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1.
确定角蝇各龄期幼虫体内的斯氏副柔线虫(Parabronema skrjabini)幼虫。通过大量剖检角蝇各龄期幼虫,收集其体内的线虫幼虫,经扩增测序获得ITS基因序列,利用DNAStar 5.0软件,将其与斯氏副柔线虫成虫的ITS基因序列进行同源性比较。结果表明,角蝇Ⅰ、Ⅱ、Ⅲ期幼虫体内的线虫幼虫确为斯氏副柔线虫幼虫。该研究结果不但为鉴定角蝇各龄期幼虫体内的斯氏副柔线虫幼虫提供了简易准确的方法,而且也为弄清斯氏副柔线虫在其传播媒介角蝇体内的发育过程奠定了基础。  相似文献   

2.
斯氏副柔线虫半胱氨酸蛋白酶Pj-CPR基因的克隆及原核表达   总被引:1,自引:0,他引:1  
为了筛选斯氏副柔线虫抗原基因用于血清学诊断和免疫防治研究,对斯氏副柔线虫半胱氨酸蛋白酶Pj-CPR基因序列进行了生物信息学分析,RT-PCR扩增获得了Pj-CPR基因,构建重组表达质粒pETCPR后,转入大肠埃希菌BL21(DE3)中并诱导表达获得重组蛋白rCPR。SDS-PAGE和Western blot检测结果表明,重组蛋白rCPR大小为17.6ku,主要以包涵体的形式表达,能与感染斯氏副柔线虫的骆驼血清中IgG特异性结合,具有良好的抗原活性,可用于斯氏副柔线虫病血清学诊断方法和免疫防控研究。  相似文献   

3.
为了解伊犁河谷区域虻的分布及其携带伊氏锥虫的情况,通过对虻的形态学鉴定及其特异性基因(CO1)和携带病原18S rRNA基因扩增、测序、同源性比对,鉴定和检测了采自伊犁河谷区域的虻及其携带病原情况。结果显示,所采集的虻为原虻属秋季原虻种,PCR扩增虻CO1基因和马伊氏锥虫18S rRNA基因序列分别为653 bp和205 bp。结果发现,秋季原虻的CO1基因与已发表的丹麦株(MT584147.1)同源性为98%,与形态学鉴定结果一致。在156只秋季原虻中携带伊氏锥虫的有9只,阳性率为5.7%(9/156),其阳性条带基因序列与GenBank中已发表的伊氏锥虫基因同源性为99%。试验结果表明,结合形态学分类和分子生物学方法对虻样品进行鉴定操作简单、准确度高。  相似文献   

4.
斯氏副柔线虫rDNA-ITS片段的克隆及序列分析   总被引:3,自引:1,他引:2  
运用PCR方法以保守引物NC5、NC13、NC13r和NC2扩增从内蒙古地区骆驼皱胃分离的3条斯氏副柔线虫(Parabronema skrjabini)rDNA的内转录间隔区1(ITS1)、5.8S序列和内转录间隔区2(ITS2)。将PCR扩增出的片段纯化后克隆至pGM-T载体,用PCR技术及酶切鉴定阳性菌落,对阳性菌落质粒DNA进行测序。结果表明线虫1(P.sk1)扩增的ITS片段大小为837 bp,包含部分的18S、28S及全部的ITS1(298 bp)、5.8S(157 bp)及ITS2(281 bp)序列;线虫2(P.sk2)扩增的ITS1片段大小为372 bp,包含部分的18S、5.8S及全部的ITS1(296 bp);线虫3(P.sk3)扩增的ITS2片段大小为484 bp,包含部分的5.8S、28S及全部的ITS2(284 bp)序列。同其它属线虫同源性比较ITS2序列同源性在30.2%-60.1%。本研究系首次报道骆驼斯氏副柔线虫的ITS序列,为斯氏副柔线虫分子生物学的进一步研究奠定基础。  相似文献   

5.
试验旨在克隆斯氏副柔线虫糖蛋白(glycoprotein,GP)抗原基因,并对其进行生物信息学分析。提取斯氏副柔线虫组织RNA,反转录合成cDNA,设计特异性引物以扩增GP基因CDS区,同时将其插入到克隆载体pMD19-T后测序,并对该基因编码蛋白的抗原表位、理化性质、信号肽、跨膜结构域等进行生物信息学预测。结果表明,GP基因开放阅读框(ORF)全长1 149bp,编码382个氨基酸,其分子式为C1760H2878N458O590S1760,理论分子质量约为40.15ku,等电点为4.37,无信号肽,总平均亲水性为0.032,不稳定系数为42.43,是疏水、不稳定蛋白;其磷酸化位点分布位于丝氨酸(Ser)、苏氨酸(Thr)和酪氨酸(Tyr)残基上;二级结构分析显示,斯氏副柔线虫GP蛋白以α-螺旋和无规则卷曲为主,与三级结构预测结果一致;抗原表位预测表明,GP蛋白可能有6个B细胞抗原表位和8个T细胞抗原表位,有望用作免疫诊断抗原和疫苗候选抗原。本研究成功克隆了斯氏副柔线虫GP基因,同时进行了系统的生物信息学分析和抗原表位预测,为斯氏副柔线虫病iELISA诊断方法的建立和DNA疫苗的研究提供理论依据。  相似文献   

6.
为阐明野猪杜氏颚口线虫分离株线粒体细胞色素b(cytb)基因的遗传变异情况,并利用该基因探究杜氏颚口线虫与其它线虫的种群遗传关系。本研究利用PCR扩增从野猪体内分离出的杜氏颚口线虫cytb基因,并对该基因序列进行分析。结果显示,8株杜氏颚口线虫分离株线粒体cytb基因序列长度均为1 067 bp,与Genbank中登录的杜氏颚口线虫分离株同源性均大于98.3%,与其它线虫的同源性均小于72.0%;通过该基因建立的系统发育树分析显示,所有的杜氏颚口线虫分离株均与已知杜氏颚口线虫属于同一大分支。表明,线粒体cytb基因序列种内相对保守,种间差异明显,可以作为分子标记应用于杜氏颚口线虫的种间遗传变异研究。本研究为杜氏颚口线虫的分子流行病学和群体遗传学奠定基础。  相似文献   

7.
本研究对安徽猪源弓形虫529 bp重复序列进行了分析,为其分子流行病学研究以及诊断方法的建立奠定基础。首先对病料虫体基因组DNA进行提取,然后对弓形虫529 bp基因进行PCR扩增、克隆、测序并对测序结果进行比对、同源性分析和构建系统进化树。结果显示,PCR扩增产物约为528 bp,与已报道的弓形虫同一基因序列具有高度同源性,与GenBank报道的EF648169.1株同源性最高,达99.5%,且遗传距离最为接近;与其他5株猪源弓形虫比对显示主要突变区域在第31~74位和第100~141位碱基。表明该猪源弓形虫与犬源弓形虫EF648169.1株为姊妹株;本基因序列碱基突变较少,保守性较好,适合作为弓形虫病诊断的靶基因。  相似文献   

8.
为了获得和田青驴线粒体DNA中细胞色素氧化酶(CO1)基因序列,试验采用PCR技术及BLAST在线平台方法对和田青驴血液线粒体DNA中CO1基因进行扩增与序列同源性分析。结果表明:DNA核苷酸序列与AJ009780.1的同源性为99.0%,与KC763190.1、CR388000.2、AB033487.1同源性为98.0%,确认是试验所需要的目的基因。  相似文献   

9.
裂头蚴病是由于裂头蚴感染引起的一种人兽共患病,为了对福建省养殖蛇类的裂头蚴感染情况进行调查并鉴定虫种,对采自福建省三明市、漳州市和南平市等地蛇场的蛇类进行剖检,分离得到了裂头蚴,记录寄生部位和数量。提取裂头蚴虫体基因组,采用PCR对虫体ITS、NAD4和COX3基因进行了扩增。同时,将扩增得到的目的基因连接到pEASY-Blunt Simple载体上,转化Trans I-T1感受态细胞,培养得到单菌落,对菌落进行扩增测序。将测序结果与NCBI公布的裂头蚴ITS、NAD4和COX3基因序列进行比对分析,测定突变率和位点,并且进行样本之间的同源性分析和测定遗传距离。结果发现,三明市、漳州市和南平市某蛇场裂头蚴的感染率分别为75%、20%和0。分离到的裂头蚴ITS基因序列长为1 360 bp~1 380 bp,与NCBI中Spirometra erinaceieuropaei(FJ886747.1)的ITS基因同源性为95.70%~98.68%,样本之间平均遗传距离为0.001 6;分离到的裂头蚴NAD4基因序列长为356 bp~650 bp,与NCBI中Spirometra erinaceieuropaei(HM475076.1)的NAD4基因同源性为96.73%~100%,样本之间平均遗传距离为0.004 1;分离到的裂头蚴COX3基因序列总长为379 bp~408 bp,与NCBI中Spirometra erinaceieuropaei(HM475033.1)的COX3基因同源性为98.94%~100%,样本之间平均遗传距离为0.003 8。结果表明,此次分离得到的裂头蚴虫体的ITS基因、NAD4基因和COX3基因与欧猥迭宫绦虫裂头蚴同源性较近,证明此次分离的蛇源裂头蚴属于欧猥迭宫绦虫裂头蚴。同时,经过对各虫体间NAD4和COX3基因分析发现,不同地区的裂头蚴虫体在进化树上存在分支。  相似文献   

10.
为筛选合适的DNA条形码对气单胞菌属(Aeromonas)进行鉴定,以33株气单胞菌为材料,选取cpn60、recA和ppsA 3个候选DNA条形码进行PCR扩增及序列分析。以种间和种内遗传距离、序列扩增测序成功率、DNA条形码间隙(DNA barcoding gap)和系统发育树作为评价条形码片段的指标,筛选出该属的DNA条形码。分析表明,cpn60基因的扩增及测序的成功率最高,种内遗传平均距离(0.017)和种间遗传平均距离(0.133)差异显著,且存在较明显的DNA barcoding gap,表明cpn60可作为气单胞菌鉴定的DNA条形码。  相似文献   

11.
The anthelmintic efficacy of ivermectin (administered subcutaneously at 200 micrograms kg-1 body weight) was assessed for control of Thelazia skrjabini in experimentally infected calves. Twenty-four uninfected male Holstein calves, 1-2 weeks old, were artificially infected with Thelazia skrjabini by placing 15 third-stage larvae under the third eyelid of calves. The challenge larvae were recovered from naturally infected face flies, Musca autumnalis. The exposed calves were randomly assigned to either an ivermectin treatment group or a control group within pairs ranked by weight. Equal numbers of calves were housed in each of four indoor fly-free rooms. The calves were treated with ivermectin or saline 35 days post-infection, then slaughtered 14 days later to determine eyeworm numbers. All eyes and associated tissues (including the lacrimal glands and ducts) were removed and examined for total number, species and viability of eyeworms. Thelazia skrjabini was found in the control group of calves only. The efficacy of ivermectin against Thelazia skrjabini was thus shown to be 100%.  相似文献   

12.
为探讨猫感染斯氏肺吸虫囊蚴后,虫体是否具有排卵规律性,以便为肺吸虫流行病学调查,临床诊断,疗效考核,实验环境灭卵等方面提供参考。用改良Kato法对猫感染斯氏肺吸虫(P.s)后定期查粪便达6个月,观察不同时间的排卵量。结果。4只感染斯氏肺吸虫猫分别于感染后第57天和第58天.在粪便中开始查到排出的P.s虫卵。用改良Kato法获得定时定量的EPG数据。结论认为Paragonimus skrjabini虫卵具有排卵高峰期,第1个高峰出现在感染后第4个月左右。第2个排卵高峰出现在感染后第5个月左右。  相似文献   

13.
试验旨在克隆斯氏副柔线虫糖蛋白(glycoprotein,GP)抗原基因,并对其进行生物信息学分析。提取斯氏副柔线虫组织RNA,反转录合成cDNA,设计特异性引物以扩增GP基因CDS区,同时将其插入到克隆载体pMD19-T后测序,并对该基因编码蛋白的抗原表位、理化性质、信号肽、跨膜结构域等进行生物信息学预测。结果表明,GP基因开放阅读框(ORF)全长1 149 bp,编码382个氨基酸,其分子式为C1760H2878N458O590S1760,理论分子质量约为40.15 ku,等电点为4.37,无信号肽,总平均亲水性为0.032,不稳定系数为42.43,是疏水、不稳定蛋白;其磷酸化位点分布位于丝氨酸(Ser)、苏氨酸(Thr)和酪氨酸(Tyr)残基上;二级结构分析显示,斯氏副柔线虫GP蛋白以α-螺旋和无规则卷曲为主,与三级结构预测结果一致;抗原表位预测表明,GP蛋白可能有6个B细胞抗原表位和8个T细胞抗原表位,有望用作免疫诊断抗原和疫苗候选抗原。本研究成功克隆了斯氏副柔线虫GP基因,同时进行了系统的生物信息学分析和抗原表位预测,为斯氏副柔线虫病iELISA诊断方法的建立和DNA疫苗的研究提供理论依据。  相似文献   

14.
Gastrointestinal helminths were collected from 49 Japanese tree sparrows (Passer montanus saturatus) in Tokyo, Japan. In 16 sparrows, 1-9 (average, 3.5) gizzard spirurid nematodes (Acuaria skrjabini Ozerskaya, 1926) were found embedded in the mucosa of the gizzard. In addition, Capillaria sp., Platynosomum passeri Yamashita et Tsumura, 1962, and a hymenolepidid cestode were collected from 1, 2, and 1 sparrows, respectively. A sexually mature A. skrjabini female and 3 males were found also in a young gray starling (Sturnus cineraceus) that was found dead in the same area after failure to leave the nest. Starlings are a new host record for this spirurid species. Until this study, this gizzard spirurid species has not been recorded in this country or the Far East region.  相似文献   

15.
A rapid and specific method for the detection of pathogenic Leptospira spp. in bovine semen using the polymerase chain reaction (PCR) is described. The primers used were derived from an EcoR1/BamH1 fragment that hybridized strongly to chromosomal DNA from the hardjobovis serovar. Three different extraction methods were evaluated in this study: phenol-chloroform extraction method, proteinase K (PK) in 1% SDS, followed by phenol-chloroform, and phenol-chloroform followed by 1% cetyltrimethylammonium bromide (CTAB). A PCR product of approximately 500 base pairs (bp) in length was obtained when DNA from pure Leptospira culture was used as a template for PCR, regardless of the DNA extraction method used. The product was consistent with that predicted from the gene sequence. However, in semen seeded in vitro, as well as in semen from infected bulls, a PCR product was obtained only when the leptospiral DNA was extracted from the specimen using the CTAB method. In contrast, other methods used for DNA extraction did not generate suitable templates for the PCR procedure. This is the first PCR protocol developed to detect Leptospira in bovine semen. The PCR protocol provided a direct and unequivocal demonstration that Leptospira can be detected in semen of infected animals. The CTAB method was also used successfully in detecting Leptospira in the urine of infected animals. The PCR procedure was shown to be more sensitive than either the fluorescent antibody test (FAT) or culture for detecting the organism in urine.  相似文献   

16.
为建立骆驼斯氏副柔线虫病间接ELISA (iELISA)诊断方法,本试验对骆驼斯氏副柔线虫半胱氨酸蛋白酶CPR基因进行重组表达,将获取的重组蛋白(rCPR)进行纯化和Western blotting检测,然后以纯化好的重组蛋白为抗原,通过棋盘滴定试验优化了抗原包被浓度、包被条件、抗体稀释度、酶标二抗稀释度、封闭液和封闭时间等,建立了骆驼斯氏副柔线虫病iELISA诊断方法,并对建立的iELISA检测方法进行了重复性、敏感性、特异性试验和临床检测。结果显示,抗原最佳包被浓度为8 μg/孔,血清最佳稀释度为1:50,酶标二抗最佳稀释度为1:5 000,最佳包被条件为4℃包被过夜,最佳封闭条件为3% BSA封闭2 h。临界值为0.235,待检血清D450 nm值>0.235则确定为阳性。重复性试验中变异系数均<10%,重复性较好;用该方法检测阳性血清的敏感性为96.3%;此方法仅与骆驼斯氏副柔线虫病阳性血清发生特异性反应,与感染了其他寄生虫的阳性血清无交叉反应,特异性为100%;对140份临床血清进行检测,阳性率为86.4%。综上可知,本试验成功建立了一种快速有效诊断骆驼斯氏副柔线虫病的iELISA方法。  相似文献   

17.
根据猪链球菌2型的mrp基因自设计和合成了一对可扩增长度为885bp目的片段的引物,成功地建立了检测溶菌酶释放蛋白(MPR)的PCR方法,用XbaⅠ内切酶进行酶切,获得了与预期一致的578bp和307bp2的2个片段,并进行了PCR的特异性试验和敏感性试验。对马链球菌兽疫亚种、猪丹毒杆菌、猪肺疫巴氏杆菌和猪肺炎支原体的PCR检测结果均呈阴性;检测的敏感度可达100个细菌。另外,对9株从病猪体内分离的猪链球菌2型菌株进行检测了8个呈阳性;对15份正常屠宰猪扁桃体分离物的检测结果是1份为阳性。结果表明此法特异性敏感性均很高,可作为MRP快速诊和流行病学调查的手段。  相似文献   

18.
从pMD18-T—HA阳性质粒中扩增出H7亚型禽流感病毒(AIV)HA1基因,并亚克隆至昆虫杆状病毒转移载体pBlueBacHis2A,将筛选的重组质粒命名为pBlueBacHisH7-HA1,与线性化杆状病毒DNA(Bac—N—BlueDNA)共转染sf9昆虫细胞,挑取蓝色蚀斑,经3次蚀斑纯化,得到重组杆状病毒rpBlue-HisH7HA1。Western-blotting和间接免疫荧光试验结果显示,HA1在昆虫细胞中得到表达,且表达产物具有抗原性。抗原特异性试验证明,重组HA1蛋白与鸡H5、H9亚型AIV抗血清不发生交叉反应。血凝试验证明,重组HA1蛋白具有良好的血凝性。  相似文献   

19.
A multiplex polymerase chain reaction (PCR) method using primer sets of G1/G2 and B64-I/B64-II was validated to detect pathogenic leptospira serovars from canine urine samples. The PCR method was found to be specific and sensitive with a detection limit of 100 cells of Leptospira icterohaemorrhagiae per milliliter of urine. The primer set previously designated and erroneously transcribed B64-I/B64-II amplified a DNA fragment of 352 base pairs from Leptospira grippotyphosa and Leptospira sejroe but not from Leptospira autumnalis, Leptospira bratislava, Leptospira canicola, Leptospira hardjo, Leptospira icterohaemorrhagiae, and Leptospira pomona. From 100 diagnostic canine urine samples, 5 were found positive for Leptospira grippotyphosalsejroe with a PCR product of 352 base pairs and 6 were positive for other pathogenic leptospira serovars with a PCR product of 285 base pairs. One 285-base pair product was sequenced and found to be 99.3% homologous to the G1/G2 PCR fragment sequence reported previously. All 352-base pair PCR products of clinical samples and pure cultures of L. grippotyphosa and L. sejroe were sequenced. The 352-base pair fragment sequences of L. grippotyphosa and L sejroe were identical. Only 2 base pairs were found different between the sequences from pure cultures and those from clinical samples. Serum samples from 3 positive cases that generated a PCR product of 352 base pairs were tested by the microscopic agglutination test, and 2 were found to be positive for L. grippotyphosa (1:10,240 and 1:5,120), 1 was positive for L. grippotyphosa (1:320) or L. icterohaemorrhagiae (1:320). The results of this study suggest that the multiplex PCR with the primer set G1/G2 and the erroneously transcribed B64-I/B64-II may be able to differentiate L. grippotyphosa or L. sejroe from other pathogenic leptospira serovars commonly tested for in Canadian diagnostic laboratories.  相似文献   

20.
小花碱茅HKT1;4基因片段的克隆与序列分析   总被引:1,自引:1,他引:0  
摘要:为研究小花碱茅(Puccinellia tenuiflora)拒Na+的分子机制,根据GenBank中已登录的植物HKT1;4基因保守序列设计一对简并引物,从小花碱茅幼根中提取总RNA,采用RT PCR方法扩增出HKT1;4基因片段并连接到pMD19 T Simple载体上,经亚克隆,PCR阳性检测后测序,得到一段长629 bp的序列。序列分析表明,该片段编码209个氨基酸,与GenBank中注册的高等植物HKT1;4基因核苷酸序列同源性在74%以上,与HKT1;4蛋白氨基酸序列同源性在60%以上,最后将其命名为PutHKT1;4。  相似文献   

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