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1. cDNA sequence is clear.
2. gDNA (2.2kb) has 6 exons with a gap (~600bp) between the 4th and 6th exon on chromosome A.
3. The newly published genome data is different from the previous version. The whole gene is spliced: exon 6 is located onto another scaffold/chromosome while exon 4 is lost in the entire new-version. And I also see big rearrangement on the chromosome A.
4. We've got three different person working on this gene...no success yet.
5. What we got: I'm able to span the first 3 exons and 2 introns, as well as the last part of this gene (exon 6 and 3'UTR), but was never able to span the gap region... If anything showing on the gel, the band size corresponds to the amplicon using cDNA as template.....though I'm sure I'm using gDNA, and no RNA/cDNA contamination..
6. I tried different optimization strategies, none had work so far. (Tm, extension time, denature time, Mg conc, enzyme digestion, different polymerases, deaza-dGTP...)
I hope I could describe this problem more clearly.....sorry in advance ~~
My question is could that be a real trans-splice? gDNA from different chromosome, spliced together to make a real cDNA? OR, is that true there is no intron at all, although the sequence information from genome database shows there must be 1-2 introns..OR, this gene is in a very "fragile" region of a chromosome, which splits easily during DNA preparation?
And how to prove/disprove for each case?
I'm in desperate now..help me out ~~~
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