Tweet
Hi all,
I have recently made de novo assemblies for the transcriptome of a plant microspore. The microspore is transcriptionally silent, so there is no new input or RNA. Basically the microspore stores all the transcripts it will need for its development and fertilization.
It is believed that this set of stored RNA is transcribed from only a very small subset of genes. If this is the case, then calculating coverage against the genome would give quite bad results (I would image).
Can any one comment on the appropriateness of estimating the coverage generated by Mbases of reads vs. Mbases of assembled sequence?
Would this even be an acceptable/informative value?
Basically I have 2145 Mbases of sequenced reads, that were assembled into 3.5 Mbases of 'unigenes.' I feel like this implies that each unigene on average should have a very large coverage ~600X but I don't know if this is a good way to look at things, or if I am just tricking myself into thinking the sequencing came out well.
Does anyone else have any suggestions for another approach?
I have recently made de novo assemblies for the transcriptome of a plant microspore. The microspore is transcriptionally silent, so there is no new input or RNA. Basically the microspore stores all the transcripts it will need for its development and fertilization.
It is believed that this set of stored RNA is transcribed from only a very small subset of genes. If this is the case, then calculating coverage against the genome would give quite bad results (I would image).
Can any one comment on the appropriateness of estimating the coverage generated by Mbases of reads vs. Mbases of assembled sequence?
Would this even be an acceptable/informative value?
Basically I have 2145 Mbases of sequenced reads, that were assembled into 3.5 Mbases of 'unigenes.' I feel like this implies that each unigene on average should have a very large coverage ~600X but I don't know if this is a good way to look at things, or if I am just tricking myself into thinking the sequencing came out well.
Does anyone else have any suggestions for another approach?
Comment