Targeted de novo phasing and long-range assembly by template mutagenesis

Author:

Li Siran1ORCID,Park Sarah1,Ye Catherine1,Danyko Cassidy1,Wroten Matthew1,Andrews Peter1,Wigler Michael1,Levy Dan1

Affiliation:

1. Cold Spring Harbor Laboratory , Cold Spring Harbor, NY  11724,  USA

Abstract

Abstract Short-read sequencers provide highly accurate reads at very low cost. Unfortunately, short reads are often inadequate for important applications such as assembly in complex regions or phasing across distant heterozygous sites. In this study, we describe novel bench protocols and algorithms to obtain haplotype-phased sequence assemblies with ultra-low error for regions 10 kb and longer using short reads only. We accomplish this by imprinting each template strand from a target region with a dense and unique mutation pattern. The mutation process randomly and independently converts ∼50% of cytosines to uracils. Sequencing libraries are made from both mutated and unmutated templates. Using de Bruijn graphs and paired-end read information, we assemble each mutated template and use the unmutated library to correct the mutated bases. Templates are partitioned into two or more haplotypes, and the final haplotypes are assembled and corrected for residual template mutations and PCR errors. With sufficient template coverage, the final assemblies have per-base error rates below 10–9. We demonstrate this method on a four-member nuclear family, correctly assembling and phasing three genomic intervals, including the highly polymorphic HLA-B gene.

Funder

Simons Foundation

SFARI

NHGRI

Publisher

Oxford University Press (OUP)

Subject

Genetics

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