Hello

I greatly thank you to all of you in this website.

I downloaded four of samples from PRJNA606815( https://www.ncbi.nlm.nih.gov/Traces/study/?acc=SRP249907&o=acc_s%3Aa ), using fasterq-dump.

The data are single-cell rna seq with 3' chemistry 10x genomics but I have one fastq file per sample.

I expected some fastq files per sample but failed.

Does anyone know how to handle it in this situation?

If you go to the Data access tab of the SRA entries for these samples you can find the original BAM files submitted: https://trace.ncbi.nlm.nih.gov/Traces/index.html?view=run_browser&acc=SRR11106929&display=data-access

Use bamtofastq (LINK) utility provided by 10x to re-create the correct R1,R2,I1 files.