Originally posted by dagmar
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Maybe the system Pippin Prep gives you another solution:
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yeah, the PAGE is very effective for that sizes (although more time consume); I did it with my small RNA libraries and apparently I get rid off all the adapter-adapter artifacts.
Maybe the system Pippin Prep gives you another solution:
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Ah... that would be a problem. For getting separation resolution like that, the beads and even an agarose gel wouldn't be that great. You might want to try PAGE or, if you have the money, the Caliper XT.Originally posted by dagmar View Post
The Caliper is capable of some very tight size separation.Leave a comment:
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Thanks.Originally posted by pbluescript View Post
I was just wondering if someone would have a little bit more percised answer.
My problem is that my fragments of interest range from 150bp up to 400bp and I need to get rid of the 120-130bp fragments. They are just so close. I tried a 1.8 :1 ratio and was successful once but starting out with less DNA I could not reporduce that.Leave a comment:
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some suggestion on gel purification
Hi, just one comment.Originally posted by pbluescript View Post
I do think the gel purification will help, if the inserted DNA size is big enough (above 100bp). And instead of using agarose gel, you can try use PAGE gel, which give you better separation. And you can just break the PAGE gel into smaller pieces and do the PCR.Leave a comment:
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Read post 16 in this thread.Originally posted by dagmar View PostLeave a comment:
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Hi everyone,
last month I used the Truseq kit for RNAseq by Illumina and it worked like a charm. Previously I had to do 2-3 gel purifications in the end, but with this kit and the AMPpure beads I got a really clean picture in the end, with no adapter dimers or anything. I am new to all this, but these beads seem to do a very good job. Here is a picture of my libraries, before size selection. The sequencing worked fine and I got ~60M reads and ~92% of them were mappable to the mm9 so I guess that I got rid of most of the dimers.Leave a comment:
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Can you give us any good advice which ratio of Ampure beads and sample one should use in oder to get rid of 120-130 bp fragments.Originally posted by Simone78 View Post
As far as I understood the more beads you use the more bigger fragments
you capture so the ratio shold be < 1.8 : 1 correct?
Thanks!Leave a comment:
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I don't usually do a PCR cleanup but if I do I just use the Qiagen PCR cleanup but this is usually just to reduce the volume so I can load everything into 1 well.Originally posted by dagmar View PostLeave a comment:
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Hello JHU-ChIPmaniac,
I am thinking about using the E-gel as well.
I have one question to the E-gel following amplification.
What kind of PCR purification do you do before running the gel cassette?
Or have you made the experience that their is no step in between needed?
Thanks!!!Leave a comment:
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I also use the E-gel 2% size select gels following amplification. This gets rid of all the adaptor species in the libraries. I typically have plenty of library for sequencing.Leave a comment:
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I was interested in the double size selection and I found this paper:Originally posted by pbluescript View Post
unfortunately, beside the batch-to-batch variability, I was never able to get a 100% pure fraction. I always had some degree of "contamination" from shorter or longer fragments (visible at Bionalyzer, I never run them on a regular agarose gel). Therefore I chose the E-gels and I am very happy with that.Leave a comment:
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At 120bp, it is almost certainly adapter-adapter ligations. They will be sequenced by the machine and you will probably end up with lots of identical reads that match the adapter sequence.Originally posted by odile View PostHello everyone,
I made libraries that I sent to some lab for sequencing and also got tons of these artefacts/adaptor dimers. My problem is that I work with very degraded DNA so my library is around 150bp...too close to get rid of the 130bp artefact. Does anyone knows the sequence of the artefact? Are the dimers truly form the adaptors or could they come from P1.1 and P2.1?
I'm at loss.
Best,
OdileLeave a comment:
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Hello everyone,
I made libraries that I sent to some lab for sequencing and also got tons of these artefacts/adaptor dimers. My problem is that I work with very degraded DNA so my library is around 150bp...too close to get rid of the 130bp artefact. Does anyone knows the sequence of the artefact? Are the dimers truly form the adaptors or could they come from P1.1 and P2.1?
I'm at loss.
Best,
OdileLeave a comment:
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