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通过聚合酶链反应(PCR)结合熔解曲线分析对绵羊朊病毒蛋白基因(PRNP)变体进行基因分型。

Genotyping of ovine prion protein gene (PRNP) variants by PCR with melting curve analysis.

作者信息

Schütz Ekkehard, Scharfenstein Melanie, Brenig Bertram

机构信息

Institute of Veterinary Medicine, Georg-August-University, Burckhardtweg 2, 37077 Göttingen, Germany.

出版信息

Clin Chem. 2006 Jul;52(7):1426-9. doi: 10.1373/clinchem.2006.069666. Epub 2006 May 11.

DOI:10.1373/clinchem.2006.069666
PMID:16690731
Abstract

BACKGROUND

Scrapie is the transmissible spongiform encephalopathy in sheep. Because genetic variants of the ovine PrP gene (PRNP) can be associated with disease risk, the European Union initiated programs to eradicate high-risk PRNP genotypes from sheep livestock. For this purpose, reliable and cost-effective genotyping is needed.

METHODS

We amplified DNA to cover the 3 risk codons in exon 3 encoding amino acids 136, 154, and 171. Amplicons were mixed with dye-labeled probe sets, and melting curves were recorded in a LightCycler by use of color and temperature multiplexing. Probe design was based on thermodynamic calculations to ensure unequivocal results for the 3 codons of interest, taking the additional F141 and T137 sequence variants into account.

RESULTS

The fluorescence resonance energy transfer (FRET) method, when compared with sequencing, gave exactly the predicted melting temperatures for all possible genotypes. When we validated the method with samples from official certification programs, it showed completely matching results. Turnaround time was approximately 5 h after receipt of a whole-blood sample. The method detected the rare sequence variants T137 and F141, which were clearly distinguishable from the other known genotypes by melting curve analysis. One scrapie sheep was ARR/ARR, which is considered the haplotype with the lowest risk.

CONCLUSIONS

The FRET-based PRNP genotyping method for sheep is rapid and can differentiate all genotypes at each locus in 1 capillary. The assay is fast and has lower costs than restriction fragment length polymorphism analysis or sequencing.

摘要

背景

羊瘙痒病是绵羊的传染性海绵状脑病。由于绵羊朊蛋白基因(PRNP)的遗传变异可能与疾病风险相关,欧盟启动了从绵羊家畜中根除高风险PRNP基因型的计划。为此,需要可靠且经济高效的基因分型方法。

方法

我们扩增DNA以覆盖编码氨基酸136、154和171的外显子3中的3个风险密码子。将扩增子与染料标记的探针组混合,并在LightCycler中通过颜色和温度多重分析记录熔解曲线。探针设计基于热力学计算,以确保对3个感兴趣的密码子能得到明确的结果,同时考虑到额外的F141和T137序列变异。

结果

与测序相比,荧光共振能量转移(FRET)方法对所有可能的基因型都给出了准确预测的熔解温度。当我们用官方认证计划的样本验证该方法时,结果完全匹配。收到全血样本后周转时间约为5小时。该方法检测到了罕见的序列变异T137和F141,通过熔解曲线分析可将它们与其他已知基因型清楚地区分开。一只患羊瘙痒病的绵羊为ARR/ARR,这被认为是风险最低的单倍型。

结论

基于FRET的绵羊PRNP基因分型方法快速,能在1根毛细管中区分每个位点的所有基因型。该检测方法速度快,且成本低于限制性片段长度多态性分析或测序。

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