From d0911a04958a04042da02a334ccc528dae79cc17 Mon Sep 17 00:00:00 2001
From: zsloan
Date: Fri, 27 Mar 2015 20:28:51 +0000
Subject: Removed everything from 'web' directory except genofiles and renamed
the directory to 'genotype_files'
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PowerPoint Presentation - Complex trait analysis, develop-ment, and
genomics
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Hars2 probe level analysis: 16 PMs
mapped
SNP
C in B6, T in D2
no SNPs
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LetŐs look at Hars2 in
more detail by mapping all of the perfect match probes (16 of them) that
target this transcript.
Go back to the Trait
Data and Editing window and select Chr 2 (rather than ALL as shown above)
and also select PM Probes. Then click on Interval Mapping button.
You will get the
illustration above, but without the sequence data that we have added.The 16 perfect match probes are
arranged in sequence (red is 5 prime, blue is the 3 prime end). For example,
the 5 prime-most primer 307387 has the sequence CACTG..... It also has a
polymorphism at the 17 nucleotide of this 25 nt probe sequence.
How do we know that the
5 prime probe is polymorphic? By looking up the sequence in the Celera
Genomics databases which often contqains sequence data for C57BL/6J (B6
above) and for DBA/2J.But two
blue probes (14 and 15) do NOT contain SNPs but still have very large LRS
scores. The other probes do not perform so wel. Highly variable probe
performance is probably a result of the very different stacking energies of
DNA-RNA duplexes.