Understanding the order of nucleotides in DNA is essential
for exploring genetics, diagnosing diseases, and developing targeted therapies.
Two classic methods for generating DNA fragments of different lengths have laid
the foundation for today’s advanced sequencing technologies.
Two Pioneering DNA Sequencing
Techniques
1. Sanger’s Chain Termination Method
Developed by Frederick Sanger, this technique uses specially modified
nucleotides called dideoxyribonucleotide triphosphates (ddNTPs). These
molecules terminate DNA synthesis at specific bases, producing fragments of
varying lengths that each end at a known base. This allows researchers to piece
together the DNA sequence by analyzing where the synthesis stops.
2. Maxam-Gilbert Chemical Cleavage Method
In this method, DNA strands are chemically treated to cleave at specific bases.
The resulting fragments of different lengths help determine the sequence by
identifying where the cuts occur. Though effective, this method has largely
been replaced by safer, more efficient techniques like Sanger sequencing.
How DNA Sequencing Works
To decode a DNA sequence, scientists first create four
separate reaction mixtures. Each contains a modified form of DNA polymerase and
is designed to randomly terminate DNA strand synthesis at one of the four
bases—adenine (A), thymine (T), cytosine (C), or guanine (G). This process
generates many fragments of different lengths, each ending at a specific base.
These fragments are then separated using gel
electrophoresis, a technique that sorts DNA fragments based on size. By
analyzing the order of the fragments, researchers can accurately determine the
sequence of the DNA strand from one end to the other.
Automation and High-Throughput
Sequencing
As the demand for DNA sequencing has skyrocketed, so has the
need for automation. Modern DNA sequencing is now fully automated, with robotic
systems performing every step—from mixing reagents to running and reading the
sequencing gel.
Today’s sequencing protocols often use fluorescently
labeled chain-terminating nucleotides, each tagged with a unique color.
This allows all four reactions to be carried out in a single tube and separated
in just one gel lane. A laser-based detector reads the color of each
fluorescent tag as DNA fragments pass by, translating the colors into
nucleotide sequences.
Advanced computers then compile and store the data, enabling
researchers to analyze entire genomes in record time.
Key Takeaways
- Sanger
sequencing uses ddNTPs to stop DNA synthesis
and generate readable fragment patterns.
- Maxam-Gilbert
sequencing relies on chemical cleavage of
DNA but is less commonly used today.
- Gel
electrophoresis helps visualize DNA fragments by
separating them based on size.
- Automation
and fluorescent labeling have revolutionized DNA sequencing, making
it faster, more accurate, and highly scalable.
- Modern
sequencers can process large volumes of DNA,
providing critical insights in research, medicine, and biotechnology.
This evolution in DNA sequencing has not only accelerated
genetic research but has also opened doors to breakthroughs in personalized
medicine, evolutionary biology, and synthetic biology.
No comments:
Post a Comment