Sanger Sequencing of DNA

Andrey K

17 Feb 201516:06

Summary

TLDRThe Sanger DNA sequencing method is a powerful technique used to determine the sequence of nucleotides in a DNA molecule. It involves the use of dideoxynucleoside triphosphates (ddNTPs), which halt DNA replication at specific points. The process includes DNA denaturation, primer binding, DNA replication with ddNTPs, and gel electrophoresis to separate fragments by size. The sequence is then read by analyzing the band patterns from the gel, allowing researchers to determine the exact order of bases in the DNA strand. This method is fundamental for gene expression studies and protein analysis.

Takeaways

😀 DNA sequencing is essential in biochemistry to determine the sequence of nucleotides in a DNA molecule, which helps understand gene expression and protein production.
😀 The Sanger DNA sequencing method involves using a modified nucleotide, ddNTP, to terminate DNA replication at specific points, helping to determine the DNA sequence.
😀 A key molecule in the Sanger method is ddNTP, which lacks a 3' hydroxyl group, preventing further nucleotide addition and thus stopping DNA replication.
😀 In DNA replication, the presence of a hydroxy group at the 3' carbon of a nucleotide is necessary for forming a phosphodiester bond; ddNTP lacks this group, halting the process.
😀 The first step in Sanger sequencing is denaturing the double-stranded DNA using sodium hydroxide to separate the strands.
😀 After denaturation, a primer complementary to the DNA sequence is added to initiate replication, and DNA polymerase builds the new strand.
😀 The Sanger method uses a mixture of normal dNTPs and a small amount (about 1%) of a single ddNTP type to selectively stop replication at specific nucleotides.
😀 The DNA polymerase synthesizes fragments of varying lengths depending on which nucleotide (normal or ddNTP) is incorporated during replication.
😀 Gel electrophoresis is used to separate the DNA fragments by size, with smaller fragments moving further down the gel, allowing visualization of the sequence.
😀 By reading the positions of the bands in the gel (from bottom to top), the sequence of the original DNA strand can be determined, starting with the primer sequence.
😀 The four ddNTPs (ddATP, ddGTP, ddCTP, ddTTP) are used in separate reactions, each targeting one base (A, G, C, or T) to stop replication at specific points.
😀 The process involves radioactive labeling of the primer, which allows detection of the fragments during gel electrophoresis and helps map the DNA sequence.

Q & A

What is the main goal of DNA sequencing in biochemistry?
-The main goal of DNA sequencing is to determine the sequence of nucleotides in a DNA molecule, which helps understand gene expression and the types of proteins produced.
What is the Sanger DNA sequencing method?
-The Sanger DNA sequencing method is a technique used to sequence DNA by incorporating dideoxynucleoside triphosphates (ddNTPs) to terminate DNA replication at specific points, allowing the sequence to be determined.
What is the role of dideoxynucleoside triphosphates (ddNTPs) in Sanger sequencing?
-ddNTPs play a critical role in stopping the DNA replication process. They lack a hydroxyl group at the 3' carbon, preventing the formation of a phosphodiester bond and halting chain elongation.
How do ddNTPs differ from normal deoxynucleoside triphosphates (dNTPs)?
-ddNTPs differ from normal dNTPs by having no hydroxyl group at the 3' carbon position of the sugar, which is necessary for continuing the DNA chain. This lack of a 3'-OH group stops the polymerase from adding further nucleotides.
What are the steps involved in Sanger DNA sequencing?
-The steps involved in Sanger DNA sequencing include: 1) DNA denaturation to separate strands, 2) DNA replication with a primer, polymerase, dNTPs, and ddNTPs, 3) Chain termination and fragment formation, 4) Gel electrophoresis to separate fragments by size, and 5) Sequence determination through band analysis.
Why is gel electrophoresis used in Sanger sequencing?
-Gel electrophoresis is used to separate DNA fragments based on their size. Smaller fragments travel further through the gel, while larger ones move more slowly. This allows the fragments to be visualized and the DNA sequence to be determined.
What is the purpose of using a radioactive DNA primer in Sanger sequencing?
-The radioactive DNA primer is used to label the starting point of the DNA sequence, allowing scientists to track the fragments produced during sequencing by visualizing them under a radioactively sensitive detector.
How are the different ddNTPs (A, G, C, T) used in Sanger sequencing?
-Each ddNTP (ddATP, ddGTP, ddCTP, ddTTP) is used in a separate reaction. These ddNTPs terminate the chain at their respective base (A, G, C, or T) when incorporated into the growing DNA strand, creating fragments that can be analyzed to determine the sequence.
How do scientists reconstruct the DNA sequence from the gel electrophoresis bands?
-The sequence is reconstructed by analyzing the positions of the bands on the gel. The smallest fragments correspond to the first nucleotide after the primer, and bands are read from bottom to top to determine the full DNA sequence.
What happens when ddNTPs are incorporated into the growing DNA chain?
-When a ddNTP is incorporated into the growing DNA chain, it causes termination of the replication process because it lacks the necessary 3'-OH group required for forming the next phosphodiester bond. This results in the formation of a DNA fragment that ends at that specific base.