Exploiting antigen receptor information to quantify index switching in single-cell transcriptome sequencing experiments.

Exploiting antigen receptor information to quantify index switching in single-cell transcriptome sequencing experiments.

By offering high sequencing speed and ultra-high-throughput at a low price, Illumina next-generation sequencing platforms have been widely adopted in recent years. However, an experiment with multiplexed library could be at risk of molecular recombination, known as "index switching", which...

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Main Authors: Ying Yao, Asima Zia, Łukasz Wyrożemski, Ida Lindeman, Geir Kjetil Sandve, Shuo-Wang Qiao
Format: Article
Language:English
Published: Public Library of Science (PLoS) 2018-01-01
Series:PLoS ONE
Online Access:https://doi.org/10.1371/journal.pone.0208484
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spelling doaj-6fb6b0eb297842d4b9d74c2c554578c52021-03-03T21:04:08ZengPublic Library of Science (PLoS)PLoS ONE1932-62032018-01-011312e020848410.1371/journal.pone.0208484Exploiting antigen receptor information to quantify index switching in single-cell transcriptome sequencing experiments.Ying YaoAsima ZiaŁukasz WyrożemskiIda LindemanGeir Kjetil SandveShuo-Wang QiaoBy offering high sequencing speed and ultra-high-throughput at a low price, Illumina next-generation sequencing platforms have been widely adopted in recent years. However, an experiment with multiplexed library could be at risk of molecular recombination, known as "index switching", which causes a proportion of the reads to be assigned to an incorrect sample. It is reported that a new advance, exclusion amplification (ExAmp) in conjunction with the patterned flow cell technology introduced on HiSeq 3000/HiSeq 4000/HiSeq X sequencing systems, potentially suffers from a higher rate of index switching than conventional bridge amplification. We took advantage of the diverse but highly cell-specific expression of antigen receptors on immune cells to quantify index switching on single cell RNA-seq data that were sequenced on HiSeq 3000 and HiSeq 4000. By utilizing the unique antigen receptor expression, we could quantify the spread-of-signal from many different wells (n = 55 from total of three batches) due to index switching. Based on full-length T cell receptor (TCR) sequences from all samples reconstructed by TraCeR and TCR gene expression quantified by Kallisto, we found index switching in all three batches of experiments investigated. The median percentage of incorrectly detected markers was estimated to be 3.9% (interquartile range (IQR): 1.7%-7.3%). We did not detect any consistent patterns of certain indices to be more prone to switching than others, suggesting that index switching is a stochastic process. Our results confirm that index switching is a problem that affects samples run in multiplexed libraries on Illumina HiSeq 3000 and HiSeq 4000 platforms.https://doi.org/10.1371/journal.pone.0208484
collection DOAJ
language English
format Article
sources DOAJ
author Ying Yao
Asima Zia
Łukasz Wyrożemski
Ida Lindeman
Geir Kjetil Sandve
Shuo-Wang Qiao
spellingShingle Ying Yao
Asima Zia
Łukasz Wyrożemski
Ida Lindeman
Geir Kjetil Sandve
Shuo-Wang Qiao
Exploiting antigen receptor information to quantify index switching in single-cell transcriptome sequencing experiments.
PLoS ONE
author_facet Ying Yao
Asima Zia
Łukasz Wyrożemski
Ida Lindeman
Geir Kjetil Sandve
Shuo-Wang Qiao
author_sort Ying Yao
title Exploiting antigen receptor information to quantify index switching in single-cell transcriptome sequencing experiments.
title_short Exploiting antigen receptor information to quantify index switching in single-cell transcriptome sequencing experiments.
title_full Exploiting antigen receptor information to quantify index switching in single-cell transcriptome sequencing experiments.
title_fullStr Exploiting antigen receptor information to quantify index switching in single-cell transcriptome sequencing experiments.
title_full_unstemmed Exploiting antigen receptor information to quantify index switching in single-cell transcriptome sequencing experiments.
title_sort exploiting antigen receptor information to quantify index switching in single-cell transcriptome sequencing experiments.
publisher Public Library of Science (PLoS)
series PLoS ONE
issn 1932-6203
publishDate 2018-01-01
description By offering high sequencing speed and ultra-high-throughput at a low price, Illumina next-generation sequencing platforms have been widely adopted in recent years. However, an experiment with multiplexed library could be at risk of molecular recombination, known as "index switching", which causes a proportion of the reads to be assigned to an incorrect sample. It is reported that a new advance, exclusion amplification (ExAmp) in conjunction with the patterned flow cell technology introduced on HiSeq 3000/HiSeq 4000/HiSeq X sequencing systems, potentially suffers from a higher rate of index switching than conventional bridge amplification. We took advantage of the diverse but highly cell-specific expression of antigen receptors on immune cells to quantify index switching on single cell RNA-seq data that were sequenced on HiSeq 3000 and HiSeq 4000. By utilizing the unique antigen receptor expression, we could quantify the spread-of-signal from many different wells (n = 55 from total of three batches) due to index switching. Based on full-length T cell receptor (TCR) sequences from all samples reconstructed by TraCeR and TCR gene expression quantified by Kallisto, we found index switching in all three batches of experiments investigated. The median percentage of incorrectly detected markers was estimated to be 3.9% (interquartile range (IQR): 1.7%-7.3%). We did not detect any consistent patterns of certain indices to be more prone to switching than others, suggesting that index switching is a stochastic process. Our results confirm that index switching is a problem that affects samples run in multiplexed libraries on Illumina HiSeq 3000 and HiSeq 4000 platforms.
url https://doi.org/10.1371/journal.pone.0208484
work_keys_str_mv AT yingyao exploitingantigenreceptorinformationtoquantifyindexswitchinginsinglecelltranscriptomesequencingexperiments
AT asimazia exploitingantigenreceptorinformationtoquantifyindexswitchinginsinglecelltranscriptomesequencingexperiments
AT łukaszwyrozemski exploitingantigenreceptorinformationtoquantifyindexswitchinginsinglecelltranscriptomesequencingexperiments
AT idalindeman exploitingantigenreceptorinformationtoquantifyindexswitchinginsinglecelltranscriptomesequencingexperiments
AT geirkjetilsandve exploitingantigenreceptorinformationtoquantifyindexswitchinginsinglecelltranscriptomesequencingexperiments
AT shuowangqiao exploitingantigenreceptorinformationtoquantifyindexswitchinginsinglecelltranscriptomesequencingexperiments
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