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**mountainogre** · 08-01-2011, 06:51 AM

Hi Jh,
Did you make any progress solving this problem?
I have just observed the same thing and i don't know why.
Have you seen this blog post: http://dnasizing.com/?p=105

**zhaoj** · 08-01-2011, 07:23 AM

Not yet, but suspect
1. RNA leftover
2. inappropriate ratio of adaptor to DNA
Frustrated, but I do not see it everytime, hope there will be an answer.

Good luck with your experiment!

**CC_seqanswers** · 08-01-2011, 07:48 AM

May I ask what sizing technique in your case?

Originally posted by zhaoj View Post

Not yet, but suspect
1. RNA leftover
2. inappropriate ratio of adaptor to DNA
Frustrated, but I do not see it everytime, hope there will be an answer.

Good luck with your experiment!

**zhaoj** · 08-01-2011, 07:54 AM

I tried cutting out from agarose gel

**mountainogre** · 08-01-2011, 08:34 AM

And in my cases I size select with the e-Gel system. I aimed for the 180-200bp range.
My situation was similar to jH, in my experiment 2 from 8 libraries had the strange appearance of a stronger band around 260bp, whereas the Bioanalyzer showed appropriate 180bp band only for the other 6 samples.
I suspect some problem with over-amplification, since the two libraries with the extra band were the ones with the most DNA at the beginning of the protocol.

**zhaoj** · 08-01-2011, 09:03 AM

How much adaptor do you use in each reaction?
I use 1ul of 10 times diluted from Illumina.

**mountainogre** · 08-01-2011, 09:17 AM

I use the same. I should also mention that I am doing ChIPseq, not RNAseq, so things could be a little different.
I think I will repeat the prep with less starting material and see if that solves the problem.
In this case I used 13-15ng on ChIPPed DNA, I think i will try <10ng.

**pmiguel** · 08-01-2011, 10:04 AM

All,
I think the extra peaks phenomenon can derive from a number of different sources. I listed ones that occurred to me here:

Help with TruSeq gDNA library prep - SEQanswers

http://seqanswers.com/forums/showpost.php?p=45116&postcount=19

Bridged amplification & clustering followed by sequencing by synthesis. (Genome Analyzer / HiSeq / MiSeq)

One odd thing in this thread -- the idea that the slower migrating peak is the single stranded one seems contrary to my intuition. But, for Agilent chips I think it is the case. For details see:

Single stranded molecules run crazy slow on a DNA Agilent Chip - SEQanswers

http://seqanswers.com/forums/showthread.php?t=12852

Techniques and protocol discussions on sample preparation, library generation, methods and ideas

dsDNA migrates crazy fast on pico RNA chip - SEQanswers

http://seqanswers.com/forums/showthread.php?t=12501

Techniques and protocol discussions on sample preparation, library generation, methods and ideas

I am just wondering are there resources that state this? The fact that the link upthread is implying that this is the case, suggests there must be. But I had not heard it previously.

--
Phillip

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