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The Fifth Generation (5G) cellular network can be considered the way to the ubiquitous Internet and pervasive paradigm.The Internet of Vehicles (IoV) uses the network infrastructure to allow cars to be connected to new radio technologies, and can be supported by 5G networks. In this way, the Vehicle-to-Everything (V2X) integration needs 5G connections unavoidably. This paper presents a 5G V2X ecosystem to provide IoV. The proposed ecosystem is based on the Software-Defined Networking (SDN) concept. Considering vehicles as entertainment consumer points, the network infrastructure must be huge enough to guarantee delivery and quality. For this purpose, this paper evaluates vehicular Internet-based video services traffic and Vehicle-to-Vehicle (V2V) communications in urban and rural scenarios. Simulations were performed through the Network Simulator ns-3, employing millimeter Wave (mmWave) communications. Three metrics, data transfer rate, transmission delay, and Packet Delivery Ratio (PDR), were analyzed and compared for rural and urban IoV scenarios. The results have shown satisfactory performance to the IoV communications requirements when adopting the 5G network with V2X communications.

In flowering plants, seed development is initiated by the fusion of the maternal egg and central cells with two paternal sperm cells, leading to the formation of embryo and endosperm, respectively. The fertilization products are surrounded by the maternally derived seed coat, whose development prior to fertilization is blocked by epigenetic regulators belonging to the Polycomb Group (PcG) protein family. Here we show that fertilization of the central cell results in the production of auxin and most likely its export to the maternal tissues, which drives seed coat development by removing PcG function. We furthermore show that mutants for the MADS-box transcription factor AGL62 have an impaired transport of auxin from the endosperm to the integuments, which results in seed abortion. We propose that AGL62 regulates auxin transport from the endosperm to the integuments, leading to the removal of the PcG block on seed coat development. The seeds of rice, wheat and other flowering plants store a variety of nutrients, largely in the form of sugars, proteins and oils. These stored reserves provide the main source of calories for humans and livestock all over the world, so they are of major social and economic importance. Seed development is an intricate process. It begins after male sperm cells fuse with female gametes inside the flower. This leads to the formation of the embryo, which will develop into a new plant, and a structure called the endosperm, which nourishes the growing embryo. A protective seed coat surrounds the embryo and endosperm, which develops from certain parts of the parent flower. In order for the seed to develop successfully, these three components have to communicate so they can coordinate their growth. Auxin is a key plant hormone that is needed for plants to grow and develop properly and is necessary for the endosperm to form. Previous research has shown that the endosperm is also required to trigger the formation of the seed coat, but the signal that triggers this process has not yet been identified. Figueiredo et al. now address this question in a small flowering plant called Arabidopsis thaliana. The experiments show that the endosperm produces auxin, which acts as a molecular signal for the seed coat to start forming. Exposing unfertilized flowers to auxin caused a seed coat to form even though the endosperm was absent. This suggests that this hormone alone is sufficient to trigger the formation of the seed coat without any other signals. Further analysis revealed that a protein called AGL62 regulates the movement of auxin to the parts of the flower that give rise to the seed coat. In the absence of AGL62, the hormone remains trapped in the endosperm and the seed coat fails to develop. The next step following on from this work is to understand how auxin moves from the endosperm to the parts of the flower that form the seed coat.

Key message The DNA methylation status at an epigenetic quantitative trait locus in the Arabidopsis chromosome 2 is linked to the formation of apomictic-like endosperms. Seed development in most angiosperms is coupled to fertilization of the maternal gametes by two sperm cells. However, apomictic species can reproduce asexually via seeds. This trait is of great agricultural interest, as it would fix complex genotypes and allow for pollen-independent seed production. However, engineering full apomixis requires three independent processes: apomeiosis, parthenogenesis and autonomous endosperm development. While the first two have been successfully engineered in some crops, the formation of autonomous endosperms remains a challenge. Although it is known that this trait is under epigenetic control, such as of DNA methylation, the underlying mechanisms remain mostly undiscovered. Here, using epigenetic recombinant inbred lines, we identified an epigenetic quantitative trait locus in the Arabidopsis chromosome 2, which correlates with permissiveness for the formation of asexual seeds: hypomethylation at this genomic region allows the formation of larger autonomous endosperms. Importantly, the methylation at this locus only correlates with asexual seed size, and not to the size of sexual seeds or that of other organs. With this, we aim to show that screening for epialleles is a promising strategy to uncover loci underlying relevant traits and could pave the way to identifying genes necessary for the engineering of apomixis.

In flowering plants, seed development is preceded by a double fertilization event, whereby two male sperm cells fuse with two female gametes: the egg and central cells. The fertilized egg cell will form the embryo, and the fertilized central cell will give rise to the triploid endosperm, whose function is to nourish and support the embryo. Even though the endosperm has an unparalleled role for human nutrition, the molecular bases for its development are yet to be understood. Our results reveal that increasing auxin levels after fertilization drive the replication of the central cell in Arabidopsis thaliana . Auxin is sufficient to trigger central cell division and is necessary for correct endosperm development, a process dependent on the MADS-box transcription factor AGL62 (AGAMOUS-LIKE 62). We propose that the epigenetic regulators of the Polycomb group (PcG) family block central cell division before fertilization by repressing the expression of auxin biosynthesis genes in the female gametophyte. Double fertilization in flowering plants produces both the embryo and the endosperm that is going to nourish it, forming a seed. Development of the endosperm is triggered by auxin production, derepressed by an epigenetic pathway after fertilization.

An angiosperm seed is formed by the embryo and endosperm, which are direct products of fertilization, and by the maternal seed coat. These tissues communicate with each other to ensure synchronized seed development. After fertilization, auxin produced in the endosperm is exported to the integuments where it drives seed coat formation. Here, we show that the seed coat signals back to the endosperm to promote its proliferation via the steroid hormones brassinosteroids (BR). We show that BR regulate cell wall-related processes in the seed coat and that the biophysical properties of this maternal organ determine the proliferation rate of the endosperm in a manner independent of the timing of its cellularization. We thus propose that maternal BR signaling tunes endosperm proliferation to seed coat expansion.

MADS-box transcription factors (TFs) are ubiquitous in eukaryotic organisms and play major roles during plant development. Nevertheless, their function in seed development remains largely unknown. Here, we show that the imprinted Arabidopsis thaliana MADS-box TF PHERES1 (PHE1) is a master regulator of paternally expressed imprinted genes, as well as of non-imprinted key regulators of endosperm development. PHE1 binding sites show distinct epigenetic modifications on maternal and paternal alleles, correlating with parental-specific transcriptional activity. Importantly, we show that the CArG-box-like DNA-binding motifs that are bound by PHE1 have been distributed by RC/Helitron transposable elements. Our data provide an example of the molecular domestication of these elements which, by distributing PHE1 binding sites throughout the genome, have facilitated the recruitment of crucial endosperm regulators into a single transcriptional network.

The BABY BOOM (BBM) AINTEGUMENTA-LIKE (AIL) AP2/ERF domain transcription factor is a major regulator of plant cell totipotency, as it induces asexual embryo formation when ectopically expressed. Surprisingly, only limited information is available on the role of BBM during zygotic embryogenesis. Here we reexamined BBM expression and function in the model plant Arabidopsis thaliana (Arabidopsis) using reporter analysis and newly developed CRISPR mutants. BBM was expressed in the embryo from the zygote stage and also in the maternal (nucellus) and filial (endosperm) seed tissues. Analysis of CRISPR mutant alleles for BBM (bbm-cr) and the redundantly acting AIL gene PLETHORA2 (PLT2) (plt2-cr) uncovered individual roles for these genes in the timing of embryo progression. We also identified redundant roles for BBM and PLT2 in endosperm proliferation and cellularization and the maintenance of zygotic embryo development. Finally, we show that ectopic BBM expression in the egg cell of Arabidopsis and the dicot crops Brassica napus and Solanum lycopersicon is sufficient to bypass the fertilization requirement for embryo development. Together these results highlight roles for BBM and PLT2 in seed development and demonstrate the utility of BBM genes for engineering asexual embryo development in dicot species.

Several pathways control time to flowering in Arabidopsis thaliana through transcriptional and posttranscriptional gene regulation. In recent years, mRNA processing has gained interest as a critical regulator of flowering time control in plants. However, the molecular mechanisms linking RNA splicing to flowering time are not well understood. In a screen for Arabidopsis early flowering mutants we identified an allele of BRR2a. BRR2 proteins are components of the spliceosome and highly conserved in eukaryotes. Arabidopsis BRR2a is ubiquitously expressed in all analyzed tissues and involved in the processing of flowering time gene transcripts, most notably FLC. A missense mutation of threonine 895 in BRR2a caused defects in FLC splicing and greatly reduced FLC transcript levels. Reduced FLC expression increased transcription of FT and SOC1 leading to early flowering in both short and long days. Genome-wide experiments established that only a small set of introns was not correctly spliced in the brr2a mutant. Compared to control introns, retained introns were often shorter and GC-poor, had low H3K4me1 and CG methylation levels, and were often derived from genes with a high-H3K27me3-low-H3K36me3 signature. We propose that BRR2a is specifically needed for efficient splicing of a subset of introns characterized by a combination of factors including intron size, sequence and chromatin, and that FLC is most sensitive to splicing defects.

Organogenesis and development of the plant body plan requires coordinated regulation of cell proliferation and fate specification to produce specialized cell types and cell lineages. Importantly, recent advances in state-of-the-art long read next generation sequencing has now opened doors to focus on non-model species. Conflict of interest The authors declare that the research was conducted in the absence of any commercial or financial relationships that could be construed as a potential conflict of interest.

Polycomb group (PcG) proteins form an epigenetic memory system in plants and animals, but interacting proteins are poorly known in plants. Here, we have identified Arabidopsis UBIQUITIN SPECIFIC PROTEASES (USP; UBP in plant and yeasts) 12 and 13 as partners of the plant-specific PcG protein LIKE HETEROCHROMATIN PROTEIN 1 (LHP1). UBP12 binds to chromatin of PcG target genes and is required for histone H3 lysine 27 trimethylation and repression of a subset of PcG target genes. Plants lacking UBP12 and UBP13 developed autonomous endosperm in the absence of fertilization. We have identified UBP12 and UBP13 as new proteins in the plant PcG regulatory network. UBP12 and UBP13 belong to an ancient gene family and represent plant homologues of metazoan USP7. We have found that Drosophila USP7 shares a function in heterochromatic gene repression with UBP12/13 and their homologue UBP26. In summary, we demonstrate that USP7-like proteins are essential for gene silencing in diverse genomic contexts. In Arabidopsis , the Polycomb proteins mediate an epigenetic memory system that is important for gene silencing via histone methylation during development. Two novel deubiquitinases, UBP12 and UBP13, have now been identified and characterized in this regulatory network.