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Development of an ammonium sulfate DNA extraction method for obtaining amplifiable DNA in a small number of cells and its application to clinical specimens. | LitMetric

Development of an ammonium sulfate DNA extraction method for obtaining amplifiable DNA in a small number of cells and its application to clinical specimens.

Biomed Res Int

Department of Animal Biotechnology, College of Animal Bioscience and Technology, Konkuk University, Gwangjin-gu, Seoul, Republic of Korea.

Published: December 2013

AI Article Synopsis

  • DNA extraction from microdissected cells is crucial for molecular pathology, especially when dealing with clinical specimens with few cells.
  • A new ammonium sulfate DNA extraction method (Method A) was developed and compared to two existing methods (B and C), proving to deliver superior DNA yield and quality.
  • Method A successfully amplified key genetic markers and mutations in limited cell samples, demonstrating its effectiveness in extracting amplifiable DNA from low-cell-number specimens.

Article Abstract

DNA extraction from microdissected cells has become essential for handling clinical specimens with advances in molecular pathology. Conventional methods have limitations for extracting amplifiable DNA from specimens containing a small number of cells. We developed an ammonium sulfate DNA extraction method (A) and compared it with two other methods (B and C). DNA quality and quantity, β-globin amplification, and detectability of two cancer associated gene mutations were evaluated. Method A showed the best DNA yield, particularly when the cell number was very low. Amplification of the β-globin gene using DNA from the SNU 790 cell line and papillary thyroid carcinoma (PTC) cells extracted with Method A demonstrated the strongest band. BRAF(V600E) mutation analysis using ethanol-fixed PTC cells from a patient demonstrated both a "T" peak increase and an adjacent "A" peak decrease when 25 and 50 cells were extracted, whereas mutant peaks were too low to be analyzed using the other two methods. EGFR mutation analysis using formalin-fixed paraffin-embedded lung cancer tissues demonstrated a mutant peak with Method A, whereas the mutant peak was undetectable with Methods B or C. Method A yielded the best DNA quantity and quality with outstanding efficiency, particularly when paucicellular specimens were used.

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Source
http://www.ncbi.nlm.nih.gov/pmc/articles/PMC3652119PMC
http://dx.doi.org/10.1155/2013/546727DOI Listing

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