MbrlCatalogueTitleDetail

Do you wish to reserve the book?
Improved characterization of 3′ single-cell RNA-seq libraries with paired-end avidity sequencing
Improved characterization of 3′ single-cell RNA-seq libraries with paired-end avidity sequencing
by Gillen, Austin E , Chamberlin, John T , Quinlan, Aaron R
in Accuracy / Avidity / Bar codes / Bioinformatics / Complementary DNA / DNA sequencing / Genomics / Medicine / Nucleotide sequence / Polyadenylation / Ribonucleic acid / RNA / RNA-directed DNA polymerase / Thymine
2024
Yes Please
Hey, we have placed the reservation for you!
Hey, we have placed the reservation for you!
By the way, why not check out events that you can attend while you pick your title.
You are currently in the queue to collect this book. You will be notified once it is your turn to collect the book.
Done
Oops! Something went wrong.
Oops! Something went wrong.
Looks like we were not able to place the reservation. Kindly try again later.
Done
Are you sure you want to remove the book from the shelf?
Improved characterization of 3′ single-cell RNA-seq libraries with paired-end avidity sequencing
by Gillen, Austin E , Chamberlin, John T , Quinlan, Aaron R
in Accuracy / Avidity / Bar codes / Bioinformatics / Complementary DNA / DNA sequencing / Genomics / Medicine / Nucleotide sequence / Polyadenylation / Ribonucleic acid / RNA / RNA-directed DNA polymerase / Thymine
2024
Confirm
Oops! Something went wrong.
Oops! Something went wrong.
While trying to remove the title from your shelf something went wrong :( Kindly try again later!
Done
Title added to your shelf!
Title added to your shelf!
View what I already have on My Shelf.
Thanks
Oops! Something went wrong.
Oops! Something went wrong.
While trying to add the title to your shelf something went wrong :( Kindly try again later!
Done
Do you wish to request the book?
Improved characterization of 3′ single-cell RNA-seq libraries with paired-end avidity sequencing
Improved characterization of 3′ single-cell RNA-seq libraries with paired-end avidity sequencing
by Gillen, Austin E , Chamberlin, John T , Quinlan, Aaron R
in Accuracy / Avidity / Bar codes / Bioinformatics / Complementary DNA / DNA sequencing / Genomics / Medicine / Nucleotide sequence / Polyadenylation / Ribonucleic acid / RNA / RNA-directed DNA polymerase / Thymine
2024

Please be aware that the book you have requested cannot be checked out. If you would like to checkout this book, you can reserve another copy
How would you like to get it?
We have requested the book for you! Sorry the robot delivery is not available at the moment
Submit
We have requested the book for you!
We have requested the book for you!
Your request is successful and it will be processed during the Library working hours. Please check the status of your request in My Requests.
Done
Oops! Something went wrong.
Oops! Something went wrong.
Looks like we were not able to place your request. Kindly try again later.
Done
Mohammed Bin Rashid Library /
Catalogue /
Improved characterization of 3′ single-cell RNA-seq libraries with paired-end avidity sequencing
Improved characterization of 3′ single-cell RNA-seq libraries with paired-end avidity sequencing
Journal Article

Improved characterization of 3′ single-cell RNA-seq libraries with paired-end avidity sequencing

Gillen, Austin E,
Chamberlin, John T,
Quinlan, Aaron R
2024
Request Book From Autostore and Choose the Collection Method
Overview
Prevailing poly(dT)-primed 3′ single-cell RNA-seq protocols generate barcoded cDNA fragments containing the reverse transcriptase priming site or in principle the polyadenylation site. Direct sequencing across this site was historically difficult because of DNA sequencing errors induced by the homopolymeric primer at the 'barcode' end. Here, we evaluate the capability of 'avidity base chemistry' DNA sequencing from Element Biosciences to sequence through the primer and enable accurate paired-end read alignment and precise quantification of polyadenylation sites. We find that the Element Aviti instrument sequences through the thymine homopolymer into the subsequent cDNA sequence without detectable loss of accuracy. The additional sequence enables direct and independent assignment of reads to polyadenylation sites, which bypasses the complexities and limitations of conventional approaches but does not consistently improve read mapping rates compared to single-end alignment. We also characterize low-level artifacts and demonstrate necessary adjustments to adapter trimming and sequence alignment regardless of platform, particularly in the context of extended read lengths. Our analyses confirm that Element avidity sequencing is an effective alternative to Illumina sequencing for standard single-cell RNA-seq, particularly for polyadenylation site measurement but do not rule out the potential for similar performance from other emerging platforms.
Share this book
Add to My Shelf
Publisher
Oxford University Press
Subject

Accuracy

/ Avidity

/ Bar codes

/ Bioinformatics

/ Complementary DNA

/ DNA sequencing

/ Genomics

/ Medicine

/ Nucleotide sequence

/ Polyadenylation

/ Ribonucleic acid

/ RNA

/ RNA-directed DNA polymerase

/ Thymine

MBRLCatalogueRelatedBooks

Related Items

Related Items

We currently cannot retrieve any items related to this title. Kindly check back at a later time.