G3: Genes|Genomes|Genetics Early Online, published on October 2, 2019 as doi:10.1534/g3.119.400705 1 Genome of Spea multiplicata, a rapidly developing, 2 phenotypically plastic, and desert-adapted spadefoot toad 3 4 Fabian Seidl1, Nicholas A. Levis2, Rachel Schell1, David W. Pfennig2,3, Karin S. Pfennig2,3, and 5 Ian M. Ehrenreich1,3 6 7 1 Molecular and Computational Biology Section, Department of Biological Sciences, University 8 of Southern California, Los Angeles, CA 90089, USA 9 10 2 Department of Biology, University of North Carolina, Chapel Hill, NC 27599, USA 11 12 3 Corresponding authors: 13 David W. Pfennig 14 Phone #: 919-962-0155 15 Email: [email protected] 16 17 Karin S. Pfennig 18 Phone #: 919-843-5590 19 Email: [email protected] 20 21 Ian M. Ehrenreich 22 Phone #: 213 – 821 – 5349 23 Email: [email protected] © The Author(s) 2013. Published by the Genetics Society of America. 24 Abstract 25 Frogs and toads (anurans) are widely used to study many biological processes. Yet, few anuran 26 genomes have been sequenced, limiting research on these organisms. Here, we produce a 27 draft genome for the Mexican spadefoot toad, Spea multiplicata, which is a member of an 28 unsequenced anuran clade. Atypically for amphibians, spadefoots inhabit deserts. 29 Consequently, they possess many unique adaptations, including rapid growth and development, 30 prolonged dormancy, phenotypic (developmental) plasticity, and adaptive, interspecies 31 hybridization. We assembled and annotated a 1.07 Gb Sp. multiplicata genome containing 32 19,639 genes. By comparing this sequence to other available anuran genomes, we found gene 33 amplifications in the gene families of nodal, hyas3, and zp3 in spadefoots, and obtained 34 evidence that anuran genome size differences are partially driven by variability in intergenic 35 DNA content. We also used the genome to identify genes experiencing positive selection and to 36 study gene expression levels in spadefoot hybrids relative to their pure-species parents. 37 Completion of the Sp. multiplicata genome advances efforts to determine the genetic bases of 38 spadefoots’ unique adaptations and enhances comparative genomic research in anurans. 39 40 2 41 Introduction 42 With at least 7,040 species (AMPHIBIAWEB 2018), frogs and toads (anurans) occur across 43 diverse habitats and exhibit a stunning array of adaptations (DUELLMAN AND TRUEB 1986; 44 HALLIDAY 2016). Moreover, anurans are critical, but increasingly threatened, components of 45 most ecosystems and thus serve as key bioindicators (STUART et al. 2004). Despite their 46 importance to fields from developmental biology and physiology to ecology and evolution, 47 genomic resources are relatively scarce for anurans. Indeed, fewer genomes are available for 48 anurans than for most other major groups of vertebrates, with only seven anurans sequenced: 49 the Western clawed frog, Xenopus tropicalis, and the closely related African clawed frog, 50 Xenopus laevis (HELLSTEN et al. 2010), the Tibetan Plateau frog, Nanorana parkeri (SUN et al. 51 2015), the American bullfrog, Rana (Lithobates) catesbeiana (HAMMOND et al. 2017), the Cane 52 toad, Rhinella marina (EDWARDS et al. 2018), the Strawberry Poison frog (Oophaga pumilio) 53 (ROGERS et al. 2018), and the African bullfrog (Pyxicephalus adspersus) (DENTON et al. 2018). 54 This paucity of genomes limits the use of anurans as model systems for many important 55 biological questions, especially given their deep levels of divergence (BOSSUYT AND ROELANTS 56 2009). 57 Here, we present a draft genome of a New World spadefoot toad, the Mexican spadefoot 58 toad, Spea multiplicata (family Scaphiopoididae; Fig. 1a,b). New World spadefoot toads 59 (hereafter, ‘spadefoots’) comprise seven diploid species, two of which––Scaphiopus holbrookii 60 and Sc. hurterii––occur in relatively mesic eastern and central North America, and five of which– 61 –Sp. multiplicata, Sp. bombifrons, Sp. hammondii, Sp. intermontana, and Sc. couchii––inhabit 62 xeric western North America. Crucially, relative to the other frogs and toads with published 63 genomes, spadefoots fill an unsequenced gap of > 200 My on the anuran phylogeny (Fig. 1a). 64 Additionally, spadefoots possess some of the smallest anuran genomes of between 1.0 and 1.4 65 Gb (GREGORY 2018). By contrast, the genomes of other sequenced diploid anurans range from 66 1.7 Gb for X. tropicalis (estimated via karyotype) (HELLSTEN et al. 2010) to a 5.8 Gb assembly 67 size for R. catesbeiana (HAMMOND et al. 2017). 68 Spadefoots serve as important models in ecology and evolution, owing to their unusual 69 ecology, rapid development, and striking phenotypic plasticity. For example, spadefoots cope 70 with their arid habitat by burrowing underground (RUIBAL et al. 1969) and estivating for a year or 71 longer (MAYHEW 1965; MCCLANAHAN 1967; SEYMOUR 1973), emerging for only a few weeks 72 following warm rains to feed and breed in short-lived pools (Fig. 1c, d) (BRAGG 1965). Although 73 these highly ephemeral pools are inaccessible to most anurans, spadefoot tadpoles can survive 74 in them by developing rapidly––in some cases metamorphosing in eight days post-hatching 3 75 (Fig. 1e) (NEWMAN 1989). Spadefoots also exhibit multiple forms of phenotypic plasticity that 76 further hastens their development and allows them to thrive in environments (such as deserts) 77 where rainfall is highly variable (TINSLEY AND TOCQUE 1995). Specifically, spadefoot tadpoles 78 can facultatively speed up (DENVER et al. 1998; MOREY AND REZNICK 2000; BOORSE AND 79 DENVER 2003; GOMEZ-MESTRE AND BUCHHOLZ 2006) or slow down (NEWMAN 1992; DENVER et 80 al. 1998; MOREY AND REZNICK 2000) development in response to the environment. Additionally, 81 whereas most anuran tadpoles are omnivores and exhibit traits adapted for feeding on detritus 82 and plankton (WELLS 2007), Spea tadpoles can develop into an alternative––and more rapidly 83 developing––‘carnivore’ ecomorph, which exhibits enlarged jaw muscles and mouthparts for 84 capturing and consuming large animal prey (Fig. 1f) (PFENNIG 1990; PFENNIG 1992a; PFENNIG 85 1992b; LEVIS et al. 2015; LEVIS et al. 2018). This carnivore morph has an additional advantage 86 in a rapidly drying pond: it can reduce competition and further enhance growth and development 87 by eating other tadpoles (PFENNIG 2000). Finally, as adults, when breeding in shallow, rapidly 88 drying ponds, Sp. bombifrons females preferentially mate with sympatric Sp. multiplicata males, 89 thereby producing hybrid tadpoles that develop even faster than pure-species tadpoles 90 (PFENNIG 2007). Genome resources for spadefoots will greatly enable further work on 91 understanding spadefoot’s unique characteristics. 92 In this paper, we performed a combination of long- and short-read sequencing on Mexican 93 spadefoots, Sp. multiplicata, and produce a draft genome for this species. By comparing this 94 genome to other available anuran genomes, we identify several distinctive gene amplifications, 95 as well as factors contributing to the substantial genome size variation found among anurans. 96 We then leverage the Sp. multiplicata genome as a platform for exploring evolution in two ways. 97 First, we produce short-read, whole genome sequencing data for three other species of 98 spadefoots: Plains spadefoots, Sp. bombifrons, Couch’s spadefoots, Sc. couchii, and Eastern 99 spadefoots, Sc. holbrookii. We obtain thousands of protein-coding gene sequences for these 100 species by mapping the data against Sp. multiplicata gene models. This allows us to identify 101 genes exhibiting different selection pressures in Spea or Scaphiopus, including positive 102 selection, thereby providing insights into specific genes underlying adaptive evolution in these 103 genera. Second, we generate transcriptome data for Sp. multiplicata and Sp. bombifrons 104 tadpoles, as well as for tadpoles produced by hybridizing these species, thereby providing 105 insights into why hybridization might be ecologically and evolutionarily significant in Spea 106 (PFENNIG 2007; PIERCE et al. 2017). 4 107 Together, our results demonstrate how the Sp. multiplicata genome can facilitate genetics 108 and genomics research in spadefoots. Ultimately, such research promises to provide key 109 insights into the distinctive phenotypes of these unique organisms. 110 111 Materials and Methods 112 Genome assembly 113 We selected an adult male Sp. multiplicata that had been collected in July 2011 at a breeding 114 aggregation in an ephemeral pond (‘410 Pond’) 20 km SSE of Portal, Arizona USA (31.7384, - 115 109.1). Immediately after euthanizing the male, we removed and homogenized his liver and 116 extracted from it high molecular weight DNA using Qiagen 500G Genomic-tip columns. 117 Additional tissue from this specimen was stored at the North Carolina Museum of Natural 118 Sciences under the identifier NCSM84230. Three types of whole genome sequencing data were 119 generated: Illumina, PacBio, and Oxford Nanopore. Illumina sequencing libraries were 120 constructed with the Illumina Nextera kit. Five replicate Illumina sequencing libraries were 121 prepared, multiplexed using barcoded adapters, and then sequenced at the USC Molecular 122 Genomics Core on an Illumina NextSeq using the 150 bp paired-end kit. PacBio libraries were 123 generated and sequenced on a Pacbio Sequel by the UC Irvine Genomics High-Throughput 124 facility. We also generated Oxford Nanopore long-read libraries, which we sequenced on two 125 2D DNA chips using a Mk1b Oxford Nanopore Minion. More information about the sequencing 126 data is provided in Supplementary Table 1. 127 Assembly was performed using all long- and short-read sequencing data, as MaSuRCA 128 includes Quorum to perform internal error correction we used the raw read data. After trying 129 multiple assemblers, we found that MaSuRCA v3.2.1 (ZIMIN et al. 2013) produced the most 130 contiguous assembly. Specifically, we employed a kmer size of 51, a cgwError rate of 0.15, and 131 a jellyfish hash size of 6x1010. 132 Following completion of the assembly, duplicate contigs were identified using the LAST 133 aligner (KIELBASA et al.
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