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**amdic2** · 07-24-2014, 08:05 AM

Which kit for RRBS

Dear lyndaben,
Have you decided which kit you are going to use?
I am also currently looking at several options.
The protocol published by Boyle et al. (2012) Genome Biology appears quite easy to optimize. I am also interested by the NextFlex kit.
By the way, Boyle et al. mentionned to used the bisulfite conversion protocol for FFPE samples with ANY samples. It thus doesn't appear to be a problem?
Cheers,
Anne-Marie

**lyndaben** · 07-24-2014, 08:09 AM

I opted for the NuGEN Ovation kit. They provided me with a protocol addition for RRBS. It was just delivered this week so I have not had the chance to try it yet

**MasterSeq** · 03-04-2015, 10:41 AM

I know this is an old thread but this could be useful for somebody: NuGEN just launched a kit specifically for RRBS which should be much better than using their Methyl-Seq kit. It uses direct ligation from MspI digestion, only one bead purification and no need for phiX spike-in to deal with the lack of diversity coming from the MspI ends.

**lyndaben** · 03-13-2015, 06:59 AM

The new kit will be better hopefully. A note of caution to anyone using the old kit with the modified RRBS protocol: The first sequencing run we multiplexed with RNAseq samples and everything was great and the data looks good. This last time we multiplexed with PhiX (in 6 of 8 lanes) as recommended by NuGEN and we are having problems with the data (only 3-10M reads for the RRBS samples). On the same flow cell, two of the lanes were multiplexed with RNAseq and we got 30M reads for the RRBS samples, so we know it was not a sequencing problem or a library problem.

**chapmandu2** · 03-20-2015, 03:27 AM

Out of interest, has anyone tried the Methyl-Seq hybrid capture sequencing method from Agilent instead of RRBS?

**nucacidhunter** · 03-20-2015, 11:40 PM

This kit does not seem to be popular. I could not find any publication that have used it nor Agilent Techsupport was able to provide any reference. It would cost more than RRBS for the same coverage of target region, noting that target or covered regions are different between two methods.

**Genohub** · 03-24-2015, 07:23 PM

Methyl-DNA Sequencing

We've posted several different flavors of Methyl-DNA sequencing. Use the links at the end of the post to see the kits that NGS service providers on Genohub use.

- Genohub

**NuGEN** · 05-15-2015, 11:40 AM

Dedicated kit for RRBS from NuGEN

I wanted to comment that NuGEN has recently launched a dedicated kit for RRBS, the Ovation RRBS Methyl-Seq System - details can found here

http://www.nugen.com/nugen/index.cfm/products/ovation/ovation-rrbs-methyl-seq-system/

**Faria** · 09-29-2015, 05:57 AM

Originally posted by lyndaben View Post

I opted for the NuGEN Ovation kit. They provided me with a protocol addition for RRBS. It was just delivered this week so I have not had the chance to try it yet

Dear lyndaben,

How did your data turn out? Did you have any issues demultiplexing your samples? We recently used the kit. The libraries looked great but we are having issues with demultiplexing. Any advice/ tricks?

Thanks for your time

**lyndaben** · 09-29-2015, 06:32 AM

We used the NuGEN Ovation kit with great results when we multiplexed our samples with RNA-seq samples. When we multiplexed some RRBS libraries with PhiX we had problems with demultiplexing but when we re-sequenced the same samples and multiplexed with RNA-seq libraries we had no problems at all.

We are now making libraries from their new Ovation RRBS Methyl-seq kit. You do not need to multiplex with high quantities of complex libraries with this kit. Library construction is working great but we haven't sequenced any yet.

BTW, we had the same demultiplexing problem when we had some TrueMethyl-seq RRBS and oxRRBS libraries sequenced with PhiX and again no problem when the same libraries were re-sequenced with some RNA-seq libraries

**nucacidhunter** · 09-29-2015, 08:37 AM

Demultiplexing rate with new kit is low with or without PhiX. Undetermined folder reads have index but it seems to have various sequences. NuGEN should have seen this issue if they sequenced libraries according to their recommendation.

**Faria** · 09-29-2015, 08:56 AM

Would you mind sharing your % undertermined reads?

**nucacidhunter** · 09-29-2015, 09:00 AM

15-30% depending on lane. Multiplexing level does not seem to have any effect.

**lyndaben** · 09-29-2015, 09:00 AM

Faria, did you use the old kit or the new kit?

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