旋毛虫各隔离种快速诊断方法的研究

提取４个旋毛虫隔离种的ＤＮＡ，应用Ｊｅａｎ设计的引物序列进行了ＰＣＲ扩增。结果黑龙江猪旋毛虫和Ｔ．ｓｐｉｒａｌｉｓ均显示出家畜型旋毛虫特异的６０２ｂｐ目的ＤＮＡ基因片段，而犬旋毛虫和Ｔ．ｎａｔｉｖａ未见此片段。扩增结果显示，黑龙江猪旋毛虫相当于Ｔ．ｓｐｉｒａｌｉｓ，犬旋毛虫相当于Ｔ．ｎａｔｉｖａ。     

东北地区4株猪,犬旋毛虫间及与国际标准虫株间的杂交试验

为了给中国旋毛虫虫株的分类提供依据，将分离自中国东北地区的４株猪，犬源旋毛虫虫株分别接种于小鼠，按常规分离出肌幼虫，纯化后，设８个杂交试验组，将每２个虫株的雌，雄幼虫体各５条混合，以食管灌注法接种于小鼠，４２ｄ后扑杀，消化，集虫，计数回收肌幼虫数。同法进行了哈尔滨猪株，犬株与国际标准虫株Ｔｒｉｃｈｉｎｅｌｌａ ｓｐｉｒａｌｉｓ（Ｔ．ｓ）．Ｔ．ｎａｔｉｖａ（Ｔ．ｎａ）之间的杂交试验。     

用随意扩增的DNA多态性鉴定中国分离的部分旋毛虫虫株

以旋毛虫国际标准虫种作对照，利用随意扩增的ＤＮＡ多态性技术对国内的部分旋毛虫分离株进行了鉴定与分析，经５条引物的单扩增及复合扩增结果显示，中国的旋毛虫猪株为Ｔ．ｓｐｉｒａｌｉｓ，大株为Ｔ．ｎａｔｉｖａ，猫株为Ｔ．ｎｅｌｓｏｎｉ。     

中国旋毛虫猫分离株SW种类归属的进一步鉴定

通过生物学特性测定及随意扩增的ＤＮＡ多态性（ＲａｎｄｏｍＡｍｐｌｉｆｅｄＰｏｌｙｍｏｒｐｈｉｃＤＮＡ,ＲＡＰＤ）技术,对中国旋毛虫猫分离株进行了进一步鉴定。结果显示：中国的猫分离株ＳＷ为Ｔｒｉｃｈｉｎｅｌｌａｎａｔｉｖａ种,而非Ｔ．ｎｅｌｓｏｎｉ种。     

旋毛虫新生幼虫cDNA文库构建及其特异性基因的筛选与鉴定

构建旋毛虫新生幼虫cDNA文库并对旋毛虫新牛幼虫期特异件基因进行筛选与鉴定,筛选出期特异性的基因片段.用λZAPⅡExpress载体成功地构建了旋毛虫新生幼虫的cDNA文库,并用放射性同位素a-38P标记cDNA探针对筛选出的阳性克隆进行鉴定.所构建的cDNA文库容量为1.92×106,重组效率为98.6%,所有的克隆片段都在0.5～2.0 kb之间,筛选获得7个阳性克隆,其大小在1.4 kb左右;用放射性同位素a-32P标记cDNA探针后,与旋毛虫成虫、肌幼虫、新生幼虫及成虫/新生幼虫cDNA文库质粒DNA进行Southern印迹杂交,结果与新生幼虫和成虫、新生幼虫cDNA文库质粒DNA有杂交而与成虫、肌幼虫cDNA文库质粒DNA不杂交.该基因是新生幼虫期所特有的cDNA片段.     

旋毛虫期特异性基因的筛选与鉴定

对旋毛虫新生幼虫 期特异性基因进行筛选与鉴定,结果表明:对新生幼虫cDNA文库进行核酸杂交筛选，获得7个阳性克隆，其大小在1.4 kb左右；用放射性同位素α³²P标记cDNA探针后，与旋毛虫成虫、肌幼虫、新生幼虫、成虫/新生幼虫cDNA文库质粒DNA进行Southern印迹杂交，结果与成虫/新生幼虫、新生幼虫cDNA文库质粒DNA有杂交而与成虫、肌幼虫cDNA文库质粒DNA不杂交，因此该探针是新生幼虫期所特有的cDNA片段。     

猪、犬旋毛虫DNA限制性片段长度多态性分析

以旋毛虫国际标准虫种Ｔ．ｓｐｉｄａｉｓ和Ｔ．ｎａｔｉｖａ作对照,应用ＤＮＡ限制性片段长度多态性（ＲＦＬＰ）技术对黑龙江省猪、大旋毛虫进行虫种鉴定。结果显示：猪旋虫和Ｔ．ｓｐｉｒｌａｉｓ酶切图谱相同;犬旋毛虫和Ｔ．ｎａｔｉｖａ酶谱一致,结果提示,黑龙江猪旋毛虫为Ｔｓｐｉｒａｌｉｓ,犬旋毛虫为Ｔ．ｎａｔｉｖａ。     

基因探针和PCR对鲤吉陶单极虫的检测

采用液氮冷冻研磨法破碎吉陶单极虫（Ｔｈｅｌｏｈａｎｅｌｕｓｋｉｔａｕｅｉ）孢子，按常规法提取其基因组ＤＮＡ。取ＤＮＡＥｃｏＲＩ消化产物，采用低熔点琼脂糖回收法制备大（３．０～１５．０ｋｂ）、小（０．５～３．０ｋｂ）片段，将其克隆于ｐＢｌｕｅｓｃｒｉｐｔｋｓＥｃｏＲＩ位点，经α－互补现象、酶切鉴定和虫体ＤＮＡ生物素标记探针筛选，构建了含２３个克隆的基因文库，克隆片段介于０．９～６．８ｋｂ之间；经阳性克隆标记筛选及特性分析，制备了长度为０．９ｋｂ（１９号质粒克隆片段）的探针，该探针具有较强的敏感性和特异性。对该探针两端ＤＮＡ序列进行分析，设计出１对引物。上游引物序列为：５′ＴＴＴＣＧＡＡＣＣＣＧＣＡＣＡＡＣＡＡＧ３′，下游引物序列为：５′ＴＧＡＧＴＧＧＡＴＡＧ－ＴＡＴＣＧＣＴＧＣ３′。应用该对引物对虫体进行了检测     

鸡传染性喉气管炎病毒中国王岗株gX基因的克隆及鉴定

以ｐＵＣ１９质粒为载体克隆鸡传染性喉气管炎病毒（ＩＬＴＶ）中国王岗株的ＤＮＡ，构建了鸡传染性喉气管炎病毒ＤＮＡ的ＫｐｎⅠＤＮＡ文库。参考ＩＬＴＶ－ＳＡ２株ｇＸ基因的核酸序列，设计并合成了分别为１２ｂｐ和１３ｂｐ的１对引物。以ＩＬＴＶ中国王岗株ＤＮＡ为模板，用ＰＣＲ方法特异性地扩增出０．８４ｋｂ的ＩＬＴＶ－ｇＸ基因片段。以地高辛标记该０．８４ｋｂ的片段为探针，经Ｓｏｕｔｈｅｒｎ杂交从ＩＬＴＶ中国王岗株ＫｐｎⅠＤＮＡ文库中筛选出３个含５．２ｋｂ外源ＩＬＴＶＤＮＡ片段的ｇＸ基因阳性重组子。经酶切分析、Ｓｏｕｔｈｅｒｎ杂交、ＰＣＲ检测和该片段部分酶谱分析表明，ＩＬＴＶ中国王岗株ＤＮＡ５．２ｋｂ的ＫｐｎⅠ片段无论是片段大小还是酶切图谱均与ＩＬＴＶ－ＳＡ２株完全相同，而且Ｓｏｕｔｈｅｒｎ杂交和ＰＣＲ检测均为ｇＸ阳性，证明其中含有完整的ｇＸ基因     

牛传染性鼻气管炎病毒TK基因缺失株与野毒株PCR鉴别诊断方法的研究

根据已发表的牛传染性敢管炎病毒（ＩＢＲＶ）ＴＫ基因和ｇＢ基因序列，应用Ｏｌｉｇｏ４．１程序设计两对引物ＰＴＫ１和ＰＴＫ２及ＰＢ１和ＰＢ２，分别对已构建的ＴＫ基因缺失（ＴＫ）ＩＢＲＶ以及ＩＢＲＶＬＡ株、洛精、美精、ＢａｒｔｈａＮｕ／６７株、Ｂ７株、云南－１和云南－２分离株进行了ＰＣＲ扩增，结果显示７株ＩＢＲＶＤＮＡ用引物ＰＴＫ１和ＰＴＫ２扩增产生４５７ｂｐ的特异性片段，而ＴＫＩＢＲＶ只出现１１０ｂｐ     

H9N2亚型禽流感病毒传播途径特性的比较及其表面基因序列分析

选择中国大陆最早分离的H9N2亚型禽流感病毒(avian influenza virus,AIV)A/Chicken/Guangdong/SS/94(H9N2)(缩写为SS株)和1998年大流行时期分离的H9N2亚型AIVA/Chicken/Shanghai/F/98(H9N2)(缩写为F株)为研究对象,对其在SPF鸡体内的复制能力和传播途径特性比较后发现,F株在4周龄SPF鸡气管中的复制能力高于SS株,F株可以经气溶胶传播途径传播,SS株不能经气溶胶传播途径传播;利用反转录-聚合酶链反应(RT-PCR)方法获取F株和SS株的HA和NA基因的cDNA,序列分析得知,F株和SS株的HA和NA基因的同源性分别是96.6%和98.1%;HA基因的裂解位点氨基酸序列都是PARSSR↓GL,但有5个氨基酸的差异,即166位N(F)→D(SS)、198位A(F)→V(SS)、217位V(F)→I(SS)、335位G(F)→R(SS)、504位L(F)→S(SS);2株病毒的NA基因在63~65位都存在氨基酸缺失,但在NA基因红细胞吸附位点的氨基酸序列不同,分别是IKKDSRSG(F)和IKEDLRSG(SS)。F株和SS株的传播特性差异是否与其表面基因序列有关,有待进一步研究。     

种鹅矛形剑带绦虫与背孔吸虫混合感染的诊治

2005年9月份,大庆市红岗区个体养鹅专业户送检6只病死的5月龄左右隆昌鹅和长白鹅,经过实验室诊断确诊为矛形剑带绦虫与背孔吸虫混合感染。矛形剑带绦虫属膜壳科     

禽类的起源、演化及我国主要家禽品种类型与分布

家禽是重要经济价值动物.本文从禽类种群进化学说出发,简介了禽类的起源、演化、动物学分类和家禽的驯化(养)与品种的形成,并对我国主要家禽(鸡、鸭、鹅)地方品种和培育品种(配套系)的分布与类型作了描述,以期为研究我国家禽起源系统,保护与利用我国家禽品种,促进家禽生产可持续发展提供参考.     

一起猪链球菌病和伪狂犬病的混合感染的诊治

近年以来,由于市场因素的刺激,生猪的存养量大幅上升,再加上由于流通环节较多,流通非常频繁,流通距离越来越远。这对繁荣经济,增加养殖效益起了重要的推动作用,但也同时给疾病的感染和传播创造了有利条件,给猪病的防治带来了困难。有的猪场感染了传染病后,由于治疗不及时不得法,而造成了惨重的经济损失。2008年7月中旬,我街道一养猪户因盲目从外地购进中猪,发生猪病疫情,引起猪只连续死亡,造成一定的经济损失。根据流行病学、临床症状、剖检变化和实验室诊断,诊断该病为猪链球菌病和猪伪狂犬病混合感染,现报告如下。     

秋冬季预防和治疗虫媒性传染病鸡白冠病和鸡痘

１前言１．１鸡白冠病鸡白冠病是由卡氏住白细胞原虫寄生于鸡的红细胞和单核细胞而引起的鸡的贫血性疾病。吸血昆虫蚋和库蠓叮咬鸡引起传播，是主要的传播媒介，一般在夏末和秋季多发，由于夏季降雨量较大，部分沟渠积水，库蠓和蚋多孳生，因此在多雨水涝的年份发病率明显增高。１９９８年中国从南到北发生洪涝灾害，吸血昆虫的孳生格外严重，出现了一个白冠病多发年，而后两年发病稍轻，并有地区性，今年８月中旬以来白冠病的发病呈抬头趋势，有一定的死亡率，对蛋鸡产蛋率也会引起一定程度的降低，应引起养鸡户的重视。１．２鸡痘鸡痘也是…     

Shape and size of teeth of dogs and cats-relevance to studies of plaque and calculus accumulation

Crown width, height and buccal surface areas were measured on heads or skulls of four dogs and four cats, and were compared with similar measurements on models of human dentition. Buccal surface area variability was greater in dogs and cats than in humans, and teeth of cats were smaller. Horizontal (gingival and occlusal halves) and vertical (mesial, middle, and distal thirds) buccal surface area variability was also greater in canine and feline teeth compared with human teeth. This increased variability suggests the need for testing of reliability and repeatability of scoring when using plaque and calculus indices based on horizontal or vertical segmentation. Buccal surface area variability between teeth also prompts questioning the validity of equal weighting of smaller, irregularly-shaped teeth when calculating a mean mouth score. Whether equal or more reliable results would be obtained from scores of whole teeth in comparison with segmentation indices used currently has yet to be determined.     

Estimations of repeatability and heritability of egg albumen antimicrobial activity and of lysozyme and ovotransferrin concentrations

1. The repeatability and heritability of growth inhibition by egg albumen of two major pathogenic bacteria, a Gram-negative (Salmonella Enteritidis) and a Gram-positive (Staphyloccocus aureus) and of two antimicrobial albumen proteins, lysozyme and ovotransferrin, were estimated in commercial pedigree hens. 2. Repeatability was evaluated in 100 egg-type hens at the beginning, middle and end of the laying cycle on eggs collected for 3 weeks. Heritabilities were estimated at 36 to 40 weeks of age on 400 pedigree hens (2 eggs/hen), which were the offspring of 25 sires each mated with 4 dams. Ovotransferrin and lysozyme were quantified by ELISA. Salmonella Enteritidis (S.E.) and Staphyloccocus aureus (S.A.) were inoculated into a sample of sterilised albumen and enumerated after incubation. 3. Total protein content in albumen decreased with age of laying hens, whereas there were increases in lysozyme or ovotransferrin concentrations and in the bacteriostatic effect of albumen. 4. Repeatability for bacterial growth in albumen ranged from 0.29 to 0.39 for the number of S.E. (log cfu/ml) one day post inoculation (p.i.) but was lower and more variable at 5 d p.i. or for S.A. number. It ranged from 0.27 to 0.38 for S.E. and S.A. number at the mid period of the laying cycle. Repeatabilities were low and variable for total egg albumen protein or lysozyme and ovotranferrin concentrations (0 to 0.22). 5. Negative phenotypic correlations were observed between lysozyme concentrations and S.E. number but that between lysozyme and S.A. number was not significant. 6. Heritabilities were low (0.01 to 0.09) for protein traits. They were 0.11 for S.A. number and 0.16 for S.E. number one day p.i. 7. It appears to be more efficient to select on global bacterial growth than on specific antimicrobial proteins. The most promising trait is the number of S.E. one day p.i.     

Evaluation of lysozyme and lactoferrin in lacrimal and other ocular glands of bison and cattle and in tears of bison

OBJECTIVE: To evaluate lactoferrin and lysozyme content in various ocular glands of bison and cattle and in tears of bison. SAMPLE POPULATION: Tissues of ocular glands obtained from 15 bison and 15 cattle and tears collected from 38 bison. PROCEDURE: Immunohistochemical analysis was used to detect lysozyme and lactoferrin in formalin-fixed, paraffin-embedded sections of the ocular glands. Protein gel electrophoresis was used to analyze ocular glands and pooled bison tears by use of a tris-glycine gel and SDS-PAGE. Western blotting was used to detect lactoferrin and lysozyme. RESULTS: Immunohistochemical staining for lactoferrin was evident in the lacrimal gland and gland of the third eyelid in cattle and bison and the deep gland of the third eyelid (Harder's gland) in cattle. Equivocal staining for lactoferrin was seen for the Harder's gland in bison. An 80-kd band (lactoferrin) was detected via electrophoresis and western blots in the lacrimal gland and gland of the third eyelid in cattle and bison, Harder's glands of cattle, and bison tears. An inconsistent band was seen in Harder's glands of bison. Lysozyme was not detected in the lacrimal gland of cattle or bison with the use of immunohistochemical analysis or western blots. Western blots of bison tears did not reveal lysozyme. CONCLUSIONS AND CLINICAL RELEVANCE: Distribution of lactoferrin and a lack of lysozyme are similar in the lacrimal gland of cattle and bison. Differences in other tear components may be responsible for variability in the susceptibility to infectious corneal diseases that exists between bison and cattle.