Pre-sampling requirements

Supporting genome team compliance with all relevant ethical and legal customary, local, regional, national, and international obligations was a priority during the infrastructure development process. Through ERGA expert committees, namely the Ethics, Legal and Social Issues (ELSI) Committee and the Sampling and Sample Processing (SSP) Committee, comprehensive documentation was developed including a ‘Sampling Code of Best Practice’ and ‘Guidelines on implementing the Traditional Knowledge and Biocultural Labels and Notices when partnering with Indigenous Peoples and Local Communities (IPLC)’^20,25. The Traditional Knowledge (TK) and Biocultural BC) Label and Notice implementation and guideline documentation was developed through a funded partnership (European Open Science Cloud Grant) with representatives of the Global Indigenous Data Alliance (https://www.gida-global.org/), Local Context Hub (https://localcontexts.org/) and the Research Data Alliance (https://www.rd-alliance.org/node/77186). Complying with this documentation was mandatory as it codifies the official ERGA standards for how to ethically and legally collect samples, as well as how to responsibly engage all interested parties (Supplementary glossary). In addition, educational webinars were used as a researcher capacity-building tool, providing more general information on pertinent topics such as the Nagoya Protocol on Access and Benefit Sharing, and Digital Sequence Information (https://www.youtube.com/@erga-consortium1001).

Sampling and metadata acquisition

During sample collection important metadata concerning the species collection event were expected to be documented by the sample collector. To standardise this process a robust metadata schema was developed, using the DToL metadata schema as a foundation²⁶. The tailored ERGA schema, including unique ERGA specimen identifiers as well as ToLID (https://id.tol.sanger.ac.uk/), was codified into a .csv formatted ‘manifest’ and made publicly available (https://github.com/ERGA-consortium/ERGA-sample-manifest). In tandem, a standard operating procedure document²⁷ was developed to provide details on how to complete all of the 81 validatable manifest fields. Inspired by the Genomic Observatories Metadatabase²⁸, ERGA also developed fields to mandate important information disclosure e.g. permanent unique identifiers (PUID) associated with ex-situ specimens, permits, and Indigenous rights and interests (TK and BC Labels and Notices)^25,29–31. Overall, samples were collected for 98 species spanning 92 genera, 81 families, 61 orders, 26 classes, and 13 phyla (https://goat.genomehubs.org/projects/ERGA-PIL, Fig. 2a). The geographic distribution of samples collected was relatively even, although some countries contributed more species than others (Fig. 2b). Altogether 89% of genome teams (n = 93) reported >90% confidence level in that they had obtained all permits required with ten Nagoya permits and three CITES (Supplementary Note 1) permits being obtained.

Sample manifest submission, validation, ex-situ storage

An accessible and streamlined metadata manifest submission system was implemented to ensure that all ERGA’s sample metadata was accurately validated and promptly submitted into the public archive. To achieve this, a user-friendly and highly customised data and metadata brokering system called Collaborative OPen Omics (COPO) (https://wellcomeopenresearch.org/articles/7-279/v1) was used³². The COPO submission system validated each manifest submitted against an ERGA-provided checklist to standardise and automate entry into the BioSamples public archive. By automating this process it ensured that all species samples collected had a permanent unique identifier (PUID) from BioSamples that can be automatically linked to the associated genomic sequencing data submitted to the European Nucleotide Archive (ENA; https://www.ebi.ac.uk/ena). Additionally, the submission system had the capability to upload permit documentation and supported its immediate transfer to a private and secure location on an internal ERGA data repository (that was built for the purposes of the pilot test) to avoid privacy concerns and data leakages. All documents were subsequently deleted from COPO’s internal servers. The internal data repository itself was constructed in partnership with the Barcelona Supercomputing Centre (BSC; https://www.bsc.es/) and was a Nextcloud instance containing a group folder with a tiered storage system, or HSM (see Supplementary glossary). All ERGA members could request access to the ERGA data repository and upon approval, members were assigned appropriate access privileges depending on their needs (read-, write-, or full file control access). To support repository utilisation, guidelines were developed detailing protocols for data upload/download as well as directory structure, to ensure standardisation, reusability, and interoperability³³.

We highly recommended that both voucher specimen(s) and cryopreserved specimen(s) be associated with all genomic resources produced during the pilot test. To support this we issued supporting guidance for biobanking and vouchering. The vouchering best practices developed recommended the deposition of both a physical and digital e-voucher(s) (high-quality, informative photographs). Through ERGA’s SSP Committee, we also supported genome teams in seek of a permanent collection for voucher deposition and a partnership with the LIB Biobank at Museum Koenig (Bonn) (https://bonn.leibniz-lib.de/en/biobank) was established to support the deposition of cryopreserved samples for those without access to a local biobank. Samples biobanked in LIB were made publicly visible via the international biodiversity biobanking portal (GGBN.org). Although not a mandatory requirement, voucher specimens were provided for 67% of the species (19% digital, 40% physical, and 40% had both physical and digital) and deposited in museum collections across 23 countries (Fig. 2c). Of the specimens, 45% had an associated cryopreserved sample that were stored in 34 biobanks in 22 countries (Fig. 2c). All 98 genome teams successfully completed, validated and uploaded their metadata publicly to BioSamples through the COPO system and manifest submissions are publicly available through the ERGA Data Portal (https://portal.erga-biodiversity.eu/) that provides intuitive search and direct links to all of the data held in the public archives ('Communication and Coordination' Section).

Sample preparation

Sample quality and shipment requirements were formalised for each data-type across ERGA sequencing facility partners, including sample requirements for long reads (Oxford Nanopore Technologies (ONT)/Pacific BioSciences (PacBio)), scaffolding (Omni-C/Hi-C), and annotation (RNA-Seq/IsoSeq) of data. Sample collectors were expected to adhere to the requirements of the ERGA sequencing facility specified and ensure that samples shipped are: 1) of a quality suitable for HMW DNA extraction, and 2) of an appropriate quantity for long-read, proximity ligation and annotation sequence data production. Two ERGA Library Preparation Hubs were established to support genome teams that required resource support for the library preparation of samples prior to sequencing. To increase the likelihood that the HMW DNA of sufficient quantity was obtained for effective sequencing, most library preparation was conducted by partnering sequencing facilities. However, the ERGA Library Preparation Hubs facilitated the production of 99 libraries: 15 libraries for proximity ligation data (Hi-C/Omni-C® kit) that were provided by 27 countries; Eight libraries for PacBio data provided by eight countries; and the remainder were for RNAseq data (Supplementary Tables 3, 4, Supplementary Figs. 1, 2).

Sequencing strategy

A key component and strength of the decentralised infrastructure was the intentional distribution of sequence data production across partnering European sequencing facilities. To initialise these partnerships, a sequencing platform landscape assessment was conducted across all of the countries that had ERGA council representation. This effort assessed the quantity, distribution, and diversity of the sequencing platforms available across Europe and specifically examined their capability to produce long read (PacBio HiFi reads/ONT reads /IsoSeq reads), and short read (Hi-C/Omni-C/RNA-Seq/PCR-free Illumina) sequencing data. This mapping indicated an uneven distribution of sequencing platforms across Europe, and so we decided that any sequencing facility with a platform to produce long read sequencing data could be an ERGA partner. We took this long read data-type agnostic approach to maximise geographic breadth and increase accessibility but also to reduce shipping costs and the likelihood of customs issues. An additional strength was that it could facilitate the development of more standardised and automated approaches for long read technologies that are currently underrepresented in generating genomic references for biodiversity genomics. Supporting a variety of technologies is important as it takes advantage of their individual characteristics (e.g. portability or lower priced solutions) to increase sequencing capability and accessibility in under-resourced countries, regions and institutions in ERGA. In the end, we partnered with a total of 26 sequencing facilities, 17 with PacBio and 9 with ONT sequencing platforms available (Fig. 2c), and documented the minimum sample collection and quality requirements for each partner. Here, we recommended the following data-type volumes for assembly generation: 30X HiFi or 60X ONT, 25X Hi-C (per haplotype) and 25X (per haplotype) Illumina (in cases where ONT data was used), and the following data-type volumes for annotation: total of 100 million reads if >five tissue types are available, or 30 million reads if tissue samples are pooled³⁴. IsoSeq production was not a mandatory requirement but was promoted, where feasible. The pilot test’s 98 species were sequenced across 25 main partnering sequencing facilities (Supplementary Table 1), and additional data was generated by Novogene for four species from the Netherlands and Hungary. 27 species were sequenced using an ONT platform, 75 using the PacBio Sequel II platform, and four by both platforms. For scaffolding and curation purposes, proximity ligation sequencing was highly recommended. A total of 76 species had some form of proximity ligation sequencing conducted, 47 species with Arima-Hi-C (Arima Genomics), 24 species with Dovetail Omni-C® (Dovetail Genomics), and five with Proximo (Phase Genomics) (Fig. 3a). Regardless of the partnering sequencing facility utilised or species being sequenced, the facilities were expected to produce sufficient data to reach at minimum EBP recommendations³⁵. An ERGA Sequencing Hub was also established at the University of Florence (Italy) Genomics Core to support the sequencing of the 99 libraries prepared by the ERGA Library Preparation Hubs (Supplementary Tables 3, 4). Upon sequencing data generation, both genomic and transcriptomic data were shared with the genome teams through the internal ERGA data repository.

Fig. 3 [Images not available. See PDF.]

Pilot test data production per species progression.

a total data production progress across all 98 species included, noting that data not planned/required for 12 species for proximity ligation, and 15 species for annotation data. b species distribution of species with genome assemblies available, both draft and curated assemblies are shown here. The data-type distribution for these species is also supplied. See Supplementary Fig. 3 for complete species tree.

Genome assembly and annotation

A requirement for becoming an ERGA reference genome was that the genome assembly reached, at minimum, the EBP standard for assembly quality³⁵. To ensure the infrastructure supported the production of genomic references to this standard, we developed assembly guidelines with workflows tailored for both ONT and HiFi-based genome assemblies³⁶. The use of these workflows was not mandatory, and any assembly workflow would be accepted if the resulting assembly met the appropriate assembly quality³⁵. To streamline the assessment and validate all ERGA genomic references, we established a stepwise procedure of 1) QC metrics assessment, 2) internal peer review, and 3) manual curation. On completion of a draft assembly, each genome team reported a set of standard QC metrics³⁷ that include a contaminant assessment, K-mer metrics, Hi-C map and graph production, gene prediction analyses, and a set of summary statistics. After this, the assembly and the associated metrics underwent an internal round of peer review from assembly experts (ERGA Sequencing and Assembly Committee). After feedback integration, each genome team uploaded the pre-curation assembly to the internal ERGA data repository along with details of the assembly construction (https://gitlab.com/wtsi-grit/documentation/-/blob/main/yaml_format.md) and each team was provided with the opportunity to submit their reference genome to an internal panel of expert curators who conducted a final manual curation³⁸.

Due to the decentralised nature of the infrastructure, all 98 species progressed through the steps at different rates, depending on the number and complexity of permits (Supplementary Note 1), difficulty of sample collection (Supplementary Note 2), need for sample specific protocol development (Supplementary Note 3), partnering sequencing facility capacity, and assembly complexity. Figure 3a highlights the current status of each species that has an assembly generated and shows that 13 complete and curated reference genomes have been generated (11 of which can be found in the INSDC), a further 17 are complete but require curation, and 8 are in non-final draft stage.

From the 30 reference genome assemblies with a ‘Curated’ or ‘Pre-curation’ status, we found 14 cases where the assemblies do not meet the quality standard 6.C.Q40 EBP standard criteria (See Supplementary glossary and Fig. 4a). For instance, Argentina silus (fArgSil1) and Knipowitschia panizzae (fKniPan1) have scaffold N50 values that meet the minimum requirement, indicating successful Hi-C scaffolding, however both fall short in terms of contig contiguity (N50 < 1 Mbp). In addition, those two pre-curation assemblies contained many small scaffolds, which increased the total number and translated to higher values of Scaffold L95. Notably, Phaeosaccion multiseriatum (uoPhaMult1) meets the contig N50 but does not meet the scaffold N50 metric (N50 > 10 Mbp). In the cases of Spongipellis delectans (gfSpoDele1) and Phakellia ventilabrum (odPhaVent1), they reached a chromosomal scale N50 scaffolding (6.C.Q40), but not the N50 threshold used as a proxy in Fig. 4a (6.7.Q40), a minimum criteria set for vertebrates but that cannot be applied to taxa with chromosome length N50 less than 10 Mbp.

Fig. 4 [Images not available. See PDF.]

Quality control and status of the 38 genome assemblies evaluated.

a Genome assemblies are represented according to their Scaffold N50 (y-axis, log₁₀) and number of the longest scaffolds that comprise at least 95% of the assembly (x-axis, log₂). Bubble size is proportional to assembly span. Empty bubbles depict HiFi-based genomes, while full bubbles are ONT-based. Colours are according to assembly status (Curated, Pre-curation, Non-final draft). Lower values for both axes indicate better assembly contiguity. Assemblies not reaching the EBP-recommended One Megabase Contig N50 (log₁₀1,000,000 = 6) or 10 Megabase Scaffold N50 (log₁₀10,000,000 = 7) here a proxy for chromosome-level scaffolds are labelled with their ToLIDs* (https://id.tol.sanger.ac.uk/). b Completed HiFi- and ONT-based genomes assemblies are represented according to their Quality value (QV, y-axis) and number of gaps per Gbp (log₁₀, x-axis). The bubble size is proportional to assembly size. Colour grade of the bubbles is according to the K-mer completeness score. ToLIDs are reported for the assemblies that are below the recommended EBP metric for QV (40), Gaps/Gbp (log₁₀1000 = 3) or K-mer completeness (90%). Quality values are calculated differently for HiFi-based assemblies than for ONT-based assemblies and should not be compared directly. c BUSCO completeness scores for genome assemblies with ‘Curated’ and ‘Pre-curation’ status. Using two orthologs databases, one for a more recent last common ancestor encompassing related species (blue), and one for all eukaryotes (grey), we seek a more comprehensive estimation of the assembly completeness. Number of single-copy orthologs present on each database is reported. *Briefly, a ToLID is a unique identifier for an individual organism within a species sampled for genome sequencing, consisting of one or two lowercase letters for high-level taxonomic rank and clade, respectively, followed by three letters for genus and species each. Thus, within insects (i), the Hemiptera (i) includes Andrena humilis (iyAndHumi1) and Osmia cornuta (iyOsmCorn1). The Coleoptera (c) contains Carabus granulatus (icCarGran1), C. intricatus (icCarIntr1), and Leptodirus hochenwarti (icLepHoch2). Ephemeroptera (e) features Epeorus assimilis (ieEpeAssi1), and among Strepsiptera (v) it is found Stylops ater (ivStyAter1). Lepidoptera (l) includes Coenonympha glycerion (ilCoeGlyc1), Helleia helle (ilHelHell1), and Parnassius mnemosyne (ilParMnem1). Within the fungi (g), Agaricomycetes (f) are represented by Spongipellis delectans (gfSpoDele1). For sponges (o), Demospongiae (d) includes Phakellia ventilabrum (odPhaVent1), and among algae (u), Heterokontophyta (o) are represented by Phaeosaccion multiseriatum (uoPhaMult1). The fishes (f) include Alburnus alburnus (fAlbAlb2), Ammodytes marinus (fAmmMar1), Anaecypris hispanica (fAnaHis1), Argentina silus (fArgSil1), Knipowitschia panizzae (fKniPan1), Perca sp.‘yellow fin Alpine’ (fPerYfa1), Salvelinus alpinus (fSalAlp1), Silurus aristotelis (fSilAri1), Solea solea (fSolSol8), Tripterygion tripteronotum (fTriTrp1), and Zingel asper (fZinAsp1). Birds (b) are represented by Haliaeetus albicilla (bHalAlb1), Oenanthe leucura (bOenLec1), and Tetrao urogallus (bTetUro2). Mammals (m) include Canis aureus (mCanAur2), Chionomys nivalis (mChiNiv1), Lepus granatensis (mLepGra1), Lepus europaeus (mLepEur2), and Mustela lutreola (mMusLut1). Among reptiles (r) is Vipera ursinii (rVipUrs1). Within dicotyledons (d), the Ericales (d) include Hottonia palustris (ddHotPalu1), and Rosales and Fabales (r) features Prunus brigantina (drPruBrig1) and Trifolium dubium (drTriDubi1), respectively. Finally, among ‘other chordates’ (k), Ascidiacea (a) includes Botryllus schlosseri (kaBotSchl2), while in the category ‘other animal phyla’ (t), Nematomorpha (f) is exemplified by Gordionus montsenyensis (tfGorSpeb1).

We found differences between HiFi- and ONT-based assemblies in the K-mer-based analyses, for example, the average quality value (QV) for HiFi-based assemblies was 61, while for ONT-based it was 38. From these ONT assemblies, five species showed values below the recommended 40, which corresponds to an error rate > 0.01% (Fig. 4b). It should be noted that in the case of ONT-based assemblies K-mers were derived from orthogonal Illumina reads from the same individual, whereas in the case of Hifi assemblies the K-mers were derived from the same data used to generate the genome assembly, likely inflating QV estimation due to data-interdependence. Further research is warranted on how to mitigate this issue. Recent unpublished results from within ERGA suggest that assembly of newer ONT data (Kit14, Q20+) consistently generates assemblies with QV > 40, perhaps side-stepping this issue. Eleven species showed K-mer completeness below 90%, with four being below 80% and one also lower than 70%. Out of these, six belonged to ONT-based assemblies while eight had curated status (Fig. 4b). A caveat to K-mer completeness is that pseudohaploid assemblies (the typical output of ONT-based assemblies) of heterozygous genomes tend to have lower K-mer completeness. This highlights the need for continued development of diploid assembly strategies to ensure high K-mer completeness.

Five genomes exceeded the recommended metric Gaps/Gbp²⁶ as they all had >1000 remaining (Argentina silus (fArgSil1), Knipowitschia panizzae (fKniPan1), Ammodytes marinus (fAmmMar1), Salvelinus alpinus (fSalAlp1) and Vipera ursinii rakosiensis (rVipUrs1)). Despite this, for all the completed assemblies, Ns accounted for less than 0.05% of the genome, with the exception of Mustela lutreola (mMusLut1). For this genome assembly, which has yet to undergo final curation (the only large ONT-based assembly evaluated >2 Gbp), 0.55% of its sequence was composed of Ns (Fig. 4b).

Besides EBP metrics, when estimating completeness using single-copy orthologs, Phakellia ventilabrum (odPhaVent1) and Gordionus montsenyensis (tfGorSpeb1) assemblies had lower values than recommended. tfGorSpeb1 is one of the first of its phylum to be sequenced³⁹, and so is therefore underrepresented in the BUSCO database (Fig. 4c)⁴⁰. Two species, Trifolium dubium (drTriDubi1) and the Salvelinus alpinus (fSalAlp1), both have higher ploidy levels (tetraploid and partial tetraploid, respectively) and had much higher BUSCO duplicate values than the recommended 5% (Supplementary Table 1).

For the pilot test, the sample collection process for the included species was ideally conducted to facilitate simultaneous genomic and transcriptomic data production. After data deposition to the ERGA data repository, we designed the infrastructure to have the flexibility necessary for each genome team to decide whether the annotation will be conducted i) by the genome team or sequencing facility, ii) with supporting expertise from the internal ERGA community, iii) or wait until the assembly and annotation data is uploaded to ENA where a gold standard annotation will be generated by Ensembl⁴¹. Although annotation was not mandatory, we produced sequencing data to support annotation data for 81 species (66 with RNA-Seq data, and 15 IsoSeq data). For those species with IsoSeq data generated, 13 also obtained RNA-Seq data. For the 30 genome teams spanning 16 countries that lacked the resources necessary to generate annotation data, we ensured that samples were shipped to a dedicated ERGA Library Preparation Hub. Here, 76 libraries were prepared and shipped to the ERGA Sequencing Hub for data production. In some groups annotation is still underway, but seven genome teams reported that they have a finalised annotation.

Phylogenetic representativeness and sampling bias

Bias was found in the representation of countries (Fig. 2), distribution of species sampled per country (even when population size is considered (Supplementary Fig. 7) and species distribution across the phylogenetic tree. Generally, non-Widening countries were more strongly represented than Widening countries and certain branches of the tree of life were overrepresented (Mammalia, Aves, Actinopterygii and Magnoliopsida), whilst others (Insecta, Amphibia Mollusca, Annelida, Fungi and most protist groups) were underrepresented. Feasibility was another obstacle. First, the production of long-read and -range sequencing on a species sample requires a significant amount of HMW DNA per 1 Gb of genome size and so small-sized species or species with very large genomes remain an unsolved challenge (Supplementary Note 2). Second, for some taxa and species, co-purification of secondary compounds resulted in sequencing chemistry interferences. Finally, ideal tissue preservation was not always possible due to sampling at remote destinations or from scientific collections where samples were preserved a long time ago (Supplementary Note 6).

Moving forward, a more robust species prioritisation process could ensure that all species are assessed using clearly specified criteria with a scoring system that is responsive to the needs of both equity deserving countries (see Supplementary glossary) and underrepresented taxa. For example, species from higher taxonomic groups without reference genomes could be prioritised over those more resource abundant groups or Widening countries could be prioritised over non-Widening countries. A more robust species prioritisation process could also facilitate knowledge transfer and serve as a seed for national investments in biodiversity genomics. Tackling these challenges will require a greater investment in research and development as well as highly-skilled personnel, additionally researchers may need incentives to prioritise the interest of species or taxa that remain underrepresented in public databases.

Enhancing end-use through genome annotation

The first hurdle in annotation is the availability of sufficient evidence (transcriptomic and protein sequence data) from focal species, databases and predictive models of repeats. Secondly, even with appropriate data, the most accurate genome annotation pipelines require advanced skills to both install and run which reduces their accessibility and ultimately their utility. Finally, robust annotation quality assessment tools are lacking particularly for species with underrepresented genomic resources, for instance gene content assessment tools such as BUSCO⁴² remain unable to account for species within taxonomic groups that have incomplete gene sets available leading to unreliable quality assessments.

Obtaining, and equitably distributing, financial resources will be required to equip researchers, labs, and regions for annotation in a manner that responds to their varying resource realities. Additionally, the development of more easily installable and reproducible pipelines are needed, and thankfully some new tools are now emerging with this in mind⁴³. Standardised and streamlined annotation pipelines are needed for consistency which is crucial for many analyses such as comparative genomics as it can facilitate more confident comparisons. Finally, sequencing more underrepresented genomes will help improve quality assessment tools. Filling in phylogenetic gaps will provide more opportunities for comparisons among taxa but also to develop better models for gene predictions. Despite these challenges, it is important that genomes are annotated. Many downstream analyses are based solely on the predicted genes from the annotation, and incomplete or incorrect results will negatively impact studies of both short-term and broad evolutionary processes.

Decentralising reference production and reproducibility

During the pilot test the reference genomics resources were produced across diverse and transdisciplinary research groups, institutes and countries. This diversity resulted in variances in accessibility, capacity and capability in sequencing technologies, computation, and software but also across different taxa. The overrepresentation of pilot sequencing facility partners located in Western Europe compared to Eastern Europe demonstrates such disparity. Furthermore, the data agnostic approach taken led to challenges in standardising assembly, annotation and curation protocols, workflows and procedures across the project. For instance, a blanket adoption of the VGP pipeline for diploid genomes based on PacBio HiFi and Hi-C sequencing (https://gxy.io/GTN:T00039; https://workflowhub.eu/workflows/325?version=1) was not appropriate as this approach would not cater for polyploid genomes nor those assemblies produced that were ONT-based. A further challenge was the provision of a centralised system for the storage and transfer of raw and final genomic and transcriptomic data. This was particularly challenging in cases where data production spanned two or more locations (e.g. PacBio sequenced at one site, Hi-C at a second, and RNA at a third) and was subsequently assembled at another site. While the Nextcloud instance created by BSC was an elegant solution for transferring vast quantities of data between parties, it required a vast amount of personnel hours to manage, in addition to its baseline system-wide maintenance requirements.

Moving forward, a key goal for ERGA is the production of standardised and reusable pipelines that are: responsive to all sequencing ‘recipes’ (PacBio, ONT, or other future technologies); written for Galaxy, Snakemake, and/or Nextflow workflow managers; made publicly available (https://github.com/ERGA-consortium/pipelines); and are actively maintained by the ERGA community with regular scheduled and versioned updates. It would also be beneficial to diversify the availability of sequencing instruments to allow for more instances where sequencing and assembly can be produced concurrently at the same location, reducing the need for transferring files that can reach up to 1 TB in size.

Building a more socially just infrastructure

Building a truly inclusive, diverse and equitable infrastructure for biodiversity genomics faces structural constraints. They are mainly twofold: first, lack of equity for and inclusion of minorities in science within the countries of Europe^18,49; second, extreme economic and political inequity between Europe and countries in the Global South⁵⁰. For the pilot test, no data was collected on race, ethnicity, religion, sexual orientation, disability, career level or the intersections of these with gender and with each other. This data deficiency made it impossible to critically evaluate the consortium in terms of inclusiveness. Some preliminary data generated in regard to sex suggested that by allowing genome teams to organically form it resulted in sex imbalances. Hence, there is a high likelihood that this also resulted in an underrepresentation of many other minoritised groups¹⁸, a known trend across European science¹⁸. The second constraint arises from a pressure to confine a biodiversity genomics consortium to the political boundary of Europe and the nation-states within. Europe, and the nations within it, are not naturally occurring units of biodiversity. In fact, Europe is part of a much wider biogeographical realm (the Palaearctic) that includes large parts of Africa and Asia⁵¹ (https://www.britannica.com/science/biogeographic-region).

As ERGA progresses, the consortium should prioritise the collection of applicable demographic data. Moreover, outreach activities should be conducted to explicitly recruit researchers from sectors of the population that are underrepresented in science. To really address the biodiversity crisis in a meaningful way, it will be important for ERGA to expand its reach globally. After all, most biodiversity by far resides not in Europe but in the Global South. Much commitment and ingenuity will be required to overcome the effects on biodiversity genomics of the equity gap that separates Europe as a block from many countries in the Global South. It will be a challenge to overcome the boundaries and constraints often dictated by scientific funding, but it is a challenge that must be overcome on the road towards a sustainable future. Through harnessing the power of its positioning in the EBP, ERGA should make efforts to become more integrated with other ongoing and related initiatives in neighbouring regions, e.g. Africa BioGenome Project⁵².

Prioritising engagement and outreach

Effective engagement is commonly seen as a constraint rather than an opportunity due to resource and time limitations, and a lack of training and awareness. Although a virtual workshop was provided during the pilot test to train researchers on 1) the significance of interested party engagement and 2) the skills to identify, map, and comprehend the needs of potential interested parties, it remained a challenge to transition researcher focus from reference genomes to the practical applications of genomics more broadly. Additionally, although the infrastructure was designed to recognise and include the rights and interests of Indigenous Peoples and Local Communities (TK and BC Labels and Notices, supporting guidelines for researcher implementation, and an ‘Open to Collaborate’ Notice on the ERGA website), researchers require more training on why and how to proactively engage and establish sustainable partnerships with Indigenous Peoples and Local Communities.

Overall, more training is needed for interested party identification, mapping, tailored engagement (varying interests and cultural perspectives), and communication. To address this, a comprehensive framework that encompasses targeted communication strategies, tailored dissemination channels, and proactive exploitation of research findings would be useful. This plan, if developed, could ensure that all interested parties receive timely and relevant information, fostering broader awareness, understanding, and utilisation of the results generated by biodiversity genomics research. Supporting ERGA members in this way could empower researchers to get more involved at the interface between biodiversity genomics research and biodiversity policy (Supplementary Note 4).

Scaling training and knowledge transfer

Financial resources are not equally distributed among countries, institutions or researchers, leading to limited access to crucial state-of-the-art training, resulting in significant disparities in terms of the expertise required to access and utilise these resources. Given the economic privilege that even the least wealthy EU countries have when compared to countries in the Global South, it is clear that access to funding for mobility is a huge barrier globally. Throughout the pilot test, several trainings were held and guidelines developed to enhance the user-friendliness of the infrastructure as well as to streamline its use; however, there was no clear long-term strategy for training and knowledge transfer.

To develop a genomics curriculum that is responsive to the needs of researchers and trainees, and promote the long-term building of capacity within these countries, an investment into a long-term strategy will be required. For instance, a publicly available knowledge transfer platform could be created to provide ERGA members with resources and training relating to each step of reference genome production, but could also provide links to complementary initiative resources e.g. EBP, Elixir (https://elixir-europe.org/), Galaxy (https://usegalaxy.org/), DSI Network (https://www.dsiscientificnetwork.org/), gBIKE (https://g-bikegenetics.eu/en), CETAF (https://cetaf.org/), etc. Such a platform could also provide a space for the sharing of relevant biodiversity genomics educational materials that could further aid collaborations between researchers who are shaping the future of biodiversity genomics curricula development globally.