4.6 Article

Evaluation and Comparison of Genomic DNA Extraction Methods and PCR Optimization on Archival Formalin-Fixed and Paraffin-Embedded Tissues of Oral Squamous Cell Carcinoma

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DIAGNOSTICS
卷 12, 期 5, 页码 -

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MDPI
DOI: 10.3390/diagnostics12051219

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oral squamous cell carcinoma; formalin-fixed tissues; formalin-fixed paraffin-embedded tissues; deparaffinization; polymerase chain reaction

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The study compares different deparaffinization methods and DNA isolation techniques, and evaluates the effectiveness of different storing methods for archived OSCC samples in terms of DNA quantity, quality, and PCR amplification of the P53 gene. It finds that xylene deparaffinization and the conventional phenol-chloroform DNA isolation method are effective for obtaining suitable DNA, and samples fixed in formalin overnight and embedded in wax yield better quality and quantity DNA.
Recovery and amplification of nucleic acids from archived formalin-fixed tissue samples is the most developing field in retrospective genetic studies. We compared different deparaffinization methods and DNA isolation techniques, and intergroup comparisons were performed to evaluate the effectiveness of different storing methods for archival OSCC samples based on obtained mean DNA quantity, quality, and PCR amplification of the P53 gene. The study comprised 75 archival histologically diagnosed OSCC samples which were divided into Group I: Formalin-fixed paraffin-embedded tissue blocks and Group II: Long-term formalin-fixed tissue. A comparison of different deparaffinization methods showed that xylene deparaffinization is an efficient method to obtain suitable DNA. Comparing different DNA isolation techniques illustrated that the conventional phenol-chloroform method gives better integrity to DNA in contrast with the kit method. Comparison between FFPET and long-term FFT samples demonstrated that samples fixed in formalin overnight and embedded in wax yield better quality and quantity DNA in comparison with long-term samples fixed in formalin. To obtain suitable integrity of DNA, tissue samples should be stored by fixing in formalin overnight followed by preparation of paraffin tissue blocks, deparaffinization by xylene, and subjecting them to the conventional phenol-chloroform DNA isolation protocol.

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