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Thanks for developing this wonderful tool! I am now using it to convert the possorted_genome_bam.bam generated by Cellranger to the fastq. I am not sure if it is paired end, should I sorted the bam file before running bamto fastq? As I have used the unsorted bam file to generate fastq, and then used the fastq file for scvelo. The scvelo show that there are about 300000 duplicated cells out of 400000 cell in total, I am not sure if it is because of the barcodes in the fastq files? Could you kindly give me some guidance?
Thanks a lot
Boyu
The text was updated successfully, but these errors were encountered:
Hi,
Thanks for developing this wonderful tool! I am now using it to convert the possorted_genome_bam.bam generated by Cellranger to the fastq. I am not sure if it is paired end, should I sorted the bam file before running bamto fastq? As I have used the unsorted bam file to generate fastq, and then used the fastq file for scvelo. The scvelo show that there are about 300000 duplicated cells out of 400000 cell in total, I am not sure if it is because of the barcodes in the fastq files? Could you kindly give me some guidance?
Thanks a lot
Boyu
The text was updated successfully, but these errors were encountered: