lecture_notes:04-01-2011
Differences
This shows you the differences between two versions of the page.
| Both sides previous revision Previous revision Next revision | Previous revision | ||
|
lecture_notes:04-01-2011 [2011/04/02 18:49] eyliaw |
lecture_notes:04-01-2011 [2011/04/03 19:28] (current) eyliaw |
||
|---|---|---|---|
| Line 6: | Line 6: | ||
| * Instruments: SAGE, Caliper | * Instruments: SAGE, Caliper | ||
| ===== Sequencing Technologies ===== | ===== Sequencing Technologies ===== | ||
| - | * Sequencing by synthesis (454 and Illumina) vs sequencing by ligation (SOLiD) | + | ==== Sequencing by synthesis (454 and Illumina) ==== |
| - | * Pyrosequencing (454) | + | * Synthesis limits sequencing 5' to 3' |
| - | * Paired tag (Illumina and SOLiD) | + | * |
| + | ==== Sequencing by ligation (SOLiD) ==== | ||
| + | * | ||
| + | ==== Pyrosequencing (454) ==== | ||
| + | * | ||
| + | ==== Paired tag (Illumina and SOLiD) ==== | ||
| + | * | ||
| + | ==== In-house ==== | ||
| + | * Nader's lab uses a method that starts by fragmenting the DNA into long fragments (aiming for ~10k). They attach a unique barcode primer to each fragment and do circular ligation, much like SOLiD. This is followed by circular replication, primer binding, and random cleavage to obtain fragments of different lengths [(cite:circular_rep>http://en.wikipedia.org/wiki/Rolling_circle_replication)]. They sequence both ends of each fragment on the Illumina, obtaining a paired read with its 10k fragment's barcode. | ||
lecture_notes/04-01-2011.1301770187.txt.gz · Last modified: 2011/04/02 18:49 by eyliaw
Except where otherwise noted, content on this wiki is licensed under the following license: CC Attribution-Noncommercial-Share Alike 3.0 Unported
