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First published online January 11, 2006; 10.1104/pp.105.074294 Plant Physiology 140:512-527 (2006) © 2006 American Society of Plant Biologists The Fertilization-Induced DNA Replication Factor MCM6 of Maize Shuttles between Cytoplasm and Nucleus, and Is Essential for Plant Growth and Development1 Developmental Biology and Biotechnology, Biocenter Klein Flottbek, University of Hamburg, 22609 Hamburg, Germany (T.D., K.S., P.G.); and Department of Molecular Biology, Faculty of Science, University of Zagreb, 10000 Zagreb, Croatia (D.L.-L.)
The eukaryotic genome is duplicated exactly once per cell division cycle. A strategy that limits every replication origin to a single initiation event is tightly regulated by a multiprotein complex, which involves at least 20 protein factors. A key player in this regulation is the evolutionary conserved hexameric MCM2-7 complex. From maize (Zea mays) zygotes, we have cloned MCM6 and characterized this essential gene in more detail. Shortly after fertilization, expression of ZmMCM6 is strongly induced. During progression of zygote and proembryo development, ZmMCM6 transcript amounts decrease and are low in vegetative tissues, where expression is restricted to tissues containing proliferating cells. The highest protein amounts are detectable about 6 to 20 d after fertilization in developing kernels. Subcellular localization studies revealed that MCM6 protein shuttles between cytoplasm and nucleoplasm in a cell cycle-dependent manner. ZmMCM6 is taken up by the nucleus during G1 phase and the highest protein levels were observed during late G1/S phase. ZmMCM6 is excluded from the nucleus during late S, G2, and mitosis. Transgenic maize was generated to overexpress and down-regulate ZmMCM6. Plants displaying minor antisense transcript amounts were reduced in size and did not develop cobs to maturity. Down-regulation of ZmMCM6 gene activity seems also to affect pollen development because antisense transgenes could not be propagated via pollen to wild-type plants. In summary, the transgenic data indicate that MCM6 is essential for both vegetative as well as reproductive growth and development in plants.
DNA replication of the eukaryotic genome in S phase is accomplished only once during each cell division cycle. This process is precisely regulated and controlled by the prereplicative complex (pre-RC) consisting of origin recognition complex (ORC), Cdt1, Cdc6, as well as minichromosome maintenance (MCM) proteins (Tye, 1999  ; Bogan et al., 2000; Hyrien et al., 2003; Arias and Walter, 2005; Blow and Dutta, 2005). The initiation of DNA synthesis is thus regulated as a multistep process involving the binding of ORC to replication origins followed by a stepwise recruitment of Cdc6, Cdt1, and MCM proteins to form the pre-RC. Finally, the pre-RC becomes activated by Cdc7/Dbf4 (DDK) and Cdc28 (Cdk2)/cyclin E protein kinases, leading to Cdc45 binding to the pre-RC to initiate DNA unwinding and DNA synthesis (Labib and Diffley, 2001; Lei and Tye, 2001; Hyrien et al., 2003). After the initiation of DNA replication in yeast (Saccharomyces cerevisiae) and animal cells, MCM proteins are displaced from chromatin and its reassociation is inhibited until cells pass through mitosis (Blow and Dutta, 2005).
Thus, the dynamic changes in the assembly and disassembly of the MCM subcomplex is critical for the regulation of DNA replication. Originally identified as proteins required for MCM in yeast, the evolutionary conserved MCM proteins are now regarded as being essential for both initiation and elongation of DNA replication in eukaryotes and archaebacteria (for review, see Tye, 1999
Compared to yeast, animals, and humans, surprisingly little is known about MCM proteins in plants. PROLIFERA (PRL) was the first MCM protein identified in plants and was shown to be required during reproduction for megagametophyte and embryo development, but is also expressed in dividing sporophytic tissues (Springer et al., 1995
Here we report the molecular cloning and functional characterization of MCM6 from maize (ZmMCM6). During our investigations about the onset of zygotic gene activation (ZGA)/embryonic gene activation (EGA), we identified a number of genes that are up-regulated or expressed de novo shortly after fertilization in the maize and wheat (Triticum aestivum) zygotes (Dresselhaus et al., 1999
Structural Properties of ZmMCM6 and Other Plant MCM Proteins We have compared all MCM proteins of Arabidopsis and the known maize MCM proteins with MCM proteins of budding yeast and African clawed frog. Yeast and frog have been selected because all MCM2 to 7 genes from these two species are known and functions of MCM proteins have been most intensely studied in these species, using genetic approaches in the case of budding yeast and biochemistry in the case of frog. As shown in Figure 1, all MCM2 to 7 proteins are encoded by single-copy genes with the exception of a duplicated MCM6 gene of frog. The expanding tree indicates that MCM proteins of fungi, animals, and plants all evolved from one ancestor molecule. Plant MCMs display a higher homology among each other compared with corresponding MCMs of other organisms. Interestingly, the Arabidopsis genome encodes two non-MCM2 to 7 proteins (MCM8 and MCM9), which show homology to MCM8 of frog and human MCM9, respectively. MCM9 of frog is not known to date.
MCM classes consist of large proteins of 716 to 1,017 amino acid residues (molecular mass between 80 and 113 kD) with the exception of Arabidopsis and human MCM9s, which are 610 and 391 amino acids in length, respectively. Table I shows a summary of characteristic features of MCM proteins. Nuclear localization sequences (NLS) have been predicted by PSORT in MCM2 and MCM3 proteins, but not in maize MCM6 and most other MCMs. We have identified potential zinc-finger motifs that might be involved in protein-protein interactions in the N-terminal regions of all MCM proteins with the exception of the MCM3 class and MCM5 from yeast. The zinc-finger motif CX2CX18-19CX4C was found in all MCM6, MCM7, and MCM8 sequences. MCM4 proteins contain either this or the CX2CX18-19CX2C motif that was also found in the MCM2 protein sequences. Deviations from these classical motifs were found as CX2CX20-24CX5-10C in the MCM5 and MCM9 classes. In addition, cyclin/cyclin-dependent kinase (CDK) phosphorylation sites (S/T)Px(K/R), which might function as cell cycle regulation motifs, were identified in some MCM proteins. Interestingly, two of the hexameric MCM2 to 7 proteins of each organism investigated in our studies contain this CDK box. For yeast, these are MCM3 and MCM4, in African clawed frog, these are MCM2 and MCM4, whereas in Arabidopsis and maize, these are MCM3 and MCM6.
We have analyzed the structural properties of MCM6 proteins in more detail. With the exception of MCM6 from rat, Figure 2 shows the alignment of all MCM6 protein sequences available in public databases. The largest and most conserved stretch of about 153 amino acids in the central region includes elements of the Walker-type nucleoside triphosphate-binding domain (Walker et al., 1982 ), which is conserved in a number of ATPases. The putative ATP-binding site of MCM6 proteins is shown by a P-loop that includes the Walker A motif (GDPS[C/T][A/S]KS) and the Walker B motif. The B motif is part of a highly conserved domain that begins with the acidic amino acid Glu preceding a stretch of hydrophobic residues predicted to form a  -strand and an acidic stretch. Finally, the conserved central domain also contains the R- or SRF (Ser-Arg-Phe)-finger. The Arg residue within the R-finger probably represents the catalytic activity (Davey et al., 2003).
In addition to an N-terminal zinc-finger motif and central catalytic domain, a cyclin/CDK phosphorylation site (S/T)Px(K/R) was found only in the N-terminal region of plant MCM6 proteins at position 107 to 110 (SPnK) in ZmMCM6 and 102 to 105 (TPnK) in AtMCM6, respectively. Finally, a conserved motif of unknown function was found at the very C terminus of most MCM6 proteins (Fig. 2, boxed region). This region of 14 to 16 amino acids consists of an aliphatic/polar core that is flanked on both sides by acidic amino acids. Although the function of this motif is unknown, it is characteristic for all MCM6 proteins expressed postfertilization in higher eukaryotes, is absent in maternal MCM6 of frog, and is different in fungi.
We have analyzed the expression, subcellular localization, and function of the fertilization-induced MCM6 gene of maize in more detail. Low gene expression levels were detected by single-cell (SC) reverse transcription (RT)-PCR in the unfertilized egg cell (Fig. 3A). Twelve hours after in vitro pollination (IVP; this stage corresponds to about 6 h after fertilization; E. Kranz, personal communication), high transcript amounts have been detected in the zygote. Later, during zygote development (21 h after IVP), ZmMCM6 transcript levels decrease and remain low 27 to 48 h after IVP. A significant oscillation of gene expression in a cell cycle-dependent manner was not observed. For comparison, another gene, ZmFEN-1a, which was also identified in our screen for fertilization-induced genes and which encodes a flap endonuclease required for DNA repair, was used to study cell cycle-dependent gene expression during zygote and proembryo development. ZmFEN-1a is a homolog of RAD27 from yeast showing up-regulation of gene expression during late G1 phase (Vallen and Cross, 1995
Compared to zygotes shortly after fertilization, expression of ZmMCM6 in vegetative and complex reproductive tissues is very low. To display significant ZmMCM6 transcript signals from a northern blot containing total RNA, hybridization with a radiolabeled probe and exposure of up to 14 d using intensifier screens was necessary (Fig. 4A). A single band slightly smaller than 3.0 kb was detected, indicating that the cloned 2,785 nucleotides of ZmMCM6 represent the full-length transcript. The strongest signals were obtained from tissues containing proliferating cells such as root tips, nodes, leaf meristem, and developing tassels, but also embryonic and nonembryogenic suspension cultures. In developing tassels, signal intensity correlates with developmental stages, while signals were absent in tassels at maturity. Moreover, signals were detected in whole-seedling tissue 4 d after germination, but were absent in leaf tissues of older seedlings (10 d after germination). Leaf meristem displayed relatively strong signals, whereas signals were absent in mature leaves. A ZmMCM6-specific peptide antibody against the less conserved C-terminal part of the protein (see also Fig. 2) was used to detect MCM6 in different tissues and developmental stages (Fig. 4B). A single band of about 90 kD was detected in protein blots, which corresponds to the expected size of 92.5 kD. Minor protein amounts could be detected in nodes, immature cobs, and ovaries, whereas significant ZmMCM6 amounts could not be detected in young and mature leaves and whole roots during tassel maturation as well as in mature pollen. The highest protein amounts are present in developing kernels. While ZmMCM6 protein amounts are relatively low in kernels prior to fertilization (0 days after pollination [DAP]), a strong increase was observed 6 DAP and highest protein levels were detected 10 to 20 DAP.
ZmMCM6 Shuttles between Cytoplasm and Nucleoplasm in a Cell Cycle-Dependent Manner
We have used a chimeric ZmMCM6 protein fused to GFP and immunocytochemistry to study the subcellular localization of ZmMCM6. First, onion epidermal cells were bombarded with a construct encoding a ZmMCM6-GFP fusion protein under the control of the strong and constitutively expressing ubiquitin (UBI) promoter of maize. As shown in Figure 5, A and B, relatively strong GFP signals accumulated in cytoplasm around the nucleus and in transvacuolar strands of the cytoplasm surrounding the nucleus. Protein localization in the nucleus was not detectable. Focusing through side views of nuclei displayed more clearly that the fusion protein accumulated in cytoplasm surrounding the nucleus, but was excluded from the nucleoplasm (Fig. 5, C and D). In contrast, the N-terminal 388 amino acids of a maize transcriptional regulator of anthocyanin biosynthesis (Ludwig et al., 1989
Immunocytochemistry with isolated BMS nuclei was performed to measure the cell cycle dependency of nuclear ZmMCM6 localization more precisely and to prove that the difference of DAPI signal intensity is not originating from problems of dye uptake. DNA and ZmMCM6 content of isolated BMS nuclei were measured after DAPI staining and by using a fluorescein isthiocyanate (FITC)-coupled secondary antibody against the ZmMCM6-specific peptide antibody described above. FITC signals of nuclei showing endoreduplication have not been measured. As shown in Figure 7, A and B, all nuclei displaying strong FITC signals were in G1 or early S phase of the cell cycle. Nuclei in late S or G2 (Fig. 7, C and D) never showed significant signals. Those signals were in the range of background signals that were also obtained after using preimmune serum instead of the serum containing the specific antibody (Fig. 7, E and F). Figure 7G shows a summary of measurements obtained from 44 nuclei. A relative DNA content of 2C (±15%) was considered as G1, a DNA content of 2C (+16% to 25%) as G1/S, and a DNA content of 4C (±15%) as G2. To determine FITC background fluorescence, DNA and FITC signal intensities of 16 randomly chosen nuclei were measured after incubation with preimmune serum (Fig. 7H). In contrast to the control, more than 50% of nuclei in G1 showed significant ZmMCM6 amounts. All nuclei in late G1/early S phase contain high ZmMCM6 levels, which decrease during S phase progression and are no longer measurable at later stages of S phase or in G2. In summary, immunocytochemistry data confirm the above finding that ZmMCM6 is taken up by the nucleus during G1 phase and protein levels are highest during late G1/S phase, while ZmMCM6 is excluded from the nucleus during late S, G2, and mitosis. Attempts to measure ZmMCM6 levels of nuclei from isolated cells of the female gametophyte were not successful, probably because only nuclei of zygotes at defined stages contain sufficient detectable protein amounts and the number of zygote nuclei was not sufficient. A very high number of nuclei, similar to the approach with the BMS suspension cells, will be necessary to determine relative ZmMCM6 protein amounts in female gametophyte nuclei.
Phenotypes of Transgenic Maize after ZmMCM6 Up- and Down-Regulation A transgenic approach was chosen to increase and to down-regulate ZmMCM6 gene expression in maize. One hundred-fifty immature hybrid embryos have been bombarded with a sense construct (UBIp:ZmMCM6) to increase ZmMCM6 transcript amounts by expressing the full-length ZmMCM6 cDNA under the control of the strong and constitutively expressing maize UBI promoter. Four plants have been regenerated (transformation efficiency of 2.7%), all representing one clonal line as they displayed the identical transgene integration pattern (plants SE1a–SE1d). The Southern blot in Figure 8A shows that this line contains multiple transgene integrations, including one or more full-length integrations. However, quantification of ZmMCM6 transcript amounts showed that there was no significant difference between the four transgenic lines compared to wild-type plants (Table II). An obvious phenotype was not observed and plants were both fully male and female fertile. We have therefore bombarded another 400 immature hybrid embryos with a sense construct carrying a GFP conjugate (UBIp:ZmMCM6-GFP) both to increase ZmMCM6 transcript amounts and to simultaneously study ZmMCM6 protein localization. Five independent transgenic lines (G1–G5) have been generated (transformation efficiency of 1.2%) containing one to two transgene integrations. Unfortunately, none of these lines contained a full-length and thus functional integration of the construct (Fig. 8A). GFP expression was therefore not detectable in any of the tissues investigated. The observation that these plants were small (Table II) was probably an effect of longer regeneration periods and growth in winter. Reproductive organs were fully developed and seed set was obtained after selfing.
In addition, we have generated transgenic maize with the aim of decreasing ZmMCM6 transcript levels. Three hundred-eighty immature embryos of the inbred line A188 have been bombarded with an antisense (AS) construct (UBIp:ZmMCM6-AS). Sixteen plants containing ZmMCM6 AS integrations were regenerated (transformation efficiency of 4.2%) representing 10 independent lines (Table II, plants AS1–AS10b). The transgene integration pattern of five plants is shown in Figure 8A. The genomic Southern blot shows multiple transgene integrations for each plant. AS4a to AS4c displayed the same pattern, indicating that they represent a clonal line. The other two plants (AS3 and AS5) show a different integration pattern. Full-length integrations could be observed in these two lines as well as in line AS6, while none of the lines AS1, AS2, and AS7 to AS10b, respectively, contained full-copy transgene integrations (Table II). Surprisingly, expression of the AS transcript could not be detected in a single line in northern blots (data not shown). The more sensitive RT-PCR method was therefore applied and showed weak AS expression after 38 PCR cycles in lines AS5 and AS6, respectively (Table II). Quantification of both sense and AS transcript amounts in transgenic AS plants by quantitative real-time RT-PCR were in the range of wild-type background sense signals, indicating that the AS transcript amounts were extremely low and not increased above wild-type sense transcript amounts. Nevertheless, those plants that showed a very weak expression of the AS transgene (AS5 and AS6) and/or contained functional copies of the transgene (AS3 and AS4a–c) were strongly reduced in size (Fig. 8B) and did either develop only immature cobs (lines AS3, AS4b, AS4c, AS5, and AS6) or no cob at all (plant AS4a). As shown in Table II, these plants were additionally male sterile due to the lack of anthers or whole male florets (AS4c and AS5). Three plants produced little pollen (AS4a, AS4b, and AS6). Pollen of the plants AS4a and AS4b was used to pollinate wild-type plants. Forty-two progeny plants (plants AS4a/1–20 and AS4b/1–22) were used to study transgene transmission and expression. Surprisingly, none of these plants contained a transgene (Table II). These findings suggest that even mild ZmMCM6 down-regulation affects both male and female gametophyte development and thus transgene transmission.
Structure and Domains of Plant MCM Proteins
Similar to fungi and animals, plants seem to possess a single gene for each subunit of the MCM hexamer complex. In addition to the classical MCM2 to 7 genes, Arabidopsis contains two additional MCM genes (AtMCM8 and AtMCM9). Homologs of these genes are not present in the yeast genome (Forsburg, 2004
All MCM proteins are likely to have evolved from a single gene, as the archeon Methanobacterium thermoautotrophicum contains a single MCM gene that is able to form a homohexamer complex and that possesses both a DNA-dependent ATPase and a 3' to 5' helicase activity to unwind 500 bp of DNA (Kelman et al., 1999
The other domains of MCM proteins are less conserved. Although the known MCM functions are within the nucleus, only a few MCM proteins were predicted to contain NLS. Experimentally, nuclear import of MCM monomers has been functionally demonstrated only for MCM2 of fission yeast (Schizosaccharomyces pombe), budding yeast, and mice, as well as for MCM3 of yeast and humans (for review, see Forsburg, 2004
Little is known about the expression and subcellular protein localization of plant MCM genes. Abundance in the expression of ZmMCM3, ZmMCM7, and AtMCM7 genes has been correlated with cell proliferation throughout vegetative plant development (Sabelli et al., 1996
Compared with frog, where distinct maternal and zygotic genes encode MCM6 (Sible et al., 1998
In yeast, it was shown that MCM proteins shuttle in and out of the nucleus during a single cell cycle. In contrast, MCM proteins in metazoans remain in the nucleus throughout the cell cycle (Blow and Dutta, 2005
ZmMCM6-GFP was evenly distributed in the nucleoplasm and we never found accumulation at certain spots that might represent pre-RC sites. It is thus likely that ZmMCM6 not only binds pre-RC sites, but is also capable of binding chromatin from all parts of the genome, excluding genomic regions containing rDNA genes, as we never observed ZmMCM6 protein in the nucleolus. Perhaps MCM6 is replaced in this chromosomal region by another MCM protein, for example, MCM8 or MCM9. Binding of human and frog MCM proteins to genomic DNA outside of ORCs, and not specifically to many sites of the chromatin, has been reported recently (Edwards et al., 2002
In fungi and animals, loss of MCM function causes severe effects, including DNA damage and genome instability. In Caenorhabditis elegans, for example, reduction of MCM5 and MCM6 function using RNAi resulted in failure of nuclear reassembly following mitosis (Gönczy et al., 2000
We have chosen an AS approach to decrease, but not to eliminate, ZmMCM6 transcript levels. Under control of the strong maize UBI promoter, transgenic maize lines usually display a broad level of transgene expression, sometimes exceeding endogenous transcript levels up to 20 times (Dresselhaus et al., 2005
A correlation of cell cycle control and plant growth as well as morphogenesis has already been reported for a number of plant cell cycle regulators including CDKs and cyclins (for review, see Hemerly et al., 1999
Plant Material, Isolation of Cells from the Female Gametophyte, and In Vitro Cultures
Maize (Zea mays) inbred lines A188 (Green and Phillips, 1975
A cDNA library of maize in vitro zygotes (Dresselhaus et al., 1996
Sequence data were compiled and compared online with EMBL, GenBank, DDBJ, Swiss-Prot, Protein Information Resource, and Protein Research Foundation databases with FASTA and BLAST algorithms (Pearson, 1990
Extraction of genomic DNA from plant tissues was performed according to Dellaporta et al. (1983)
Capillary Southern and northern blots, as well as labeling, hybridization, washing, and autoradiographic exposures, were performed as described in Dresselhaus et al. (2005)
SC RT-PCR analysis was performed as described by Cordts et al. (2001)
Plant tissue was ground in liquid nitrogen. One volume of extraction buffer (250 mM KCl, 20 mM Tris-HCl, pH 6.8, 50% v/v glycerol, 2.5% w/v polyvinylpyrrolidone, 5 mM dithiothreitol, and one mini protease inhibitor tablet [Roche] in 10 mL extraction buffer) was added and mixed until material thawed. Samples were centrifuged at 13,000 rpm for 30 min at 4°C. This step was repeated twice with the supernatant. Protein concentrations were measured after adding 100 µL Bradford reagent (Bradford, 1976
SDS-PAGE in a discontinuous Tris-Gly buffer system was performed according to Sambrook et al. (1989)
For immunodetection, a rabbit peptide antibody (anti-MCM6-Ab) was generated by BioTrend against a ZmMCM6 C-terminal-specific region (VPSESDAGQPAEEDA) between position 680 and 694 (Fig. 2) and tested for specificity by ELISA. Protein blots were blocked overnight in 5% phosphate-buffered saline (PBS)-Blotto at 4°C or for 1 h at room temperature. Blots were incubated with a 1:500 dilution of anti-MCM6-Ab in 5% PBS-Blotto for 2 h at room temperature, rinsed twice with PBS for 5 min each, followed by a 1-h treatment at room temperature with a 1:5,000 dilution of the secondary antibody, a mouse monoclonal anti-rabbit IgG ( Immunocytochemistry to determine ZmMCM6 levels during the cell cycle were performed as follows. Each 2-mL BMS cell was collected by centrifugation at 1,000 rpm for 4 min. Supernatants were removed and cell pellets immediately fixed in 1 mL 4% paraformaldehyde and 0.25% glutaraldehyde in PBS, and incubated for 1 h at room temperature. Fixed cells were centrifuged at 1,000 rpm, supernatant discarded, and pellets rinsed four times with PBS (containing 1% Triton) and each time centrifuged for 10 min at 1,000 rpm to collect cells. Cell walls were degraded for 30 min at room temperature after adding 500 µL of enzyme mixture, which contained 1.5% pectinase, 0.5% pectolyase, 1.0% hemicellulase, and 1.0% cellulase in mannitol solution (570 milliosmolar; pH 4.9–5.0). Digested cells were resuspended with a pipette, nuclei collected after centrifugation at 1,000 rpm, and supernatants removed. Nuclei were washed four times in 1 mL PBS containing 0.1% Triton for 10 min during centrifugation at 1,000 rpm at 4°C. The pellets were resuspended in 500 µL PBS containing the 1:250 diluted anti-MCM6-Ab and incubated at 4°C overnight. Nuclei were washed three times in 1 mL PBS and centrifuged at 1,000 rpm for 10 min. After a final wash, pellets containing nuclei were resuspended in 500 µL PBS containing an FITC-coupled anti-rabbit antibody (1:500) and incubated for 4 h at 4°C. Nuclei were collected after centrifugation at 1,000 rpm for 10 min and washed five times each in 1 mL PBS as described above. Finally, nuclei were resuspended in 500 µL PBS and centrifuged at 500 rpm for 1 min. Twenty-microliter fractions containing nuclei were collected from the bottom of the tubes and transferred to microscopic slides after adding 0.25 µL DAPI solution.
To generate an AS construct (UBIp:MCM6-AS) of ZmMCM6, the full-length cDNA of ZmMCM6 was excised from pK19U2 (see above) using the enzymes SstI and BamHI and cloned into the corresponding restriction sites of the vector pUbi.Cas (Christensen and Quail, 1996
Epidermal onion cell layers were bombarded with 2 to 5 µg plasmid DNA, according to the procedure described by Scott et al. (1999)
Embryos of the maize inbred line A188 were used 12 to 14 DAP for stable transformation using the construct UBIp:MCM6-AS. Hybrid embryos from both lines A188 and H99 were used for stable transformation experiments with the constructs UBIp:MCM6 and UBIp:MCM6-GFP. Constructs were cotransformed with the plasmid construct 35Sp:PAT carrying the selectable marker PAT for glufosinate ammonium resistance. Particle bombardment, tissue culture, and selection of transgenic maize plants were performed according to Brettschneider et al. (1997)
Axiovert 35 M or Axiovert 200 fluorescence microscopes (Zeiss) with the filter set 01 (FITC filter with excitation at 450–490 nm; emission at >515 nm) or filter set 38 (GFP filter with excitation at 470–495 nm; emission at 525 nm) were used to observe GFP fluorescence in onion epidermal and maize BMS cells, as well as FITC fluorescence of isolated BMS nuclei after immunostaining. A DAPI filter (Zeiss, excitation at 359–371 nm and emission >397 nm) was used to visualize DNA and cell wall material. Samples were excited with UV light produced by a HBO 50/Ac lamp and images taken with a Nikon DS-5Mc camera. Nikon software EclipseNet plug in MCF was used to obtain and merge fluorescence images. ImageJ software was used to measure DAPI, GFP, and FITC fluorescence. CLSM was performed using the Leica TCS 4D CLSM (Leica-Laser-Technologie). Samples were excited by 488 nm with an Argon laser as described in Knebel et al. (1990). Sequence data from this article can be found in the GenBank/EMBL data libraries under accession numbers AY862320 (ZmMCM6 cDNA), AAW55593 (ZmMCM6 protein), and DQ138311 (ZmFEN-1a cDNA).
We are grateful to Stefanie Sprunck for critical comments on the manuscript and to Gislind Bräcker for excellent technical support. We thank Natascha Techen for the 35Sp:Lc-GFP construct and Hartmut Quader for help with the CLSM studies. Received November 17, 2005; returned for revision December 8, 2005; accepted December 11, 2005.
1 This work was supported by the Deutsche Forschungsgemeinschaft (grant Dr334/2 to T.D.), the Südwestdeutsche Saatzucht, Rastatt, Germany (to D.N.S.), a Roman Herzog research fellowship (to D.L.-L.), and a postgraduate Hamburg (HmbNFG) fellowship (to K.S.). 
2 Present address: Department of Biology, National University of Ireland, Maynooth, County Kildare, Ireland. The author responsible for distribution of materials integral to the findings presented in this article in accordance with the policy described in the Instructions for Authors (www.plantphysiol.org) is: Thomas Dresselhaus (dresselh{at}botanik.uni-hamburg.de). Article, publication date, and citation information can be found at www.plantphysiol.org/cgi/doi/10.1104/pp.105.074294. * Corresponding author; e-mail dresselh{at}botanik.uni-hamburg.de; fax 49–40–42816–229.
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ABSTRACT
RESULTS
-vector UniZAP II, and packed using the Gigapack-Gold II extract (Stratagene) to generate a cDNA library from zygotes containing full-length cDNAs. The 5' region (2 kb) of ZmMCM6 was amplified from this library using the T3 vector primer and the gene-specific primer 19A (5'-CATGATGTAGACCAGATCAA-3') in a standard PCR reaction with Taq DNA polymerase. PCR products were blunted, purified, and cloned into the pPCR-Script vector (Stratagene), according to the manufacturer's specifications. The full-length cDNA of ZmMCM6 was amplified from 1 µg poly(A)+ RNA extracted from root tips. Twenty nanograms of the primer 19U2 (5'-GTCAGACTACAGATGCTAATT-3') derived from the 3' end of the ZmMCM6 transcript was incubated with poly(A)+ RNA and SuperScript reverse transcriptase according to the protocol of the 5'-RACE system (Life Technologies). PCR was performed with proofreading pfu DNA polymerase (Stratagene) as well as primers 19U2 and GB19A (5'-TGCCAATCTCCAACTCATACCC-3'), the latter derived from the 5' region of the ZmMCM6 transcript. The PCR product was cloned into the pPCR-script vector (see above) generating the plasmid pK19U2 and fully sequenced. The full-length ZmMCM6 nucleotide sequence data reported in this article is available in the EMBL, GenBank, and DNA Data Bank of Japan (DDJB) nucleotide sequence databases under accession number 
-chain-specific) horseradish peroxidase conjugate clone RG-96 (Sigma). Blots were rinsed twice with PBS for 5 min, incubated for 5 min in 1:1 luminol:peroxide solution from Pierce in the dark, followed by exposure to autoradiographic films, according to the manufacturer's instructions. 
