鸡毒支原体 Taq Man实时荧光定量PCR检测方法的建立

为快速检测鸡毒支原体,根据鸡毒支原体的保守基因设计特异性引物和Taq Man探针,建立鸡毒支原体Taq Man实时荧光定量PCR方法并分析鸡毒支原体培养过程中颜色单位改变法(color change unit,CCU)和荧光定量PCR检测的相关性。结果显示,标准曲线y=-3.646x+44.208,相关系数R^(2)=0.998,最低检测限度为1 copy/μL;与其他菌株等均无交叉反应;组内和组间变异系数均小于3%,表明该方法具有良好的稳定性和可重复性。用建立的实时荧光定量PCR检测方法对26份临床样品进行检测,该方法较普通PCR方法检出率更高。建立的荧光定量PCR与CCU显示鸡毒支原体在对数生长期时,两者具有一定的对应关系。表明建立了鸡毒支原体Taq Man探针实时荧光定量PCR检测方法,可实现对鸡毒支原体的快速检测,为鸡毒支原体感染的防控提供技术基础。

不同品种辣椒营养品质、辣椒红素含量的差异比较及聚类分析

为了提高辣椒资源的利用,得到适合不同辣椒的加工方式,以64种新品种辣椒为实验材料,研究不同品种辣椒果实营养成分的差异,并利用超声波辅助法提取辣椒红素,将辣椒进行聚类分析。结果表明辣椒中富含Vc、脂肪、粗纤维等营养物质;相关性结果表明营养成分之间存在显著相关关系(P<0.05),其中Vc与水分、总糖呈极显著正相关关系(P<0.01),与灰分呈显著正相关关系(P<0.05),与粗纤维呈极显著负相关关系(P<0.01);通过单因素实验和正交实验,确定辣椒红素的最佳提取工艺为料液比1∶9、提取温度60℃、微波功率500 W、提取时间30 min,在此条件下辣椒红素的含量在30.24~562.29 mg/100 g之间。聚类分析结果显示,以营养品质为指标可将64种辣椒分成4类,以辣椒红素为指标可将其分成3类。

2019年滨州地区及周边规模化场牛支原体血清流行病学调查

[目的]为了了解山东省滨州地区及周边规模化牛场支原体流行的基本情况,[方法]对该区域14个规模化奶牛场和肉牛场进行了血清采集,采用牛支原体IgG抗体ELISA检测方法进行牛支原体血清抗体检测,并使用SPSS 20进行卡方统计学检验。[结果]山东省规模化牛场的牛支原体IgG抗体总阳性率为77.86%,奶牛场的阳性率为74.29%,肉牛场的阳性率为81.43%,奶牛场牛支原体IgG阳性率与肉牛场的统计学差异不显著(P>0.05);奶牛场不同场区,肉牛场不同场区之间,牛支原体的IgG阳性率差异显著(P<0.05)。[结论]山东省滨州地区及周边规模化牛场存在不同程度的牛支原体感染,牛支原体感染可能成为危害国内规模化奶牛场奶牛健康的主要疫病之一。

一株牛源副干酪乳杆菌的分离与鉴定

为了分离有研究价值的益生菌,从牛肠道中分离到1株疑似乳酸菌,通过对参考菌株的16S r RNA基因序列的归纳分析,证实存在种间特异性可变区,最终确定为副干酪乳杆菌,分离菌作为一种益生菌在饲料添加剂方面存在重要研究价值。

滑液囊支原体研究进展

滑液囊支原体感染病是严重危害养禽业的一种重要病原,近年该病在国内发病增多,对养禽业造成了一定程度的危害。论文就滑液囊支原体病的病原学、流行病学、致病机理、临床症状、诊断、综合防控措施等几个方面进行综述,并对其未来发展进行展望,以期为该病的临床诊断、病原学研究、疫苗开发和防治研究提供参考。

一种高稳定性钆类核磁共振成像造影剂的合成

合成了一种基于氮氧化二乙烯三胺五乙酸(DTPA)二异丙胺双酰胺的钆配合物,兼具高弛豫率和高稳定性。通过高分辨质谱、核磁谱图确认了氮氧化配体及对应的钆配合物的结构,并通过电位滴定法测得其配位稳定性常数。实验结果表明此配合物的水合常数为3,弛豫率(16.39mM^(-1)·s^(-1))达到商用造影剂的3倍,稳定性优于商用造影剂Gd-DTPA-BMA(Omniscan~)且表现出良好的成像效果以及优异的生物相容性,具有投入临床应用的巨大潜力。

Prokaryotic Expression of Gene Encoding Glutamate Dehydrogenase of Streptococcus suis Serotype 2 and Preparation of Polyclonal Antibodies against Its Expressed Products

[ Objective] To obtain detection antigen for diagnosis of Streptococcus suis infection. [ Method] The complete ORF of glutamate dehy- drogenase （GDH） gene was amplified from the genomic DNA of Streptococcus suis serotype 2 strain SC22 isolated in Sichuan Province by poly- merase chain reaction （PCR）. The resulting product was cloned into the prokaryotic expression vector pET-30a, which was then transformed into E. coil BL21 （DE3）. The identified positive transformants were screened for expression induced by IPTG. The expression products were subjected to SDS-PAGE and the recombinant protein was purified by nickel ion-agarose affinity chromatography. New Zealand rabbits were immunized with the purified recombinant GDH protein to prepare polyclonal antibodies. Titers of the anti-serum were determined by indirect ELISA and Western blot assay. [ Result] The recombinant GDH protein was effectively expressed in the host bacteria, and highly pure recombinant protein was obtained by nickel ion-agarose affinity chromatography. High-titer anti-serum against the recombinant protein was obtained. As evidenced by western blot as- say, the sera could react specifically with the lysates of all detected Streptococcus suis strains. In addition, the recombinant GDH protein could re- act specifically with serum samples collected from five pigs experimentally infected by strain SC22. [ Conclusion] The expressed GDH fusion protein has some common epitopes of natural GDH and can be used as detection antigen to develop ELISA and other diagnostic methods.