Improved haplotype resolution of highly duplicated MHC genes in a long-read genome assembly using MiSeq amplicons

Mellinger, Samantha; Stervander, Martin; Lundberg, Max; Drews, Anna; Westerdahl, Helena

Improved haplotype resolution of highly duplicated MHC genes in a long-read genome assembly using MiSeq amplicons

Mark

Mellinger, Samantha ^LU ; Stervander, Martin ^LU ; Lundberg, Max ^LU ; Drews, Anna ^LU and Westerdahl, Helena ^LU (2023) In PeerJ 11.

Abstract: Long-read sequencing offers a great improvement in the assembly of complex genomic regions, such as the major histocompatibility complex (MHC) region, which can contain both tandemly duplicated MHC genes (paralogs) and high repeat content. The MHC genes have expanded in passerine birds, resulting in numerous MHC paralogs, with relatively high sequence similarity, making the assembly of the MHC region challenging even with long-read sequencing. In addition, MHC genes show rather high sequence divergence between alleles, making diploid-aware assemblers incorrectly classify haplotypes from the same locus as sequences originating from different genomic regions. Consequently, the number of MHC paralogs can easily be over- or underestimated... (More); Long-read sequencing offers a great improvement in the assembly of complex genomic regions, such as the major histocompatibility complex (MHC) region, which can contain both tandemly duplicated MHC genes (paralogs) and high repeat content. The MHC genes have expanded in passerine birds, resulting in numerous MHC paralogs, with relatively high sequence similarity, making the assembly of the MHC region challenging even with long-read sequencing. In addition, MHC genes show rather high sequence divergence between alleles, making diploid-aware assemblers incorrectly classify haplotypes from the same locus as sequences originating from different genomic regions. Consequently, the number of MHC paralogs can easily be over- or underestimated in long-read assemblies. We therefore set out to verify the MHC diversity in an original and a haplotype-purged long-read assembly of one great reed warbler Acrocephalus arundinaceus individual (the focal individual) by using Illumina MiSeq amplicon sequencing. Single exons, representing MHC class I (MHC-I) and class IIB (MHC-IIB) alleles, were sequenced in the focal individual and mapped to the annotated MHC alleles in the original long-read genome assembly. Eighty-four percent of the annotated MHC-I alleles in the original long-read genome assembly were detected using 55% of the amplicon alleles and likewise, 78% of the annotated MHC-IIB alleles were detected using 61% of the amplicon alleles, indicating an incomplete annotation of MHC genes. In the haploid genome assembly, each MHC-IIB gene should be represented by one allele. The parental origin of the MHC-IIB amplicon alleles in the focal individual was determined by sequencing MHC-IIB in its parents. Two of five larger scaffolds, containing 6–19 MHC-IIB paralogs, had a maternal and paternal origin, respectively, as well as a high nucleotide similarity, which suggests that these scaffolds had been incorrectly assigned as belonging to different loci in the genome rather than as alternate haplotypes of the same locus. Therefore, the number of MHC-IIB paralogs was overestimated in the haploid genome assembly. Based on our findings we propose amplicon sequencing as a suitable complement to long-read sequencing for independent validation of the number of paralogs in general and for haplotype inference in multigene families in particular.
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Please use this url to cite or link to this publication: https://lup.lub.lu.se/record/b2d4e762-8180-4b98-b9db-2839de19a19d

author

Mellinger, Samantha ^LU ; Stervander, Martin ^LU ; Lundberg, Max ^LU ; Drews, Anna ^LU and Westerdahl, Helena ^LU

organization

publishing date

2023

type

Contribution to journal

publication status

published

subject

keywords

Amplicon sequencing, Copy number variation, Family, Haploid genome assembly, Linkage analysis, Major histocompatibility complex, MHC diversity

in

PeerJ

volume

11

article number

e15480

publisher

PeerJ

external identifiers

pmid:37456901
scopus:85168601901

ISSN

2167-8359

DOI

10.7717/peerj.15480

language

English

LU publication?

yes

id

b2d4e762-8180-4b98-b9db-2839de19a19d

date added to LUP

2023-12-01 12:51:29

date last changed

2024-04-14 13:17:00

@article{b2d4e762-8180-4b98-b9db-2839de19a19d,
  abstract     = {{<p>Long-read sequencing offers a great improvement in the assembly of complex genomic regions, such as the major histocompatibility complex (MHC) region, which can contain both tandemly duplicated MHC genes (paralogs) and high repeat content. The MHC genes have expanded in passerine birds, resulting in numerous MHC paralogs, with relatively high sequence similarity, making the assembly of the MHC region challenging even with long-read sequencing. In addition, MHC genes show rather high sequence divergence between alleles, making diploid-aware assemblers incorrectly classify haplotypes from the same locus as sequences originating from different genomic regions. Consequently, the number of MHC paralogs can easily be over- or underestimated in long-read assemblies. We therefore set out to verify the MHC diversity in an original and a haplotype-purged long-read assembly of one great reed warbler Acrocephalus arundinaceus individual (the focal individual) by using Illumina MiSeq amplicon sequencing. Single exons, representing MHC class I (MHC-I) and class IIB (MHC-IIB) alleles, were sequenced in the focal individual and mapped to the annotated MHC alleles in the original long-read genome assembly. Eighty-four percent of the annotated MHC-I alleles in the original long-read genome assembly were detected using 55% of the amplicon alleles and likewise, 78% of the annotated MHC-IIB alleles were detected using 61% of the amplicon alleles, indicating an incomplete annotation of MHC genes. In the haploid genome assembly, each MHC-IIB gene should be represented by one allele. The parental origin of the MHC-IIB amplicon alleles in the focal individual was determined by sequencing MHC-IIB in its parents. Two of five larger scaffolds, containing 6–19 MHC-IIB paralogs, had a maternal and paternal origin, respectively, as well as a high nucleotide similarity, which suggests that these scaffolds had been incorrectly assigned as belonging to different loci in the genome rather than as alternate haplotypes of the same locus. Therefore, the number of MHC-IIB paralogs was overestimated in the haploid genome assembly. Based on our findings we propose amplicon sequencing as a suitable complement to long-read sequencing for independent validation of the number of paralogs in general and for haplotype inference in multigene families in particular.</p>}},
  author       = {{Mellinger, Samantha and Stervander, Martin and Lundberg, Max and Drews, Anna and Westerdahl, Helena}},
  issn         = {{2167-8359}},
  keywords     = {{Amplicon sequencing; Copy number variation; Family; Haploid genome assembly; Linkage analysis; Major histocompatibility complex; MHC diversity}},
  language     = {{eng}},
  publisher    = {{PeerJ}},
  series       = {{PeerJ}},
  title        = {{Improved haplotype resolution of highly duplicated MHC genes in a long-read genome assembly using MiSeq amplicons}},
  url          = {{http://dx.doi.org/10.7717/peerj.15480}},
  doi          = {{10.7717/peerj.15480}},
  volume       = {{11}},
  year         = {{2023}},
}

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Improved haplotype resolution of highly duplicated MHC genes in a long-read genome assembly using MiSeq amplicons