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Hi, https://github.com/TreesLab/NCLscan/pull/32/files Still, thanks for the kindly report! Best, |
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Interesting. Has it ever been there? I first cloned the repo a couple years
ago and struggled to get past that point, not knowing what caused the empty
output. I only found it recently by tracing and mapping every step of the
workflow, with the same input.
Removing that line made it run to the end. Maybe my former self put it in;
I can't remember. Sorry about the noise if that's what I did. But then
there is a mystery of what broke the workflow originally.
Since we are on the topic (almost), do you see an easy way to discover
circRNAs that do not result from canonical splicing? I have a sample with a
massive amount of RNA concatemer made of a fragment of ROS1 exon 37. The
repeat unit is a fraction of that exon that does not include a splice site.
I can only discover such things by clicking around in a browser.
Thank you,
…--Gene
On Tue, 12 Dec 2023 at 07:26, Tai-Wei Chiang ***@***.***> wrote:
Hi,
Thank you for trying to report bugs for NCLscan,
but the print() call was not appeared in the original file.
https://github.com/TreesLab/NCLscan/pull/32/files
Still, thanks for the kindly report!
Best,
tw
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This print call in
AssembleJSeq.pywas contaminated one of the intermediate outputs, leading to the ivalid (empty) novoindex:print(common_IDs)This results in this error condition at the following step
does not appear to be a valid novoindex