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**doxologist** · 02-24-2009, 02:03 PM

are you willing to amplify?

we also work with samples with low RNA but go through one or two rounds of amplifications.

**neethav** · 05-24-2010, 08:18 AM

Which kit do you use for mRNA amplification?

**james hadfield** · 05-26-2010, 11:51 PM

Have you looked at Nugens Ovation kit (http://www.nugeninc.com/nugen/index....-seq-system/)?
Looks good but we have not tried it yet.

**krobison** · 05-27-2010, 09:00 AM

A few papers have done SOLiD sequencing from a single cell: Cell Stem Cell. 2010 May 7;6(5):468-78, J Biomol Tech. 2009 Dec;20(5):266-71, Nat Protoc. 2010;5(3):516-35. Epub 2010 Feb 25, Nat Methods. 2009 May;6(5):377-82. Epub 2009 Apr 6.

**kainsteven** · 06-10-2010, 08:26 AM

Users of Ovation RNA-Seq

We have had several users generate good results using low input amounts of total RNA with the Ovation RNA-Seq System. If you are interested, we have several customer posters and webinars from recent conferences on the NuGEN website: http://www.nugeninc.com/nugen/index....en-sequencing/

Also note that today we announced our Encore NGS Library Systems which integrate directly with the RNA-Seq protocol, or can be used to construct libraries for any NGS application.

Best,
Steve

**paul z** · 06-10-2010, 10:12 AM

Illumina is said to have started with as low a 1 ng total RNA.
Internally, I have started with as low as 10 ng total RNA.

I don't think the problem is obtaining sequencing material (that's pretty easy) -- I think the problem is, how accurate of a representation what it is that ends up being sequenced is of its origin, whether starting with 1 ng, 10 ug, or using the Ovation System. Unfortunately, the received determination of this is typically through correlation coefficients, which are inappropriate as measures of agreement, but agreement (and not association) is what I take as intended to assess when we compare the efficaciousness of starting with 1 ng vs 10 ug, e.g.

**wenhuang** · 06-15-2010, 06:49 AM

I have used messageAmp from Ambion for amplification and was able to get sequencing to work, sort of...

One problem I have is reads are severely biased towards the 3'end. So recovery of full length transcript is very difficult.

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