 72 hr declined to 71.79%. The reliable identification with the highest score from the first measurement was 100% only for OTE from BA (24 hr), whereas OTE from TSA gave 84.61% (24 hr), 76.92% (48 hr) and 84.61% (72 hr). The reliable MALDI‐TOF MS identification of Ph. damselae subsp. piscicida is incubation time, media, target plate preparation and replicate‐dependent.     

内蒙古马铃薯黑胫病病原菌的分离和鉴定

 马铃薯是我国的第四大主粮。内蒙古是我国最大的马铃薯生产基地,马铃薯产业是当地农民收入的主要来源。2017年8月,内蒙古锡林郭勒盟部分马铃薯田块发生了一种细菌性黑胫病,发病面积约为200亩,发病率约为20%。发病初期,植株的茎基部变色、发黑,伴有臭味,严重时茎秆腐烂,植株死亡。为明确该地区马铃薯细菌性黑胫病的病原菌种类,本研究对该病原菌进行了分离,并利用生理生化测定,Biolog分析和分子生物学手段将该病原菌鉴定为胡萝卜软腐果胶杆菌巴西亚种(Pectobacterium carotovorum subsp. brasiliense)。据以往报道,我国马铃薯黑胫病主要由黑腐果胶杆菌(P. atrosepticum)和胡萝卜软腐果胶杆菌胡萝卜亚种(P. carotovorum subsp. carotovorum)两种病原菌引起,本研究是P. carotovorum subsp. brasiliense引起马铃薯黑胫病在国内的首次报道。     

高效微生物杀虫剂对蚊虫的杀灭作用

新疆阿勒泰北屯地区位于额尔齐斯河下游,夏季蚊虫泛滥,严重威胁当地人民的身体健康.本研究跟踪调查了各种水体的幼蚊滋生情况,确定了幼蚊发生的2个高峰期分别出现在5月下旬至6月上旬及6月下旬至7月上旬,同时确定了洪水型积水、排碱渠积水和漫灌林带积水是幼蚊高发的孳生地类型.采集并对蚊虫样品进行形态学鉴定,确定了该地区的优势蚊种为刺扰伊蚊Aedes vexans.用苏云金芽胞杆菌以色列亚种Bacillus thuringiensis subsp.israelensis(Bti)水剂对该蚊种进行了室内生测,其LC50和LC90分别为0.055和0.198 mg/L.分别选取3种高发孳生地的3处积水进行野外试验,发现48 h后该药剂对幼蚊的杀灭率均在96％以上,对大面积孳生地也有很好的杀灭作用.监测显示成蚊出现的高峰时间是每年的6月上旬至6月中旬及7月中旬至7月下旬.连续施药3年后,2013年的成蚊数量相比2011年时下降幅度超过50％.本研究对于北屯地区蚊虫的进一步控制以及Bti制剂在新疆的推广有重要的意义.     

双重PCR检测马铃薯晚疫病和环腐病方法的建立

通过克隆马铃薯环腐病菌和晚疫病菌转录间隔区(ITS)序列,并对测序结果进行同源性比较,选取差异位点分别设计了两对引物P.IN1/P.IN2和C.IN1/C.IN2,并检测了引物的特异性及方法的灵敏度。引物P.IN1/P.IN2可扩增出1条363bp马铃薯晚疫病菌的特异性条带,在DNA水平上其灵敏度达18fg/μL;引物C.IN1/C.IN2可扩增出1条218bp马铃薯环腐病菌的特异性条带,在细菌数上检测灵敏度为104 cfu/mL。混合这两对引物构建双重PCR反应体系,能从马铃薯环腐病菌和晚疫病菌的混合DNA及感染这两种菌的马铃薯植株中同时扩增到363bp和218bp的特异片段。实现了同时对马铃薯晚疫病菌和环腐病菌的快速可靠检测。     

玉米细菌性枯萎病菌的环介导恒温扩增(LAMP)检测方法

为了提高口岸和基层实验室检疫和监测玉米细菌性枯萎病菌的准确性和工作效率,利用环介导恒温扩增技术(LAMP),根据内切葡聚糖酶(EGase)基因前导序列,设计2个内引物和2个外引物,对玉米细菌性枯萎病菌进行快速检测。结果表明,使用玉米细菌性枯萎病菌的近缘种或引致相似症状的病原菌菊欧文氏菌玉米致病变种Erwinia chrysanthemi pv.zeae、玉米内州萎蔫病菌Clavibacter michiganensis subsp.nebraskensis、燕麦假单胞菌Pseudomonas avenae、杓兰欧文氏菌Erwinia cypripedii检测其特异性,仅玉米细菌性枯萎病菌有扩增。LAMP检测灵敏度达到2 pg DNA,为普通PCR的100倍;与其它检测方法相比,LAMP方法检测时间短,效率高,不仅降低了设备投入,易于操作,而且具有较高的灵敏度和特异性,适合玉米细菌性枯萎病菌的现场检疫和大规模检测。     

固定化唾液链球菌生产γ-氨基丁酸的研究

以唾液链球茵嗜热亚种(Streptococcus salivarius subsp.thermophilus Y-2)为供试菌株,考察了卡拉胶、明胶和海藻酸钙等材料将此菌株固定化的效果,并通过比较固定化细胞的谷氨酸脱羧酶(glutamatedecarboxylase,GAD)活性及γ-氨基丁酸的产量和载体机械强度,确定了海藻酸钙作为固定化细胞的适宜载体.优化后得到的最适固定化条件(W/V)为:海藻酸钠2%,CaCl_2 14%,茵体25%,凝胶平均颗粒直径1.64 mm,在此条件下测得固定化细胞的GAD活性为游离细胞的1.2倍.细胞多批次应用稳定性试验证明:固定化细胞较游离细胞有着更稳定的GAD活性,反复使用60 h后,固定化细胞GAD活性仍能保持其初始活性的90%以上,γ-氨基丁酸的积累量达到7.97 g/L.     

Growth pattern and partial proteome of Mycobacterium avium subsp. paratuberculosis during the stress response to hypoxia and nutrient starvation

Mycobacterium avium subsp. paratuberculosis is an important pathogen that causes Johne's disease in animals and has been implicated in Crohn's disease in man yet few data exist on its physiological adaptation in either the host or the environment. In this study, the proteomic responses of the two distinct strains of M. a. paratuberculosis, cattle (C) and sheep (S), to hypoxia and starvation were studied in vitro. Nutrient starvation inhibited growth of both strains and was lethal for S strain after 12 weeks. Hypoxia induced a state of very low metabolic activity but rapid resuscitation occurred upon restoration of an aerobic atmosphere, consistent with the dormancy response of other mycobacteria. A total of 55 protein spots differentially expressed in response to starvation and/or hypoxic stress in one or both strains were identified from 2D gels and classified based on biological function. Antioxidant enzymes, oxidoreducatse enzymes and proteins involved in amino acid metabolism, fatty acid metabolism, ATP and purine biosynthesis, proteolysis, cell wall synthesis, protein synthesis, signal recognition and hypothetical proteins with putative functions including dormancy response regulators and universal stress proteins were identified. These proteins are potential screening targets for future diagnosis, prevention and control of M. a. paratuberculosis infection and their identification will assist understanding the pathogenesis of diseases caused by this organism.