Pyrosequencing

Quick Biochemistry Basics

29 Nov 201903:43

Summary

TLDRThis video explains the pyrosequencing technique, a method for DNA sequencing where the incorporation of nucleotides (dNTPs) into DNA is detected via light emission. The release of pyrophosphate during nucleotide addition is converted into ATP, which powers a luciferase enzyme to produce light. To determine which nucleotide is incorporated, the reaction is performed in a flow cell, introducing one dNTP at a time. The template DNA is immobilized on a bead, and multiple copies are made using PCR. Light detection allows for sequencing, and unused dNTPs are removed to ensure accuracy.

Takeaways

🔬 Pyrosequencing is a DNA sequencing technique where the incorporation of dNTPs is detected by the emission of light.
💡 When a nucleotide (dNTP) is added to the template DNA, pyrophosphate is released, which can be converted into ATP.
🧬 The ATP is then used by the enzyme luciferase to generate light, similar to the light produced by fireflies.
⚙️ Only one dNTP (A, T, G, or C) is added at a time during the sequencing process to determine which nucleotide is incorporated.
💻 The sequencing reaction takes place in a flow cell controlled by a computer, which monitors which dNTP is added.
🔗 The template DNA is immobilized on a bead to prevent it from being washed away during the flow cell process.
🧪 Multiple copies of the same template DNA are produced by PCR, increasing the intensity of the light signal for detection.
🚫 If no nucleotide is incorporated, no light is produced, which helps determine the DNA sequence.
🧹 Unused dNTPs in the flow cell are removed by an enzyme called apyrase.
🧫 Advanced pyrosequencing allows for the sequencing of multiple DNA templates in a single run using beads placed in a PicoTiter plate.

Q & A

What is pyrosequencing?
-Pyrosequencing is a DNA sequencing technique that detects the incorporation of dNTPs into DNA by observing light generated as a result of enzymatic reactions.
How is light generated in pyrosequencing?
-When a nucleotide is added to the template DNA, pyrophosphate is released, which is converted into ATP by ATP sulfurylase. The ATP is then used by the luciferase enzyme, which, along with oxygen and luciferin, generates light.
Why is the release of pyrophosphate important in pyrosequencing?
-The release of pyrophosphate is crucial because it initiates the enzymatic reaction that generates light, which is the signal used to detect whether a nucleotide has been incorporated.
How does pyrosequencing determine which nucleotide was added?
-Only one type of dNTP (A, T, G, or C) is added at a time in a controlled manner by a computer, and if the correct nucleotide is incorporated, light is generated. This helps determine which nucleotide was added.
What is the purpose of the flow cell in pyrosequencing?
-The flow cell allows the reagents to be added and flushed out, but to prevent the template DNA from being washed away, it is immobilized on a bead.
Why is the DNA template immobilized on a bead in pyrosequencing?
-The DNA template is immobilized on a bead to prevent it from being flushed out of the flow cell during the sequencing process.
What role does PCR play in pyrosequencing?
-PCR is used to generate multiple copies of the same DNA template, ensuring that enough pyrophosphate is released when a nucleotide is incorporated, resulting in a detectable light signal.
What happens if a dNTP is not incorporated during pyrosequencing?
-If a dNTP is not incorporated, no pyrophosphate is released, and therefore no light is generated. This lack of light indicates that the dNTP added was not complementary to the template DNA.
How is unused dNTP removed from the flow cell?
-Unused dNTP is removed by an enzyme called apyrase, which degrades the remaining dNTPs to prevent interference with subsequent cycles.
How does advanced pyrosequencing handle multiple DNA templates in one run?
-In advanced pyrosequencing, different DNA templates are immobilized on separate beads, which are placed in wells of a PicoTiter plate. Each well contains a single bead with many copies of the same DNA template, allowing multiple templates to be sequenced in a single run.