A deep dive into genome assemblies of non-vertebrate animals
Diving, and even digging, into the wild jungle of annotation pathways for non-vertebrate animalsRecommended by Francois Sabot based on reviews by Yann Bourgeois, Benjamin Istace, Cécile Monat and Valentina Peona
In their paper, Guiglielmoni et al. propose we pick up our snorkels and palms and take "A deep dive into genome assemblies of non-vertebrate animals" (1). Indeed, while numerous assembly-related tools were developed and tested for human genomes (or at least vertebrates such as mice), very few were tested on non-vertebrate animals so far. Moreover, most of the benchmarks are aimed at raw assembly tools, and very few offer a guide from raw reads to an almost finished assembly, including quality control and phasing.
This huge and exhaustive review starts with an overview of the current sequencing technologies, followed by the theory of the different approaches for assembly and their implementation. For each approach, the authors present some of the most representative tools, as well as the limits of the approach.
The authors additionally present all the steps required to obtain an almost complete assembly at a chromosome-scale, with all the different technologies currently available for scaffolding, QC, and phasing, and the way these tools can be applied to non-vertebrates animals. Finally, they propose some useful advice on the choice of the different approaches (but not always tools, see below), and advocate for a robust genome database with all information on the way the assembly was obtained.
This review is a very complete one for now and is a very good starting point for any student or scientist interested to start working on genome assembly, from either model or non-model organisms. However, the authors do not provide a list of tools or a benchmark of them as a recommendation. Why? Because such a proposal may be obsolete in less than a year.... Indeed, with the explosion of the 3rd generation of sequencing technology, assembly tools (from different steps) are constantly evolving, and their relative performance increases on a monthly basis. In addition, some tools are really efficient at the time of a review or of an article, but are not further developed later on, and thus will not evolve with the technology. We have all seen it with wonderful tools such as Chiron (2) or TopHat (3), which were very promising ones, but cannot be developed further due to the stop of the project, the end of the contract of the post-doc in charge of the development, or the decision of the developer to switch to another paradigm. Such advice would, therefore, need to be constantly updated.
Thus, the manuscript from Guiglielmoni et al will be an almost intemporal one (up to the next sequencing revolution at last), and as they advocated for a more informed genome database, I think we should consider a rolling benchmarking system (tools, genome and sequence dataset) allowing to keep the performance of the tools up-to-date, and to propose the best set of assembly tools for a given type of genome.
1. Guiglielmoni N, Rivera-Vicéns R, Koszul R, Flot J-F (2022) A Deep Dive into Genome Assemblies of Non-vertebrate Animals. Preprints, 2021110170, ver. 3 peer-reviewed and recommended by Peer Community in Genomics. https://doi.org/10.20944/preprints202111.0170
2. Teng H, Cao MD, Hall MB, Duarte T, Wang S, Coin LJM (2018) Chiron: translating nanopore raw signal directly into nucleotide sequence using deep learning. GigaScience, 7, giy037. https://doi.org/10.1093/gigascience/giy037
3. Trapnell C, Pachter L, Salzberg SL (2009) TopHat: discovering splice junctions with RNA-Seq. Bioinformatics, 25, 1105–1111. https://doi.org/10.1093/bioinformatics/btp120
Phylogenetics in the Genomic Era
“Phylogenetics in the Genomic Era” brings together experts in the field to present a comprehensive synthesisRecommended by Robert Waterhouse and Karen Meusemann
E-book: Phylogenetics in the Genomic Era (Scornavacca et al. 2021)
This book was not peer-reviewed by PCI Genomics. It has undergone an internal review by the editors.
Accurate reconstructions of the relationships amongst species and the genes encoded in their genomes are an essential foundation for almost all evolutionary inferences emerging from downstream analyses. Molecular phylogenetics has developed as a field over many decades to build suites of models and methods to reconstruct reliable trees that explain, support, or refute such inferences. The genomic era has brought new challenges and opportunities to the field, opening up new areas of research and algorithm development to take advantage of the accumulating large-scale data. Such ‘big-data’ phylogenetics has come to be known as phylogenomics, which broadly aims to connect molecular and evolutionary biology research to address questions centred on relationships amongst taxa, mechanisms of molecular evolution, and the biological functions of genes and other genomic elements. This book brings together experts in the field to present a comprehensive synthesis of Phylogenetics in the Genomic Era, covering key conceptual and methodological aspects of how to build accurate phylogenies and how to apply them in molecular and evolutionary research. The paragraphs below briefly summarise the five constituent parts of the book, highlighting the key concepts, methods, and applications that each part addresses. Being organised in an accessible style, while presenting details to provide depth where necessary, and including guides describing real-world examples of major phylogenomic tools, this collection represents an invaluable resource, particularly for students and newcomers to the field of phylogenomics.
Part 1: Phylogenetic analyses in the genomic era
Modelling how sequences evolve is a fundamental cornerstone of phylogenetic reconstructions. This part of the book introduces the reader to phylogenetic inference methods and algorithmic optimisations in the contexts of Markov, Maximum Likelihood, and Bayesian models of sequence evolution. The main concepts and theoretical considerations are mapped out for probabilistic Markov models, efficient tree building with Maximum Likelihood methods, and the flexibility and robustness of Bayesian approaches. These are supported with practical examples of phylogenomic applications using the popular tools RAxML and PhyloBayes. By considering theoretical, algorithmic, and practical aspects, these chapters provide readers with a holistic overview of the challenges and recent advances in developing scalable phylogenetic analyses in the genomic era.
Part 2: Data quality, model adequacy
This part focuses on the importance of considering the appropriateness of the evolutionary models used and the accuracy of the underlying molecular and genomic data. Both these aspects can profoundly affect the results when applying current phylogenomic methods to make inferences about complex biological and evolutionary processes. A clear example is presented for methods for building multiple sequence alignments and subsequent filtering approaches that can greatly impact phylogeny inference. The importance of error detection in (meta)barcode sequencing data is also highlighted, with solutions offered by the MACSE_BARCODE pipeline for accurate taxonomic assignments. Orthology datasets are essential markers for phylogenomic inferences, but the overview of concepts and methods presented shows that they too face challenges with respect to model selection and data quality. Finally, an innovative approach using ancestral gene order reconstructions provides new perspectives on how to assess gene tree accuracy for phylogenomic analyses. By emphasising through examples the importance of using appropriate evolutionary models and assessing input data quality, these chapters alert readers to key limitations that the field as a whole strives to address.
Part 3: Resolving phylogenomic conflicts
Conflicting phylogenetic signals are commonplace and may derive from statistical or systematic bias. This part of the book addresses possible causes of conflict, discordance between gene trees and species trees and how processes that lead to such conflicts can be described by phylogenetic models. Furthermore, it provides an overview of various models and methods with examples in phylogenomics including their pros and cons. Outlined in detail is the multispecies coalescent model (MSC) and its applications in phylogenomics. An interesting aspect is that different phylogenetic signals leading to conflict are in fact a key source of information rather than a problem that can – and should – be used to point to events like introgression or hybridisation, highlighting possible future trends in this research area. Last but not least, this part of the book also addresses inferring species trees by concatenating single multiple sequence alignments (gene alignments) versus inferring the species tree based on ensembles of single gene trees pointing out advantages and disadvantages of both approaches. As an important take home message from these chapters, it is recommended to be flexible and identify the most appropriate approach for each dataset to be analysed since this may tremendously differ depending on the dataset, setting, taxa, and phylogenetic level addressed by the researcher.
Part 4: Functional evolutionary genomics
In this part of the book the focus shifts to functional considerations of phylogenomics approaches both in terms of molecular evolution and adaptation and with respect to gene expression. The utility of multi-species analysis is clearly presented in the context of annotating functional genomic elements through quantifying evolutionary constraint and protein-coding potential. An historical perspective on characterising rates of change highlights how phylogenomic datasets help to understand the modes of molecular evolution across the genome, over time, and between lineages. These are contextualised with respect to the specific aim of detecting signatures of adaptation from protein-coding DNA alignments using the example of the MutSelDP-ω∗ model. This is extended with the presentation of the generally rare case of adaptive sequence convergence, where consideration of appropriate models and knowledge of gene functions and phenotypic effects are needed. Constrained or relaxed, selection pressures on sequence or copy-number affect genomic elements in different ways, making the very concept of function difficult to pin down despite it being fundamental to relate the genome to the phenotype and organismal fitness. Here gene expression provides a measurable intermediate, for which the Expression Comparison tool from the Bgee suite allows exploration of expression patterns across multiple animal species taking into account anatomical homology. Overall, phylogenomics applications in functional evolutionary genomics build on a rich theoretical history from molecular analyses where integration with knowledge of gene functions is challenging but critical.
Part 5: Phylogenomic applications
Rather than attempting to review the full extent of applications linked to phylogenomics, this part of the book focuses on providing detailed specific insights into selected examples and methods concerning i) estimating divergence times, and ii) species delimitation in the era of ‘omics’ data. With respect to estimating divergence times, an exemplary overview is provided for fossil data recovered from geological records, either using fossil data as calibration points with an extant-species-inferred phylogeny, or using a fossilised birth-death process as a mechanistic model that accounts for lineage diversification. Included is a tutorial for a joint approach to infer phylogenies and estimate divergence times using the RevBayes software with various models implemented for different applications and datasets incorporating molecular and morphological data. An interesting excursion is outlined focusing on timescale estimates with respect to viral evolution introducing BEAGLE, a high-performance likelihood-calculation platform that can be used on multi-core systems. As a second major subject, species delimitation is addressed since currently the increasing amount of available genomic data enables extensive inferences, for instance about the degree of genetic isolation among species and ancient and recent introgression events. Describing the history of molecular species delimitation up to the current genomic era and presenting widely used computational methods incorporating single- and multi-locus genomic data, pros and cons are addressed. Finally, a proposal for a new method for delimiting species based on empirical criteria is outlined. In the closing chapter of this part of the book, BPP (Bayesian Markov chain Monte Carlo program) for analysing multi-locus sequence data under the multispecies coalescent (MSC) model with and without introgression is introduced, including a tutorial. These examples together provide accessible details on key conceptual and methodological aspects related to the application of phylogenetics in the genomic era.
Scornavacca C, Delsuc F, Galtier N (2021) Phylogenetics in the Genomic Era. https://hal.inria.fr/PGE/
Chromosomal rearrangements with stable repertoires of genes and transposable elements in an invasive forest-pathogenic fungus
Comparative genomics in the chestnut blight fungus Cryphonectria parasitica reveals large chromosomal rearrangements and a stable genome organizationRecommended by Sebastien Duplessis based on reviews by Benjamin Schwessinger and 1 anonymous reviewer
About twenty-five years after the sequencing of the first fungal genome and a dozen years after the first plant pathogenic fungi genomes were sequenced, unprecedented international efforts have led to an impressive collection of genomes available for the community of mycologists in international databases (Goffeau et al. 1996, Dean et al. 2005; Spatafora et al. 2017). For instance, to date, the Joint Genome Institute Mycocosm database has collected more than 2,100 fungal genomes over the fungal tree of life (https://mycocosm.jgi.doe.gov). Such resources are paving the way for comparative genomics, population genomics and phylogenomics to address a large panel of questions regarding the biology and the ecology of fungal species. Early on, population genomics applied to pathogenic fungi revealed a great diversity of genome content and organization and a wide variety of variants and rearrangements (Raffaele and Kamoun 2012, Hartmann 2022). Such plasticity raises questions about how to choose a representative genome to serve as an ideal reference to address pertinent biological questions.
Cryphonectria parasitica is a fungal pathogen that is infamous for the devastation of chestnut forests in North America after its accidental introduction more than a century ago (Anagnostakis 1987). Since then, it has been a quarantine species under surveillance in various parts of the world. As for other fungi causing diseases on forest trees, the study of adaptation to its host in the forest ecosystem and of its reproduction and dissemination modes is more complex than for crop-targeting pathogens. A first reference genome was published in 2020 for the chestnut blight fungus C. parasitica strain EP155 in the frame of an international project with the DOE JGI (Crouch et al. 2020). Another genome was then sequenced from the French isolate YVO003, which showed a few differences in the assembly suggesting possible rearrangements (Demené et al. 2019). Here the sequencing of a third isolate ESM015 from the native area of C. parasitica in Japan allows to draw broader comparative analysis and particularly to compare between native and introduced isolates (Demené et al. 2022).
Demené and collaborators report on a new genome sequence using up-to-date long-read sequencing technologies and they provide an improved genome assembly. Comparison with previously published C. parasitica genomes did not reveal dramatic changes in the overall chromosomal landscapes, but large rearrangements could be spotted. Despite these rearrangements, the genome content and organization – i.e. genes and repeats – remain stable, with a limited number of genes gains and losses. As in any fungal plant pathogen genome, the repertoire of candidate effectors predicted among secreted proteins was more particularly scrutinized. Such effector genes have previously been reported in other pathogens in repeat-enriched plastic genomic regions with accelerated evolutionary rates under the pressure of the host immune system (Raffaele and Kamoun 2012). Demené and collaborators established a list of priority candidate effectors in the C. parasitica gene catalog likely involved in the interaction with the host plant which will require more attention in future functional studies. Six major inter-chromosomal translocations were detected and are likely associated with double break strands repairs. The authors speculate on the possible effects that these translocations may have on gene organization and expression regulation leading to dramatic phenotypic changes in relation to introduction and invasion in new continents and the impact regarding sexual reproduction in this fungus (Demené et al. 2022).
I recommend this article not only because it is providing an improved assembly of a reference genome for C. parasitica, but also because it adds diversity in terms of genome references availability, with a third high-quality assembly. Such an effort in the tree pathology community for a pathogen under surveillance is of particular importance for future progress in post-genomic analysis, e.g. in further genomic population studies (Hartmann 2022).
Anagnostakis SL (1987) Chestnut Blight: The Classical Problem of an Introduced Pathogen. Mycologia, 79, 23–37. https://doi.org/10.2307/3807741
Crouch JA, Dawe A, Aerts A, Barry K, Churchill ACL, Grimwood J, Hillman BI, Milgroom MG, Pangilinan J, Smith M, Salamov A, Schmutz J, Yadav JS, Grigoriev IV, Nuss DL (2020) Genome Sequence of the Chestnut Blight Fungus Cryphonectria parasitica EP155: A Fundamental Resource for an Archetypical Invasive Plant Pathogen. Phytopathology®, 110, 1180–1188. https://doi.org/10.1094/PHYTO-12-19-0478-A
Dean RA, Talbot NJ, Ebbole DJ, Farman ML, Mitchell TK, Orbach MJ, Thon M, Kulkarni R, Xu J-R, Pan H, Read ND, Lee Y-H, Carbone I, Brown D, Oh YY, Donofrio N, Jeong JS, Soanes DM, Djonovic S, Kolomiets E, Rehmeyer C, Li W, Harding M, Kim S, Lebrun M-H, Bohnert H, Coughlan S, Butler J, Calvo S, Ma L-J, Nicol R, Purcell S, Nusbaum C, Galagan JE, Birren BW (2005) The genome sequence of the rice blast fungus Magnaporthe grisea. Nature, 434, 980–986. https://doi.org/10.1038/nature03449
Demené A., Laurent B., Cros-Arteil S., Boury C. and Dutech C. 2022. Chromosomal rearrangements with stable repertoires of genes and transposable elements in an invasive forest-pathogenic fungus. bioRxiv, 2021.03.09.434572, ver.6 peer-reviewed and recommended by Peer Community in Genomics. https://doi.org/10.1101/2021.03.09.434572
Goffeau A, Barrell BG, Bussey H, Davis RW, Dujon B, Feldmann H, Galibert F, Hoheisel JD, Jacq C, Johnston M, Louis EJ, Mewes HW, Murakami Y, Philippsen P, Tettelin H, Oliver SG (1996) Life with 6000 Genes. Science, 274, 546–567. https://doi.org/10.1126/science.274.5287.546
Hartmann FE (2022) Using structural variants to understand the ecological and evolutionary dynamics of fungal plant pathogens. New Phytologist, 234, 43–49. https://doi.org/10.1111/nph.17907
Raffaele S, Kamoun S (2012) Genome evolution in filamentous plant pathogens: why bigger can be better. Nature Reviews Microbiology, 10, 417–430. https://doi.org/10.1038/nrmicro2790
Spatafora JW, Aime MC, Grigoriev IV, Martin F, Stajich JE, Blackwell M (2017) The Fungal Tree of Life: from Molecular Systematics to Genome-Scale Phylogenies. Microbiology Spectrum, 5, 5.5.03. https://doi.org/10.1128/microbiolspec.FUNK-0053-2016
Fine-scale quantification of GC-biased gene conversion intensity in mammals
A systematic approach to the study of GC-biased gene conversion in mammalsRecommended by Carina Farah Mugal based on reviews by David Castellano, Fanny Pouyet and 1 anonymous reviewer
The role of GC-biased gene conversion (gBGC) in molecular evolution has interested scientists for the last two decades since its discovery in 1999 (Eyre-Walker 1999; Galtier et al. 2001). gBGC is a process that is associated with meiotic recombination, and is characterized by a transmission distortion in favor of G and C over A and T alleles at GC/AT heterozygous sites that occur in the vicinity of recombination-inducing double-strand breaks (Duret and Galtier 2009; Mugal et al. 2015). This transmission distortion results in a fixation bias of G and C alleles, equivalent to directional selection for G and C (Nagylaki 1983). The fixation bias subsequently leads to a correlation between recombination rate and GC content across the genome, which has served as indirect evidence for the prevalence of gBGC in many organisms. The fixation bias also produces shifts in the allele frequency spectrum (AFS) towards higher frequencies of G and C alleles.
These molecular signatures of gBGC provide a means to quantify the strength of gBGC and study its variation among species and across the genome. Following this idea, first Lartillot (2013) and Capra et al. (2013) developed phylogenetic methodology to quantify gBGC based on substitutions, and De Maio et al. (2013) combined information on polymorphism into a phylogenetic setting. Complementary to the phylogenetic methods, later Glemin et al. (2015) developed a method that draws information solely from polymorphism data and the shape of the AFS. Application of these methods to primates (Capra et al. 2013; De Maio et al. 2013; Glemin et al. 2015) and mammals (Lartillot 2013) supported the notion that variation in the strength of gBGC across the genome reflects the dynamics of the recombination landscape, while variation among species correlates with proxies of the effective population size. However, application of the polymorphism-based method by Glemin et al. (2015) to distantly related Metazoa did not confirm the correlation with effective population size (Galtier et al. 2018).
Here, Galtier (2021) introduces a novel phylogenetic approach applicable to the study of closely related species. Specifically, Galtier introduces a statistical framework that enables the systematic study of variation in the strength of gBGC among species and among genes. In addition, Galtier assesses fine-scale variation of gBGC across the genome by means of spatial autocorrelation analysis. This puts Galtier in a position to study variation in the strength of gBGC at three different scales, i) among species, ii) among genes, and iii) within genes. Galtier applies his method to four families of mammals, Hominidae, Cercopithecidae, Bovidae, and Muridae and provides a thorough discussion of his findings and methodology.
Galtier found that the strength of gBGC correlates with proxies of the effective population size (Ne), but that the slope of the relationship differs among the four families of mammals. Given the relationship between the population-scaled strength of gBGC B = 4Neb, this finding suggests that the conversion bias (b) could vary among mammalian species. Variation in b could either result from differences in the strength of the transmission distortion (Galtier et al. 2018) or evolutionary changes in the rate of recombination (Boman et al. 2021). Alternatively, Galtier suggests that also systematic variation in proxies of Ne could lead to similar observations. Finally, the present study reports intriguing inter-species differences between the extent of variation in the strength of gBGC among and within genes, which are interpreted in consideration of the recombination dynamics in mammals.
Boman J, Mugal CF, Backström N (2021) The Effects of GC-Biased Gene Conversion on Patterns of Genetic Diversity among and across Butterfly Genomes. Genome Biology and Evolution, 13. https://doi.org/10.1093/gbe/evab064
Capra JA, Hubisz MJ, Kostka D, Pollard KS, Siepel A (2013) A Model-Based Analysis of GC-Biased Gene Conversion in the Human and Chimpanzee Genomes. PLOS Genetics, 9, e1003684. https://doi.org/10.1371/journal.pgen.1003684
De Maio N, Schlötterer C, Kosiol C (2013) Linking Great Apes Genome Evolution across Time Scales Using Polymorphism-Aware Phylogenetic Models. Molecular Biology and Evolution, 30, 2249–2262. https://doi.org/10.1093/molbev/mst131
Duret L, Galtier N (2009) Biased Gene Conversion and the Evolution of Mammalian Genomic Landscapes. Annual Review of Genomics and Human Genetics, 10, 285–311. https://doi.org/10.1146/annurev-genom-082908-150001
Eyre-Walker A (1999) Evidence of Selection on Silent Site Base Composition in Mammals: Potential Implications for the Evolution of Isochores and Junk DNA. Genetics, 152, 675–683. https://doi.org/10.1093/genetics/152.2.675
Galtier N (2021) Fine-scale quantification of GC-biased gene conversion intensity in mammals. bioRxiv, 2021.05.05.442789, ver. 5 peer-reviewed and recommended by Peer Community in Genomics. https://doi.org/10.1101/2021.05.05.442789
Galtier N, Piganeau G, Mouchiroud D, Duret L (2001) GC-Content Evolution in Mammalian Genomes: The Biased Gene Conversion Hypothesis. Genetics, 159, 907–911. https://doi.org/10.1093/genetics/159.2.907
Galtier N, Roux C, Rousselle M, Romiguier J, Figuet E, Glémin S, Bierne N, Duret L (2018) Codon Usage Bias in Animals: Disentangling the Effects of Natural Selection, Effective Population Size, and GC-Biased Gene Conversion. Molecular Biology and Evolution, 35, 1092–1103. https://doi.org/10.1093/molbev/msy015
Glémin S, Arndt PF, Messer PW, Petrov D, Galtier N, Duret L (2015) Quantification of GC-biased gene conversion in the human genome. Genome Research, 25, 1215–1228. https://doi.org/10.1101/gr.185488.114
Lartillot N (2013) Phylogenetic Patterns of GC-Biased Gene Conversion in Placental Mammals and the Evolutionary Dynamics of Recombination Landscapes. Molecular Biology and Evolution, 30, 489–502. https://doi.org/10.1093/molbev/mss239
Mugal CF, Weber CC, Ellegren H (2015) GC-biased gene conversion links the recombination landscape and demography to genomic base composition. BioEssays, 37, 1317–1326. https://doi.org/10.1002/bies.201500058
Nagylaki T (1983) Evolution of a finite population under gene conversion. Proceedings of the National Academy of Sciences, 80, 6278–6281. https://doi.org/10.1073/pnas.80.20.6278
Genetic mapping of sex and self-incompatibility determinants in the androdioecious plant Phillyrea angustifolia
Identification of distinct YX-like loci for sex determination and self-incompatibility in an androdioecious shrubRecommended by Tatiana Giraud and Ricardo C. Rodríguez de la Vega based on reviews by 2 anonymous reviewers
A wide variety of systems have evolved to control mating compatibility in sexual organisms. Their genetic determinism and the factors controlling their evolution represent fascinating questions in evolutionary biology and genomics. The plant Phillyrea angustifolia (Oleaeceae family) represents an exciting model organism, as it displays two distinct and rare mating compatibility systems : 1) males and hermaphrodites co-occur in populations of this shrub (a rare system called androdioecy), while the evolution and maintenance of purely hermaphroditic plants or mixtures of females and hermaphrodites (a system called gynodioecy) are easier to explain ; 2) a homomorphic diallelic self-incompatibility system acts in hermaphrodites, while such systems are usually multi-allelic, as rare alleles are advantageous, being compatible with all other alleles. Previous analyses of crosses brought some interesting answers to these puzzles, showing that males benefit from the ability to mate with all hermaphrodites regardless of their allele at the self-incompatibility system, and suggesting that both sex and self incompatibility are determined by XY-like genetic systems, i.e. with each a dominant allele; homozygotes for a single allele and heterozygotes therefore co-occur in natural populations at both sex and self-incompatibility loci .
Here, Carré et al. used genotyping-by-sequencing to build a genome linkage map of P. angustifolia . The elegant and original use of a probabilistic model of segregating alleles (implemented in the SEX-DETector method) allowed to identify both the sex and self-incompatibility loci , while this tool was initially developed for detecting sex-linked genes in species with strictly separated sexes (dioecy) . Carré et al.  confirmed that the sex and self-incompatibility loci are located in two distinct linkage groups and correspond to XY-like systems. A comparison with the genome of the closely related Olive tree indicated that their self-incompatibility systems were homologous. Such a XY-like system represents a rare genetic determination mechanism for self-incompatibility and has also been recently found to control mating types in oomycetes .
This study  paves the way for identifying the genes controlling the sex and self-incompatibility phenotypes and for understanding why and how self-incompatibility is only expressed in hermaphrodites and not in males. It will also be fascinating to study more finely the degree and extent of genomic differentiation at these two loci and to assess whether recombination suppression has extended stepwise away from the sex and self-incompatibility loci, as can be expected under some hypotheses, such as the sheltering of deleterious alleles near permanently heterozygous alleles . Furthermore, the co-occurrence in P. angustifolia of sex and mating types can contribute to our understanding of the factor controlling their evolution .
 Saumitou-Laprade P, Vernet P, Vassiliadis C, Hoareau Y, Magny G de, Dommée B, Lepart J (2010) A Self-Incompatibility System Explains High Male Frequencies in an Androdioecious Plant. Science, 327, 1648–1650. https://doi.org/10.1126/science.1186687
 Pannell JR, Voillemot M (2015) Plant Mating Systems: Female Sterility in the Driver’s Seat. Current Biology, 25, R511–R514. https://doi.org/10.1016/j.cub.2015.04.044
 Billiard S, Husse L, Lepercq P, Godé C, Bourceaux A, Lepart J, Vernet P, Saumitou-Laprade P (2015) Selfish male-determining element favors the transition from hermaphroditism to androdioecy. Evolution, 69, 683–693. https://doi.org/10.1111/evo.12613
 Carre A, Gallina S, Santoni S, Vernet P, Gode C, Castric V, Saumitou-Laprade P (2021) Genetic mapping of sex and self-incompatibility determinants in the androdioecious plant Phillyrea angustifolia. bioRxiv, 2021.04.15.439943, ver. 7 peer-reviewed and recommended by Peer Community in Genomics. https://doi.org/10.1101/2021.04.15.439943
 Muyle A, Käfer J, Zemp N, Mousset S, Picard F, Marais GA (2016) SEX-DETector: A Probabilistic Approach to Study Sex Chromosomes in Non-Model Organisms. Genome Biology and Evolution, 8, 2530–2543. https://doi.org/10.1093/gbe/evw172
 Dussert Y, Legrand L, Mazet ID, Couture C, Piron M-C, Serre R-F, Bouchez O, Mestre P, Toffolatti SL, Giraud T, Delmotte F (2020) Identification of the First Oomycete Mating-type Locus Sequence in the Grapevine Downy Mildew Pathogen, Plasmopara viticola. Current Biology, 30, 3897-3907.e4. https://doi.org/10.1016/j.cub.2020.07.057
 Jay P, Tezenas E, Giraud T (2021) A deleterious mutation-sheltering theory for the evolution of sex chromosomes and supergenes. bioRxiv, 2021.05.17.444504. https://doi.org/10.1101/2021.05.17.444504
 Billiard S, López-Villavicencio M, Devier B, Hood ME, Fairhead C, Giraud T (2011) Having sex, yes, but with whom? Inferences from fungi on the evolution of anisogamy and mating types. Biological Reviews, 86, 421–442. https://doi.org/10.1111/j.1469-185X.2010.00153.x
TransPi - a comprehensive TRanscriptome ANalysiS PIpeline for de novo transcriptome assembly
TransPI: A balancing act between transcriptome assemblersRecommended by Oleg Simakov based on reviews by Juan Daniel Montenegro Cabrera and Gustavo Sanchez
Ever since the introduction of the first widely usable assemblers for transcriptomic reads (Huang and Madan 1999; Schulz et al. 2012; Simpson et al. 2009; Trapnell et al. 2010, and many more), it has been a technical challenge to compare different methods and to choose the “right” or “best” assembly. It took years until the first widely accepted set of benchmarks beyond raw statistical evaluation became available (e.g., Parra, Bradnam, and Korf 2007; Simão et al. 2015). However, an approach to find the right balance between the number of transcripts or isoforms vs. evolutionary completeness measures has been lacking. This has been particularly pronounced in the field of non-model organisms (i.e., wild species that lack a genomic reference). Often, studies in this area employed only one set of assembly tools (the most often used to this day being Trinity, Haas et al. 2013; Grabherr et al. 2011). While it was relatively straightforward to obtain an initial assembly, its validation, annotation, as well its application to the particular purpose that the study was designed for (phylogenetics, differential gene expression, etc) lacked a clear workflow. This led to many studies using a custom set of tools with ensuing various degrees of reproducibility.
TransPi (Rivera-Vicéns et al. 2021) fills this gap by first employing a meta approach using several available transcriptome assemblers and algorithms to produce a combined and reduced transcriptome assembly, then validating and annotating the resulting transcriptome. Notably, TransPI performs an extensive analysis/detection of chimeric transcripts, the results of which show that this new tool often produces fewer misassemblies compared to Trinity. TransPI not only generates a final report that includes the most important plots (in clickable/zoomable format) but also stores all relevant intermediate files, allowing advanced users to take a deeper look and/or experiment with different settings. As running TransPi is largely automated (including its installation via several popular package managers), it is very user-friendly and is likely to become the new "gold standard" for transcriptome analyses, especially of non-model organisms.
Grabherr MG, Haas BJ, Yassour M, Levin JZ, Thompson DA, Amit I, Adiconis X, Fan L, Raychowdhury R, Zeng Q, Chen Z, Mauceli E, Hacohen N, Gnirke A, Rhind N, di Palma F, Birren BW, Nusbaum C, Lindblad-Toh K, Friedman N, Regev A (2011) Full-length transcriptome assembly from RNA-Seq data without a reference genome. Nature Biotechnology, 29, 644–652. https://doi.org/10.1038/nbt.1883
Haas BJ, Papanicolaou A, Yassour M, Grabherr M, Blood PD, Bowden J, Couger MB, Eccles D, Li B, Lieber M, MacManes MD, Ott M, Orvis J, Pochet N, Strozzi F, Weeks N, Westerman R, William T, Dewey CN, Henschel R, LeDuc RD, Friedman N, Regev A (2013) De novo transcript sequence reconstruction from RNA-seq using the Trinity platform for reference generation and analysis. Nature Protocols, 8, 1494–1512. https://doi.org/10.1038/nprot.2013.084
Huang X, Madan A (1999) CAP3: A DNA Sequence Assembly Program. Genome Research, 9, 868–877. https://doi.org/10.1101/gr.9.9.868
Parra G, Bradnam K, Korf I (2007) CEGMA: a pipeline to accurately annotate core genes in eukaryotic genomes. Bioinformatics, 23, 1061–1067. https://doi.org/10.1093/bioinformatics/btm071
Rivera-Vicéns RE, Garcia-Escudero CA, Conci N, Eitel M, Wörheide G (2021) TransPi – a comprehensive TRanscriptome ANalysiS PIpeline for de novo transcriptome assembly. bioRxiv, 2021.02.18.431773, ver. 3 peer-reviewed and recommended by Peer Community in Genomics. https://doi.org/10.1101/2021.02.18.431773
Schulz MH, Zerbino DR, Vingron M, Birney E (2012) Oases: robust de novo RNA-seq assembly across the dynamic range of expression levels. Bioinformatics, 28, 1086–1092. https://doi.org/10.1093/bioinformatics/bts094
Simão FA, Waterhouse RM, Ioannidis P, Kriventseva EV, Zdobnov EM (2015) BUSCO: assessing genome assembly and annotation completeness with single-copy orthologs. Bioinformatics, 31, 3210–3212. https://doi.org/10.1093/bioinformatics/btv351
Simpson JT, Wong K, Jackman SD, Schein JE, Jones SJM, Birol İ (2009) ABySS: A parallel assembler for short read sequence data. Genome Research, 19, 1117–1123. https://doi.org/10.1101/gr.089532.108
Trapnell C, Williams BA, Pertea G, Mortazavi A, Kwan G, van Baren MJ, Salzberg SL, Wold BJ, Pachter L (2010) Transcript assembly and quantification by RNA-Seq reveals unannotated transcripts and isoform switching during cell differentiation. Nature Biotechnology, 28, 511–515. https://doi.org/10.1038/nbt.1621
A pipeline to detect the relationship between transposable elements and adjacent genes in host genomes
A new tool to cross and analyze TE and gene annotationsRecommended by Emmanuelle Lerat based on reviews by 2 anonymous reviewers
Transposable elements (TEs) are important components of genomes. Indeed, they are now recognized as having a major role in gene and genome evolution (Biémont 2010). In particular, several examples have shown that the presence of TEs near genes may influence their functioning, either by recruiting particular epigenetic modifications (Guio et al. 2018) or by directly providing new regulatory sequences allowing new expression patterns (Chung et al. 2007; Sundaram et al. 2014). Therefore, the study of the interaction between TEs and their host genome requires tools to easily cross-annotate both types of entities. In particular, one needs to be able to identify all TEs located in the close vicinity of genes or inside them. Such task may not always be obvious for many biologists, as it requires informatics knowledge to develop their own script codes.
In their work, Meguerdichian et al. (2021) propose a command-line pipeline that takes as input the annotations of both genes and TEs for a given genome, then detects and reports the positional relationships between each TE insertion and their closest genes. The results are processed into an R script to provide tables displaying some statistics and graphs to visualize these relationships.
This tool has the potential to be very useful for performing preliminary analyses before studying the impact of TEs on gene functioning, especially for biologists. Indeed, it makes it possible to identify genes close to TE insertions. These identified genes could then be specifically considered in order to study in more detail the link between the presence of TEs and their functioning. For example, the identification of TEs close to genes may allow to determine their potential role on gene expression.
Biémont C (2010). A brief history of the status of transposable elements: from junk DNA to major players in evolution. Genetics, 186, 1085–1093. https://doi.org/10.1534/genetics.110.124180
Chung H, Bogwitz MR, McCart C, Andrianopoulos A, ffrench-Constant RH, Batterham P, Daborn PJ (2007). Cis-regulatory elements in the Accord retrotransposon result in tissue-specific expression of the Drosophila melanogaster insecticide resistance gene Cyp6g1. Genetics, 175, 1071–1077. https://doi.org/10.1534/genetics.106.066597
Guio L, Vieira C, González J (2018). Stress affects the epigenetic marks added by natural transposable element insertions in Drosophila melanogaster. Scientific Reports, 8, 12197. https://doi.org/10.1038/s41598-018-30491-w
Meguerditchian C, Ergun A, Decroocq V, Lefebvre M, Bui Q-T (2021). A pipeline to detect the relationship between transposable elements and adjacent genes in host genomes. bioRxiv, 2021.02.25.432867, ver. 4 peer-reviewed and recommended by Peer Community In Genomics. https://doi.org/10.1101/2021.02.25.432867
Sundaram V, Cheng Y, Ma Z, Li D, Xing X, Edge P, Snyder MP, Wang T (2014). Widespread contribution of transposable elements to the innovation of gene regulatory networks. Genome Research, 24, 1963–1976. https://doi.org/10.1101/gr.168872.113
A primer and discussion on DNA-based microbiome data and related bioinformatics analyses
A hitchhiker’s guide to DNA-based microbiome analysisRecommended by Danny Ionescu based on reviews by Rafael Cuadrat, Nicolas Pollet and 1 anonymous reviewer
In the last two decades, microbial research in its different fields has been increasingly focusing on microbiome studies. These are defined as studies of complete assemblages of microorganisms in given environments and have been benefiting from increases in sequencing length, quality, and yield, coupled with ever-dropping prices per sequenced nucleotide. Alongside localized microbiome studies, several global collaborative efforts have emerged, including the Human Microbiome Project , the Earth Microbiome Project , the Extreme Microbiome Project, and MetaSUB .
Coupled with the development of sequencing technologies and the ever-increasing amount of data output, multiple standalone or online bioinformatic tools have been designed to analyze these data. Often these tools have been focusing on either of two main tasks: 1) Community analysis, providing information on the organisms present in the microbiome, or 2) Functionality, in the case of shotgun metagenomic data, providing information on the metabolic potential of the microbiome. Bridging between the two types of data, often extracted from the same dataset, is typically a daunting task that has been addressed by a handful of tools only.
The extent of tools and approaches to analyze microbiome data is great and may be overwhelming to researchers new to microbiome or bioinformatic studies. In their paper “A primer and discussion on DNA-based microbiome data and related bioinformatics analyses”, Douglas and Langille  guide us through the different sequencing approaches useful for microbiome studies. alongside their advantages and caveats and a selection of tools to analyze these data, coupled with examples from their own field of research.
Standing out in their primer-style review is the emphasis on the coupling between taxonomic/phylogenetic identification of the organisms and their functionality. This type of analysis, though highly important to understand the role of different microorganisms in an environment as well as to identify potential functional redundancy, is often not conducted. For this, the authors identify two approaches. The first, using shotgun metagenomics, has higher chances of attributing a function to the correct taxon. The second, using amplicon sequencing of marker genes, allows for a deeper coverage of the microbiome at a lower cost, and extrapolates the amplicon data to close relatives with a sequenced genome. As clearly stated, this approach makes the leap between taxonomy and functionality and has been shown to be erroneous in cases where the core genome of the bacterial genus or family does not encompass the functional diversity of the different included species. This practice was already common before the genomic era, but its accuracy is improving thanks to the increasing availability of sequenced reference genomes from cultures, environmentally picked single cells or metagenome-assembled genome.
In addition to their description of standalone tools useful for linking taxonomy and functionality, one should mention the existence of online tools that may appeal to researchers who do not have access to adequate bioinformatics infrastructure. Among these are the Integrated Microbial Genomes and Microbiomes (IMG) from the Joint Genome Institute , KBase  and MG-RAST .
A second important point arising from this review is the need for standardization in microbiome data analyses and the complexity of achieving this. As Douglas and Langille  state, this has been previously addressed, highlighting the variability in results obtained with different tools. It is often the case that papers describing new bioinformatic tools display their superiority relative to existing alternatives, potentially misleading newcomers to the field that the newest tool is the best and only one to be used. This is often not the case, and while benchmarking against well-defined datasets serves as a powerful testing tool, “real-life” samples are often not comparable. Thus, as done here, future primer-like reviews should highlight possible cross-field caveats, encouraging researchers to employ and test several approaches and validate their results whenever possible.
In summary, Douglas and Langille  offer both the novice and experienced researcher a detailed guide along the paths of microbiome data analysis, accompanied by informative background information, suggested tools with which analyses can be started, and an insightful view on where the field should be heading.
 Turnbaugh PJ, Ley RE, Hamady M, Fraser-Liggett CM, Knight R, Gordon JI (2007) The Human Microbiome Project. Nature, 449, 804–810. https://doi.org/10.1038/nature06244
 Gilbert JA, Jansson JK, Knight R (2014) The Earth Microbiome project: successes and aspirations. BMC Biology, 12, 69. https://doi.org/10.1186/s12915-014-0069-1
 Mason C, Afshinnekoo E, Ahsannudin S, Ghedin E, Read T, Fraser C, Dudley J, Hernandez M, Bowler C, Stolovitzky G, Chernonetz A, Gray A, Darling A, Burke C, Łabaj PP, Graf A, Noushmehr H, Moraes s., Dias-Neto E, Ugalde J, Guo Y, Zhou Y, Xie Z, Zheng D, Zhou H, Shi L, Zhu S, Tang A, Ivanković T, Siam R, Rascovan N, Richard H, Lafontaine I, Baron C, Nedunuri N, Prithiviraj B, Hyat S, Mehr S, Banihashemi K, Segata N, Suzuki H, Alpuche Aranda CM, Martinez J, Christopher Dada A, Osuolale O, Oguntoyinbo F, Dybwad M, Oliveira M, Fernandes A, Oliveira M, Fernandes A, Chatziefthimiou AD, Chaker S, Alexeev D, Chuvelev D, Kurilshikov A, Schuster S, Siwo GH, Jang S, Seo SC, Hwang SH, Ossowski S, Bezdan D, Udekwu K, Udekwu K, Lungjdahl PO, Nikolayeva O, Sezerman U, Kelly F, Metrustry S, Elhaik E, Gonnet G, Schriml L, Mongodin E, Huttenhower C, Gilbert J, Hernandez M, Vayndorf E, Blaser M, Schadt E, Eisen J, Beitel C, Hirschberg D, Schriml L, Mongodin E, The MetaSUB International Consortium (2016) The Metagenomics and Metadesign of the Subways and Urban Biomes (MetaSUB) International Consortium inaugural meeting report. Microbiome, 4, 24. https://doi.org/10.1186/s40168-016-0168-z
 Douglas GM, Langille MGI (2021) A primer and discussion on DNA-based microbiome data and related bioinformatics analyses. OSF Preprints, ver. 4 peer-reviewed and recommended by Peer Community In Genomics. https://doi.org/10.31219/osf.io/3dybg
 Chen I-MA, Markowitz VM, Chu K, Palaniappan K, Szeto E, Pillay M, Ratner A, Huang J, Andersen E, Huntemann M, Varghese N, Hadjithomas M, Tennessen K, Nielsen T, Ivanova NN, Kyrpides NC (2017) IMG/M: integrated genome and metagenome comparative data analysis system. Nucleic Acids Research, 45, D507–D516. https://doi.org/10.1093/nar/gkw929
 Arkin AP, Cottingham RW, Henry CS, Harris NL, Stevens RL, Maslov S, Dehal P, Ware D, Perez F, Canon S, Sneddon MW, Henderson ML, Riehl WJ, Murphy-Olson D, Chan SY, Kamimura RT, Kumari S, Drake MM, Brettin TS, Glass EM, Chivian D, Gunter D, Weston DJ, Allen BH, Baumohl J, Best AA, Bowen B, Brenner SE, Bun CC, Chandonia J-M, Chia J-M, Colasanti R, Conrad N, Davis JJ, Davison BH, DeJongh M, Devoid S, Dietrich E, Dubchak I, Edirisinghe JN, Fang G, Faria JP, Frybarger PM, Gerlach W, Gerstein M, Greiner A, Gurtowski J, Haun HL, He F, Jain R, Joachimiak MP, Keegan KP, Kondo S, Kumar V, Land ML, Meyer F, Mills M, Novichkov PS, Oh T, Olsen GJ, Olson R, Parrello B, Pasternak S, Pearson E, Poon SS, Price GA, Ramakrishnan S, Ranjan P, Ronald PC, Schatz MC, Seaver SMD, Shukla M, Sutormin RA, Syed MH, Thomason J, Tintle NL, Wang D, Xia F, Yoo H, Yoo S, Yu D (2018) KBase: The United States Department of Energy Systems Biology Knowledgebase. Nature Biotechnology, 36, 566–569. https://doi.org/10.1038/nbt.4163
 Wilke A, Bischof J, Gerlach W, Glass E, Harrison T, Keegan KP, Paczian T, Trimble WL, Bagchi S, Grama A, Chaterji S, Meyer F (2016) The MG-RAST metagenomics database and portal in 2015. Nucleic Acids Research, 44, D590–D594. https://doi.org/10.1093/nar/gkv1322
Uncovering transposable element variants and their potential adaptive impact in urban populations of the malaria vector Anopheles coluzzii
Anopheles coluzzii, a new system to study how transposable elements may foster adaptation to urban environmentsRecommended by Anne Roulin based on reviews by Yann Bourgeois and 1 anonymous reviewer
Transposable elements (TEs) are mobile DNA sequences that can increase their copy number and move from one location to another within the genome . Because of their transposition dynamics, TEs constitute a significant fraction of eukaryotic genomes. TEs are also known to play an important functional role and a wealth of studies has now reported how TEs may influence single host traits [e.g. 2–4]. Given that TEs are more likely than classical point mutations to cause extreme changes in gene expression and phenotypes, they might therefore be especially prone to produce the raw diversity necessary for individuals to respond to challenging environments [5,6] such as the ones found in urban area.
In their study , Vargas et al. establish the foundation to investigate how TEs may help Anopheles coluzzii - the primary vectors of human malaria in sub-Saharan Africa - adapt to urban environments. To cover natural breeding sites in major Central Africa cities, they made use of the previously available An. coluzzii genome from Yaoundé (Cameroon) and sequenced with long-read technology six additional ones originating from Douala (Cameroon) and Libreville (Gabon). The de novo annotation of TEs in these genomes revealed 64 new anopheline TE families and allowed to identify seven active families. As a first step towards characterizing the potential role of TEs in the adaptation of An. coluzzii to urban environments, they further analyzed the distribution of TEs across the seven genomes. By doing so, they identified a significant number of polymorphic or fixed TE insertions located in the vicinity of genes involved in insecticide resistance and immune response genes.
The availability of seven An. coluzzii genomes allowed the authors to explore how TE diversity may affect genes functionally relevant for the adaptation to urban environments and provide ground for further functional validation studies. More and more studies have demonstrated the impact of TEs on adaptation and as such, the work of Vargas et al. contributes to fostering our understanding of the link between TEs and gain of function in a species facing strong anthropogenic pressures.
 Wicker T, Sabot F, Hua-Van A, Bennetzen JL, Capy P, Chalhoub B, Flavell A, Leroy P, Morgante M, Panaud O, Paux E, SanMiguel P, Schulman AH (2007) A unified classification system for eukaryotic transposable elements. Nature Reviews Genetics, 8, 973–982. https://doi.org/10.1038/nrg2165
 van’t Hof AE, Campagne P, Rigden DJ, Yung CJ, Lingley J, Quail MA, Hall N, Darby AC, Saccheri IJ (2016) The industrial melanism mutation in British peppered moths is a transposable element. Nature, 534, 102–105. https://doi.org/10.1038/nature17951
 González J, Karasov TL, Messer PW, Petrov DA (2010) Genome-wide patterns of adaptation to temperate environments associated with transposable elements in Drosophila. PLOS Genetics, 6, e1000905. https://doi.org/10.1371/journal.pgen.1000905
 Lisch D (2013) How important are transposons for plant evolution? Nature Reviews Genetics, 14, 49–61. https://doi.org/10.1038/nrg3374
 Bonchev G, Parisod C (2013) Transposable elements and microevolutionary changes in natural populations. Molecular Ecology Resources, 13, 765–775. https://doi.org/10.1111/1755-0998.12133
 Casacuberta E, González J (2013) The impact of transposable elements in environmental adaptation. Molecular Ecology, 22, 1503–1517. https://doi.org/10.1111/mec.12170
 Vargas-Chavez C, Pendy NML, Nsango SE, Aguilera L, Ayala D, González J (2021). Uncovering transposable element variants and their potential adaptive impact in urban populations of the malaria vector Anopheles coluzzii. bioRxiv, 2020.11.22.393231, ver. 3 peer-reviewed and recommended by Peer community in Genomics. https://doi.org/10.1101/2020.11.22.393231
Evidence for shared ancestry between Actinobacteria and Firmicutes bacteriophages
Viruses of bacteria: phages evolution across phylum boundariesRecommended by Denis Tagu based on reviews by 3 anonymous reviewers
Bacteria and phages have coexisted and coevolved for a long time. Phages are bacteria-infecting viruses, with a symbiotic status sensu lato, meaning they can be pathogenic, commensal or mutualistic. Thus, the association between bacteria phages has probably played a key role in the high adaptability of bacteria to most - if not all – of Earth’s ecosystems, including other living organisms (such as eukaryotes), and also regulate bacterial community size (for instance during bacterial blooms).
As genetic entities, phages are submitted to mutations and natural selection, which changes their DNA sequence. Therefore, comparative genomic analyses of contemporary phages can be useful to understand their evolutionary dynamics. International initiatives such as SEA-PHAGES have started to tackle the issue of history of phage-bacteria interactions and to describe the dynamics of the co-evolution between bacterial hosts and their associated viruses. Indeed, the understanding of this cross-talk has many potential implications in terms of health and agriculture, among others.
The work of Koert et al. (2021) deals with one of the largest groups of bacteria (Actinobacteria), which are Gram-positive bacteria mainly found in soil and water. Some soil-born Actinobacteria develop filamentous structures reminiscent of the mycelium of eukaryotic fungi. In this study, the authors focused on the Streptomyces clade, a large genus of Actinobacteria colonized by phages known for their high level of genetic diversity.
The authors tested the hypothesis that large exchanges of genetic material occurred between Streptomyces and diverse phages associated with bacterial hosts. Using public datasets, their comparative phylogenomic analyses identified a new cluster among Actinobacteria–infecting phages closely related to phages of Firmicutes. Moreover, the GC content and codon-usage biases of this group of phages of Actinobacteria are similar to those of Firmicutes.
This work demonstrates for the first time the transfer of a bacteriophage lineage from one bacterial phylum to another one. The results presented here suggest that the age of the described transfer is probably recent since several genomic characteristics of the phage are not fully adapted to their new hosts. However, the frequency of such transfer events remains an open question. If frequent, such exchanges would mean that pools of bacteriophages are regularly fueled by genetic material coming from external sources, which would have important implications for the co-evolutionary dynamics of phages and bacteria.
Koert, M., López-Pérez, J., Courtney Mattson, C., Caruso, S. and Erill, I. (2021) Evidence for shared ancestry between Actinobacteria and Firmicutes bacteriophages. bioRxiv, 842583, version 5 peer-reviewed and recommended by Peer community in Genomics. doi: https://doi.org/10.1101/842583
Semi-artificial datasets as a resource for validation of bioinformatics pipelines for plant virus detection
Toward a critical assessment of virus detection in plantsRecommended by Hadi Quesneville based on reviews by Alexander Suh and 1 anonymous reviewer
The advent of High Throughput Sequencing (HTS) since the last decade has revealed previously unsuspected diversity of viruses as well as their (sometimes) unexpected presence in some healthy individuals. These results demonstrate that genomics offers a powerful tool for studying viruses at the individual level, allowing an in-depth inventory of those that are infecting an organism. Such approaches make it possible to study viromes with an unprecedented level of detail, both qualitative and quantitative, which opens new venues for analyses of viruses of humans, animals and plants. Consequently, the diagnostic field is using more and more HTS, fueling the need for efficient and reliable bioinformatics tools.
Many such tools have already been developed, but in plant disease diagnostics, validation of the bioinformatics pipelines used for the detection of viruses in HTS datasets is still in its infancy. There is an urgent need for benchmarking the different tools and algorithms using well-designed reference datasets generated for this purpose. This is a crucial step to move forward and to improve existing solutions toward well-standardized bioinformatics protocols. This context has led to the creation of the Plant Health Bioinformatics Network (PHBN), a Euphresco network project aiming to build a bioinformatics community working on plant health. One of their objectives is to provide researchers with open-access reference datasets allowing to compare and validate virus detection pipelines.
In this framework, Tamisier et al.  present real, semi-artificial, and completely artificial datasets, each aimed at addressing challenges that could affect virus detection. These datasets comprise real RNA-seq reads from virus-infected plants as well as simulated virus reads. Such a work, providing open-access datasets for benchmarking bioinformatics tools, should be encouraged as they are key to software improvement as demonstrated by the well-known success story of the protein structure prediction community: their pioneer community-wide effort, called Critical Assessment of protein Structure Prediction (CASP), has been providing research groups since 1994 with an invaluable way to objectively test their structure prediction methods, thereby delivering an independent assessment of state-of-art protein-structure modelling tools. Following this success, many other bioinformatic community developed similar “competitions”, such as RNA-puzzles  to predict RNA structures, Critical Assessment of Function Annotation  to predict gene functions, Critical Assessment of Prediction of Interactions  to predict protein-protein interactions, Assemblathon  for genome assembly, etc. These are just a few examples from a long list of successful initiatives. Such efforts enable rigorous assessments of tools, stimulate the developers’ creativity, but also provide user communities with a state-of-art evaluation of available tools.
Inspired by these success stories, the authors propose a “VIROMOCK challenge” , asking researchers in the field to test their tools and to provide feedback on each dataset through a repository. This initiative, if well followed, will undoubtedly improve the field of virus detection in plants, but also probably in many other organisms. This will be a major contribution to the field of viruses, leading to better diagnostics and, consequently, a better understanding of viral diseases, thus participating in promoting human, animal and plant health.
 Tamisier, L., Haegeman, A., Foucart, Y., Fouillien, N., Al Rwahnih, M., Buzkan, N., Candresse, T., Chiumenti, M., De Jonghe, K., Lefebvre, M., Margaria, P., Reynard, J.-S., Stevens, K., Kutnjak, D. and Massart, S. (2021) Semi-artificial datasets as a resource for validation of bioinformatics pipelines for plant virus detection. Zenodo, 4273791, version 4 peer-reviewed and recommended by Peer community in Genomics. doi: https://doi.org/10.5281/zenodo.4273791
 Critical Assessment of protein Structure Prediction” (CASP) - https://en.wikipedia.org/wiki/CASP
 RNA-puzzles - https://www.rnapuzzles.org
 Critical Assessment of Function Annotation (CAFA) - https://en.wikipedia.org/wiki/Critical_Assessment_of_Function_Annotation
 Critical Assessment of Prediction of Interactions (CAPI) - https://en.wikipedia.org/wiki/Critical_Assessment_of_Prediction_of_Interactions
 Assemblathon - https://assemblathon.org
 VIROMOCK challenge - https://gitlab.com/ilvo/VIROMOCKchallenge
Gut microbial ecology of Xenopus tadpoles across life stages
A comprehensive look at Xenopus gut microbiota: effects of feed, developmental stages and parental transmissionRecommended by Wirulda Pootakham based on reviews by Vanessa Marcelino and 1 anonymous reviewer
It is well established that the gut microbiota play an important role in the overall health of their hosts (Jandhyala et al. 2015). To date, there are still a limited number of studies on the complex microbial communites inhabiting vertebrate digestive systems, especially the ones that also explored the functional diversity of the microbial community (Bletz et al. 2016).
This preprint by Scalvenzi et al. (2021) reports a comprehensive study on the phylogenetic and metabolic profiles of the Xenopus gut microbiota. The author describes significant changes in the gut microbiome communities at different developmental stages and demonstrates different microbial community composition across organs. In addition, the study also investigates the impact of diet on the Xenopus tadpole gut microbiome communities as well as how the bacterial communities are transmitted from parents to the next generation.
This is one of the first studies that addresses the interactions between gut bacteria and tadpoles during the development. The authors observe the dynamics of gut microbiome communities during tadpole growth and metamorphosis. They also explore host-gut microbial community metabolic interactions and demostrate the capacity of the microbiome to complement the metabolic pathways of the Xenopus genome. Although this study is limited by the use of Xenopus tadpoles in a laboratory, which are probably different from those in nature, I believe it still provides important and valuable information for the research community working on vertebrate’s microbiota and their interaction with the host.
Bletz et al. (2016). Amphibian gut microbiota shifts differentially in community structure but converges on habitat-specific predicted functions. Nature Communications, 7(1), 1-12. doi: https://doi.org/10.1038/ncomms13699
Jandhyala, S. M., Talukdar, R., Subramanyam, C., Vuyyuru, H., Sasikala, M., & Reddy, D. N. (2015). Role of the normal gut microbiota. World journal of gastroenterology: WJG, 21(29), 8787. doi: https://dx.doi.org/10.3748%2Fwjg.v21.i29.8787
Scalvenzi, T., Clavereau, I., Bourge, M. & Pollet, N. (2021) Gut microbial ecology of Xenopus tadpoles across life stages. bioRxiv, 2020.05.25.110734, ver. 4 peer-reviewed and recommended by Peer community in Geonmics. https://doi.org/10.1101/2020.05.25.110734
Traces of transposable element in genome dark matter co-opted by flowering gene regulation networks
Using small fragments to discover old TE remnants: the Duster approach empowers the TE detectionRecommended by Francois Sabot based on reviews by Josep Casacuberta and 1 anonymous reviewer
Transposable elements are the raw material of the dark matter of the genome, the foundation of the next generation of genes and regulation networks". This sentence could be the essence of the paper of Baud et al. (2021). Transposable elements (TEs) are endogenous mobile genetic elements found in almost all genomes, which were discovered in 1948 by Barbara McClintock (awarded in 1983 the only unshared Medicine Nobel Prize so far). TEs are present everywhere, from a single isolated copy for some elements to more than millions for others, such as Alu. They are founders of major gene lineages (HET-A, TART and telomerases, RAG1/RAG2 proteins from mammals immune system; Diwash et al, 2017), and even of retroviruses (Xiong & Eickbush, 1988). However, most TEs appear as selfish elements that replicate, land in a new genomic region, then start to decay and finally disappear in the midst of the genome, turning into genomic ‘dark matter’ (Vitte et al, 2007). The mutations (single point, deletion, recombination, and so on) that occur during this slow death erase some of their most notable features and signature sequences, rendering them completely unrecognizable after a few million years. Numerous TE detection tools have tried to optimize their detection (Goerner-Potvin & Bourque, 2018), but further improvement is definitely challenging. This is what Baud et al. (2021) accomplished in their paper. They used a simple, elegant and efficient k-mer based approach to find small signatures that, when accumulated, allow identifying very old TEs. Using this method, called Duster, they improved the amount of annotated TEs in the model plant Arabidopsis thaliana by 20%, pushing the part of this genome occupied by TEs up from 40 to almost 50%. They further observed that these very old Duster-specific TEs (i.e., TEs that are only detected by Duster) are, among other properties, close to genes (much more than recent TEs), not targeted by small RNA pathways, and highly associated with conserved regions across the rosid family. In addition, they are highly associated with flowering or stress response genes, and may be involved through exaptation in the evolution of responses to environmental changes. TEs are not just selfish elements: more and more studies have shown their key role in the evolution of their hosts, and tools such as Duster will help us better understand their impact.
Baud, A., Wan, M., Nouaud, D., Francillonne, N., Anxolabéhère, D. and Quesneville, H. (2021). Traces of transposable elements in genome dark matter co-opted by flowering gene regulation networks. bioRxiv, 547877, ver. 5 peer-reviewed and recommended by PCI Genomics.doi: https://doi.org/10.1101/547877
Bourque, G., Burns, K.H., Gehring, M. et al. (2018) Ten things you should know about transposable elements. Genome Biology 19:199. doi: https://doi.org/10.1186/s13059-018-1577-z
Goerner-Potvin, P., Bourque, G. Computational tools to unmask transposable elements. Nature Reviews Genetics 19:688–704 (2018) https://doi.org/10.1038/s41576-018-0050-x
Jangam, D., Feschotte, C. and Betrán, E. (2017) Transposable element domestication as an adaptation to evolutionary conflicts. Trends in Genetics 33:817-831. doi: https://doi.org/10.1016/j.tig.2017.07.011
Vitte, C., Panaud, O. and Quesneville, H. (2007) LTR retrotransposons in rice (Oryza sativa, L.): recent burst amplifications followed by rapid DNA loss. BMC Genomics 8:218. doi: https://doi.org/10.1186/1471-2164-8-218
Xiong, Y. and Eickbush, T. H. (1988) Similarity of reverse transcriptase-like sequences of viruses, transposable elements, and mitochondrial introns. Molecular Biology and Evolution 5: 675–690. doi: https://doi.org/10.1093/oxfordjournals.molbev.a040521
An evaluation of pool-sequencing transcriptome-based exon capture for population genomics in non-model species
Assessing a novel sequencing-based approach for population genomics in non-model speciesRecommended by Thomas Derrien and Sebastian E. Ramos-Onsins based on reviews by Valentin Wucher and 1 anonymous reviewer
Developing new sequencing and bioinformatic strategies for non-model species is of great interest in many applications, such as phylogenetic studies of diverse related species, but also for studies in population genomics, where a relatively large number of individuals is necessary. Different approaches have been developed and used in these last two decades, such as RAD-Seq (e.g., Miller et al. 2007), exome sequencing (e.g., Teer and Mullikin 2010) and other genome reduced representation methods that avoid the use of a good reference and well annotated genome (reviewed at Davey et al. 2011). However, population genomics studies require the analysis of numerous individuals, which makes the studies still expensive. Pooling samples was thought as an inexpensive strategy to obtain estimates of variability and other related to the frequency spectrum, thus allowing the study of variability at population level (e.g., Van Tassell et al. 2008), although the major drawback was the loss of information related to the linkage of the variants. In addition, population analysis using all these sequencing strategies require statistical and empirical validations that are not always fully performed. A number of studies aiming to obtain unbiased estimates of variability using reduced representation libraries and/or with pooled data have been performed (e.g., Futschik and Schlötterer 2010, Gautier et al. 2013, Ferretti et al. 2013, Lynch et al. 2014), as well as validation of new sequencing methods for population genetic analyses (e.g., Gautier et al. 2013, Nevado et al. 2014). Nevertheless, empirical validation using both pooled and individual experimental approaches combined with different bioinformatic methods has not been always performed.
Here, Deleury et al. (2020) proposed an efficient and elegant way of quantifying the single-nucleotide polymorphisms (SNPs) of exon-derived sequences in a non-model species (i.e. for which no reference genome sequence is available) at the population level scale. They also designed a new procedure to capture exon-derived sequences based on a reference transcriptome. In addition, they were able to make predictions of intron-exon boundaries for de novo transcripts based on the decay of read depth at the ends of the coding regions.
Based on theoretical predictions (Gautier et al. 2013), Deleury et al. (2020) designed a procedure to test the accuracy of variant allele frequencies (AFs) with pooled samples, in a reduced genome-sequence library made with transcriptome regions, and additionally testing the effects of new bioinformatic methods in contrast to standardized methods. They applied their strategy on the non-model species Asian ladybird (Harmonia axyridis), for which a draft genome is available, thereby allowing them to benchmark their method with regard to a traditional mapping-based approach. Based on species-specific de novo transcriptomes, they designed capture probes which are then used to call SNPx and then compared the resulting SNP AFs at the individual (multiplexed) versus population (pooled) levels. Interestingly, they showed that SNP AFs in the pool sequencing strategy nicely correlate with the individual ones but obviously in a cost-effective way. Studies of population genomics for non-model species have usually limited budgets. The number of individuals required for population genomics analysis multiply the costs of the project, making pooling samples an interesting option. Furthermore, the use of pool sequencing is not always a choice, as many organisms are too small and/or individuals are too sticked each other to be individually sequenced (e.g., Choquet et al. 2019, Kurland et al. 2019). In addition, the study of a reduced section of the genome is cheaper and often sufficient for a number of population genetic questions, such as the understanding of general demographic events, or the estimation of the effects of positive and/or negative selection at functional coding regions. Studies on population genomics of non-model species have many applications in related fields, such as conservation genetics, control of invasive species, etc. The work of Deleury et al. (2020) is an elegant contribution to the assessment and validation of new methodologies used for the analysis of genome variations at the intra-population variability level, highlighting straight bioinformatic and reliable sequencing methods for population genomics studies.
 Choquet et al. (2019). Towards population genomics in non-model species with large genomes: a case study of the marine zooplankton Calanus finmarchicus. Royal Society open science, 6(2), 180608. doi: https://doi.org/10.1098/rsos.180608
 Davey, J. W., Hohenlohe, P. A., Etter, P. D., Boone, J. Q., Catchen, J. M. and Blaxter, M. L. (2011). Genome-wide genetic marker discovery and genotyping using next-generation sequencing. Nature Reviews Genetics, 12(7), 499-510. doi: https://doi.org/10.1038/nrg3012
 Deleury, E., Guillemaud, T., Blin, A. and Lombaert, E. (2020) An evaluation of pool-sequencing transcriptome-based exon capture for population genomics in non-model species. bioRxiv, 10.1101/583534, ver. 7 peer-reviewed and recommended by PCI Genomics. https://doi.org/10.1101/583534
 Ferretti, L., Ramos‐Onsins, S. E. and Pérez‐Enciso, M. (2013). Population genomics from pool sequencing. Molecular ecology, 22(22), 5561-5576. doi: https://doi.org/10.1111/mec.12522
 Futschik, A. and Schlötterer, C. (2010). Massively parallel sequencing of pooled DNA samples—the next generation of molecular markers. Genetics, 186 (1), 207-218. doi: https://doi.org/10.1534/genetics.110.114397
 Gautier et al. (2013). Estimation of population allele frequencies from next‐generation sequencing data: pool‐versus individual‐based genotyping. Molecular Ecology, 22(14), 3766-3779. doi: https://doi.org/10.1111/mec.12360
 Kurland et al. (2019). Exploring a Pool‐seq‐only approach for gaining population genomic insights in nonmodel species. Ecology and evolution, 9(19), 11448-11463. doi: https://doi.org/10.1002/ece3.5646
 Lynch, M., Bost, D., Wilson, S., Maruki, T. and Harrison, S. (2014). Population-genetic inference from pooled-sequencing data. Genome biology and evolution, 6(5), 1210-1218. doi: https://doi.org/10.1093/gbe/evu085
 Miller, M. R., Dunham, J. P., Amores, A., Cresko, W. A. and Johnson, E. A. (2007). Rapid and cost-effective polymorphism identification and genotyping using restriction site associated DNA (RAD) markers. Genome research, 17(2), 240-248. doi: https://doi.org/10.1101%2Fgr.5681207
 Nevado, B., Ramos‐Onsins, S. E. and Perez‐Enciso, M. (2014). Resequencing studies of nonmodel organisms using closely related reference genomes: optimal experimental designs and bioinformatics approaches for population genomics. Molecular ecology, 23(7), 1764-1779. doi: https://doi.org/10.1111/mec.12693
 Teer, J. K. and Mullikin, J. C. (2010). Exome sequencing: the sweet spot before whole genomes. Human molecular genetics, 19(R2), R145-R151. doi: https://doi.org/10.1093/hmg/ddq333
 Van Tassell et al. (2008). SNP discovery and allele frequency estimation by deep sequencing of reduced representation libraries. Nature methods, 5(3), 247-252. doi: https://doi.org/10.1038/nmeth.1185
A rapid and simple method for assessing and representing genome sequence relatedness
A quick alternative method for resolving bacterial taxonomy using short identical DNA sequences in genomes or metagenomesRecommended by B. Jesse Shapiro based on reviews by Gavin Douglas and 1 anonymous reviewer
The bacterial species problem can be summarized as follows: bacteria recombine too little, and yet too much (Shapiro 2019).
Too little in the sense that recombination is not obligately coupled with reproduction, as in sexual eukaryotes. So the Biological Species Concept (BSC) of reproductive isolation does not strictly apply to clonally reproducing organisms like bacteria. Too much in the sense that genetic exchange can occur promiscuously across species (or even Domains), potentially obscuring species boundaries.
In parallel to such theoretical considerations, several research groups have taken more pragmatic approaches to defining bacterial species based on sequence similarity cutoffs, such as genome-wide average nucleotide identity (ANI). At a cutoff above 95% ANI, genomes are considered to come from the same species. While this cutoff may appear arbitrary, a discontinuity around 95% in the distribution of ANI values has been argued to provide a 'natural' cutoff (Jain et al. 2018). This discontinuity has been criticized as being an artefact of various biases in genome databases (Murray, Gao, and Wu 2020), but appears to be a general feature of relatively unbiased metagenome-assembled genomes as well (Olm et al. 2020). The 95% cutoff has been suggested to represent a barrier to homologous recombination (Olm et al. 2020), although clusters of genetic exchange consistent with BSC-like species are observed at much finer identity cutoffs (Shapiro 2019; Arevalo et al. 2019).
Although 95% ANI is the most widely used genomic standard for species delimitation, it is by no means the only plausible approach. In particular, tracts of identical DNA provide evidence for recent genetic exchange, which in turn helps define BSC-like clusters of genomes (Arevalo et al. 2019). In this spirit, Briand et al. (2020) introduce a genome-clustering method based on the number of shared identical DNA sequences of length k (or k-mers). Using a test dataset of Pseudomonas genomes, they find that 95% ANI corresponds to approximately 50% of shared 15-mers. Applying this cutoff yields 350 Pseudomonas species, whereas the current taxonomy only includes 207 recognized species. To determine whether splitting the genus into a greater number of species is at all useful, they compare their new classification scheme to the traditional one in terms of the ability to taxonomically classify metagenomic sequencing reads from three Pseudomonas-rich environments. In all cases, the new scheme (termed K-IS for "Kinship relationships Identification with Shared k-mers") yielded a higher number of classified reads, with an average improvement of 1.4-fold. This is important because increasing the number of genome sequences in a reference database – without consistent taxonomic annotation of these genomes – paradoxically leads to fewer classified metagenomic reads. Thus a rapid, automated taxonomy such as the one proposed here offers an opportunity to more fully harness the information from metagenomes.
KI-S is also fast to run, so it is feasible to test several values of k and quickly visualize the clustering using an interactive, zoomable circle-packing display (that resembles a cross-section of densely packed, three-dimensional dendrogram). This interface allows the rapid flagging of misidentified species, or understudied species with few sequenced representatives as targets for future study. Hopefully these initial Pseudomonas results will inspire future studies to apply the method to additional taxa, and to further characterize the relationship between ANI and shared identical k-mers. Ultimately, I hope that such investigations will resolve the issue of whether or not there is a 'natural' discontinuity for bacterial species, and what evolutionary forces maintain this cutoff.
Arevalo P, VanInsberghe D, Elsherbini J, Gore J, Polz MF (2019) A Reverse Ecology Approach Based on a Biological Definition of Microbial Populations. Cell, 178, 820-834.e14. https://doi.org/10.1016/j.cell.2019.06.033
Briand M, Bouzid M, Hunault G, Legeay M, Saux MF-L, Barret M (2020) A rapid and simple method for assessing and representing genome sequence relatedness. bioRxiv, 569640, ver. 5 peer-reveiwed and recommended by PCI Genomics. https://doi.org/10.1101/569640
Jain C, Rodriguez-R LM, Phillippy AM, Konstantinidis KT, Aluru S (2018) High throughput ANI analysis of 90K prokaryotic genomes reveals clear species boundaries. Nature Communications, 9, 5114. https://doi.org/10.1038/s41467-018-07641-9
Murray CS, Gao Y, Wu M (2020) There is no evidence of a universal genetic boundary among microbial species. bioRxiv, 2020.07.27.223511. https://doi.org/10.1101/2020.07.27.223511
Olm MR, Crits-Christoph A, Diamond S, Lavy A, Carnevali PBM, Banfield JF (2020) Consistent Metagenome-Derived Metrics Verify and Delineate Bacterial Species Boundaries. mSystems, 5. https://doi.org/10.1128/mSystems.00731-19
Shapiro BJ (2019) What Microbial Population Genomics Has Taught Us About Speciation. In: Population Genomics: Microorganisms Population Genomics. (eds Polz MF, Rajora OP), pp. 31–47. Springer International Publishing, Cham. https://doi.org/10.1007/13836201810