- Pyrosequencing
Pyrosequencing is a method of
DNA sequencing (determining the order ofnucleotides in DNA) based on the "sequencing by synthesis" principle. The technique was developed byMostafa Ronaghi andPål Nyrén at theRoyal Institute of Technology in Stockholm in the 1990s.] [cite journal|author=Ronaghi et al.|title=Real-time DNA sequencing using detection of pyrophosphate release| journal=Analytical Biochemistry|date=1996 |volume=242 |page=84-89 |pmid=8923969|pages=84|doi=10.1006/abio.1996.0432] [cite journal|author=Nyrén, P. |title=The History of Pyrosequencing|journal=Methods Mol Biology |date=2007|volume=373| pmid=17185753|pages=1–14]Procedure
"Sequencing by synthesis" involves taking a single strand of the DNA to be sequenced and then synthesizing its complementary strand enzymatically. The Pyrosequencing method is based on detecting the activity of
DNA polymerase (a DNA synthesizing enzyme) with anotherchemiluminescent enzyme . Essentially, the method allows sequencing of a single strand ofDNA by synthesizing the complementary strand along it, one base pair at a time, and detecting which base was actually added at each step. The template DNA is immobilized, and solutions of A, C, G, and Tnucleotides are added and removed after the reaction, sequentially. Light is produced only when the nucleotide solution complements the first unpaired base of the template. The sequence of solutions which produce chemiluminescent signals allows the determination of the sequence of the template.ssDNA template is hybridized to a sequencingprimer and incubated with the enzymesDNA polymerase ,ATP sulfurylase ,luciferase andapyrase , and with the substratesadenosine 5´ phosphosulfate (APS) andluciferin .
# The addition of one of the fourdeoxynucleotide triphosphate s (dNTP s)(in the case of dATP we add dATPαS which is not a substrate for a luciferase) initiates the second step. DNA polymerase incorporates the correct, complementary dNTPs onto the template. This incorporation releasespyrophosphate (PPi) stoichiometrically.
# ATP sulfurylase quantitatively converts PPi to ATP in the presence of adenosine 5´ phosphosulfate. This ATP acts as fuel to the luciferase-mediated conversion of luciferin to oxyluciferin that generates visible light in amounts that are proportional to the amount of ATP. The light produced in the luciferase-catalyzed reaction is detected by a camera and analyzed in a program.
# Unincorporated nucleotides and ATP are degraded by the apyrase, and the reaction can restart with another nucleotide.Currently, a limitation of the method is that the lengths of individual reads of DNA sequence are in the neighborhood of 300-500 nucleotides, shorter than the 800-1000 obtainable with chain termination methods (e.g. Sanger sequencing). This can make the process of
genome assembly more difficult, particularly for sequence containing a large amount ofrepetitive DNA . As of 2007, pyrosequencing is most commonly used for resequencing or sequencing of genomes for which the sequence of a close relative is already available.The templates for pyrosequencing can be made both by solid phase template preparation (Streptavidin coated magnetic beads) and enzymatic template preparation (Apyrase+Exonuclease).
Licensing
Pyrosequencing AB in Uppsala. Sweden, was started to commercialize the machine and reagent for sequencing of short stretches of DNA. Pyrosequencing AB was renamed to Biotage in 2003. Pyrosequencing technology was further licensed to
454 Life Sciences . 454 developed an array-based Pyrosequencing which has emerged as a rapid platform for large-scale DNA sequencing. Most notable are the applications for genome sequencing and metagenomics. "GS FLX", the latest pyrosequencing platform by 454 Life Sciences (owned by Roche), can generate 100 million nucleotide data in a 7 hour run with a single machine. It is anticipated that the throughput would increase by 5-10 fold with the next release. Each run would cost about 5,000-6,000 USD, pushing de novo sequencing of mammalian genomes into the million dollar range.Use in research
In September 2007, 454 pyrosequencing was used in a study implicating
Israel acute paralysis virus in honeybeeColony Collapse Disorder [ [http://www.washingtonpost.com/wp-dyn/content/article/2007/09/06/AR2007090601471.html?tid=informbox AP, Virus May Be Cause of Honeybees' Deaths. The Washington Post, September 6th, 2007.] ] .External links and references
* http://www.454.com
*cite journal| author=Ronaghi M. |url=http://www.genome.org/cgi/content/full/11/1/3 |title=Pyrosequencing sheds light on DNA sequencing|journal=
Genome Research |date=2001 Jan|volume=11 |pmid=11156611|pages=3–11 |doi=10.1101/gr.11.1.3
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References
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