Regardless of the number of samples, they can be submitted either in individual tubes or 96-well plates. Please follow these easy steps to prepare and submit your samples:
The total amount of DNA template needed for sequencing depends on the type of DNA (PCR, plasmid, cosmid or BAC) and the size of fragment to be sequenced. If you send pre-mixed DNAs with primers, we recommend that you use at least 50 ng, but no more than 1000 ng for plasmids in the size range 3-30 kbp per tube or well. The optimal amount is 100-250 ng/reaction. For PCR fragments, regardless of the size, use 5 to 500 ng per tube/well. The optimum amount is 25 ng/reaction. Using less or significantly more of the template will result in sub-optimal or even no data.
For cosmids (typically ~ 40 kbp) or BACs (typically 100-150 kbp), use minimally 1000 ng of DNA per tube/well. Adjust the amount accordingly, if multiple reactions are required.
Insert Size (Kbp) | # of Seq Reactions (minimum) | ng of Plasmid DNA (minimum/optimal) | ng of PCR Fragment (minimum/optimal) |
---|---|---|---|
0.2 - 0.8 | 2 | 100/500 | 10/50 |
0.8 - 1.6 | 4 | 200/1000 | 20/100 |
1.6 - 2.4 | 6 | 300/1500 | 30/150 |
2.4 - 3.2 | 8 | 400/2000 | 40/200 |
3.2 - 4.0 | 10 | 500/2500 | 50/250 |
4.0 - 4.8 | 12 | 600/3000 | 60/300 |
4.8 - 5.6 | 14 | 700/3500 | 70/350 |
5.6 - 6.4 | 16 | 800/4000 | 80/400 |
6.4 - 7.2 | 18 | 900/4500 | 90/450 |
We strongly recommend that your templates be re-suspended in 10 mM Tris, pH 7-8. Please remember that EDTA (as for example in TE buffer = 10 mM Tris, 1 mM EDTA, pH 8) interferes with sequencing, although a low amount, 0.1 mM or less, is tolerated. These conditions assure that your templates are stable for a long time under most storage conditions. Templates stored in water deteriorate within a few weeks, which may pose problems, if additional sequencing on the same sample is required in the future. We appreciate that you advise us on the type of storage solution you use, particularly if your samples are in water or if the buffer contains EDTA.
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