A high-quality assembly of the nine-spined stickleback (Pungitius pungitius) genome

Varadharajan, Srinidhi; Rastas, Pasi; Löytynoja, Ari; Matschiner, Michael; Calboli, Federico C. F.; Guo, Baocheng; Nederbragt, Alexander Johan; Jakobsen, Kjetill S.; Merilä, Juha

doi:10.1093/gbe/evz240

Cited by 56 publications

(113 citation statements)

References 93 publications

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“…Divergence times for each of the strata can be approximated based on divergence rates 461 between the threespine stickleback fish and the ninespine stickleback fish (Pungitius pungitius), al. 2009; Varadharajan et al 2019). Combined with a mean genome-wide estimate of Using the same calibration, stratum two formed less than 5.9 million years ago and stratum three 467 formed less than 4.7 million years ago.…”

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confidence: 99%

Assembly of a young vertebrate Y chromosome reveals convergent signatures of sex chromosome evolution

Peichel

McCann

Ross

et al. 2019

Preprint

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Heteromorphic sex chromosomes have evolved repeatedly across diverse species. Suppression of recombination between X and Y chromosomes leads to rapid degeneration of the Y chromosome. However, these early stages of degeneration are not well understood, as complete Y chromosome sequence assemblies have only been generated across a handful of taxa with ancient sex chromosomes. Here we describe the assembly of the threespine stickleback (Gasterosteus aculeatus) Y chromosome, which is less than 26 million years old. Our previous work identified that the non-recombining region between the X and the Y spans ∼17.5 Mb on the X chromosome. Here, we combined long-read PacBio sequencing with a Hi-C-based proximity guided assembly to generate a 15.87 Mb assembly of the Y chromosome. Our assembly is concordant with cytogenetic maps and Sanger sequences of over 90 Y chromosome clones from a bacterial artificial chromosome (BAC) library. We found three evolutionary strata on the Y chromosome, consistent with the three inversions identified by our previous cytogenetic analyses. The young threespine stickleback Y shows convergence with older sex chromosomes in the retention of haploinsufficient genes and the accumulation of genes with testis-biased expression, many of which are recent duplicates. However, we found no evidence for large amplicons found in other sex chromosome systems. We also report an excellent candidate for the master sex-determination gene: a translocated copy of Amh (Amhy). Together, our work shows that the same evolutionary forces shaping older sex chromosomes can cause remarkably rapid changes in the overall genetic architecture on young Y chromosomes.

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confidence: 99%

Assembly of a young vertebrate Y chromosome reveals convergent signatures of sex chromosome evolution

Peichel

McCann

Ross

et al. 2019

Preprint

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“…The improved assembly brings noticeable gains, and we could now successfully map the centromere associated repeat and unambiguously identify the centromere positions in all linkage groups (previously missing from LG1 and LG16, and incoherent in LG10 and LG14, Fig. 1b; see reference (17)). Removal of haplotypes and other changes in the genome assembly affects read mapping and single nucleotide variant calling.…”

Section: Resultsmentioning

confidence: 99%

“…The starting point for this reference was the genomic DNA sequence data from Varadharajan et al (17) In short, sequence data on one male individual from Pyöreälampi pond (66 a large inversion in LG19 was characterized and the region was reassembled (see below), and the mitochondrial genome was reassembled (see below). The resulting contig-assembly was anchored using Lep-Anchor (9) following the standard pipeline (https://sourceforge.net/p/lep-anchor/wiki/Home) with default parameters (exception: minQuality=1 for Map2Bed to assign more contigs into chromosomes).…”

Section: Nine-spined Stickleback Assemblymentioning

confidence: 99%

“…The parental genotypes were called using ParentCall2 module utilizing half-sib families (halfsibs=1) and calling also sex markers (XLimit=2). After running Fil-tering2 on default parameters, 50568 markers were retained and SeparateChromosomes2 module with LOD score limit 40 (lodLimit) clustered these markers into 21 linkage groups (LGs), matching the chromosome number of the species (33,17). JoinSingles2All with lodLimit=20 and lodDifference=4 assigned 22753 markers to the LGs and each LG was then ordered with OrderMarkers2, producing the first maps.…”

Section: Nine-spined Stickleback Linkage Mapmentioning

confidence: 99%

“…JoinSingles2All with lodLimit=20 and lodDifference=4 assigned 22753 markers to the LGs and each LG was then ordered with OrderMarkers2, producing the first maps. After genome anchoring with the novel maps and maps from Varadharajan et al (17), OrderMarkers2 was run one more time, separately for each LG, with physically ordered markers (parameter evaluateOrder). This yielded the final map from which the crossover locations were acquired.…”

Section: Nine-spined Stickleback Linkage Mapmentioning

confidence: 99%

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Automated improvement of stickleback reference genome assemblies with Lep-Anchor software

Kivikoski

Rastas

Löytynoja

et al. 2020

Preprint

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The utility of genome-wide sequencing data in biological research depends heavily on the quality of the reference genome. Although the reference genomes have improved, it is evident that the assemblies could still be refined, especially in non-model study organisms. Here, we describe an integrative approach to improve contiguity and haploidy of a reference genome assembly. With two novel features of Lep-Anchor software and a combination of dense linkage maps, overlap detection and bridging long reads we generated an improved assembly of the nine-spined stickleback (Pungitius pungitius) reference genome. We were able to remove a significant number of haplotypic contigs, detect more genetic variation and improve the contiguity of the genome, especially that of X chromosome. However, improved scaffolding cannot correct for mosaicism of erroneously assembled contigs, demonstrated by a de novo assembly of a 1.7 Mbp inversion. Qualitatively similar gains were obtained with the genome of three-spined stickleback (Gasterosteus aculeatus).

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Pelvic spine reduction affects diet but not gill raker morphology in two polymorphic brook stickleback (Culaea inconstans) populations

Mee,

Yap,

Wuitchik

2023

Ecology and Evolution

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Pelvic spine polymorphism occurs in several species in the stickleback family (Gasterosteidae). Given the similar phenotypic polymorphisms in multiple stickleback species, we sought to determine the extent of parallelism in the ecological correlates of pelvic spine reduction. Based on a metabarcoding analysis of brook stickleback gut contents in two polymorphic populations, we found that significant diet differences were associated with pelvic spine reduction, but we found no clear or consistent trend supporting a tendency for benthic feeding in pelvic‐reduced brook sticklebacks. These results contrast with those found in threespine sticklebacks where pelvic spine reduction is often associated with a benthic diet. Hence, we found non‐parallel consequences of spine polymorphism across species. Furthermore, a difference in gill raker morphology has been frequently observed between ecomorphs with different diets in many fish species. However, we found no evidence of any difference in gill raker morphology associated with pelvic spine polymorphism in brook sticklebacks.

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A high-quality assembly of the nine-spined stickleback (Pungitius pungitius) genome

Cited by 56 publications

References 93 publications

Assembly of a young vertebrate Y chromosome reveals convergent signatures of sex chromosome evolution

Assembly of a young vertebrate Y chromosome reveals convergent signatures of sex chromosome evolution

Automated improvement of stickleback reference genome assemblies with Lep-Anchor software

Pelvic spine reduction affects diet but not gill raker morphology in two polymorphic brook stickleback (Culaea inconstans) populations

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