2007-2008 a lot more advanced biotechnology tools (part 1) sequencing
TRANSCRIPT
2007-2008
A Lot More Advanced Biotechnology Tools(Part 1)
Sequencing
• Sanger method– determine the base sequence of DNA– based on replication– dideoxynucleotides• ddATP, ddGTP, ddTTP, ddCTP• missing O for bonding of next
nucleotide• terminates the growing chain
DNA Sequencing
DNA Sequencing• Sanger method– synthesize
complementary DNA strand in vitro
– in each tube:• “normal” N-bases• dideoxy N-bases
– ddA, ddC, ddG, ddT
• DNA polymerase• primer• buffers & salt
2
1
3
42
Reading the sequence• Load gel with sequences from ddA, ddT,
ddC, ddG in separate lanes– read lanes manually & carefully– polyacrylamide gel
Fred Sanger 1978 | 1980
This was his 2nd Nobel Prize!!– 1st was in 1958 for the structure of
insulin
Advancements to sequencing• Fluorescent tagging– no more radioactivity– all 4 bases in 1 lane• each base a different color
• Automated reading
Advancements to sequencing• Fluorescent tagging sequence data• Computer read & analyzed
Applied Biosystems, Inc (ABI) built an industry on these machines
Advancements to sequencing Capillary tube electrophoresis
no more pouring gels higher capacity & faster
384 lanes
PUBLIC Joint Genome Institute
(DOE) MIT Washington University of St.
Louis Baylor College of Medicine Sanger Center (UK)PRIVATE Celera Genomics
Big labs! economy of scale
Automated Sequencing machines Really BIG labs!
Human Genome Project• U.S government project– begun in 1990
• estimated to be a 15 year project– DOE & NIH
• initiated by Jim Watson• led by Francis Collins
– goal was to sequence entire human genome• 3 billion base pairs
• Celera Genomics– Craig Venter challenged gov’t – would do it faster, cheaper– private company
Different approaches
3. Assemble DNA sequence using overlapping sequences.
“map-based method”gov’t method
“shotgun method”Craig Venter’s method
1. Cut DNA entire chromosome into small fragments and clone.
2. Sequence each segment & arrange based on overlapping nucleotide sequences.
1. Cut DNA segment into fragments, arrange based on overlapping nucleotide sequences, and clone fragments.
2. Cut and clone into smaller fragments.