Identification of genes expressed in the Arabidopsis female gametophyte

Steffen, Joshua G.; Kang, Il-Ho; Macfarlane, Jane L.; Drews, Gary N.

doi:10.1111/j.1365-313x.2007.03137.x

Cited by 252 publications

(303 citation statements)

References 72 publications

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“…These results indicate that expression of the pBiP1::BiP1 construct complemented the defect in fusion of the polar nuclei, and that this defect arose from the bip1 bip2 double mutation. We produced BiP1 cDNA constructs driven by the promoters of various genes expressed in specific cells of the female gametophyte (15) and used the constructs to transform b1/+ b2/b2 plants. We found that BiP1 expression in the central cell, but not in other female gametophytic cells, suppressed the seed abortion phenotype (Table S3).…”

Section: Resultsmentioning

confidence: 99%

BiP-mediated polar nuclei fusion is essential for the regulation of endosperm nuclei proliferation in Arabidopsis thaliana

Maruyama

Endo

Nishikawa

2010

Proc. Natl. Acad. Sci. U.S.A.

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Nuclear fusion is an essential process in the sexual reproduction of animals and plants. In flowering plants, nuclear fusion occurs three times: once during female gametogenesis, when the two polar nuclei fuse to produce the diploid central cell nucleus, and twice during double fertilization. The yeast Ig binding protein (BiP) is a molecular chaperone Hsp70 in the endoplasmic reticulum that regulates nuclear membrane fusion during mating. Here we report that in Arabidopsis thaliana, BiP is involved in the fusion of polar nuclei during female gametophyte development. BiP-deficient mature female gametophytes contain two unfused polar nuclei, in spite of their close contact. This indicates a surprising conservation of BiP function in nuclear fusion between plants and yeasts. We also found that endosperm nuclear division becomes aberrant after fertilization of the BiP-deficient female gametophytes with wild-type pollen. This is experimental evidence for the importance of fusion of the polar nuclei in the proliferation of endosperm nuclei.endoplasmic reticulum | molecular chaperone | nuclear fusion | fertilization | female gametogenesis N uclear fusion is the process by which two nuclei fuse to produce a single nucleus. This process is essential for the sexual reproduction of various organisms including animals and plants. During the life cycle of angiosperms, nuclear fusion occurs three times: twice during double fertilization, when two sperm cells fertilize the egg and the central cell, and once during the development of female gametophytes (1).The female gametophyte, also referred to as the embryo sac, develops within the ovule. The developmental pattern of female gametophytes in most angiosperm species, including Arabidopsis thaliana, is the Polygonum type: a single megaspore produced by meiosis undergoes three rounds of mitosis to produce an eightnucleate cell. The subsequent migration of nuclei and cellularizations result in a seven-celled female gametophyte consisting of one egg cell, two synergid cells, three antipodal cells, and one central cell containing two polar nuclei (2). In A. thaliana and other species, the polar nuclei fuse before pollination to form the secondary nucleus in the central cell.Mutants affecting the fusion of polar nuclei have been isolated; however, little is known about the molecular mechanisms of this fusion process (3-6). The mating of budding yeast involves one of the best-characterized nuclear fusion processes in eukaryotic cells. In yeast, the Ig binding protein (BiP), which is a molecular chaperone Hsp70 in the endoplasmic reticulum (ER), was shown to play key roles in the nuclear membrane fusion process (7,8). Furthermore, a nuclear membrane protein that possibly functions in this process was identified (9). This prompted us to assess the effects of mutations in BiP on the fusion of polar nuclei during female gametophyte development in A. thaliana.A. thaliana contains three BiP genes (10) (BiP1, BiP2, and BiP3/ BiP-L), two of which (BiP1 and BiP2) encode proteins that are 99% ...

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Section: Resultsmentioning

confidence: 99%

BiP-mediated polar nuclei fusion is essential for the regulation of endosperm nuclei proliferation in Arabidopsis thaliana

Maruyama

Endo

Nishikawa

2010

Proc. Natl. Acad. Sci. U.S.A.

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“…A primary transcriptomic comparison of UP, ovules, and siliques enriched the UP and ovule data sets for stage-specific transcripts by excluding common sporophyte-expressed genes potentially involved in carpel and ovule determination, such as SEEDSTICK (STK; Rounsley et al, 1995) and SHATTERPROOF1 (SHP1; Flanagan et al, 1996), a phosphogluconolactonase (At5g24420) that is expressed in ovule integuments and in the ovary wall (Scutt et al, 2003), as well as genes involved in later stages of seed development, such as MEDEA (MEA; Vielle-Calzada et al, 1999), FERTILIZATION INDE-PENDENT SEED2 (Luo et al, 1999), and FLOWERING WAGENINGEN (Kinoshita et al, 2004). Using the parameters outlined in "Materials and Methods" and further comparison with publicly available data sets (Zimmermann et al, 2004;Tung et al, 2005;Yu et al, 2005;Steffen et al, 2007;Borges et al, 2008;Wang et al, 2008;Qin et al, 2009;Wuest et al, 2010), a total of 42 genes were considered enriched or preferentially expressed in ovules (Supplemental File S1). As anticipated, 27 out of 42 transcripts preferentially expressed in ovules and 96 out of 1,275 ovule-enriched transcripts were previously reported to be expressed specifically in the embryo sac or enriched in female gametophytic cells (Supplemental File S1; Yu et al, 2005;Johnston et al, 2007;Punwani et al, 2007;Steffen et al, 2007;Wuest et al, 2010).…”

Section: Prediction Of Stage-specific and Reproductive Organ-enrichedmentioning

confidence: 99%

“…Using the parameters outlined in "Materials and Methods" and further comparison with publicly available data sets (Zimmermann et al, 2004;Tung et al, 2005;Yu et al, 2005;Steffen et al, 2007;Borges et al, 2008;Wang et al, 2008;Qin et al, 2009;Wuest et al, 2010), a total of 42 genes were considered enriched or preferentially expressed in ovules (Supplemental File S1). As anticipated, 27 out of 42 transcripts preferentially expressed in ovules and 96 out of 1,275 ovule-enriched transcripts were previously reported to be expressed specifically in the embryo sac or enriched in female gametophytic cells (Supplemental File S1; Yu et al, 2005;Johnston et al, 2007;Punwani et al, 2007;Steffen et al, 2007;Wuest et al, 2010). Ovule-expressed transcripts likely include plausible candidates for shortrange pollen tube attractants expressed in the embryo sac (Higashiyama et al, 2001(Higashiyama et al, , 2003Chen et al, 2007;Okuda et al, 2009) but also of other modulators expressed in the surrounding sporophytic tissues that could function as long-range pollen tube attractants.…”

Section: Prediction Of Stage-specific and Reproductive Organ-enrichedmentioning

confidence: 99%

“…The transcriptional profiles of pollen (Becker et al, 2003;Twell, 2003, 2004;Pina et al, 2005; for review, see Becker and Feijó , 2007), embryo sac (Yu et al, 2005;Johnston et al, 2007;Jones-Rhoades et al, 2007;Steffen et al, 2007), pistil (Scutt et al, 2003;Tung et al, 2005), and embryo or seed developmental stages (Chen et al, 2001;Hennig et al, 2004;Yoshida et al, 2005, Le et al, 2010 were recently analyzed. More notably, recent progress in the isolation of Arabidopsis (Arabidopsis thaliana) gametes allowed genomewide expression profiling of purified sperm cells (Borges et al, 2008) as well as of isolated egg and central cells (Wuest et al, 2010).…”

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Whole Genome Analysis of Gene Expression Reveals Coordinated Activation of Signaling and Metabolic Pathways during Pollen-Pistil Interactions in Arabidopsis

et al. 2011

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Plant reproduction depends on the concerted activation of many genes to ensure correct communication between pollen and pistil. Here, we queried the whole transcriptome of Arabidopsis (Arabidopsis thaliana) in order to identify genes with specific reproductive functions. We used the Affymetrix ATH1 whole genome array to profile wild-type unpollinated pistils and unfertilized ovules. By comparing the expression profile of pistils at 0.5, 3.5, and 8.0 h after pollination and applying a number of statistical and bioinformatics criteria, we found 1,373 genes differentially regulated during pollen-pistil interactions. Robust clustering analysis grouped these genes in 16 time-course clusters representing distinct patterns of regulation. Coregulation within each cluster suggests the presence of distinct genetic pathways, which might be under the control of specific transcriptional regulators. A total of 78% of the regulated genes were expressed initially in unpollinated pistil and/or ovules, 15% were initially detected in the pollen data sets as enriched or preferentially expressed, and 7% were induced upon pollination. Among those, we found a particular enrichment for unknown transcripts predicted to encode secreted proteins or representing signaling and cell wall-related proteins, which may function by remodeling the extracellular matrix or as extracellular signaling molecules. A strict regulatory control in various metabolic pathways suggests that fine-tuning of the biochemical and physiological cellular environment is crucial for reproductive success. Our study provides a unique and detailed temporal and spatial gene expression profile of in vivo pollen-pistil interactions, providing a framework to better understand the basis of the molecular mechanisms operating during the reproductive process in higher plants.

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“…To confirm that synergid degeneration was not properly executed upon pollen tube arrival by AP1G loss of function, we expressed NLS-YFP under a synergid-specific promoter Pro DD39 (27). Synergid nuclei were labeled in both unfertilized wild-type and ap1g/+ ovules ( Fig.…”

Section: Resultsmentioning

confidence: 98%

AP1G mediates vacuolar acidification during synergid-controlled pollen tube reception

Wang

Feng

Liu

et al. 2017

Proc. Natl. Acad. Sci. U.S.A.

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Double fertilization in angiosperms requires the delivery of immotile sperm through pollen tubes, which enter embryo sacs to initiate synergid degeneration and to discharge. This fascinating process, called pollen tube reception, involves extensive communications between pollen tubes and synergids, within which few intracellular regulators involved have been revealed. Here, we report that vacuolar acidification in synergids mediated by AP1G and V-ATPases might be critical for pollen tube reception. Functional loss of AP1G or VHA-A, encoding the γ subunit of adaptor protein 1 or the shared component of two endomembrane V-ATPases, respectively, impaired synergid-controlled pollen tube reception and caused partial female sterility. AP1G works in parallel to the plasma membrane-associated receptor FERONIA in synergids, suggesting that synergid-mediated pollen tube reception requires proper sorting of vacuolar cargos by AP1G. Although AP1G did not mediate the targeting of V-ATPases, AP1G loss of function or the expression of AP1G-RNAi compromised vacuolar acidification mediated by V-ATPases, implying their genetic interaction. We propose that vacuolar acidification might represent a distinct cell-death mechanism specifically adopted by the plant phylum, which is critical for synergid degeneration during pollen tube reception. . The female gametophyte (FG), i.e., the embryo sac, is formed inside the ovules and contains an egg cell, a central cell, two synergid cells, and three antipodal cells (3). Upon landing on a receptive pistil, a pollen grain forms a long cylindrical extension, called a pollen tube, which extends inside female sporophytic tissues. To deliver immotile sperm, pollen tubes perceive attractive signals sent out by the FG, change their growth axis, and finally enter the embryo sacs through the micropyle (1-4). A process called "pollen tube reception" instructs the cessation and discharge of the penetrating pollen tube, leading to sperm release and fertilization (1-4).Studies have uncovered key female factors controlling pollen tube reception, including FERONIA (FER) (5-7), LORELEI (LRE) (8, 9), and early nodulin-like proteins (ENODLs) (10) and NORTIA (NTA) (11). These synergid receptors likely operate in the same genetic pathway (10-12) whose functional loss caused the failure of pollen tube discharge and led to reduced female fertility (5-9, 11). Male ligands are yet to be identified. However, recent studies showed that the production of reactive oxygen species (ROS) and Ca 2+ spiking are downstream events of FER-controlled pollen tube reception (13-16).Synergid degeneration, a form of programmed cell death (PCD), is a key step during pollen tube reception. Between the two synergid cells, a receptive synergid cell is the one that succeeds in interacting with the pollen tube and induces it to burst and undergoes cell death first. The other synergid cell that continues to persist and then undergoes cell death orchestrated by the fertilized egg cell and the central cell is the persistent synergid (3,11,1...

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Identification of genes expressed in the Arabidopsis female gametophyte

Cited by 252 publications

References 72 publications

BiP-mediated polar nuclei fusion is essential for the regulation of endosperm nuclei proliferation in Arabidopsis thaliana

BiP-mediated polar nuclei fusion is essential for the regulation of endosperm nuclei proliferation in Arabidopsis thaliana

Whole Genome Analysis of Gene Expression Reveals Coordinated Activation of Signaling and Metabolic Pathways during Pollen-Pistil Interactions in Arabidopsis

AP1G mediates vacuolar acidification during synergid-controlled pollen tube reception

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