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In addition to input RNA quality and accurate quantification, the clean-up and size selection steps are critical to generating a successful RNA-Seq library.
The ~ 70 bp or ~90 bp peak is likely standard or barcoded adapter dimers, respectively. Adapter dimers may form during the adapter ligation step and are usually removed during the size selection process. The adapter dimers will amplify on the Ion Torrent™ Ion Sphere™ particles during template preparation and decrease the overall throughput of usable sequencing reads; thus, we highly recommend removing the adapter dimers by performing an additional clean-up step prior to template preparation.
We recommend using the qPCR result, as quantification by qPCR is generally more accurate than quantification using the Bioanalyzer instrument.
No, the Ion Library Quantitation Kit for qPCR library quantification is unable to differentiate amplifiable primer-dimers from library fragments. We recommend assessing the library size distribution, including checking for the presence of adapter dimers, using the Bioanalyzer instrument. Libraries containing adapter dimers will have a sharp peak at ~70 bp for non-barcoded libraries or ~90 bp for barcoded libraries.
Make sure that you are using the recommended seals and compression pads (depending on the thermal cycler being used). If you are able to avoid it, we recommend against using Rows A and H (depending on the thermocycler, there can be more evaporation in these outer wells).
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