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I have designed targeted primers and amplified specific DNA fragments using the Smart-seq3 pipeline, resulting in FASTQ files. Since DNA lacks splicing events, I am wondering if it is possible to use zUMIs for processing these data to obtain BAM files for variant calling.
Here are some specific questions:
Can zUMIs stop the workflow before the counting step?
Is it possible to omit the GTF annotation file when using zUMIs? Since DNA-seq does not involve transcripts.
How can I modify the STAR aligner parameters within zUMIs to better suit DNA-seq data? I assume certain RNA-seq-specific options (like handling splice junctions) should be disabled.
The text was updated successfully, but these errors were encountered:
Hi,
I have designed targeted primers and amplified specific DNA fragments using the Smart-seq3 pipeline, resulting in FASTQ files. Since DNA lacks splicing events, I am wondering if it is possible to use zUMIs for processing these data to obtain BAM files for variant calling.
Here are some specific questions:
Can zUMIs stop the workflow before the counting step?
Is it possible to omit the GTF annotation file when using zUMIs? Since DNA-seq does not involve transcripts.
How can I modify the STAR aligner parameters within zUMIs to better suit DNA-seq data? I assume certain RNA-seq-specific options (like handling splice junctions) should be disabled.
The text was updated successfully, but these errors were encountered: