Scientific article
OA Policy
English

Elimination of PCR duplicates in RNA-seq and small RNA-seq using unique molecular identifiers

Published inBMC genomics, vol. 19, no. 1, 531
Publication date2018-07-13
First online date2018-07-13
Abstract

Background: RNA-seq and small RNA-seq are powerful, quantitative tools to study gene regulation and function. Common high-throughput sequencing methods rely on polymerase chain reaction (PCR) to expand the starting material, but not every molecule amplifies equally, causing some to be overrepresented. Unique molecular identifiers (UMIs) can be used to distinguish undesirable PCR duplicates derived from a single molecule and identical but biologically meaningful reads from different molecules.

Results: We have incorporated UMIs into RNA-seq and small RNA-seq protocols and developed tools to analyze the resulting data. Our UMIs contain stretches of random nucleotides whose lengths sufficiently capture diverse molecule species in both RNA-seq and small RNA-seq libraries generated from mouse testis. Our approach yields high-quality data while allowing unique tagging of all molecules in high-depth libraries.

Conclusions: Using simulated and real datasets, we demonstrate that our methods increase the reproducibility of RNA-seq and small RNA-seq data. Notably, we find that the amount of starting material and sequencing depth, but not the number of PCR cycles, determine PCR duplicate frequency. Finally, we show that computational removal of PCR duplicates based only on their mapping coordinates introduces substantial bias into data analysis.

Keywords
  • PCR cycle
  • PCR duplicates
  • RNA-seq
  • Ribognome
  • Sequencing depth
  • Small RNA-seq
  • Starting material
  • Transcriptome
  • UMI
  • Unique molecular identifier
  • Animals
  • Gene Library
  • Male
  • Mice
  • Polymerase Chain Reaction
  • RNA / chemistry
  • RNA / isolation & purification
  • RNA / metabolism
  • Reproducibility of Results
  • Sequence Analysis, RNA / methods
  • Testis / metabolism
Affiliation entities Not a UNIGE publication
Funding
  • NICHD NIH HHS - [P01 HD078253]
  • NIGMS NIH HHS - [R37 GM062862]
  • National Institute of General Medical Sciences - [R37GM062862]
  • Eunice Kennedy Shriver National Institute of Child Health and Human Development - [HD078253]
  • Howard Hughes Medical Institute -
Citation (ISO format)
FU, Yu et al. Elimination of PCR duplicates in RNA-seq and small RNA-seq using unique molecular identifiers. In: BMC genomics, 2018, vol. 19, n° 1, p. 531. doi: 10.1186/s12864-018-4933-1
Main files (1)
Article (Published version)
Secondary files (3)
Identifiers
Journal ISSN1471-2164
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