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Originally posted by nucacidhunter
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It only works for applications that are not sensitive to crosstalk. Personally, I would never multiplex samples of the same genus on a NovaSeq unless all libraries had dual unique barcodes. The current system of unique pairs, in which multiple libraries share the same first barcode and multiple libraries share the same second barcode, and any pair of first and second barcodes lands a read in a specific library, is insufficient for NovaSeq. To be honest, it was insufficient for the HiSeq 2500 as well, in situations where low-frequency variants were important (or for multiplexed single-cell sequencing). But it's more insufficient now, where multiplexing is desired on a NovaSeq, due to the substantially increased crosstalk rate.Last edited by Brian Bushnell; 10-10-2017, 01:10 AM. -
I agree Brian. It will be even worse if they release S4 flow cells without individual lane loading device/fix which currently is in beta testing.Comment
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Adding 4-5 diversity base is possible but two points to consider:Originally posted by Markiyan View Post
1- it will be difficult to obtain good oligo annealing to form adapters and also there will unpaired oligos which would require further purification
2- Illumina is unlikely to change their established indexing strategy and also there might be some patents on inline barcoding
Unique duel indexing (every library with different index 1 and 2) should enable identification and filtering of any fragments resulting from index hopping.
Actually in patterned flow cells position of each nano-well which would have clusters is already known. I have not thought about the need for sequence diversity but it could be related to background signal.Comment
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You can buy the UDI 96 and/or the UDI 384 kit from IDT as a custom order. Just contact their sales. We bought the UDI 96. Made libraries (both no Amp DNA and RNAseq libraries) from them. Ran them on our NovaSeq.Originally posted by nucacidhunter View Post
The UDI 384 are 10 base indexes though. So you would have to reduce your sequence insert reads by 2 bases each to compensate...
NuGEN sales reps told me that their adapters don't use T/A tailing. So they wouldn't work with most other kits.
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PhillipComment
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Did you see much phiX index hopping? Searching the "undetermined" fastq for index hops involving one of i7/i5 GGGGGGGG/TCGTAGTG I tentatively identified a fair number. Of course they may just be the result of signal bleed.Originally posted by Brian Bushnell View Post
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PhillipComment
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How did you come up with that 10^-6 figure? In an RNASeq or CHIPseq experiment that's only about 20-30 reads.Originally posted by Markiyan View PostComment
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I have not looked into that yet. Actually, I don't even know if we are spiking PhiX into our Novaseq runs, but that rate is worth examining, after I find out whether there is actually any PhiX present.Originally posted by pmiguel View PostComment
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I am not sure that index hopping onto PhiX reads would be a good measure. As far as I remember the Illumina PhiX adapter sequences are quite different from TruSeq or Nextera sequences.Comment
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Well, not as different as you might think. Please see the attachment.Originally posted by luc View Post
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PhillipComment
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For those with NovaSeqs, are you allowed to say how much the consumables are? Based on what people are charging for a lane, it looks like about $40K per run...Comment
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I was told by an Illumina rep at Queenstown Research week about a month ago that NovaSeq run cost would be similar to HiSeq, but produce about double the output.Comment
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List price on S4 reagent kits is about $30K. For NovaSeq sites with ≥5 NovaSeq instruments, they're able to get a discount large enough to achieve the "20% cheaper than HiSeq X" statement Francis deSouza made when they announced this platform. Something tells me this is factoring in how many samples could be run per year on NovaSeq than HiSeq X due to the throughput and runtime, so their discount is likely not more than 20% off of list. Everyone else likely gets <10% discount. HiSeq 4000 (300 cycle) kits are about $17K list price, so they're not the same price but S4 will give you about 5x the output (in about half the time).Comment
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I’m not a sequencing expert. I’m a purification scientist who uses NGS to evaluate workflows my group develops. With this perspective, we think about the sample first and the NGS workflow second. The sequencer is an exceptionally honest reporter, but it can only report on what you give it, so whether you get clean, interpretable data from an NGS workflow is largely determined before you begin.
Here are nine questions we think about, in roughly the order they matter, before...06-18-2026, 07:11 AM -
Data variability is still an issue in sequencing technologies despite the advances in reproducibility and accuracy of these platforms. But the problem does not originate in the sequencing itself, but in the previous steps, before the sample reaches the sequencer.
The first step is collection, followed by preservation and sample preparation for analysis. Most scientists overlook those steps, but not being careful might just be skewing the experiment’s results.
...06-02-2026, 10:05 AM
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