Short tandem repeat stutter model inferred from direct measurement of in vitro stutter noise

Ofir Raz; Tamir Biezuner; Adam Spiro; Shiran Amir; Lilach Milo; Alon Titelman; Amos Onn; Noa Chapal-Ilani; Liming Tao; Tzipy Marx; Uriel Feige; Ehud Shapiro

doi:10.1093/nar/gky1318

Short tandem repeat stutter model inferred from direct measurement of in vitro stutter noise

Ofir Raz, Tamir Biezuner, Adam Spiro, Shiran Amir, Lilach Milo, Alon Titelman, Amos Onn, Noa Chapal-Ilani, Liming Tao, Tzipy Marx, Uriel Feige, Ehud Shapiro

Department of Computer Science and Applied Mathematics

Weizmann Institute of Science

Research output: Contribution to journal › Article › peer-review

Abstract

Short tandem repeats (STRs) are polymorphic genomic loci valuable for various applications such as research, diagnostics and forensics. However, their polymorphic nature also introduces noise duringin vitroamplification, making them difficult to analyze. Although it is possible to overcome stutter noise by using amplification-free library preparation, such protocols are presently incompatible with single cell analysis and with targeted-enrichment protocols. To address this challenge, we have designed a method for direct measurement of in vitro noise. Using a synthetic STR sequencing library, we have calibrated a Markov model for the prediction of stutter patterns at any amplification cycle. By employing this model, we have managed to genotype accurately cases of severe amplification bias, and biallelic STR signals, and validated our model for several high-fidelity PCR enzymes. Finally, we compared this model in the context of a naive STR genotyping strategy against the state-of-the-art on a benchmark of single cells, demonstrating superior accuracy.

Original language	English
Pages (from-to)	2436-2445
Number of pages	10
Journal	Nucleic acids research
Volume	47
Issue number	5
DOIs	https://doi.org/10.1093/nar/gky1318
State	Published Online - 30 Jan 2019

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10.1093/nar/gky1318License: CC BY

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title = "Short tandem repeat stutter model inferred from direct measurement of in vitro stutter noise",

abstract = "Short tandem repeats (STRs) are polymorphic genomic loci valuable for various applications such as research, diagnostics and forensics. However, their polymorphic nature also introduces noise duringin vitroamplification, making them difficult to analyze. Although it is possible to overcome stutter noise by using amplification-free library preparation, such protocols are presently incompatible with single cell analysis and with targeted-enrichment protocols. To address this challenge, we have designed a method for direct measurement of in vitro noise. Using a synthetic STR sequencing library, we have calibrated a Markov model for the prediction of stutter patterns at any amplification cycle. By employing this model, we have managed to genotype accurately cases of severe amplification bias, and biallelic STR signals, and validated our model for several high-fidelity PCR enzymes. Finally, we compared this model in the context of a naive STR genotyping strategy against the state-of-the-art on a benchmark of single cells, demonstrating superior accuracy.",

author = "Ofir Raz and Tamir Biezuner and Adam Spiro and Shiran Amir and Lilach Milo and Alon Titelman and Amos Onn and Noa Chapal-Ilani and Liming Tao and Tzipy Marx and Uriel Feige and Ehud Shapiro",

note = "We thank O. Bechar for the prompt design of figures. FUNDING: European Union [ERC-2008-AdG (Project No. 233047) and ERC-2014-AdG (Project No. 670535)]; Israel Science Foundation grants: Individual Research Grant [456/13]; Joint Broad-ISF Research [422/14 and 2012/15]; German Research Foundation [DFG SH grant 867/1-1]; Kenneth and Sally Leafman Appelbaum Discovery Fund. E.S. is the Incumbent of The Harry Weinrebe Professorial Chair of Computer Science and Biology. Funding for open access charge: European Union [ERC-2014-AdG [Project No. 670535)].",

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doi = "10.1093/nar/gky1318",

language = "الإنجليزيّة",

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T1 - Short tandem repeat stutter model inferred from direct measurement of in vitro stutter noise

AU - Raz, Ofir

AU - Biezuner, Tamir

AU - Spiro, Adam

AU - Amir, Shiran

AU - Milo, Lilach

AU - Titelman, Alon

AU - Onn, Amos

AU - Chapal-Ilani, Noa

AU - Tao, Liming

AU - Marx, Tzipy

AU - Feige, Uriel

AU - Shapiro, Ehud

N1 - We thank O. Bechar for the prompt design of figures. FUNDING: European Union [ERC-2008-AdG (Project No. 233047) and ERC-2014-AdG (Project No. 670535)]; Israel Science Foundation grants: Individual Research Grant [456/13]; Joint Broad-ISF Research [422/14 and 2012/15]; German Research Foundation [DFG SH grant 867/1-1]; Kenneth and Sally Leafman Appelbaum Discovery Fund. E.S. is the Incumbent of The Harry Weinrebe Professorial Chair of Computer Science and Biology. Funding for open access charge: European Union [ERC-2014-AdG [Project No. 670535)].

PY - 2019/1/30

Y1 - 2019/1/30

N2 - Short tandem repeats (STRs) are polymorphic genomic loci valuable for various applications such as research, diagnostics and forensics. However, their polymorphic nature also introduces noise duringin vitroamplification, making them difficult to analyze. Although it is possible to overcome stutter noise by using amplification-free library preparation, such protocols are presently incompatible with single cell analysis and with targeted-enrichment protocols. To address this challenge, we have designed a method for direct measurement of in vitro noise. Using a synthetic STR sequencing library, we have calibrated a Markov model for the prediction of stutter patterns at any amplification cycle. By employing this model, we have managed to genotype accurately cases of severe amplification bias, and biallelic STR signals, and validated our model for several high-fidelity PCR enzymes. Finally, we compared this model in the context of a naive STR genotyping strategy against the state-of-the-art on a benchmark of single cells, demonstrating superior accuracy.

AB - Short tandem repeats (STRs) are polymorphic genomic loci valuable for various applications such as research, diagnostics and forensics. However, their polymorphic nature also introduces noise duringin vitroamplification, making them difficult to analyze. Although it is possible to overcome stutter noise by using amplification-free library preparation, such protocols are presently incompatible with single cell analysis and with targeted-enrichment protocols. To address this challenge, we have designed a method for direct measurement of in vitro noise. Using a synthetic STR sequencing library, we have calibrated a Markov model for the prediction of stutter patterns at any amplification cycle. By employing this model, we have managed to genotype accurately cases of severe amplification bias, and biallelic STR signals, and validated our model for several high-fidelity PCR enzymes. Finally, we compared this model in the context of a naive STR genotyping strategy against the state-of-the-art on a benchmark of single cells, demonstrating superior accuracy.

U2 - 10.1093/nar/gky1318

DO - 10.1093/nar/gky1318

M3 - مقالة

SN - 0305-1048

VL - 47

SP - 2436

EP - 2445

JO - Nucleic acids research

JF - Nucleic acids research

IS - 5

ER -

Short tandem repeat stutter model inferred from direct measurement of in vitro stutter noise

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