Number of aligned reads distinct between preset rna-seq and generic-amplicon-with-umi #1650
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AntonellaGuo
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Hi, The difference you are seeing is because the It's hard to determine which preset would be best for this type of data. Did you mean that instead of using a cell suspension, you extracted bulk RNA from multiple cells and used this solution with the 10x Genomics microfluidics cartridge? |
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Hi there,
I got a bulk rna-seq data of T cells with 10X Single Cell Mouse TCR Amplification Kit. Although it's a weird way to build the library, I still would like to do the analysis. Since the library has 16bp 10x barcode and 10bp UMI in read 1, I treated this 26bp as a unique UMI and used the following setting
And I got this report, which shows that only 5.2% reads aligned.
Total sequencing reads: 16382057
Successfully aligned reads: 784470 (4.79%)
Coverage (percent of successfully aligned):
CDR3: 716849 (91.38%)
FR3_TO_FR4: 103 (0.01%)
CDR2_TO_FR4: 82 (0.01%)
FR2_TO_FR4: 707 (0.09%)
CDR1_TO_FR4: 590 (0.08%)
VDJRegion: 222 (0.03%)
Alignment failed: no hits (not TCR/IG?): 10151902 (61.97%)
Alignment failed: absence of J hits: 5442259 (33.22%)
Alignment failed: absent barcode: 3426 (0.02%)
Instead of using the
generic-amplicon-with-umi
, I also triedrna-seq
The report shows that 55.8% reads aligned.
Total sequencing reads: 16382057
Successfully aligned reads: 9141188 (55.8%)
Coverage (percent of successfully aligned):
CDR3: 719411 (7.87%)
FR3_TO_FR4: 178 (0%)
CDR2_TO_FR4: 908 (0.01%)
FR2_TO_FR4: 407 (0%)
CDR1_TO_FR4: 955 (0.01%)
VDJRegion: 465 (0.01%)
Alignment failed: no hits (not TCR/IG?): 2071405 (12.55%)
Alignment failed: no CDR3 parts: 4813938 (29.18%)
Alignment failed: low total score: 406572 (2.46%)
I would like to know why there is a big difference between the two results and to analyze this data which preset do you preferred.
Thx
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