PCR-based evaluation of sequence specificity of DNA fragmentation by ultrasound
- Authors: Chemeris A.V.1, Garafutdinov R.R.1, Galimova A.A.1, Sakhabutdinova A.R.1
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Affiliations:
- Institute of Biochemistry and Genetics of Ufa Science Center of Russian Academy of Sciences
- Issue: Vol 50, No 2 (2016)
- Pages: 236-241
- Section: Genomics. Transcriptomics
- URL: https://journal-vniispk.ru/0026-8933/article/view/162578
- DOI: https://doi.org/10.1134/S0026893316020059
- ID: 162578
Cite item
Abstract
Ultrasonic fragmentation, which is a simple and convenient method for the mechanical degradation of DNA, is widely used in modern genome studies as one of the sample preparation steps. It has been recently found that the DNA breaks occur more often in the regions containing 5'-CG-3' dinucleotides. We studied the influence of the 5'-CG-3' dinucleotides on the efficiency of the 28S rRNA gene amplification during PCR with sonicated DNA of Mantis religiosa. It was shown that the amplification rate depends on the template length and the number of 5'-CG-3' dinucleotides. Amplification of the DNA regions with a higher 5'-CG-3' density is less efficient because of their higher sensitivity to ultrasound. The amount of the amplified DNA templates is inversely proportional to the 5'-CG-3'number.
About the authors
A. V. Chemeris
Institute of Biochemistry and Genetics of Ufa Science Center of Russian Academy of Sciences
Email: garafutdinovr@gmail.com
Russian Federation, Ufa, 450054
R. R. Garafutdinov
Institute of Biochemistry and Genetics of Ufa Science Center of Russian Academy of Sciences
Author for correspondence.
Email: garafutdinovr@gmail.com
Russian Federation, Ufa, 450054
A. A. Galimova
Institute of Biochemistry and Genetics of Ufa Science Center of Russian Academy of Sciences
Email: garafutdinovr@gmail.com
Russian Federation, Ufa, 450054
A. R. Sakhabutdinova
Institute of Biochemistry and Genetics of Ufa Science Center of Russian Academy of Sciences
Email: garafutdinovr@gmail.com
Russian Federation, Ufa, 450054
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