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首页> 外文期刊>International Journal of Clinical and Experimental Pathology >Improved PCR amplification for molecular analysis using DNA from long-term preserved formalin-fixed, paraffin-embedded lung cancer tissue specimens
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Improved PCR amplification for molecular analysis using DNA from long-term preserved formalin-fixed, paraffin-embedded lung cancer tissue specimens

机译:使用长期保存的福尔马林固定,石蜡包埋的肺癌组织标本中的DNA进行分子分析的改进的PCR扩增

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Archival tissue specimens are valuable resources of materials for molecular biological analyses in retrospective studies, especially for rare diseases or those associated with exposure to uncommon environmental events. Although successful amplification with PCR is essential for analysis of DNA extracted from archival formalin-fixed, paraffin-embedded (FFPE) tissue specimens, we have often encountered problems with poor PCR amplification of target fragments. To overcome this, we examined whether heat treatment in alkaline solution could efficiently restore the PCR template activity of DNA that had already been extracted from FFPE lung cancer tissue specimens. The effect of the heat treatment was assessed by PCR for the emTP53/em gene and other lung cancer-related gene loci. The heat treatment of DNA samples in borate buffer resulted in successful PCR amplification of DNA fragments ranging from 91 to 152 bp. This technique for restoration of template activity of DNA for PCR amplification is very simple and economical, and requires no special apparatus, so it may be applicable for molecular analysis of DNA samples from FFPE tissue specimens at various laboratories.
机译:档案组织标本是进行回顾性研究(尤其是罕见疾病或与罕见环境事件相关的疾病)进行分子生物学分析的宝贵材料资源。尽管成功进行PCR扩增对于分析从福尔马林固定档案,石蜡包埋(FFPE)组织样本中提取的DNA至关重要,但我们经常遇到目标片段PCR扩增不良的问题。为了克服这个问题,我们检查了在碱性溶液中进行热处理是否可以有效地恢复已经从FFPE肺癌组织标本中提取的DNA的PCR模板活性。通过PCR评估 TP53 基因和其他肺癌相关基因位点的热处理效果。在硼酸盐缓冲液中对DNA样品进行热处理导致成功地PCR扩增了91至152 bp的DNA片段。该用于PCR扩增的DNA的模板活性的恢复技术非常简单且经济,并且不需要特殊的设备,因此其可适用于在各种实验室中对来自FFPE组织样品的DNA样品进行分子分析。

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