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**DNADEB** · 03-09-2011, 08:52 AM

We worked with FAS and it started working again. Even working one on one at the same time, the FAS and tech could never spot any differences! Many Many controls were run including tubes, slides, reagents, water etc. Talked to another lab with this problem as well --haven't heard back.
So we are in business again!

**pmiguel** · 03-11-2011, 06:33 AM

Okay thanks for your reply.
Our FAS replaced our deposition kit and now everything seems back to normal for us as well.

--
Phillip

**niceday** · 03-11-2011, 07:14 AM

This is something to do with the 3 prime modification. The enzyme might be faulty. Before you even get to the bead deposition stage you should look at the beads and they should clump together. After doing the terminal transferase reaction check for clumpiness. You can't miss it. If the beads don't appear clumpy you have a problem.

This should save you wasting time and beads.

**pmiguel** · 03-11-2011, 07:54 AM

Probably, yes. Although sometimes we have problems with beads being too clumpy--as that can interfere with deposition also.

BTW, any idea what the basis of the binding of the beads to the slide is? During training in Foster City the trainers went all inscrutable when asked. So I presume they are using someones IP with promise of keeping it secret. Irritating though.

Terminal transferase just takes a double stranded end and adds a bunch of bases to it--from dNTPs, I presume. Why would that cause beads to "clump" anyway? Physical tangling, or something else?

--
Phillip

**niceday** · 03-11-2011, 08:03 AM

So with the beads being too clumpy. I have used the new protocol of splitting the E80 beads in two, 3 lots of declump 1, combine and 3 lots of declump 3.

We have worked out that the best deposition, ie best quality QV is off 240K per panel. We have got a few slides with 270K per panel but the QV values are low.

I setting up some experiments of the same library, beads but with a 240K depo and a 170K depo. We will then know the difference. We suspect the lower density give higher QV. Sorry we know this but we need to show the experiment with no other variables to get the point across.

Strangely quads and octs don't have any depo problem. This is due to the lower bead density.

AB don't acknowledge this but I don't care. We continue on regardless.

**pmiguel** · 03-11-2011, 08:21 AM

Very interesting.

We basically gave up trying to get above ~210K/panel--not because the QVs were lower, but because nothing we did seemed to get us there. For our current run we deposited 1 billion beads and the result is just under 500 million usable beads total (208K/panel). We tried depositing more, but then we were seeing lots of slides breaking--no idea why, but it doesn't take too many occurrences of losing a run 10 days in to dim the appetite for experimentation.

--
Phillip

**ngs-user** · 03-29-2011, 08:02 AM

Originally posted by niceday View Post

Strangely quads and octs don't have any depo problem. This is due to the lower bead density.

AB don't acknowledge this but I don't care. We continue on regardless.

This phenomenon has been acknowledged (i.e. the higher bead:volume ratio for E80 causes a greater degree of clumping)! - this is why the modified protocol for E80 scale was written!

**niceday** · 03-29-2011, 08:05 AM

Officially?

**ngs-user** · 03-29-2011, 08:12 AM

Did they give you a modified protocol?

**niceday** · 03-29-2011, 08:15 AM

not directly. We now have one and it works better. Still not close to 300K per panel. We know what the problem is. An official explanation would be useful and some indiciation that the problem will have been solved before the 5500 hit the shelves.

**ngs-user** · 03-29-2011, 08:26 AM

That's odd - our FAS gave us an official recommendation a few months ago...

**pmiguel** · 03-30-2011, 10:47 AM

Is your FAS named Merlin, perchance? I mean, if he is living backwards through time that could explain how he had access to a protocol not released to the rest of us.

Seriously, though, we get modified protocols of one sort or another all the time. Hard to know exactly what is being discussed here. What differences were there in the new protocol?

--
Phillip

**DNADEB** · 04-08-2011, 07:20 AM

It turns out that the REAL reason ours failed has to do with the CONTROL! When the FAS came to work at our site with our tech and new reagents etc, everything worked. These were our samples. However, later we came to find out it is actually the CONTROL DNA that they supply that does not work. The tech used it when she was starting to use the EZ Bead system and the manual suggested starting with their Control DNA.
WELL.....................

**SeqAA** · 04-08-2011, 08:17 AM

The Control DNA would still not explain beads coming off the slide.

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