nobody knows ?

it will help me a lot.

Thanks

You can try clipRead program at our deepBase database ( http://deepbase.sysu.edu.cn/ ), which were developed to discover small and long ncRNAs from deep-sequencing data.

you can download clipRead program at http://deepbase.sysu.edu.cn/clipRead/. More detailed information, please see the readme file ( http://deepbase.sysu.edu.cn/clipRead/readme.txt ).

See
http://seqanswers.com/forums/showthread.php?t=198&highlight=sticky


It should be a sticky but doesn't "stick" to the top

thanks, I found the adapter I expect

3'RNA adapter : UCGUAUGCCGUCUUCUGCUUGU

In my fastq file, I've got about 19M reads. When I sort the reads on the number of occurences, I found that the sequence with the most important occurence is :

adapter

TCGTATGCCGTCTTCTGCTTGTAAAAAAAAAAAAAA (I remplace U by T)

and the next sequence in the list are similar (It seems that one mismatch appears in the 3! part of the reads )

I found some other reads with high occurence like that :

adapter in green and a mismatch in the adapter seq in red

TCGTATGCCGTCTTCTGCTTGTAAAAAAAAAAAAAA

and even ( just a part of the adapter is present, the N represent an non-readable nucleotide )

AGTACAGTCTCGTATGCCGTCTNNNNNNNNN

the last example appears even with mismatches.

what is the best method to trim this adapter ?

Thanks

hellö, I have the same problem now, then how did you deal with finally?