Project description:Genome-wide gene expression atlas of maize inbred line B73. Maize inbred B73 was used for constructing the gene atlas. Plants were grown in Plano silt loam soil at the West Madison Agricultural Research Station, Verona, WI during Summer 2008. During field preparation, 200 kg/acre of Urea (46-0-0) was applied. One day after planting, herbicides including Callisto (142 g/acre), Dual II (710 ml/acre), and Simazine (227 g/acre) were applied. For collection of seed tissues, shoots were covered before silk emergence avoiding any injury to the plants. Plants were self-pollinated on the same day to establish a common time initiation point for the harvest timeline. Greenhouse-grown plants were propagated by growing five plants per pot (30 cm top diameter, 28 cm height, 14.5 L volume) containing Metro-Mix 300 (Sun Gro Horticulture, Bellevue, WA, USA) with no additional fertilization. The growing conditions were 27 deg. C day and 24 deg. C night temperature with a 16h light (5:00am to 9:00pm) and 8h dark regime. Germinating seed tissue was generated by soaking seeds in distilled water in a Petri dish for 12h and then placing seeds between layers of moist paper towels for another 12h to allow germination. The field samples were collected between 8:00am and 10:00am, approximately 3 hours after sunrise. The greenhouse samples were collected between 8:00am and 9:00am, three hours after turning on the lights. Three biological replicates were collected for each tissue type. For all the tissues except germinating seeds, a biological replicate was constituted by collecting and pooling samples from three competitive randomly chosen plants. For germinating seed, ten randomly chosen seeds were pooled to form a biological replicate. The harvested tissues were immediately frozen in liquid nitrogen and stored at -80 deg. C. Total RNA was extracted using TRIZOL reagent (Invitrogen, http://www.invitrogen.com) following the manufacturer's protocol, and purified using RNeasy MinElute Cleanup Kit (Qiagen, http://www.qiagen.com) following the manufacturer's instructions. PLEXdb (http://www.plexdb.org) has submitted this series at GEO on behalf of the original contributor, Rajandeep S Sekhon. The equivalent experiment is ZM29 at PLEXdb. organism part name: 24H_Germinating Seed(3-replications); organism part name: 6DAS_GH_Coleoptile(3-replications); organism part name: 6DAS_GH_Primary Root(3-replications); organism part name: V1_GH_Primary Root(3-replications); organism part name: VE_Whole Seedling(3-replications); organism part name: VE_Primary Root(3-replications); organism part name: V1_Pooled Leaves(3-replications); organism part name: V1_Stem and SAM(3-replications); organism part name: V4_Stem and SAM(3-replications); organism part name: V3_Stem and SAM(3-replications); organism part name: V3_First Leaf and Sheath(3-replications); organism part name: V3_Topmost Leaf(3-replications); organism part name: V5_Shoot Tip(3-replications); organism part name: V5_First Internode(3-replications); organism part name: V5_Tip of stage-2 Leaf(3-replications); organism part name: V5_Base of stage-2 Leaf(3-replications); organism part name: V7_First Internode(3-replications); organism part name: V7_Tip of stage-2 Leaf(3-replications); organism part name: V7_Base of stage-2 Leaf(3-replications); organism part name: V9_Fourth Internode(3-replications); organism part name: V9_Eighth Leaf(3-replications); organism part name: V9_Eleventh Leaf(3-replications); organism part name: V9_Thirteenth Leaf(3-replications); organism part name: V9_Immature Leaves(3-replications); organism part name: V13_Immature Tassel(3-replications); organism part name: V18_Meiotic Tassel(3-replications); organism part name: V18_Immature Cob(3-replications); organism part name: VT_Thirteenth Leaf(3-replications); organism part name: R1_Pre-pollination Cob(3-replications); organism part name: R1_Silks(3-replications); organism part name: R1_Anthers(3-replications); organism part name: R1_Innermost Husk(3-replications); organism part name: R2_Thirteenth Leaf(3-replications); organism part name: R2_Outer Husk(3-replications); organism part name: R2_Innermost Husk(3-replications); organism part name: 2DAP_Whole Seed(3-replications); organism part name: 4DAP_Whole Seed(3-replications); organism part name: 6DAP_Whole Seed(3-replications); organism part name: 8DAP_Whole Seed(3-replications); organism part name: 10DAP_Whole Seed(3-replications); organism part name: 12DAP_Whole Seed(3-replications); organism part name: 12DAP_Endosperm(3-replications); organism part name: 14DAP_Whole Seed(3-replications); organism part name: 14DAP_Endosperm(3-replications); organism part name: 16DAP_Whole Seed(3-replications); organism part name: 16DAP_Endosperm(3-replications); organism part name: 16DAP_Embryo(3-replications); organism part name: 18DAP_Whole Seed(3-replications); organism part name: 18DAP_Endosperm(3-replications); organism part name: 18DAP_Embryo(3-replications); organism part name: 18DAP_Pericarp(3-replications); organism part name: 20DAP_Whole Seed(3-replications); organism part name: 20DAP_Endosperm(3-replications); organism part name: 20DAP_Embryo(3-replications); organism part name: 22DAP_Whole Seed(3-replications); organism part name: 22DAP_Endosperm(3-replications); organism part name: 22DAP_Embryo(3-replications); organism part name: 24DAP_Whole Seed(3-replications); organism part name: 24DAP_Endosperm(3-replications); organism part name: 24DAP_Embryo(3-replications)

Project description:Transcriptional profiling of seeds of Medicago truncatula during maturation. To identify genes that are regulated during seed maturation in the model legume Medicago truncatula, plants at flowering stage were grown at variable light and temperature conditions under greenhouse environment (period March-June). Seeds were then collected at different stages of development. Using the Medicago NimbleGen chip, a transcriptomic analysis was performed to follow the differential expression of genes during seed maturation.

Project description:Transcriptional profiling of seeds of Medicago truncatula during maturation. To identify genes that are regulated during seed maturation in the model legume Medicago truncatula, plants at flowering stage were grown at variable light and temperature conditions under greenhouse environment (period March-June). Seeds were then collected at different stages of development. Using the Medicago NimbleGen chip, a transcriptomic analysis was performed to follow the differential expression of genes during seed maturation.

Project description:To shed light on the genetic events downstream of DELLA proteins, we have employed a microarray expression profiling of Arabidopsis thaliana seeds to identify target genes of the DELLA protein RGL2. Seeds of the germinating ga1-3 rga-t2 rgl2-1 and the non-germinating ga1-3 rga-t2 mutant were stratified, and RNA was extracted after five days. Transcript profiles of the non-germinating seeds closely resemble profiles of dormant seeds, and several transcription factors involved in light- and phytohormone-regulated signalling pathways appear to be up-regulated, suggesting that RGL2 controls various physiological aspects to inhibit seed germination.

Project description:Seed germination triggers a transition of growth and metabolic activities from quiescent to active statuses. Germinating seeds is a good system to study many biological and biochemical processes including hormone metabolic activities and cell wall biosynthesis. Next generation sequence technology is used to study these processes. We have examined gene transcription activities and alternative splicing events in germinating embryos

Project description:MicroRNAs (miRNAs) are important post-transcriptional regulators of plant development. In soybean (Glycine max), an important edible oil crop, valuable lipids are synthesized and stored in the cotyledons during embryogenesis .This storage lipids are used as energy source of the emerging seeds, during the germination procces. Until now, there are no microRNAs related to lipid metabolism in soybean or any other plant. This work aims to describe the miRNAome of germinating seeds of B. napus by identifying plant-conserved and novel miRNAs and comparing miRNA abundance in mature versus germinating seeds. A total of 183 familes were detected through a computational analysis of a large number of reads obtained from deep sequencing from two small RNA libraries of (i) pooled germintaing seeds stages and (ii) mature soybean seeds. We have found 39 new mirna precursors which produce 41 new mature forms. The present work also have identified isomiRNAs and mirnas offset (moRNAs). This work presents a comprehensive study of the miRNA transcriptome of soybean germinating seeds and will provide a basis for future research on more targeted studies of individual miRNAs and their functions in lipid consumption in development soybean seeds. MicroRNA profiles in 2 different seed libraries (mature seeds and a pool of germinating seed stages) of Glycine max by deep sequencing (Illumina GAII).

Project description:We analyzed dual-transcriptome changes in germinating Arabidopsis seeds at three development stages (3, 6 and 10 days after sowing) with or without Alternaria brassicicola. Differentailly expressed genes were identified from both seed and fungus.

Project description:Plant seeds prepare for germination already during seed maturation. We performed a detailed transcriptome analysis of barley grain maturation, desiccation and germination in two tissue fractions (endosperm/aleurone = e/a and embryo = em) using the Affymetrix barley1 chip. Experiment Overall Design: Barley developing and germinating seeds were harvested at different time points after flowering (developing) and imbibition (germinating). To further disseect the influence of different tissues, seeds were dissecte and tissues were analyzed individually.

Project description:During the embryonic-to-vegetative transition in plants, many genes that were active in seeds become transcriptionally turned off. Recently, we reported a new transcriptional corepressor of the embryonic program, SEED DORMANCY 4-LIKE (AtSDR4L). Multiple lines of evidence suggest that AtSDR4L plays an essential role in regulating the transition from seed to seedling, possibly by collaborating with components of Polycomb Repressive Complexes (PRCs) and PRC-associated proteins VIVIPAROUS1/ABI3-LIKE (VAL) proteins. Through yeast-two-hybrid (Y2H) assays and genome-wide binding analysis, we demonstrated that AtSDR4L and DIG1 physically interact with VAL2 but not with VAL1. The interactions depend on the C-terminal halves of AtSDR4L and DIG1, and the N-terminal half of VAL2. AtSDR4L binds to target loci in germinating seeds, preceding reduced accumulation of H3K27me3 Atsdr4l seedlings at a few loci important for seed development. These findings suggest AtSDR4L, and potentially DIG1, facilitate the recruitment of PRC2 through VAL2 to inactivate seed development genes, thus promoting the seed-to-seedling transition.

Project description:Seed germination is a complicated physiological process, during which structures of mitochondria and plastids are recovered, and metabolisms are re-activated (Han and Yang, 2015). It has been shown that metabolism reactivation is very important for rice germination (He et al., 2011b;Han et al., 2014a). It is still unknown if protein acetylation involved in and regulate these metabolisms during rice seed germination. To answer this question, we globally profiled the acetylome in rice embryos from the germinating seeds. A number of acetylated enzymes were identified. The results provide more information about the metabolism regulation in germinating seeds.