Hi Alexis,

Typically, we choose whether to use bowtie 1 or 2 depending on the read length of the library. As ChIP-Seq libraries are often sequenced using relatively short reads (around 50bp or less), bowtie 1 is probably more suitable for alignment.

The --best parameter isn't really applicable in bowtie2 because it handles alignments differently to bowtie1. The defaults in bowtie2 are pretty sensible, so if your results look correct then you're probably fine.

Phil

Great.
Thanks for your answer tallphil.
I feel better that I'm not delivering results that are completely false.

I've been using bowtie2 simply because 2 sounds better, and bowtie2 can handle compressed FASTQ files directly.

My reads are paired end 50 bases. The documentation on the bowtie2 website is a bit ambiguous since they recommend bowtie2 for reads longer than 50 bases, and say that bowtie1 may or may not be better for reads shorter than 50 bases. I may be a bit picky but they don't say anything about reads exactly 50 bases long.

I should probably switch to bowtie1 for my 50 bases long paired end ChIP-Seq, since it seems to be much more widely used that bowtie2.

It would be interesting to do a comparison of the 2 programs on 50 bases paired end ChIP-Seq, but since the programs are constantly being updated the comparison would have to be repeated for each update.