Hello, I planned to explore diverse T cell receptor transcripts using long-read sequencing. So I transfected TCR mini gene into cells and got sequencing data.

I mapped my data to genome reference and visualize it via IGV. But I couldn't see any transcripts from TCR plasmid on the chromosome 7 where T cell receptor locus is.

How can I detect reads from transfected plasmid? Shall I make custom reference file using plasmid map?

Or should I use any specific ways to detect TCR transcripts like IGMT, MiXCR, IgBLAST and so on?

I just want to see the diversity of splicing patterns using tools like FLAIR.

I need your advice! Thank you.

Hi, as you said, you could add the sequence of your minigene to your reference fasta. After uploading it to IGV, there will be a new option in the chromosome select field to view reads mapping on the mini-gene.

Maybe you have artificial subsequences in your minigene, which makes it different from the original locus.

Since the TCR locus is rearranged (compared to the genome in other cells) in mature receptor genes you should use a specialized software to reconstruct the CDR3 region and rearrangement.

You can use MiXCR for that. We have recently added support for long-read data also.

If you can give more details on the sequencing platform and library structure I can help you with running MiXCR.

Feel free to ask us on github: https://github.com/milaboratory/mixcr

or e-mail:

support@milaboratories.com

In general it shouldn't be hard, e.g.:

mixcr analyze generic-tcr-amplicon \
--species mmu \
--rna \
--rigid-left-alignment-boundary \
--floating-right-alignment-boundary C \
  input_R1.fastq.gz \
  input_R2.fastq.gz \
  result

But certain library structures (or long reads sequencing platform) might need some tweaks. You can also check our new documentation portal: https://docs.milaboratories.com/