1st BASE is using ABI PRISM 3730xl Genetic Analyzer developed by Applied Biosystems, USA.

Fragment sizing run times are 45 minutes with single base resolution up to 500 base pairs and 0.15 base pair standard deviation.

The promised size resolution is between the range of ≥75bp and ≤490 bp.
Please contact us separately if you have sample size > 500bp to be analysed using our Standard Fragment Analysis service.

You can indicate the DNA Size Standard to be used in the order form. Alternatively, we will select the DNA Size Standard based on your experiment setup. We provide the following size standard:

GS500-ROX (recommended for 3-dye multiplexing)
GS500-LIZ (recommended for 4-dye multiplexing)

Please enquire for other DNA Size Standards.

Please check the sizing precision first. After which, display your DNA size Standard peaks (up to sixteen different samples) in one display panel and align by size. All the peaks should overlap exactly. If it doesn’t, please redefine the size standards for those lanes that do not line up, and then re-check the sizing precision. Once the DNA Size Standard peaks superimpose exactly, then the sizing precision is correct, and the data can be considered reliable. At 1st BASE, we will perform this check before releasing the raw data to our customers.

Yes, each order will be attached with our control reaction using our control DNA and control labelled oligo, which is Blue (5' 6-FAM).

Only ONE primer of your PCR (either Forward or Reverse) needs to be labelled.

Please enquire if your dye combination is different from below:

Yes, you can. However, do ensure that the expected allele size ranges do not overlap, and be at least >10bp apart.

No, you do not need to purify your PCR product. Purification is only required when your samples contain high salts (usually from RE buffers used in TRFLP analysis) which will interfere with the electro-kinetic injection.

Yes, you can. For targets with a similar allele size range, please use different dyes. However, do ensure it is from the same filter set.

1. For new projects, please send in separate tubes and we will do the pooling for you.
2. For repeat projects, please ensure similar intensity of each dye before pooling all the different dyes together. Please send in 1 plate.

Note: 6-FAM, VIC and TET generate higher signals than NED or HEX. 
For (1) and (2), the extent of the spectral optimization is different but charges are the same as per dye.

The accuracy of sizing provided in our analysis is +/- 0.5 bp. We can achieve much higher level of accuracy and automation in sizing as size standard is included in every sample, unlike manual gels where size standard is loaded in only one lane of the gel.

Results are downloadable via an email with the password protected weblink. You can download the compressed file in .zip format (for Windows).
The run files were saved as *.fsa files, and the sizing tables are available in *.xls and *.txt files. You may open and analyze the *.fsa files with ABI freeware, Peak Scanner™ Software.

If you have requested the run report, it contains the analyzed electropherograms. They are presented in *.pdf files.

Applied Biosystems® has changed the matrix condition bounds of the spectral calibration kit for Filter F (catalogue number: 4345831). Please refer to:
http://www3.appliedbiosystems.com/cms/groups/mcb_marketing/documents/generaldocuments/cms_042198.pdf

Thus, please ensure that you are using the recommended amplification kits from Applied Biosystems® for Filter F. Else, you would need to provide us with the matrix calibration from your supplier to calibrate our machine separately.

Based on the user manual of GeneMapper® Software Version 4.0 for Microsatellite Analysis Getting Started Guide (page no. 24):

“Depending on the type of instrument, type of polymer and its primer, it may be appropriate to choose one of the other size standards that omit peaks. Specifically, the 35bp-peak can be eclipsed by the neighbouring primer peak, or the 250bp and 340bp peaks can migrate abnormally on the capillary electrophoresis instrument”.

For the fragment analysis done by 1st BASE, we set the size range from 50bp to 500bp and we omit the 35bp and 250bp peaks during the sizing analysis. As such, you would still be able to view the 250bp peak from the raw data without the size call. If you check the sizing precision according to what we described in Question no. 3 of this FAQ session, you will see the abnormal migration for this 250bp peak. For the 340bp peak, we found that it is still consistent along our runs and thus we did not omit this peak during our size call program.