Replies: 9 comments 3 replies
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Hi @pmenzel , That sounds interesting. We haven't tried with any of those kits or looked into the flongle unfortunately. I assume the data quality is similar? Jody |
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Hi, I just wanted to piggy back on this thread. Does the tbprofiler support ONT reads after base calling? I am hoping to start some work on the Flongle and want to compare with my MiSeq runs. |
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Yep if you change the if you add |
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oh amazing. I haven't started yet but planing to soon to compare ONT with previous Illumina. The plan is that for query DR isolates we get in the hospital I can run then quicker on a Flongle than batching on a MiSeq run! I'll keep you posted as and when I try! |
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Hey Jody, Just confirm the command would be; tb-profiler --nanopore profile -1 I have some Nanopore reads from last year that I was going to play around with! |
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Hi @peflanag, Almost, usually we would just one set of reads so it should be somehting like: Jody |
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Sorry yes! I just did a copy and paste from one of my scripts and forgot that its one set of reads! I assume there's no need to run Unicycler to assemble and I can directly use the Fast5 files that where basecalled to Fastq? |
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Oh no it should just work direct with the fastq data! |
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Cool, I might give it a go today! |
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Dear Jody,
we are looking into sequencing MTB cultures with Nanopore, first with the MinION and possibly later with the Flongle.
I saw that in your 2019 paper, that you used the SQK-LWB001 kit from ONT. This low input DNA kit is no longer available, so I wanted to ask if you already tried some of the currently available kits?
Probably many cultures would only yield low amounts of DNA, so that one likely needs a PCR-based kit, such as the Rapid PCR Barcoding Kit (SQK-RPB004) or the PCR Sequencing Kit (SQK-PSK004), which has higher yield in Gbp.
Second, the flongle seems quite useful for sequencing one or maybe two multiplexed samples at lower cost. Did you maybe already give it a try?
thanks and best wishes,
Peter
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