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Universal direct PCR amplification system: a time- and cost-effective tool for high-throughput applications

机译:通用直接PCR扩增系统:适用于高通量应用的节省时间和成本的工具

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摘要

Taking into account the limits of current genotyping methodologies, we have established a versatile direct PCR method on intact microtissue samples without prior DNA isolation. A simple and standard protocol was developed and validated on a wide range of living organisms including bacterial and fungal strains, plant species and human samples. This allows reliable amplification of target genomic DNA fragment directly from source material using minimal amount of tissue which makes DNA purification irrelevant for a number of biological applications. The direct PCR technique established here represents an excellent alternative to traditional amplification methods used for real-time detection. Since this approach was efficiently and universally applied for high-throughput molecular screening, its implementation will offer new insights for several investigations in human health, biomedical diagnosis, plant biotechnology, as well as in applied environmental and food microbiology.
机译:考虑到当前基因分型方法的局限性,我们已经建立了一种完整的直接PCR方法,无需预先进行DNA分离即可对完整的微组织样品进行检测。开发了一种简单而标准的方案,并已在包括细菌和真菌菌株,植物物种和人类样品在内的多种生物中进行了验证。这允许使用最少的组织直接从源材料可靠地扩增靶基因组DNA片段,这使得DNA纯化与许多生物学应用无关。此处建立的直接PCR技术代表了用于实时检测的传统扩增方法的绝佳替代品。由于这种方法已有效且普遍地用于高通量分子筛查,因此其实施将为人类健康,生物医学诊断,植物生物技术以及应用环境和食品微生物学领域的多项研究提供新的见识。

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