Your search keyword '"Hénaff E"' showing total 13 results

1. FloodNet: low-cost ultrasonic sensors for real-time measurement of hyperlocal, street-level floods in New York City

Author

Mydlarz, Charlie, primary, Challagonda, P., additional, Steers, B., additional, Rucker, J., additional, Brain, T., additional, Branco, Brett, additional, Burnett, Hannah Eisler, additional, Kaur, A., additional, Fischman, R., additional, Graziano, K., additional, Kreuger, K., additional, Hénaff, E., additional, Ignace, V., additional, Jozwiak, E., additional, Palchuri, J., additional, Pierone, P., additional, Rothman, P., additional, Toledo-Crow, R., additional, and Silverman, Andrea I., additional

Published

2023

2. Sequencing of 6.7 Mb of the melon genome using a BAC pooling strategy

Author

Garcia-Mas Jordi, Casacuberta Josep M, Mir Gisela, Hénaff Elizabeth, Benjak Andrej, González Víctor M, and Puigdomènech Pere

Subjects

Botany, QK1-989

Abstract

Abstract Background Cucumis melo (melon) belongs to the Cucurbitaceae family, whose economic importance among horticulture crops is second only to Solanaceae. Melon has a high intra-specific genetic variation, morphologic diversity and a small genome size (454 Mb), which make it suitable for a great variety of molecular and genetic studies. A number of genetic and genomic resources have already been developed, such as several genetic maps, BAC genomic libraries, a BAC-based physical map and EST collections. Sequence information would be invaluable to complete the picture of the melon genomic landscape, furthering our understanding of this species' evolution from its relatives and providing an important genetic tool. However, to this day there is little sequence data available, only a few melon genes and genomic regions are deposited in public databases. The development of massively parallel sequencing methods allows envisaging new strategies to obtain long fragments of genomic sequence at higher speed and lower cost than previous Sanger-based methods. Results In order to gain insight into the structure of a significant portion of the melon genome we set out to perform massive sequencing of pools of BAC clones. For this, a set of 57 BAC clones from a double haploid line was sequenced in two pools with the 454 system using both shotgun and paired-end approaches. The final assembly consists of an estimated 95% of the actual size of the melon BAC clones, with most likely complete sequences for 50 of the BACs, and a total sequence coverage of 39x. The accuracy of the assembly was assessed by comparing the previously available Sanger sequence of one of the BACs against its 454 sequence, and the polymorphisms found involved only 1.7 differences every 10,000 bp that were localized in 15 homopolymeric regions and two dinucleotide tandem repeats. Overall, the study provides approximately 6.7 Mb or 1.5% of the melon genome. The analysis of this new data has allowed us to gain further insight into characteristics of the melon genome such as gene density, average protein length, or microsatellite and transposon content. The annotation of the BAC sequences revealed a high degree of collinearity and protein sequence identity between melon and its close relative Cucumis sativus (cucumber). Transposon content analysis of the syntenic regions suggests that transposition activity after the split of both cucurbit species has been low in cucumber but very high in melon. Conclusions The results presented here show that the strategy followed, which combines shotgun and BAC-end sequencing together with anchored marker information, is an excellent method for sequencing specific genomic regions, especially from relatively compact genomes such as that of melon. However, in agreement with other results, this map-based, BAC approach is confirmed to be an expensive way of sequencing a whole plant genome. Our results also provide a partial description of the melon genome's structure. Namely, our analysis shows that the melon genome is highly collinear with the smaller one of cucumber, the size difference being mainly due to the expansion of intergenic regions and proliferation of transposable elements.

Published

2010

3. Holobiont Urbanism: sampling urban beehives reveals cities' metagenomes.

Author

Hénaff E, Najjar D, Perez M, Flores R, Woebken C, Mason CE, and Slavin K

Abstract

Background: Over half of the world's population lives in urban areas with, according to the United Nations, nearly 70% expected to live in cities by 2050. Our cities are built by and for humans, but are also complex, adaptive biological systems involving a diversity of other living species. The majority of these species are invisible and constitute the city's microbiome. Our design decisions for the built environment shape these invisible populations, and as inhabitants we interact with them on a constant basis. A growing body of evidence shows us that human health and well-being are dependent on these interactions. Indeed, multicellular organisms owe meaningful aspects of their development and phenotype to interactions with the microorganisms-bacteria or fungi-with which they live in continual exchange and symbiosis. Therefore, it is meaningful to establish microbial maps of the cities we inhabit. While the processing and sequencing of environmental microbiome samples can be high-throughput, gathering samples is still labor and time intensive, and can require mobilizing large numbers of volunteers to get a snapshot of the microbial landscape of a city., Results: Here we postulate that honeybees may be effective collaborators in gathering samples of urban microbiota, as they forage daily within a 2-mile radius of their hive. We describe the results of a pilot study conducted with three rooftop beehives in Brooklyn, NY, where we evaluated the potential of various hive materials (honey, debris, hive swabs, bee bodies) to reveal information as to the surrounding metagenomic landscape, and where we conclude that the bee debris are the richest substrate. Based on these results, we profiled 4 additional cities through collected hive debris: Sydney, Melbourne, Venice and Tokyo. We show that each city displays a unique metagenomic profile as seen by honeybees. These profiles yield information relevant to hive health such as known bee symbionts and pathogens. Additionally, we show that this method can be used for human pathogen surveillance, with a proof-of-concept example in which we recover the majority of virulence factor genes for Rickettsia felis, a pathogen known to be responsible for "cat scratch fever"., Conclusions: We show that this method yields information relevant to hive health and human health, providing a strategy to monitor environmental microbiomes on a city scale. Here we present the results of this study, and discuss them in terms of architectural implications, as well as the potential of this method for epidemic surveillance., (© 2023. The Author(s).)

Published

2023

4. Making waves: Uses of real-time, hyperlocal flood sensor data for emergency management, resiliency planning, and flood impact mitigation.

Author

Silverman AI, Brain T, Branco B, Challagonda PSV, Choi P, Fischman R, Graziano K, Hénaff E, Mydlarz C, Rothman P, and Toledo-Crow R

Subjects

Floods, Urbanization

Abstract

Flooding is expected to increase due to intensification of extreme precipitation events, sea-level rise, and urbanization. Low-cost water level sensors have the ability to fill a critical data gap on the presence, depth, and duration of street-level floods by measuring flood profiles (i.e., flood stage hydrographs) in real-time with a time interval on the order of minutes. Hyperlocal flood data collected by low-cost sensors have many use cases for a variety of stakeholders including municipal agencies, community members, and researchers. Here we outline examples of potential uses of flood sensor data before, during, and after flood events, based on dialog with stakeholders in New York City. These uses include inputs to predictive flood models, generation of real-time flood alerts for community members and emergency response teams, storm recovery assistance and cataloging of storm impacts, and informing infrastructure design and investment for long-term flood resilience project planning., (Copyright © 2022 Elsevier Ltd. All rights reserved.)

Published

2022

5. Correction to: Comprehensive benchmarking and ensemble approaches for metagenomic classifiers.

Author

McIntyre ABR, Ounit R, Afshinnekoo E, Prill RJ, Hénaff E, Alexander N, Minot SS, Danko D, Foox J, Ahsanuddin S, Tighe S, Hasan NA, Subramanian P, Moffat K, Levy S, Lonardi S, Greenfield N, Colwell RR, Rosen GL, and Mason CE

Abstract

Following publication of the original article [1], the authors would like to highlight the following two corrections.

Published

2019

6. Comprehensive benchmarking and ensemble approaches for metagenomic classifiers.

Author

McIntyre ABR, Ounit R, Afshinnekoo E, Prill RJ, Hénaff E, Alexander N, Minot SS, Danko D, Foox J, Ahsanuddin S, Tighe S, Hasan NA, Subramanian P, Moffat K, Levy S, Lonardi S, Greenfield N, Colwell RR, Rosen GL, and Mason CE

Subjects

Benchmarking standards, Contig Mapping standards, DNA Barcoding, Taxonomic standards, Humans, Microbiota, Phylogeny, Sequence Analysis, DNA standards, Benchmarking methods, Contig Mapping methods, DNA Barcoding, Taxonomic methods, Metagenome, Sequence Analysis, DNA methods, Software

Abstract

Background: One of the main challenges in metagenomics is the identification of microorganisms in clinical and environmental samples. While an extensive and heterogeneous set of computational tools is available to classify microorganisms using whole-genome shotgun sequencing data, comprehensive comparisons of these methods are limited., Results: In this study, we use the largest-to-date set of laboratory-generated and simulated controls across 846 species to evaluate the performance of 11 metagenomic classifiers. Tools were characterized on the basis of their ability to identify taxa at the genus, species, and strain levels, quantify relative abundances of taxa, and classify individual reads to the species level. Strikingly, the number of species identified by the 11 tools can differ by over three orders of magnitude on the same datasets. Various strategies can ameliorate taxonomic misclassification, including abundance filtering, ensemble approaches, and tool intersection. Nevertheless, these strategies were often insufficient to completely eliminate false positives from environmental samples, which are especially important where they concern medically relevant species. Overall, pairing tools with different classification strategies (k-mer, alignment, marker) can combine their respective advantages., Conclusions: This study provides positive and negative controls, titrated standards, and a guide for selecting tools for metagenomic analyses by comparing ranges of precision, accuracy, and recall. We show that proper experimental design and analysis parameters can reduce false positives, provide greater resolution of species in complex metagenomic samples, and improve the interpretation of results.

Published

2017

7. Retrotransposons are specified as DNA replication origins in the gene-poor regions of Arabidopsis heterochromatin.

Author

Vergara Z, Sequeira-Mendes J, Morata J, Peiró R, Hénaff E, Costas C, Casacuberta JM, and Gutierrez C

Subjects

Arabidopsis cytology, Arabidopsis metabolism, Cell Line, Chromatin genetics, Chromatin metabolism, Chromosome Mapping, DNA, Plant genetics, DNA, Plant metabolism, GC Rich Sequence genetics, Genome, Plant genetics, Heterochromatin metabolism, Histones metabolism, Lysine metabolism, Methylation, Microscopy, Confocal, Reverse Transcriptase Polymerase Chain Reaction, Transcription, Genetic, Arabidopsis genetics, DNA Replication, Heterochromatin genetics, Replication Origin genetics, Retroelements genetics

Abstract

Genomic stability depends on faithful genome replication. This is achieved by the concerted activity of thousands of DNA replication origins (ORIs) scattered throughout the genome. The DNA and chromatin features determining ORI specification are not presently known. We have generated a high-resolution genome-wide map of 3230 ORIs in cultured Arabidopsis thaliana cells. Here, we focused on defining the features associated with ORIs in heterochromatin. In pericentromeric gene-poor domains ORIs associate almost exclusively with the retrotransposon class of transposable elements (TEs), in particular of the Gypsy family. ORI activity in retrotransposons occurs independently of TE expression and while maintaining high levels of H3K9me2 and H3K27me1, typical marks of repressed heterochromatin. ORI-TEs largely colocalize with chromatin signatures defining GC-rich heterochromatin. Importantly, TEs with active ORIs contain a local GC content higher than the TEs lacking them. Our results lead us to conclude that ORI colocalization with retrotransposons is determined by their transposition mechanism based on transcription, and a specific chromatin landscape. Our detailed analysis of ORIs responsible for heterochromatin replication has implications on the mechanisms of ORI specification in other multicellular organisms in which retrotransposons are major components of heterochromatin and of the entire genome., (© The Author(s) 2017. Published by Oxford University Press on behalf of Nucleic Acids Research.)

Published

2017

8. Jitterbug: somatic and germline transposon insertion detection at single-nucleotide resolution.

Author

Hénaff E, Zapata L, Casacuberta JM, and Ossowski S

Subjects

Algorithms, Arabidopsis genetics, Computer Simulation, Genome, Human, Homozygote, Humans, Neoplasms genetics, Polymorphism, Genetic, Reproducibility of Results, Software, Computational Biology methods, DNA Transposable Elements, Genomics methods, Germ Cells metabolism, Mutagenesis, Insertional

Abstract

Background: Transposable elements are major players in genome evolution. Transposon insertion polymorphisms can translate into phenotypic differences in plants and animals and are linked to different diseases including human cancer, making their characterization highly relevant to the study of genome evolution and genetic diseases., Results: Here we present Jitterbug, a novel tool that identifies transposable element insertion sites at single-nucleotide resolution based on the pairedend mapping and clipped-read signatures produced by NGS alignments. Jitterbug can be easily integrated into existing NGS analysis pipelines, using the standard BAM format produced by frequently applied alignment tools (e.g. bwa, bowtie2), with no need to realign reads to a set of consensus transposon sequences. Jitterbug is highly sensitive and able to recall transposon insertions with a very high specificity, as demonstrated by benchmarks in the human and Arabidopsis genomes, and validation using long PacBio reads. In addition, Jitterbug estimates the zygosity of transposon insertions with high accuracy and can also identify somatic insertions., Conclusions: We demonstrate that Jitterbug can identify mosaic somatic transposon movement using sequenced tumor-normal sample pairs and allows for estimating the cancer cell fraction of clones containing a somatic TE insertion. We suggest that the independent methods we use to evaluate performance are a step towards creating a gold standard dataset for benchmarking structural variant prediction tools.

Published

2015

9. Transposon Insertions, Structural Variations, and SNPs Contribute to the Evolution of the Melon Genome.

Author

Sanseverino W, Hénaff E, Vives C, Pinosio S, Burgos-Paz W, Morgante M, Ramos-Onsins SE, Garcia-Mas J, and Casacuberta JM

Subjects

Cucumis sativus genetics, Gene Deletion, Genetic Loci, Nucleotides genetics, Phylogeny, Selection, Genetic, Cucurbitaceae genetics, DNA Transposable Elements genetics, Evolution, Molecular, Genome, Plant, Mutagenesis, Insertional genetics, Polymorphism, Single Nucleotide genetics

Abstract

The availability of extensive databases of crop genome sequences should allow analysis of crop variability at an unprecedented scale, which should have an important impact in plant breeding. However, up to now the analysis of genetic variability at the whole-genome scale has been mainly restricted to single nucleotide polymorphisms (SNPs). This is a strong limitation as structural variation (SV) and transposon insertion polymorphisms are frequent in plant species and have had an important mutational role in crop domestication and breeding. Here, we present the first comprehensive analysis of melon genetic diversity, which includes a detailed analysis of SNPs, SV, and transposon insertion polymorphisms. The variability found among seven melon varieties representing the species diversity and including wild accessions and highly breed lines, is relatively high due in part to the marked divergence of some lineages. The diversity is distributed nonuniformly across the genome, being lower at the extremes of the chromosomes and higher in the pericentromeric regions, which is compatible with the effect of purifying selection and recombination forces over functional regions. Additionally, this variability is greatly reduced among elite varieties, probably due to selection during breeding. We have found some chromosomal regions showing a high differentiation of the elite varieties versus the rest, which could be considered as strongly selected candidate regions. Our data also suggest that transposons and SV may be at the origin of an important fraction of the variability in melon, which highlights the importance of analyzing all types of genetic variability to understand crop genome evolution., (© The Author 2015. Published by Oxford University Press on behalf of the Society for Molecular Biology and Evolution. All rights reserved. For permissions, please e-mail: journals.permissions@oup.com.)

Published

2015

10. Extensive amplification of the E2F transcription factor binding sites by transposons during evolution of Brassica species.

Author

Hénaff E, Vives C, Desvoyes B, Chaurasia A, Payet J, Gutierrez C, and Casacuberta JM

Subjects

Base Sequence, Binding Sites, Evolution, Molecular, Gene Amplification, Genetic Speciation, Inverted Repeat Sequences genetics, Molecular Sequence Data, Plant Proteins genetics, Promoter Regions, Genetic genetics, Brassica genetics, DNA Transposable Elements genetics, E2F Transcription Factors genetics, Gene Expression Regulation, Plant, Genome, Plant genetics

Abstract

Transposable elements (TEs) are major players in genome evolution. The effects of their movement vary from gene knockouts to more subtle effects such as changes in gene expression. It has recently been shown that TEs may contain transcription factor binding sites (TFBSs), and it has been proposed that they may rewire new genes into existing transcriptional networks. However, little is known about the dynamics of this process and its effect on transcription factor binding. Here we show that TEs have extensively amplified the number of sequences that match the E2F TFBS during Brassica speciation, and, as a result, as many as 85% of the sequences that fit the E2F TFBS consensus are within TEs in some Brassica species. We show that these sequences found within TEs bind E2Fa in vivo, which indicates a direct effect of these TEs on E2F-mediated gene regulation. Our results suggest that the TEs located close to genes may directly participate in gene promoters, whereas those located far from genes may have an indirect effect by diluting the effective amount of E2F protein able to bind to its cognate promoters. These results illustrate an extreme case of the effect of TEs in TFBS evolution, and suggest a singular way by which they affect host genes by modulating essential transcriptional networks., (© 2014 The Authors The Plant Journal © 2014 John Wiley & Sons Ltd.)

Published

2014

11. Next-generation sequencing, FISH mapping and synteny-based modeling reveal mechanisms of decreasing dysploidy in Cucumis.

Author

Yang L, Koo DH, Li D, Zhang T, Jiang J, Luan F, Renner SS, Hénaff E, Sanseverino W, Garcia-Mas J, Casacuberta J, Senalik DA, Simon PW, Chen J, and Weng Y

Subjects

Chromosome Mapping, Cucumis cytology, Gene Rearrangement, High-Throughput Nucleotide Sequencing, In Situ Hybridization, Fluorescence, Models, Genetic, Phylogeny, Ploidies, Sequence Analysis, DNA, Species Specificity, Chromosomes, Plant genetics, Cucumis genetics, Genome, Plant genetics, Synteny genetics

Abstract

In the large Cucurbitaceae genus Cucumis, cucumber (C. sativus) is the only species with 2n = 2x = 14 chromosomes. The majority of the remaining species, including melon (C. melo) and the sister species of cucumber, C. hystrix, have 2n = 2x = 24 chromosomes, implying a reduction from n = 12 to n = 7. To understand the underlying mechanisms, we investigated chromosome synteny among cucumber, C. hystrix and melon using integrated and complementary approaches. We identified 14 inversions and a C. hystrix lineage-specific reciprocal inversion between C. hystrix and melon. The results reveal the location and orientation of 53 C. hystrix syntenic blocks on the seven cucumber chromosomes, and allow us to infer at least 59 chromosome rearrangement events that led to the seven cucumber chromosomes, including five fusions, four translocations, and 50 inversions. The 12 inferred chromosomes (AK1-AK12) of an ancestor similar to melon and C. hystrix had strikingly different evolutionary fates, with cucumber chromosome C1 apparently resulting from insertion of chromosome AK12 into the centromeric region of translocated AK2/AK8, cucumber chromosome C3 originating from a Robertsonian-like translocation between AK4 and AK6, and cucumber chromosome C5 originating from fusion of AK9 and AK10. Chromosomes C2, C4 and C6 were the result of complex reshuffling of syntenic blocks from three (AK3, AK5 and AK11), three (AK5, AK7 and AK8) and five (AK2, AK3, AK5, AK8 and AK11) ancestral chromosomes, respectively, through 33 fusion, translocation and inversion events. Previous results (Huang, S., Li, R., Zhang, Z. et al., , Nat. Genet. 41, 1275-1281; Li, D., Cuevas, H.E., Yang, L., Li, Y., Garcia-Mas, J., Zalapa, J., Staub, J.E., Luan, F., Reddy, U., He, X., Gong, Z., Weng, Y. 2011a, BMC Genomics, 12, 396) showing that cucumber C7 stayed largely intact during the entire evolution of Cucumis are supported. Results from this study allow a fine-scale understanding of the mechanisms of dysploid chromosome reduction that has not been achieved previously., (© 2013 The Authors The Plant Journal © 2013 John Wiley & Sons Ltd.)

Published

2014

12. The genome of melon (Cucumis melo L.).

Author

Garcia-Mas J, Benjak A, Sanseverino W, Bourgeois M, Mir G, González VM, Hénaff E, Câmara F, Cozzuto L, Lowy E, Alioto T, Capella-Gutiérrez S, Blanca J, Cañizares J, Ziarsolo P, Gonzalez-Ibeas D, Rodríguez-Moreno L, Droege M, Du L, Alvarez-Tejado M, Lorente-Galdos B, Melé M, Yang L, Weng Y, Navarro A, Marques-Bonet T, Aranda MA, Nuez F, Picó B, Gabaldón T, Roma G, Guigó R, Casacuberta JM, Arús P, and Puigdomènech P

Subjects

Base Sequence, Chromosome Mapping, Chromosomes, Artificial, Bacterial genetics, DNA Transposable Elements genetics, Disease Resistance genetics, Genes, Duplicate genetics, Genes, Plant genetics, Genomics methods, Likelihood Functions, Models, Genetic, Molecular Sequence Annotation, Molecular Sequence Data, Sequence Alignment, Sequence Analysis, DNA, Biological Evolution, Cucumis melo genetics, Genome, Plant genetics, Phylogeny

Abstract

We report the genome sequence of melon, an important horticultural crop worldwide. We assembled 375 Mb of the double-haploid line DHL92, representing 83.3% of the estimated melon genome. We predicted 27,427 protein-coding genes, which we analyzed by reconstructing 22,218 phylogenetic trees, allowing mapping of the orthology and paralogy relationships of sequenced plant genomes. We observed the absence of recent whole-genome duplications in the melon lineage since the ancient eudicot triplication, and our data suggest that transposon amplification may in part explain the increased size of the melon genome compared with the close relative cucumber. A low number of nucleotide-binding site-leucine-rich repeat disease resistance genes were annotated, suggesting the existence of specific defense mechanisms in this species. The DHL92 genome was compared with that of its parental lines allowing the quantification of sequence variability in the species. The use of the genome sequence in future investigations will facilitate the understanding of evolution of cucurbits and the improvement of breeding strategies.

Published

2012

13. The Tnt1 retrotransposon escapes silencing in tobacco, its natural host.

Author

Hernández-Pinzón I, Cifuentes M, Hénaff E, Santiago N, Espinás ML, and Casacuberta JM

Subjects

Chromatin metabolism, DNA Methylation, Epigenesis, Genetic, Gene Expression Regulation, Gene Order, Histones metabolism, Methyltransferases metabolism, Promoter Regions, Genetic, Stress, Physiological genetics, Nicotiana metabolism, Transcription, Genetic, Gene Silencing, Retroelements genetics, Nicotiana genetics

Abstract

Retrotransposons' high capacity for mutagenesis is a threat that genomes need to control tightly. Transcriptional gene silencing is a general and highly effective control of retrotransposon expression. Yet, some retrotransposons manage to transpose and proliferate in plant genomes, suggesting that, as shown for plant viruses, retrotransposons can escape silencing. However no evidence of retrotransposon silencing escape has been reported. Here we analyze the silencing control of the tobacco Tnt1 retrotransposon and report that even though constructs driven by the Tnt1 promoter become silenced when stably integrated in tobacco, the endogenous Tnt1 elements remain active. Silencing of Tnt1-containing transgenes correlates with high DNA methylation and the inability to incorporate H2A.Z into their promoters, whereas the endogenous Tnt1 elements remain partially methylated at asymmetrical positions and incorporate H2A.Z upon induction. Our results show that the promoter of Tnt1 is a target of silencing in tobacco, but also that endogenous Tnt1 elements can escape this control and be expressed in their natural host.

Published

2012