虾夷扇贝脓胞病病原的分离、鉴定与致病性

开展对大连市长海县附近养殖海域近几年夏季出现的大规模虾夷扇贝死亡现象的研究,能为虾夷扇贝养殖过程中的疾病防治提供基础理论支持。以患病虾夷扇贝为研究对象,通过对病变组织进行细菌分离、提纯培养,并采用人工感染试验确定虾夷扇贝脓胞病的病原性质;通过生理生化特性、16SrRNA基因部分序列和药物敏感性测定,对虾夷扇贝脓胞病进行了鉴定。结果表明,从患病组织中分离出的其中一株细菌经人工感染试验证实为虾夷扇贝脓胞病的病原菌,在水温19℃、注射浓度为1.09×105CFU/mL的条件下,该菌有较强的致病性。通过对该病原菌的生理生化特性测定和16SrRNA基因部分序列分析,确定虾夷扇贝脓胞病的病原为查氏弧菌。

虾夷扇贝脓胞病病原查氏弧菌的PCR快速检测

应用PCR技术,建立一种能够快速有效检测出虾夷扇贝脓胞病致病病原查氏弧菌的方法。根据查氏弧菌的GyrB基因的高保守区序列,设计1对扩增片段为144bp的引物,并利用PCR技术对其进行了特异性和敏感性检测。试验结果表明,该方法对查氏弧菌DNA的检测呈特异性,每个PCR反应检测的敏感度为0.43pg的DNA和3.9cuf的细菌。由人工感染和海区取样的虾夷扇贝的病灶组织中可以检测出相应的病原菌,说明本方法有效可行。

骆驼脓胞病防治之我见

骆驼脓疱病是目前国内外危害养驼业十分严重的传染性疾病。早在六十年代初期,甘肃省阿克塞地区就开始有本病流行,以后波及到内蒙古、青海、宁夏、新疆以及甘肃省的其他各县。1979年,非洲地区报导,当地单峰驼也有脓疱病发生。骆驼发生脓疱病不但体质衰弱,使役能力降低,而且绒毛数量减少,质量下降,使养驼业造成严重损失。 关于骆驼脓疱病的病原问题,目前国内外尚无统一的认识。

疱疹样脓疱病23例临床疗效观察

疱疹样脓疱病２３例临床疗效观察刘梦飞①黄利军②周毅成①张晓娟①史语实①王晓惠①郑淑云①孙丽梅①我科自１９７０年～１９９４年底共收治疱疹样脓疱病２３例，现将治疗情况报道如下。１临床资料和治疗方法１．１病例：２３例全为本院皮肤科住院患者，男性５人，女性１...

五大连池矿泉水治疗银屑病868例

本文报道了用低温铁硅质钙镁型矿泉水治疗 868例银屑病患者 ,收到满意疗效 ,总有效率 98 1 6%。

妊娠期间好发的皮肤病

妇女在妊娠期间.由于内分泌改变及胎儿生长发育的需要,母体会发生一系列适应性的变化,皮肤也会发生明显的变化,有的甚至产生疾病。与妊娠有关的皮肤病有以下几种。 妊娠性黄褐斑 妊娠由于黑促素增加,促使黑色素增多,可引起皮肤色素加深,在面部可出现妊娠性黄褐斑。一般在分娩后即渐消退,但不易完全恢复本色。

Up-regulation interleukin-6 and interleukin-8 by activated protein C in lipopolysaccharide-treated human umbilical vein endothelial cells

Objective: To investigate the effect of activated protein C (APC) on inflammatory responses in human umbilical vein endothelial cells (HUVEC) stimulated with lipopolysaccharide (LPS). Methods: The second passage of collagenase digested HUVEC was divided into the following groups: serum free medium control group (SFM control), phosphate buffer solution control group (PBS control), LPS group with final concentration of 1 μg/ml (LPS group), APC group with final concentration of 7 μg/ml, Pre-APC group (APC pretreatment for 30 min prior to LPS challenge), and Post-APC group (APC administration 30 min after LPS challenge). Supernatant was harvested at 0, 4, 8, 12 and 24 h after LPS challenge. Interleukin-6 (IL-6) and Interleukin-8 (IL-8) levels were analyzed with ELISA. Cells were harvested at 24 h after LPS challenge, and total RNA was extracted. Mes-senger RNA levels for IL-6 and IL-8 were semi-quantitatively determined by RT-PCR. Results: Compared with control group, IL-6 and IL-8 levels steadily increased 4 to 24 h after LPS stimulation. APC treatment could increase LPS-induced IL-6 and IL-8 production. The mRNA levels of IL-6 and IL-8 exhibited a similar change. Conclusion: APC can further increase the level of IL-6 and IL-8 induced by LPS. The effect of these elevated cytokines is still under investigation.