I wouldn't go that far! Cheap (no-agarose-gel) Illumina mate-pair libraries are still legitimate, if trailing-edge, technologies.
454 is *dead*, dead.
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Phillip
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In the age of long read sequencing (PacBio, Nanopore) and linked reads (10X Genomics), "mate pair" sequencing is as obsolete as 454.Leave a comment:
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Is the 454 Paired End technology beginner friendly, so to speak? How difficult is it to get into?Leave a comment:
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Originally posted by soungalo View Post
Wow, time to fire up the WayBack Machine Mr. Peabody.
Yes, 454 "Paired End" technology is similar in design to Illumina Mate Pair tech. A large fragment is circularized with a linker, the circular DNA is fragmented and the piece with the linker is enriched. It is then sequenced and the linker sequence is identified to separate the "forward" and "reverse" reads. I have attached a 454 data processing manual; look at section 4.6 for information about paired end data.
Here are some links to previous thread on SeqAnswers discussing 454 paired end reads:
This latter thread includes a post with the linker sequences (post #2). There are different linker sequencing depending which generation of the library prep kit was used, FLX or Titanium.Leave a comment:
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454 GS FLX Titanium 'paired end' protocol
Hi,
I know this is an obsolete technology, but I came across some data produced on the 454 instrument (archived in SRA/ENA) which I'd like to use for assembly.
According to the meta data, insert sizes are 8kb and 20kb, but I wasn't able to figure out the protocol used to produce the libraries. I gather that this is some variant on what we'd now call mate-pair, but I'm not sure if I can treat the data exactly the same way as data coming from Illumina mate-pair libraries, in terms of read orientation, insert size distribution etc.
Had anyone worked with such data, or can direct me to some documentation about it? I failed to find anything in the current Roche docs.
Thanks!
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