I'm afraid that this is incorrect.

First 'fr' does not mean 'forward read'. What it means is the the two reads are arranged in the FR (Foward/Reverse) as opposed to the RF (Reverse/Forward) orientation. FR means that the read pairs are oriented with the 3' end point toward each other when aligned to the reference and RF means they are pointing away from each other.

Firststrand means that read #1 matches the first strand of cDNA generated during conversion of the single stranded mRNA to ds-cDNA. In other words the R1 is the reverse complement of the mRNA. Note that all of these reference landmarks are relative to transcript, not the genome. For Illumina strand specific, paired end mRNA-Seq reads the orientation of the reads relative to their original RNA is:

Looks like Jim Robinson had it backwards for the color legends. Actually

red=positive,
blue=negative

He has clarified here:

I always thought that blue=positive and red=negative. See screen shots of my data in IGV.

I used Illumina dUTP-type stranded library prep and fr-firststrand with Tophat2. I find several places that say dUTP libraries should use fr-firststrand with Tophat, for example: http://onetipperday.sterding.com/201...pe-to-use.html


Is anyone able to clear this up?

Thanks

Tablet has a "read concordance" mode for viewing strand direction on reads. Both pairs of reads that are consistent with a mapped direction following the reference sequence are coloured green (customisable), and reads that are consistent with the reverse complement of the reference sequence are coloured red.