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I am working with RNA-seq data generated using the SMARTer Human TCR α/β Profiling Kit. Some of my samples show issues with adapter content and/or low Phred scores (<20-25) at the longer read lengths.
I need to align my data with the version 3.0.13 to ensure compatibility with previously analyzed samples. Before running MiXCR alignment with -rna seq preset option, would you recommend performing a trimming step to remove adapters and low-quality bases, or does MiXCR internally handle these issues effectively?
If trimming is recommended, is there a quality score threshold below which it becomes necessary?
Thank you in advance for your insights and for the quality of the documentation provided for MiXCR—it's greatly appreciated!
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Hello everyone,
I am working with RNA-seq data generated using the SMARTer Human TCR α/β Profiling Kit. Some of my samples show issues with adapter content and/or low Phred scores (<20-25) at the longer read lengths.
I need to align my data with the version 3.0.13 to ensure compatibility with previously analyzed samples. Before running MiXCR alignment with -rna seq preset option, would you recommend performing a trimming step to remove adapters and low-quality bases, or does MiXCR internally handle these issues effectively?
If trimming is recommended, is there a quality score threshold below which it becomes necessary?
Thank you in advance for your insights and for the quality of the documentation provided for MiXCR—it's greatly appreciated!
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