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**C.R.** · 09-24-2013, 04:55 AM

here is an example: http://www.zymoresearch.com/epigenet...ylated-dna-set

You probably used a 2% agarose gel to get a nice separation of the 100 bp ladder and the small fragments which you want to excise. Unfortunatley, under these conditions the pattern of the digest looks very similar to uncleaved DNA. Try a lower concentrated gel and you will see a better separation of the bigger fragments.

**DonDolowy** · 10-28-2013, 09:03 AM

Hey again, I have now tried several times to digest gDNA with MspI but I never get fragments in the low range (>500bp).
I have tried MspI enzyme from both NEB and Fermentas, which I have tested on commercial human and mouse DNA. Incubation time was 12 hours at 37C.

Since it is just a simple restriction digestion, what can possibly go wrong?

I have attached the bioanalyzer results (high sensitivity DNA chip).

Attached Files

Screen Shot 2013-10-28 at 5.38.07 PM.png (120.1 KB, 389 views)

**C.R.** · 10-28-2013, 09:13 AM

Hey, the digest just works so good, that I already omit to check it on a gel to safe DNA for some samples. I also used NEB and Fermentas and prepared Libaries with both. If you really want to see the smear after digest: take 500ng to 1 µg DNA and incubate at 37C. 2 hours are already enough. Important: put the digested DNA on a 0.7 to 1 percent agarose gel. Do not use the Bioanalyzer CHIP here. If this does not help: can you cut the DNA with other enzymes? Do you really have pure DNA?

**DonDolowy** · 10-28-2013, 09:19 AM

Hi C.R, thanks for the quick reply. The DNA I am working on now is completely pure, since it is commercial DNA bought only for optimization to exclude potential problems with impure DNA.
I have also tried to load on a 0.5% gel and I get kind of a smear, but when I continue with the Biooscientific RRBS-seq protocol and do size-selection (300-500bp) using beads, I end up with nothing.
To eliminate rookie mistakes when handling the beads, I asked our sequencing facility to test the protocol, since they are very experienced in library prep for all kind of applications. They as well failed, so it suggests that there really is no small bands.

What is the reason for not using bioanalyzer chips for this purpose? Maybe because the undigested gDNA is taking up such a huge fraction that the chip won't show the small amount of fragmented DNA there might is?

Thanks a lot!

**C.R.** · 10-28-2013, 09:29 AM

Yes, I was also very confused when I looked at my first digest on a 2 percent gel, since I thought that it did not work. Basically what I saw was an accumulation of long fragments which made me think that the digest did not work. I am still doing the traditional gel-excise method, but I think that in principle the bead based method also should work.

**DonDolowy** · 10-29-2013, 07:38 AM

I now performed another MspI digestion on commercial available mouse gDNA.

2ug DNA
5uL Cutsmart buffer
1.5uL MspI enzyme
------
Total volume 50uL. 37C, 2hours.

Followed by cleanup using phenol/chloroform/isoamyl alcohol and EtOH precipitation.

I then loaded 1ug on a 0.7% gel, ran 90min @ 100V. The ladder is Fermentas 100bp ladder.

To me there is basically no fragments in the desired range 200-400bp.

I would very much appreciate your inputs!

Attached Files

MspI_2hrs_1ug_gDNA.png (36.0 KB, 397 views)

**C.R.** · 10-29-2013, 08:08 AM

I am not too sure about your image, because the undigested control is missing. In fact I think, that you can see a smear of fragments on your gel picture.

Please have a look at the attached image. MspI was included to the samples on the left side. The right side is the same DNA without any treatment as control. You can clearly see that the enzyme was active and created a smear of fragments ranging from very long fragments to very short ones. Next you see that there is no real enrichment of small fragments visible in this resolution.

Attached Files

MspI_digested_DNA.jpg (71.8 KB, 415 views)

**DonDolowy** · 10-29-2013, 10:50 PM

That gel looks great. Far from what I am getting!
How do you extract your DNA? And are you also using MspI from NEB?

**C.R.** · 10-30-2013, 12:50 AM

Yes it is from NEB. For the gel I used 3µg DNA, 5µl buffer 4, 2µl MspI in a total volume of 50µl. 1/3 of the digest was directly used for the gel without phenol-extraction. The gel is 0.7% Agarose in TAE and the ladder is the GeneRuler DNA Ladder Mix (100-10000). I just realized that I am still using an old stock of the enzyme with buffer 4 instead of the new CutSmart version. I doubt that the buffer system change evokes a big difference. But maybe it is worth to ask NEB if this might explain your results.

**DonDolowy** · 10-30-2013, 08:40 AM

Finally, it seems like it is working now!

Using a heat block or water bath instead of thermo cycler seems to do the trick. Incredible

No big changes between Fermentas and NEB's MspI enzyme.

Attached Files

MspI_2hrs_1ug_gDNA_Heatblock.png (89.4 KB, 408 views)

**rosatoc** · 06-24-2014, 11:44 AM

Very interesting... We are trying the PstI/MspI double digest, and as we are not getting any library that we can detect (due to humongous adapter dimers) we are trying a number of optimizing experiments. Perhaps the waterbath/heat block could be another variable we can use. Thanks for posting

**JeremyDay** · 06-24-2014, 02:42 PM

Hi rosatoc,

We struggled with RRBS for a couple of months. The input was DNA from 64-cell embryos, so ~200pg. Eventually we ended up using Nugen's ultra-low Ovation kit. We never saw the digestion, but DID see traces after library prep that resembled Nugen's trace @ 200pg. If I remember correctly we only needed 7-8 cycles of amp, in comparison to above 25 in previous attempts. We were observing what looked like adapter concatemers (evenly spaced ladder, unlike MSPI traces), which were verified by sequencing. 99% adapter dimers! Anyhow, we had a couple of small issues with the indexes and sequencing quality, but the library prep was much better. They have a proprietary blunt-end ligation chemistry, but somehow improves efficiency. It's expensive, but they were very generous on a trial kit.

**Castrolsc** · 05-18-2018, 10:16 AM

Doubts about MspI digestion

Hi all!

I'm having the same situation described before. I'm trying to use the Premium RRBS kit (Diagenode) to analyze bovine DNA samples and it seems the restriction enzyme from the kit is not working well for my DNA (sperm DNA in the picture). I got gDNA from fish testes from another lab which worked for this kit before, and the digestion looks fine.
I'm doing the incubation in water bath (as suggested here before), 37°C overnight, and following the kit instructions (100 ng of DNA in 26 uL of water, 1 uL of restriction enzyme and 3 uL of the buffer).
The person who gave me this gDNA recommended to do a clean-up DNA with beads and elute the DNA in water, so I did that for both DNAs, so it should not be a problem related to the sample buffer.
Any suggestions? I tried to look in the literature some profile of bovine DNA digested with MspI but I couldn't find anything, so I don't know what expect.

Attached Files

MspI digestion.jpg (68.4 KB, 329 views)

**JeremyDay** · 05-18-2018, 11:24 AM

I hope you mean 100ng of DNA

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MspI digestion - how is it supposed to look?

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