Many reasons can cause this issue. For example, DNA from the same species but from different populations or individuals might be quite different. If the DNA is from a PCR product, mismatch errors during the amplification process should also be taken into consideration. We always guarantee the 100% correctness of sequencing results based on the received samples, but we cannot guarantee the identical sequences to the ones from the references.
Articles in this section
- Will the primers degrade at room temperature during transportation? Can we use dry ice for transporting to maintain stability?
- Why there is a difference between my sequencing data and the one from the references?
- Why the short PCR product is not suitable for direct sequencing?
- Why target gene products are seen in control sample with no template?
- Why my sequence results are reverse complement to the template DNA, while I demand a 5’ to 3’ orientation?
- Why is the TM value for primers of Genscript different from the TM value I obtained from other software?
- Why is the sequence of primers in the sequencing results different from the expected sequence?
- Why is my gene sequence different from the standard sequence?
- Why I got a sequencing result that was not I want?
- Why does the sequencing primer need to be site-specific on the DNA template?