I've just started constructing 5500 Mate Paired libraries, the first few worked well but lately I have been unable to generate any library even though the trial PCR shows a band at 300bp. Has anyone else had this problem or any ideas? Thank you.
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Yes, I was told by a ABI FAS that the beads are inhibitory. One work around might be to denature the steptavidin and recover the library molecules in the absence of the beads. See:Originally posted by SeqAA View Postincrease the number of cycles for fullscale amplification. For some reason the trial PCR seems to work better. I almost always have to add a few more cycles to the full scale PCR. Maybe something with the beads inhibits PCR?
Electrophoresis 2005, 26, 501–510, Anders Holmberg, Anna Blomstergren, Olof Nord, Morten Lukacs, Joakim Lundeberg, Mathias Uhlén, The biotin-streptavidin interaction can be reversiblybroken using water at elevated temperatures.
for details.
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Phillip
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Final PCR Troubleshooting
Hi clissold,
How many cycles did you do your final amplification for? Typically you don't have to do that many cycles to get slighty more than a faint band with your remaining 26 uL of beads to do a lot of sequencing. I haven't had any problems with final amplifications as long as the trial PCR went well (easily identifiable bands for at least the 14 cycle trial PCR with low input, and a faint or strong band for the 10 cycle trial PCR depending on DNA input quantities). Did you see decent bands both at 10 and 14 cycles of trial PCR?
As long as you didn't forget the 20 minute/72 Celsius nick translation step for the final amplification (a new change in the 5500 protocol), and you used the same amplification mix and primers as you did for your successful trial PCR reactions, the results for the final amplification shouldn't be any different. However, the bead mass (26 uL of beads versus 4 uL of beads) for the final amplification is much greater for the final amp versus the trial PCR, so make sure you pulse vortex at full speed right before the final PCR, and do not pulse centrifuge to the point of bead pelleting. You can examine the PCR tube bottom before you put it into the thermocycler for the final amplification to see if any pelleting of beads occured during pulse centrifugation.
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Yes, that is strange.
Either the P1-T and P2-T adapters are not 5' phosphorylated which would be bizarre (the "T" overhands should prevent their ligating), or the insert is not 5' phosphorylated prior to adapter ligation?
The insert results from and earlier nick translation of circularized DNA followed by treatment with BstT7 nuclease and S1 nuclease. So the 5' end of the insert is generated by S1. S1 should remove 5' mononucleotides in single stranded regions, so I would expect the 5' phosphate to remain attached to insert.
I guess the 5' insert phosphate might be removed during dA tailing somehow?
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Phillip
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by GATTACATLove this - good data definitely starts from good input, and poor input can only give relatively poor data. I particularly like the mention of Nanodrop/absorbance based methods for quantification. It's such a toss up if you'll get an accurate reading or what amounts to a randomly generated number, and a lot of library/sequencing related issues can be traced back to poor quant.
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by SEQadmin2
I’m not a sequencing expert. I’m a purification scientist who uses NGS to evaluate workflows my group develops. With this perspective, we think about the sample first and the NGS workflow second. The sequencer is an exceptionally honest reporter, but it can only report on what you give it, so whether you get clean, interpretable data from an NGS workflow is largely determined before you begin.
Here are nine questions we think about, in roughly the order they matter, before...-
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