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First published online May 1, 2003; 10.1105/tpc.010447 American Society of Plant Biologists The Arabidopsis MALE MEIOCYTE DEATH1 Gene Encodes a PHD-Finger Protein That Is Required for Male Meiosis
a Department of Chemistry and Biochemistry, Miami University, Oxford, Ohio 45056 2 To whom correspondence should be addressed. E-mail hxm16{at}psu.edu; fax 814-863-1357; or e-mail makaroca{at}muohio.edu; fax 814-863-1357
In plants, reproductive development requires normal meiosis, which involved several highly coordinated events. Such meiotic events are regulated in a number of ways in yeast and animal systems, including transcriptional and checkpoint control mechanisms. Although a number of mutations that affect different aspects of meiosis have been characterized in plants, very little is known about the regulation of plant meiosis at the molecular level. In particular, no meiosis-specific transcriptional regulators have been identified in plants, and checkpoint control has not been observed during plant meiosis. We report here the isolation and characterization of a new Arabidopsis male-sterile mutant that exhibits meiotic defects. Meiocytes from mutant plants appeared normal up to diakinesis, when they exhibited signs of apoptosis, including defects in chromosome behavior, cytoplasmic shrinkage, and chromatin fragmentation, followed by cell death before cytokinesis. Therefore, the mutant was named male meiocyte death1 (mmd1). The MMD1 gene was cloned using Dissociation transposon tagging and encodes a plant homeo domain domain–containing protein. MMD1 is expressed preferentially during male meiosis. Our results suggest that MMD1 may be involved in the regulation of gene expression during meiosis and that the mmd1 mutation triggers cell death in male meiocytes.
Meiosis has been characterized extensively in a number of organisms, including plants. It consists of a highly coordinated series of events, all of which are essential for the proper segregation of chromosomes. The establishment of cohesion between sister chromatids, which is essential for the correct attachment of chromosomes to the spindles, occurs during meiotic S-phase. Homologous chromosome pairing and synaptonemal complex formation and recombination occur during zygotene and pachytene, respectively. During diplonema and diakinesis, chromosomes desynapse and condense. The reorganization of chromosomes from long thin fibers into highly condensed, compact structures, which begins during leptonema and is completed during diakinesis, is one of the most striking but least understood events of meiosis. The condensin complex and topoisomerase II participate in chromosome condensation during mitosis and likely are involved in meiosis (Hirano, 2000  ; Cuvier and Hirano, 2003); however, how this process is controlled is unknown at present. Once condensed, the chromosomes align and attach to the meiotic spindle during metaphase, followed by segregation of homologous copies of each chromosome pair at anaphase I. Finally, during meiosis II, the sister chromosomes segregate in an equational division similar to that observed during mitosis.
Considerable progress has been made in understanding meiosis and elucidating factors associated with a number of meiotic events. Many meiotic processes are highly conserved among organisms (reviewed by Ashley and Plug, 1998
However, one aspect of meiosis that may vary significantly between organisms concerns how the cell controls the progression through the meiotic cell cycle. Regulation of the meiotic cell cycle is best understood in yeast (reviewed by Lee and Amon, 2001
In Arabidopsis, maize, and other plants, genetic studies have identified a number of mutants that affect either meiocyte formation or the process of meiosis (Scott et al., 1991
In contrast to meiotic mutants in yeast and animals that cause meiotic cell arrest and/or cell death, most plant meiotic mutants complete meiosis and cytokinesis and produce abnormal microspores. The abnormal microspores produced in these plant meiotic mutants typically degenerate during pollen development, resulting in male sterility or reduced male fertility, suggesting that plants may not use meiotic checkpoint control. However, a number of maize male-sterile mutants have been isolated that show defects in male meiocytes, including ab-normal morphology and cell degeneration before cytokinesis (Albertsen and Phillips, 1981 As part of studies to better understand meiosis and its control in plants, we have characterized male-sterile mutants in Arabidopsis. Here, we describe the isolation and detailed characterization of one mutant, male meiocyte death1 (mmd1), that exhibited alterations in meiosis that resulted in male meiocyte arrest and cell death. We show that MMD1 encodes a plant homeo domain (PHD) domain–containing protein and that it is expressed preferentially in male meiocytes. The mutant phenotype and molecular characteristics of MMD1 suggest that it may participate in chromatin remodeling and/or transcriptional events required for successful progression through meiosis.
Isolation and Characterization of a Male Meiotic Mutant Arabidopsis lines carrying Dissociation (Ds) insertions were generated and screened for mutant plants that exhibit defects in fertility and meiosis. Progeny of one line (Y9287) segregated for fertile and sterile plants with a ratio of  3:1, suggesting that the parental plant was heterozygous for a recessive mutation. Mutant flowers failed to produce pollen but produced apparently normal seeds when cross-pollinated (data not shown), suggesting that the mutation affects male meiosis and/or pollen development but not female reproduction. Although most flowers resembled those of the wild type (Figure 1A), a fraction of flowers (30%) contained four or five stamens (Figure 1B) instead of the normal six stamens. In addition, the filaments of mutant flowers were consistently shorter than those of wild-type plants.
Light microscopic analysis indicated that anther development was normal through stage 8 (as defined by Smyth et al., 1990 ), just before male meiosis. In particular, compared with wild-type anthers (Figure 1C), no alterations were observed in the epidermis, endothecium, middle layer, tapetum, or meiocytes of mutant plants before meiosis (Figure 1D). In anthers of stage-9 flowers, when normal male meiosis occurs to form tetrads (Figure 1E), the four outer layers of the anther again appeared normal in the mutant (Figure 1F). However, arrested and/or degenerating male meiocytes were observed in the locules of mutant plants (Figure 1F). In anthers of stage-10 flowers from wild-type plants, tetrads (Figure 1G) and developing microspores were observed. By contrast, only shrunken and collapsed male meiocytes were observed in stage-10 and later flowers from the mutant (Figure 1H). Tetrads were not observed in the anthers of mutant plants, suggesting that meiocytes fail to undergo cytokinesis. Because no alterations were observed in the remaining four layers of the anther before, during, or after defects were observed in meiocytes, other aspects of anther development seem normal in the mutant. However, we cannot exclude the possibility that subtle alterations in anther development were present and not detected. Because the main defects associated with the mutant were meiotic arrest and cell death in male meiocytes (see below for more details), we named the mutant mmd1 for male meiocyte death1.
To further understand the major effect of the mmd1 mutation, male meiosis in mmd1 plants was analyzed using 4',6-diamidino-2-phenylindole (DAPI) staining of spreads of meiotic chromosomes and was compared with wild-type meiosis (Ross et al., 1996
Regardless of chromosomal morphology, all mmd1 cells observed at diakinesis exhibited signs of cytoplasmic shrinkage (Figures 2AA to 2DD), indicating that they are clearly defective by this stage. This finding is in contrast to the results seen in mmd1 meiocytes before diakinesis, which did not exhibit cytoplasmic shrinkage (Figure 2Z). Some mmd1 meiocytes appeared to arrest and undergo nuclear degradation at diakinesis (Figure 2U), whereas others progressed past diakinesis and exhibited several different alterations. Cells with fewer than five bivalents were observed at metaphase I and early anaphase I (Figures 2J and 2P). Uneven distribution of chromosomes, chromosome bridges, and chromosome fragmentation also was observed (Figures 2V to 2X). These defects in chromosome segregation may result from alterations in the resolution of nonhomologous chromosomes observed at diakinesis. Small numbers of meiocytes also were observed at metaphase II and at anaphase II/telophase II with two or three clusters of degrading chromosomes (Figures 2R and 2S), suggesting that in some cells chromosomes are able to complete meiosis I and progress into meiosis II. Finally, a considerable number of collapsing cells were observed with two to four DAPI-staining areas (data not shown). In these cells, which typically were surrounded by a thin callose wall, vesicles sometimes were observed partitioning the cytoplasm (Figure 2T), in contrast to the typical cell membrane and callose wall that surrounded wild-type cells at the tetrad stage (Figure 2O). No evidence of cytokinesis or the formation of the callose wall associated with cytokinesis was observed in mmd1 meiocytes. Ultimately, all mmd1 meiocytes underwent nuclear degradation and collapse before anthesis. In contrast to most meiotic mutants characterized in plants, microspores were not formed in mmd1 plants.
One of the more notable alterations during meiosis in mmd1 meiocytes was observed from telophase I to telophase II. In wild-type meiocytes, a distinct organelle band formed between the separated chromosomes along what would become the division plane (Figures 2L and 2M). This organelle band was not observed in meiocytes of mmd1 plants (Figures 2Q to 2S), although DAPI-staining material was detected in the cytoplasm. Therefore, it is not clear whether the organelles are degraded in the mutant or just dispersed throughout the cytoplasm. The absence of an organelle band in mmd1 meiocytes may be associated with the failure of meiocytes to form normal cell/callose walls during cytokinesis. It is worth noting that programmed cell death in animal cells often is associated with mitochondrial degeneration (Green and Reed, 1998
Our observation that mmd1 meiocytes exhibited cytoplasmic shrinkage and signs of chromosome degradation at diakinesis raised the possibility that the mutation may evoke a meiotic checkpoint control mechanism, which may arrest meiosis or cause a delay in the progression of meiosis. To investigate this possibility, we examined the distribution of meiocytes at various substages of prophase I in stage-9 flowers and compared these numbers with those observed for wild-type plants. When data from samples containing only or largely prophase I cells were analyzed, we found that in wild-type anthers (six flowers), nearly half of the meiocytes (1374 of 2885) were pachytene cells (Figure 3). Moderate numbers of cells at zygotene (29%) and diakinesis (13%) were observed, with considerably fewer cells at leptotene (7%) and diplotene (2%). A similar distribution of meiotic cells during prophase was reported previously for wild-type Arabidopsis (Azumi et al., 2002
In contrast to the alterations in male fertility observed in mmd1 plants, female fertility appeared to be relatively normal. Nevertheless, we examined female meiosis in wild-type and mmd1 mutant plants. At least 150 female meiocytes ranging from early prophase I to telophase II were examined in mmd1 plants and compared with wild-type meiocytes. Female meiosis appeared completely normal in mmd1 plants (data not shown). Therefore, the mmd1 mutation disrupts male meiosis starting at approximately diakinesis in microsporocytes but does not affect female meiosis.
Male Meiocytes in mmd1 Plants Undergo Chromosome Fragmentation
By contrast, TUNEL labeling of DNA was first detected at approximately mid to late diakinesis in mmd1 male meiocytes (Figure 4J), which is consistent with when we first observed cytoplasmic shrinkage in mmd1 meiocytes. Strong labeling was observed in cells at metaphase I and anaphase I and in cells arrested at diakinesis and the dyad stage (Figures 4K, 4L, 4Q, and 4R). Labeling was observed typically throughout the chromosomes in these cells. Weak labeling also was detected in degenerating meiotic cells from anthers of stage-10 flowers (Figures 4S and 4T). The labeling patterns of these cells typically appeared as foci concentrated around the periphery of the nucleus. The foci also stained positive with DAPI and propidium iodide, confirming that they contained DNA. This finding is reminiscent of the apoptotic bodies—membrane-bound bodies that contain fragmented DNA—that are observed in animal cells undergoing apoptosis (Bursch et al., 1990 ). The TUNEL-positive results, coupled with the cytoplasmic shrinkage and the lack of an organelle band in degenerating mmd1 male meiocytes, are consistent with the hypothesis that they are apoptotic. However, we cannot exclude the possibility that TUNEL labeling is the result of cell death unrelated to a specific apoptosis-related pathway.
The mmd1 Mutation Was Caused by a Ds Insertion
To determine whether Ds-mmd1 caused the meiotic defects observed in mmd1 plants, further linkage analysis was performed. PCR with Ds and plant-specific primers indicated that all 63 sterile plants analyzed were homozygous for the Ds-mmd1 insertion, demonstrating a linkage of <1 centimorgan between the sterility defect and the Ds insertion. Furthermore, revertant analysis was conducted to ascertain if the Ds-mmd1 insertion caused the sterility defect observed in mmd1 plants by searching for fertile flowers and elongated siliques on mutant plants carrying an active Activator (Ac). Of the 58 mmd1 mutant plants examined, 26 produced one or more elongated siliques, whereas mutant plants lacking Ac produced none. Flowers of one large revertant sector produced significant amounts of pollen, demonstrating that the fertility was caused by reversion and not by cross-pollination. The progeny of six independent revertant sectors were planted and segregated for both wild-type and mutant plants. DNA sequence analysis of PCR fragments flanking the Ds insertion site in plants from 10 independent reversion events identified only the wild-type sequence, suggesting that restoration of the wild-type MMD1 sequence might be required for functional reversion. Complementation experiments also were performed. A 4.8-kb wild-type genomic DNA fragment containing MMD1 and 1.5 and 1.0 kb of upstream and downstream DNA, respectively, was introduced into a segregating population of mmd1 plants. Thirty-six transgenic plants were obtained and analyzed for the presence of the complementation clone and Ds-mmd1. PCR using Ds and MMD1 primers showed that of 36 transgenic plants analyzed, 9 were homozygous for Ds-mmd1, 10 were heterozygous, and the remaining 17 were wild type. All of the nine mmd1 homozygous lines were confirmed to contain the complementation clone. Of these nine lines, two lines were completely fertile, three lines were semifertile, and four lines were sterile (data not shown). Therefore, male sterility can be restored by the 4.8-kb fragment containing a wild-type copy of MMD1. At this time, it is not clear why several of the lines showed no or partial restoration of fertility; however, it is possible that the transgene may not be expressed properly in these lines.
MMD1 Encodes a Novel PHD-Containing Nuclear Protein
The predicted protein also contains two potential nuclear localization signals (amino acids 11 to 15 and 432 to 435), suggesting that the protein is targeted to the nucleus. To investigate this possibility, a translational fusion of MMD1 to
The MMD1 Transcript Accumulates Preferentially in Male Meiocytes To obtain additional clues about the mechanism of MMD1 function, we analyzed its expression pattern. MMD1 transcripts were not detectable on RNA gel blots of poly(A+) RNA (1.5 µg) isolated from various Arabidopsis organs, including flower buds (data not shown), indicating that MMD1 is expressed at low levels. Using RT-PCR, MMD1 transcripts were detected only in RNA samples from young buds (24 cycles of PCR; Figure 7). However, 45 cycles of amplification also resulted in the detection of MMD1 transcripts in RNA samples from roots, leaves, and seedlings (data not shown). Therefore, MMD1 transcript levels were highest in floral buds. Amplification was not obtained with bud RNA isolated from mmd1 plants (Figure 7), indicating that the Ds element completely inactivated MMD1 expression.
The temporal and spatial expression patterns of MMD1 in flowers were determined by RNA in situ hybridization experiments. Our results show that MMD1 transcripts were below detection levels in reproductive meristems, early floral primordia, and floral buds before the formation of meiocytes (Figures 8A and 8B). Approximately at the time of male meiosis, MMD1 transcripts clearly were present inside anther locules in areas corresponding to meiocytes but not in other anther tissues or other organs (Figures 8C and 8D) or in postmeiotic anthers (Figure 8E). Binding of both the antisense and sense (negative control) probes to the sepals also was observed. This nonspecific sticking of RNA probes to sepals has been reported previously (Yanofsky et al., 1990 ; Chen et al., 2002). These observations indicate that MMD1 transcripts are highest in male meiocytes at approximately the time of meiosis.
The MMD1 Gene Is Required for Normal Male Meiosis The mmd1 mutant is male sterile but female fertile. The mutation has its greatest effect on meiosis. Male meiosis appeared to proceed normally in mmd1 plants through pachytene. No alterations were observed in >1300 cells observed in leptotene, zygotene, and pachytene. In particular, sister chromosome cohesion and the synapsis of homologous chromosomes appeared normal in meiotic chromosome spreads of mmd1 meiocytes (Figure 2). Consistent with our conclusion that mmd1 meiocytes proceed normally through pachytene was our observation that the distribution of SYN1, the meiotic cohesin protein (Bai et al., 1999 ), was normal on mmd1 meiotic chromosomes up to diakinesis, when chromosomes began to exhibit signs of fragmentation (data not shown). At approximately diakinesis, male meiocytes began to exhibit a general breakdown in meiosis and signs of cell death, including cytoplasmic shrinkage and chromatin fragmentation. Numerous meiotic defects were observed in mmd1 male meiocytes beginning at diakinesis, including alterations in chromosome condensation and difficulties in resolving nonhomologous chromosomes, which resulted in missegregation of chromosomes, chromosome bridges, and fragmentation of chromosomes at anaphase I. In addition, mmd1 meiocytes lacked the distinctive organelle band found in normal meiocytes from telophase I to telophase II. Male meiocytes in mmd1 plants arrested at various stages of meiosis I and II, and none of them underwent cytokinesis. All of our analyses indicate that alterations associated with the mmd1 mutation are first manifest at diakinesis. However, we cannot exclude the possibility that minor alterations in an earlier stage of meiosis may be present in mmd1 meiocytes.
To our knowledge, mmd1 is the only example of a meiotic mutation in Arabidopsis that exhibits apoptosis-like phenotypes before cytokinesis. However, several maize male-sterile mutants have been isolated that show abnormal male meiocyte morphology and cell degeneration. For example, in ms8 mutants, meiotic defects are observed as early as leptotene; a few pollen mother cells complete meiosis, but microspores degenerate soon afterward (Albertsen and Phillips, 1981 In contrast to the meiotic defects observed during male meiosis, no alterations were detected during female meiosis, and female fertility appeared normal in mmd1 plants. In addition, no alterations were observed in the epidermis, endothecium, or middle layer of the anther. These observations, along with the fact that MMD1 transcripts were detected mainly in male meiocytes, suggest that MMD1 is essential only for male meiosis. However, very low levels of MMD1 transcript were detected in other tissues, raising the possibility that it may play an additional minor role outside of male meiosis. Consistent with this possibility is our observation that 30% of mmd1 flowers contained abnormal numbers of stamens and that filaments in mmd1 flowers were somewhat shorter than those in wild-type flowers. This finding suggests that mmd1 also could play a minor role in flower development.
Does the Absence of MMD1 Trigger Meiotic Cell Cycle Control and Associated Apoptosis?
It is possible that the mmd1 mutation may trigger a checkpoint control mechanism other than the classic meiotic checkpoint. For example, mutations in mice that cause telomere dysfunction trigger a germ cell surveillance system that results in developmentally regulated germ cell apoptosis (Hemann et al., 2001
What Is the Role of MMD1?
Recently, PHD domains were found to be associated with E3 ubiquitin ligase activity. Several PHD-containing viral proteins that are targeted to cellular membranes and the cytosol have been shown to function as E3 ubiquitin ligases (Cosoy and Ganem, 2003
To date, PHD domain–containing proteins have not been linked with chromatin-remodeling events associated with chromosome condensation during either mitosis or meiosis. However, it should be noted that although it is clear that topoisomerase II and the condensin complex are required for chromosome condensation (Hirano, 2000
As discussed above, Arabidopsis contains four MMD1-related genes, including MS1, which is required for microspore development (Wilson et al., 2001
Generation of Dissociation Insertional Lines, Isolation of the mmd1 Mutant, and Reversion Analysis Plants used in this study were of the Arabidopsis thaliana ecotype Landsberg erecta. They were grown in the greenhouse or growth chambers with a 16-h-light/8-h-dark cycle at 22 to 24°C. Seeds were plated onto Murashige and Skoog (1962) agar medium with or without appropriate antibiotics under continuous light at 22°C.
Arabidopsis Dissociation insertional lines were generated according to Sundaresan et al. (1995)
Putative revertant sectors were identified as fertile siliques on otherwise sterile F2 plants carrying both the mmd1 mutation and a recombinant Ac element, Ac1 (Sundaresan et al., 1995 PCR was conducted on DNA isolated from 63 sterile plants segregating from a cross between mmd1 and wild-type Columbia plants to test linkage between the Ds and male sterility. Two gene-specific primers flanking the Ds insertion site, oMC462 and oMC465, and a Ds-specific primer, oMC432, were used in separate PCR procedures to determine if the plants contained the mutant mmd1 or the wild-type MMD1 allele.
Phenotypic Characterization of Meiocytes
Isolation and Characterization of MMD1 Genomic and cDNA Clones The MMD1 cDNA was amplified in successive rounds of PCR using the primer pairs oMC465/oMC473 and oMC465/oMC472 on first-strand cDNA generated by reverse transcription with an oligo(dT) adaptor primer (oCM162) on poly(A+) RNAs isolated from wild-type buds (Figure 5A). The 3' end of the mmd1 cDNA was amplified using primer oMC468 and the adaptor primer (oCM176). Amplification products were cloned and sequenced. The Arabidopsis BAC clone F15E21 was obtained from the Arabidopsis Stock Center (Columbus, OH). Primers used in this study are described in Table 1.
The Ds insertion site was analyzed by DNA gel blot hybridization with  -32P-dCTP–labeled probes for either the Ds element (1.8-kb EcoRI fragment) or the MMD1 genomic locus (2.4-kb PCR-derived genomic clone). Hybridized membranes were exposed to x-ray film.
A 4.8-kb wild-type genomic DNA fragment containing MMD1 and 1.5 and 1.0 kb of upstream and downstream DNAs, respectively, was cloned into the plant transformation vector pCAMBIA1390 (Hajdukiewicz et al., 1994
Expression Studies and Protein Localization
In situ RNA hybridization experiments were performed as described previously (Drews et al., 1991
Nuclear localization of the MMD1 protein was tested by transient expression of the MMD1– Upon request, all novel materials described in this article will be made available in a timely manner for noncommercial research purposes.
Accession Number
We thank Y. Hu for generating F2 families for the screening of Ds insertional lines and for performing the RNA in situ hybridization experiment, A. Richardson for help with mutant screening, A. Omeis for plant care, W. Li for assistance in phenotypic analysis, and B. Bliss, W. Li, and D. Zhao for comments and critical reading of the manuscript. The Miami University Electron Microscope Facility provided resources for this work. This work was supported by grants from the National Science Foundation (MCB-9896340) and the National Institutes of Health (R01 GM63871-01) to H.M., by funds from the Department of Biology and the Huck Institute of Life Sciences at Pennsylvania State University, and by Grant R15 GM55956-02 from the National Institutes of Health to C.A.M.
Article, publication date, and citation information can be found at www.plantcell.org/cgi/doi/10.1105/tpc.010447.
1 Current address: Department of Chemistry and Biochemistry, Miami University, Oxford, OH 45056. Received January 9, 2003; accepted March 27, 2003.
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Abstract
INTRODUCTION
-gluc-uronidase (GUS) was generated for transient expression in plant cells driven by the 35S promoter. Introduction of the MMD1-GUS fusion into onion epidermal cells by particle bombardment resulted in GUS staining in the nucleus (
