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Hello, I have a pre-processed, paired-end snRNASeq dataset I want to to align in which the first read is 26bp and the second read is 91bp. How do I generate a single splici index for two different read lengths? Thank you, ~ Mark |
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Replies: 2 comments 5 replies
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Hi @lawsonvt, In this case, the first read is techinal (UMI and barcode) and not relevant to the index construction. You should treat 91 as your read length. Best, |
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Thanks Rob. Does this mean the reads should be aligned as single reads or still as paired? |
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What protocol were they sequenced with? Best, |
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"snRNA-seq libraries were obtained using 10X Genomics Chromium Single Cell 5′ v2 chemistry following nuclear dissociation" Is that enough info? |
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Yes; this is sufficient information. Basically, it means you should run Then, when you perform the --Rob |
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I ran into something similar. I have FASTQs with different read lengths: Do I have to create different reference indices? I am using simpleaf (alevin-fry). |
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I just had a look at the following post. Since the specific length does not seem to make a difference, I will use 91. If I am mistaken, please correct me. Based on the following tutorial, you recommend checking and using the exact read length of the processed dataset. I am still confused. A response would be much appreciated. |
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Hi @lawsonvt,
In this case, the first read is techinal (UMI and barcode) and not relevant to the index construction. You should treat 91 as your read length.
Best,
Rob