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**mpappas** · 12-17-2012, 05:11 PM

Hi all

I have the very same problem with plant RNA. The 28s/18s ratio is no that high but I have consistently ratios of 3 to 4. Traces looks ok, even leaves samples(BR3-F), with chloroplast rRNA peaks don´t seem to be degraded, RIN values are ok. But I can´t understand the high 28s intensity.

Attached are traces from xylem (BR3-X) and leaves (BR3-F).

I hope to have some help form the experts.

Attached Files

bioanalyzer-BR3.ppt (623.5 KB, 85 views)

**pmiguel** · 12-18-2012, 04:35 AM

I would speculated that in some cases the nuclear (25S) rRNA is co-migrating with the large chloroplast (23S) rRNA. However, one would expect to see either both 18S (nuclear) and 16S (chloroplast) or a combination peak there as well. In some cases you do. But in other cases you don't.
--
Phillip

**mpappas** · 12-18-2012, 04:49 AM

Thanks for your answer, Philip

Do you have any experience with degradome sequencing? I´m afraid to use this RNA samples. I also tried to use Qiagen columns at the end of my CTAB/BME extraction but I got low 260/230 ratio and I´m afraid to lose important RNAs for degradome sequencing due to size exclusion. What do you think about it?

PS: Send the traces for samples extracted with qiagen columns.

Attached Files

bioanalyzer-BR3-qiagen.ppt (440.0 KB, 50 views)

**pmiguel** · 12-19-2012, 04:32 AM

Originally posted by mpappas View Post

Thanks for your answer, Philip

Do you have any experience with degradome sequencing? I´m afraid to use this RNA samples. I also tried to use Qiagen columns at the end of my CTAB/BME extraction but I got low 260/230 ratio and I´m afraid to lose important RNAs for degradome sequencing due to size exclusion. What do you think about it?

PS: Send the traces for samples extracted with qiagen columns.

Why do you think that a low 260/230 ratio is an issue? Please be specific -- what contaminating solute that absorbs at 230 nm will interfere with downstream steps?

--
Phillip

**mpappas** · 12-19-2012, 12:58 PM

I´m just trying to attend all the requirements the company that will prepare the degradome library and sequence it is asking. But, as I mentioned, I´m afraid of using the cloumn and exclude important cleaved RNA for degradome data. That´s why I prefer to use CTAB protocol with isopropanol precipitation. In this case, baseline seemed just a little higher but I think that all the DNA present can higly contribute to that.

Do you understand my point? Is it worth using the columns if I seem to loose lots of information and besides that I have a worse 260/230 ratio? I´m betting I shouldn´t use it.

Marília

**pmiguel** · 12-20-2012, 04:30 AM

Originally posted by mpappas View Post

I´m just trying to attend all the requirements the company that will prepare the degradome library and sequence it is asking. But, as I mentioned, I´m afraid of using the cloumn and exclude important cleaved RNA for degradome data. That´s why I prefer to use CTAB protocol with isopropanol precipitation. In this case, baseline seemed just a little higher but I think that all the DNA present can higly contribute to that.

Do you understand my point? Is it worth using the columns if I seem to loose lots of information and besides that I have a worse 260/230 ratio? I´m betting I shouldn´t use it.

Marília

You mean that you want sequence from very short RNA fragments in your sample? If so, most library construction protocols are not going to discard the shorter fragments anyway, using Ampure low-size cut-off purifications after various steps.

--
Phillip

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