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The Sanger sequencing Genetic Analyzer method relies on the incorporation of chain-terminating dideoxynucleotides (ddNTPs) during DNA synthesis. These ddNTPs lack the 3'-OH group necessary for further DNA chain elongation, effectively terminating the DNA strand at specific positions. The DNA is first divided into multiple identical fragments, and each fragment is subjected to DNA synthesis with normal nucleotides (dNTPs) and a small amount of one of the four ddNTPs labeled with different fluorophores. As a result, the DNA synthesis reaction produces a set of fragments of varying lengths, each terminating with a specific ddNTP. The fragments are then separated by capillary electrophoresis, allowing for the determination of the DNA sequence based on the fluorescent signals emitted by the different labeled ddNTPs.
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