Custom TaqMan® Gene Expression Assay

Possible causes of no amplification when using Custom TaqMan Gene Expression Assays include (select one):

• You may not have performed bioinformatic validation of your sequences.
• If you performed bioinformatic validation correctly, you may have problems with reverse transcription.
• I used the correct reverse transcription method and kit.

This section applies to TaqMan® assay design and SYBR® Green assay design.

Custom TaqMan® Gene Expression Assay design is based on a template sequence provided by the customer. You can also design your own assays using other programs, and send the oligonucleotide sequences to Applied Biosystems for synthesis. You must perform bioinformatic evaluation of the sequences prior to submission to avoid PCR failure.

Read Bioinformatic Evaluation of a Sequence for Custom TaqMan® Gene Expression Assays to understand how to run a bioinformatics evaluation of a template sequence.

Bioinformatic evaluation allows you to accomplish three tasks:

1. Identify a unique sequence by using BLAST (basic local alignment search tool). If the sequence submitted is unique (or from a non-homologous region), the assay that is designed on this template only detects the transcript of interest.
2. Mask low complexity regions by using RepeatMasker. Low complexity regions, such as ALU sequences, are usually found within genomic DNA sequences. If you design your assay over these regions, the primers or probe will be depleted quickly if there is any genomic DNA in the samples.
3. Mask SNP sites in the sequence, so that primers and probes will not be designed over SNP sites.