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首页> 外文期刊>Journal of Virological Methods >QUANTITATION OF FELINE IMMUNODEFICIENCY PROVIRUSES IN DOUBLY INFECTED CATS USING COMPETITIVE PCR AND A FLUORESCENCE-BASED RFLP
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QUANTITATION OF FELINE IMMUNODEFICIENCY PROVIRUSES IN DOUBLY INFECTED CATS USING COMPETITIVE PCR AND A FLUORESCENCE-BASED RFLP

机译:使用竞争性PCR和荧光的RFLP定量双层感染猫的猫直接免疫缺陷潜水术

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A nested polymerase chain reaction assay, which amplifies a region of the gag gene, was developed for the direct detection of feline immunodeficiency virus (FIV) DNA sequences in the blood of infected cats. This method detects as few as ten copies of a plasmid containing the whole genome of the FIV-Pet isolate on agarose gel. To distinguish two FIV isolates in double infected cats: we devised an RFLP analysis on PCR amplified products exploiting sequence differences in the gag gene of the two strains. To quantitate the two strains, a fluorescent inner-sense primer was used in the second amplification step. Amplicons were subsequently digested, heat-denatured and loaded on a polyacrylamide gel in an automated DNA sequencer. The proportion of the two isolates was determined using the laser-excited fluorescence of labelled strain specific fragments. These data were used to extrapolate the numbers of proviral genomes from the total viral load as estimated by using a competitive PCR assay, These sensitive and specific assays complement virological detection of FIV and enable superinfection studies to be evaluated; a prerequisite for the testing of live attenuated immunodeficiency virus vaccines.
机译:嵌套的聚合酶链反应测定,其扩增GAG基因的区域,用于直接检测感染猫的血液中的猫免疫缺陷病毒(FIV)DNA序列。该方法检测到含有琼脂糖凝胶上的FIV-PET分离物的全部基因组的质粒的10份。将两只FIV分离物区分开进行双重感染的猫:我们设计了对PCR扩增产物的RFLP分析,其利用两种菌株的GAG基因的序列差异。为了定量两种菌株,在第二扩增步骤中使用荧光内部感觉引物。随后消化,在自动DNA测序仪中消化并在聚丙烯酰胺凝胶上被消化,热变性和装载。使用标记的应变特异性碎片的激光激发荧光测定两种分离株的比例。这些数据用于从总病毒载量来推断出通过使用竞争性PCR测定的总病毒载量,这些敏感和具体的测定补体检测FIV的补体检测并实现待评估的超蛋白研究;实时减毒免疫缺陷病毒疫苗测试的先决条件。

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