Abstract
Rf1 is a nuclear gene that controls fertility restoration in cases of cytoplasmic male sterility caused by the Owen cytoplasm in sugar beet. In order to isolate the gene by positional cloning, a BAC library was constructed from a restorer line, NK198, with the genotype Rf1Rf1. The library contained 32,180 clones with an average insert size of 97.8 kb, providing 3.4 genome equivalents. Five AFLP markers closely linked to Rf1 were used to screen the library. As a result, we identified eight different BAC clones that were clustered into two contigs. The gap between the two contigs was filled by chromosome walking. To map the Rf1 region in more detail, we developed five cleaved amplified polymorphic sequence (CAPS) markers from the BAC DNAs identified, and carried out genotyping of 509 plants in the mapping population with the Rf1-flanking AFLP and CAPS markers. Thirteen plants in which recombination events had occurred in the vicinity of the Rf1 locus were identified and used to map the molecular markers relative to each other and to Rf1. In this way, we were able to restrict the possible location of the Rf1 gene to a minimum of six BAC clones spanning an interval of approximately 250 kb.
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Introduction
Cytoplasmic male sterility (CMS) in higher plants represents one of the few systems in which interactions between mitochondrial and nuclear genomes, and their role in developmental processes, can be investigated (Hanson and Bentolila 2004). CMS is a maternally inherited defect in pollen production that is thought to result from the expression of unusual or aberrant mitochondrial genes (Schnable and Wise 1998). The mitochondrial defect can be compensated for by specific nuclear genes, termed Restorer of fertility (Rf) genes (Hanson and Bentolila 2004). In several of the cases that have been analyzed in detail, these Rf genes appear to inhibit the expression of the CMS-associated mitochondrial gene at a post-transcriptional level (Hanson and Bentolila 2004).
The occurrence of CMS in sugar beet was first documented by Owen (1945). He reported that the CMS (Owen CMS) is controlled by interaction between at least two restorer genes (designated X and Z) and the sterilizing cytoplasm. Owen CMS has been used to produce nearly all commercial beet hybrids (Bosemark 1993), but the molecular mechanism of this CMS remains to be fully defined. We recently found, using in organello translation experiments, that a 35-kDa mitochondrial protein is associated with Owen CMS (Yamamoto et al. 2005). Interestingly, this protein proved to be antigenically related to the 387-codon mitochondrial ORF (designated preSatp6) which is fused in frame with the downstream atp6 ORF (Yamamoto et al. 2005). However, in contrast to the situation in other CMS systems, the presence of Rf genes has no detectable effect on the expression of preSatp6 (Yamamoto et al. 2005). In order to understand the mechanism of fertility restoration in Owen CMS, we therefore decided to clone the Rf genes involved using a positional cloning approach. This approach has allowed the isolation of Rf genes in petunia (Bentolila et al. 2002), radish (Koizuka et al. 2003; Brown et al. 2003; Desloire et al. 2003), and rice (Kazama and Toriyama 2003; Komori et al. 2004; Akagi et al. 2004). All of these Rf genes were reported to encode a pentatricopeptide repeat protein that may prevent the accumulation of the mitochondrial protein responsible for male sterility.
As sugar beet possesses a relatively small genome of 758 Mb (Arumuganathan and Earle 1991), positional cloning is technically feasible if the molecular resources are available (Cai et al. 1997). We identified AFLP markers tightly linked to an Rf gene (named Rf1, probably the same as X) for Owen CMS by employing bulked segregant analysis (Hagihara et al. 2005). These markers provide one tool required for map-based cloning. This report describes the construction of a sugar beet BAC library, which is another resource necessary for the cloning strategy (Gindullis et al. 2001; Hohmann et al. 2003; Fang et al. 2004; McGrath et al. 2004). We also describe the use of the BAC library in the assembly of a 250 kb contig spanning Rf1.
Materials and methods
Plant materials
TK76-MS and TK81-MS are male-sterile Owen cytoplasm lines, while NK198 is a restorer line with the genotype Rf1Rf1. Pollen from NK198 was used to pollinate TK76-MS. A male-fertile F1 plant was then crossed with TK81-MS instead of TK76-MS because of failure to synchronize the flowering between the F1 plant and TK76-MS. The resultant (three-way cross) population consisted of 509 plants and segregated in a 1:1 ratio for the presence/absence of Rf1. Male fertility was determined by visual observation of anther color and pollen dehiscence, and by microscopic observation of the percentage of cotton-blue stained pollen (Hagihara et al. 2005).
Isolation of high molecular weight DNA
About 10 g of fresh green leaves was collected from NK198 and used to isolate nuclei according to Liu and Whittier (1994) with minor modifications: our nuclear isolation buffer consisted of 10 mM Tris–HCl (pH 9.5), 20 mM EDTA (pH 8.0), 80 mM KCl, 0.5 M sucrose, 4 mM spermidine, 1 mM spermine and 0.1% mercaptoethanol; the leaf homogenate was filtered through miracloth (Calbiochem, La Jolla, CA, USA) instead of nylon mesh; the isolation buffer added to the filtrate was not supplemented with Triton X-100. The nuclei were pelleted at 600 g for 10 min. Plugs of high molecular weight DNA were prepared after adding 1.5% low-melting agarose (45°C). Plugs were equilibrated in lysis buffer (1% Sarkosyl, 0.2 M EDTA pH 8.0, 0.1 mg/ml proteinase K) at 50°C for 48 h with one change of lysis buffer, followed by dialysis with TE50 buffer (10 mM Tris–HCl pH 8.0, 50 mM EDTA) at 4°C for more than 2 h. The proteinase K was inactivated by a 2 h incubation at 50°C in TE50 buffer supplemented with phenylmethylsulfonyl fluoride (PMSF) (final concentration 2 mM). Plugs were then washed in TE50 buffer and stored at 4°C until use. Plugs were equilibrated in TE buffer (10 mM Tris–HCl pH 8.0, 1 mM EDTA) and then kept in buffer containing 10 mM TRIS–HCl pH 7.5, 1 mM DTT, 50 mM NaCl, 0.01% BSA and 15 U/ml HindIII (Takara Bio, Otsu, Japan) at 4°C for 5 h. After incubation in the presence of 10 mM MgCl2 at 4°C for a further hour, plugs were kept at 37°C for 10 min. Restriction digestion was terminated by adding 0.5 M EDTA (pH 8.0) and chilling the reaction. The partially digested DNA was fractionated by pulsed-field gel electrophoresis (PFGE) using a CHEF-DRII apparatus (Bio-Rad, Hercules, CA, USA): electrophoresis was done at 14°C in a 1.0% pulsed-field certified agarose gel (Bio-Rad) at 6 V/cm with a switch time of 90 s for 8 h, followed by a switch time of 6 s for 16 h. Gel pieces containing DNA fragments ranging in size from 200 to 500 kb were excised, and the DNA was electroeluted as described by Strong et al. (1997).
Construction of the BAC library
The vector pBeloBAC11 (Kim et al. 1994) was prepared as described by Woo et al. (1994). The size-fractionated, HindIII-digested sugar beet DNA was ligated to pBeloBAC11 at a molar ratio of 1 (beet DNA) to 10 (vector DNA) and the ligation mixture was dialyzed according to Woo et al. (1994). The ligated DNA was utilized to transform E. coli Electro Max DH10B cells (Invitrogen, Carlsbad, CA, USA). The BAC clones were picked manually with sterile toothpicks and addressed in 96- or 384-well microtiter plates. BAC DNA was prepared from 2 ml cultures in LB medium by an alkaline lysis method (Woo et al. 1994), and electrophoresed in a 1% gel using the CHEF-DRII apparatus (6 V/cm, 5–15 s switch time, 14 h run-time, 14°C).
Screening of the BAC library based on AFLP analysis
The BAC library was screened with the AFLPs using plate pools, and then row and column sub-pools of BAC DNAs. The library stored in 384-well plates was replicated onto LB-plates using a 384-pin replicator, and colonies were grown at 37°C for 16 h. The plates were washed with liquid LB medium to collect clones and the BAC DNAs were isolated. The resultant plate pools of BAC DNA were subjected to AFLP analysis (Vos et al. 1995; Habu et al. 1997) using AFLP Analysis System I (Invitrogen) with 32P-labeled primers. Pooled DNA was digested with EcoRI and MseI. The adaptor-ligated DNA was pre-amplified using primers without selective nucleotides. The selective-amplification was performed using primers with two selective nucleotides. Plate pools containing clone(s) of interest were further subdivided in 16 rows and 24 columns to give 40 sub-pools, which were subsequently used for AFLP-based screening to identify individual positive clones.
Screening of the BAC library based on colony hybridization
Using a 384-pin replicator, BAC clones were spotted onto Hybond N membranes (Amersham Biosciences, Piscataway, N J, USA) placed on LB agar plates. Colonies were grown at 37°C for 12 h. Colony filters were processed and hybridized using standard protocols (Sambrook et al. 1989) according to the manufacturer’s instruction manual. The hybridization probe was labeled with 32P using the Megaprime DNA labeling system (Amersham Biosciences).
Sub-cloning of BAC insert ends
About 50 ng aliquots of BAC DNA were digested with BamHI or SphI, and then self-ligated. BAC insert ends were generated by vectorette-PCR (Riley et al. 1990), using BR3 (5′-TGACCATGATTACGCCAAGC-3′) and BL3 (5′-ACCTGCAGGCATGCAAGCTT-3′) primers. TAIL-PCR (Liu and Whittier 1995) was also used to isolate BAC ends. The specific primers used to amplify the right ends were BR1 (5′-CACTTTATGCTTCCGGCTCG-3′), BR2 (5′-GTTGTGTGGAATTGTGAGCG-3′) and BR3, while the left ends were amplified with BL1 (5′-GGGATGTGCTGCAAGGCGAT-3′), BL2 (5′-GGTTTTCCCAGTCACGACGT-3′) and BL3. The resultant PCR products were cloned into pBluescript vector (Stratagene, La Jolla, CA, USA).
Cloning of AFLP fragments
AFLP products were electrophoresed on a standard sequencing gel. After exposure, the autoradiogram was aligned with the dried gel to isolate the amplified fragment of interest from the gel. The gel piece was then boiled in water for 15 min as described by Habu et al. (1997). After a brief centrifugation, the supernatant was subjected to PCR amplification using the same sets of AFLP primers. The amplification products were recovered from the agarose gel and cloned into pBluescript vector.
Cleaved amplified polymorphic sequence (CAPS) analysis
Primer sequences and restriction enzymes used for CAPS analysis are listed in Table 1. About 20 ng of total cellular DNA was subjected to PCR amplification using the following reaction parameters: 35 cycles of 30 s at 94°C, 30 s at 54°C and 90 s at 70°C. The amplification products were digested with appropriate restriction endonucleases and resolved by electrophoresis in 1.5% agarose gels.
Other molecular analyses
Cellular DNA extraction, DNA and RNA gel blot analyses and DNA sequencing followed standard techniques (Sambrook et al. 1989; Kubo et al. 2000; Hagihara et al. 2005).
Results and discussion
Construction of the NK198 BAC library
A restorer line, NK198, was chosen as the source of genomic DNA for the construction of the BAC library. Using three different ligation mixes, a total of 32,180 BAC clones was collected and constitutes the library. The insert-size distribution of the library was evaluated by analyzing 100 randomly selected individual clones. Figure 1a shows an ethidium bromide-stained pulsed-field gel of 16 of these clones digested with NotI. The average size of the inserts in the 100 clones was 97.8 kb, and the range was 20–180 kb. Approximately 58% of the clones carried inserts larger than 80 kb, though a significant number of clones (30%) had inserts smaller than 40 kb (Fig. 1b).
To examine the stability of sugar beet DNA fragments maintained as BACs in E. coli, four BAC clones with inserts larger than 100 kb were selected and grown for about 100 generations (3 days). We analyzed the HindIII restriction digestion patterns of the four BAC clones after 16 and 100 generations. No obvious changes were observed (data not shown), proving that the BAC cloning vector could stably maintain large DNA fragments in E. coli.
The NK198 BAC library was further investigated to determine the extent of contamination with clones originating from chloroplast DNA. For this purpose, 1,536 randomly chosen clones were hybridized with three sugar beet chloroplast DNA probes, ndhG (located within the small single-copy region), psbB (within the large single-copy region) and ycf2 (within the large inverted repeat regions), simultaneously. These three probes are approximately equidistant from each other in the chloroplast genome, so that any BAC insert larger than 60 kb should hybridize with one of the probes.
Some 19% of the BACs hybridized with this probe set (data not shown), indicating that these positive clones contained chloroplast sequences. Based on a haploid genome size of 758 Mb for sugar beet (Arumuganathan and Earle 1991), the NK198 BAC library represents 3.4-fold genome equivalents, if the chloroplast fraction is subtracted out. Assuming that the BAC inserts are randomly distributed in the genome, the probability of detecting any given sequence can be calculated (Clarke and Carbon 1976) as 96.7%.
A BAC contig containing the Rf1 locus
We previously identified five AFLP-markers (mAFEM972, mAFEM984, mAFEM004, mAFEM976 and mAFEM985) that show close linkage to the Rf1 locus (Hagihara et al. 2005). The AFLP marker fragments were recovered from the gel and cloned, and the resultant clones were used as probes for hybridization with sugar beet genomic DNA. Two markers, mAFEM976 and mAFEM985, showed single-copy fragment patterns (Fig. 2) and therefore these markers were deemed suitable for use in colony-hybridization-based screening of the NK198 library. The remaining three markers were less suitable as probes for the same screening approach because they were shown to represent repetitive DNA (Fig. 2). We therefore attempted to screen the library with AFLP primer combinations using pools of BAC DNA as templates. Our pooling strategy utilized three different pool types: plate pools of 384 single BAC clones, rows of sub-pools comprising 16 single clones each, and columns of sub-pools comprising 24 single clones each. A total of 324 pools (84 plate pools, and 240 sub-pools derived from rows and columns) were screened with the three AFLP markers. As summarized in Table 2, eight different BAC clones were identified after both hybridization- and AFLP-based screens.
In the next step, the ends of these BAC clones were sub-cloned. The BAC end clones obtained were then used for hybridization to Southern blots of HindIII-digested BAC DNAs. The results allowed us to assemble the eight BAC clones into two contigs (5A3/9C23/37O9/33E19/9O3/51L1 and 1M13/36I20). In order to join the two contigs, we further screened the library with the outermost ends of the contigs. This led to the identification of six additional, overlapping BACs, one (41H8) of which was found to be a bridging clone connecting the two contigs (Fig. 3). As shown in Fig. 3, a physical map of the Rf1 region could be constructed, encompassing 14 BACs anchored by the five AFLP loci mentioned above. The genomic region of interest is flanked by the AFLP-markers mAFEM984 and mAFEM004, which are located 3.5 cM apart.
BAC-derived markers
In order to more precisely locate the Rf1 gene in the BAC contig, we attempted to derive additional molecular markers from the BAC clones spanning the Rf1 region. The HindIII sub-fragments of BAC DNAs were utilized as probes for genomic Southern hybridization. In total, 23 sub-fragments were regarded as single-copy and some of these sub-fragments were end-sequenced to design the primers for CAPS analysis. The CAPS primer pairs were used to amplify DNAs from the Owen CMS lines (TK81-MS and TK76-MS, rf1rf1) and the restorer line NK198 (Rf1Rf1) involved in the three-way cross (see “Materials and methods”). The amplification products were further digested with four-base-cutters to detect polymorphisms, resulting in the development of five CAPS markers, mCP-A54, mP-A16, mCP-K2, mCP-L6 and mCP-L45 (Fig. 3). Using a subset of the three-way cross population [TK81-MS × (TK76-MS × NK198)], we confirmed that all the CAPS markers segregated according to the expected ratio of 1:1 and co-segregated with Rf1 (data not shown).
Candidate Rf1-containing clones
We next wished to identify members of the three-way cross population that had undergone recombination close to the Rf1 locus. We therefore determined the genotypes of DNA samples from 509 plants in the three-way cross population using eight Rf1-flanking markers. The screen enabled us to identify 13 plants in which recombination had occurred in the vicinity of Rf1, and these plants were then used to map the eight markers relative to each other and to Rf1. As shown in Table 3 and Fig. 3, Rf1 could be restricted to the 250-kb region that is delimited by the markers mP-A16 and mCP-L6. Two BACs, 37O9 and 33E19, with insert sizes of 220 and 210 kb, respectively, are candidates for cloning the Rf1 gene.
As mentioned above, a number of HindIII sub-fragments from the BAC DNAs covering the Rf1 region were labeled for Southern hybridization. These fragments were also used to probe Northern blots of RNA prepared from flower buds, leaves and roots of the Rf1Rf1 (NK198) and rf1rf1 (TK81-MS) plants in an attempt to identify regions which were transcribed in the Rf1Rf1 plants but not in the rf1rf1 plants. Interestingly, a transcript difference was detected when a 7.0 kb HindIII fragment derived from the BAC 37O9 was utilized as a probe against flower bud RNA. This probe hybridized to a 1.7-kb transcript in NK198, but no transcripts were observed in TK81-MS (Fig. 4). It should also be noted that the 1.7-kb transcript was not detectable in leaves or roots of Rf1Rf1 plants (Fig. 4). To pinpoint the location of the Rf1 gene, sequencing of BAC DNAs and identification of candidate sequences will be required. Such investigations are presently underway in this laboratory.
References
Akagi H, Nakamura A, Yokozeki-Misono Y, Inagaki A, Takahashi H, Mori K, Fujimura T (2004) Positional cloning of the rice Rf-1 gene, a restorer of BT-type cytoplasmic male sterility that encodes a mitochondria-targeting PPR protein. Theor Appl Genet 108:1449–1457
Arumuganathan K, Earle ED (1991) Nuclear DNA content of some important plant species. Plant Mol Biol Rep 9:211–215
Bentolila S, Alfonso AA, Hanson MR (2002) A pentatricopeptide repeat-containing gene restores fertility to cytoplasmic male-sterile plants. Proc Natl Acad Sci USA 99:10887–10892
Bosemark NO (1993) Genetics and breeding. In: Cooke DA, Scott RK (eds) The sugar beet crops. Chapman and Hall, London, pp 66–119
Brown GG, Formanova N, Jin H, Wargachuk R, Dendy C, Patil P, Laforest M, Zhang J, Cheung WY, Landry BS (2003) The radish Rfo restorer gene of Ogura cytoplasmic male sterility encodes a protein with multiple pentatricopeptide repeats. Plant J 35:262–272
Cai D, Kleine M, Kifle S, Harloff HJ, Sandal NN, Marcker KA, Klein-Lankhorst RM, Salentijn EM, Lange W, Stiekema WJ, Wyss U, Grundler FM, Jung C (1997) Positional cloning of a gene for nematode resistance in sugar beet. Science 275:832–834
Clarke L, Carbon J (1976) A colony bank containing synthetic ColE1 hybrid plasmids representative of the entire E. coli genome. Cell 9:91–99
Desloire S, Gherbi H, Laloui W, Marhadour S, Clouet V, Cattollico L, Falentin C, Giancola S, Renard M, Budar F, Small I, Caboche M, Delourme R, Bendahmane A (2003) Identification of the fertility restoration locus, Rfo, in radish, as a member of the pentatricopeptide-repeat protein family. EMBO Rep 4:588–594
Fang X, Gu S, Xu Z, Chen F, Guo D, Zhang H-B, Wu N (2004) Construction of a binary BAC library for an apomictic monosomic addition line of Beta corolliflora in sugar beet and identification of the clones derived from the alien chromosome. Theor Appl Genet 108:1420–1425
Gindullis F, Dechveva D, Schmidt T (2001) Construction and characterization of a BAC library for the molecular dissection of a single wild beet centromere and sugar beet (Beta vulgaris) genome analysis. Genome 44:846–855
Habu Y, Fukada-Tanaka S, Hisatomi Y, Iida S (1997) Amplified restriction fragment length polymorphism-based mRNA fingerprinting using a single restriction enzyme that recognizes a 4-bp sequence. Biochem Biophys Res Commun 234:516–521
Hagihara E, Itchoda N, Habu Y, Iida S, Mikami T, Kubo T (2005) Molecular mapping of a fertility restorer gene for Owen cytoplasmic male sterility in sugar beet. Theor Appl Genet (in press)
Hanson MR, Bentolila S (2004) Interactions of mitochondrial and nuclear genes that affect male gametophyte development. Plant Cell 16:S154–S169
Hohmann U, Jacobs G, Telgmann A, Gaafar RM, Alam S, Jung C (2003) A bacterial artificial chromosome (BAC) library of sugar beet and a physical map of the region encompassing the bolting gene B. Mol Genet Genomics 269:126–136
Kazama T, Toriyama K (2003) A pentatricopeptide repeat-containing gene that promotes the processing of aberrant atp6 RNA of cytoplasmic male-sterile rice. FEBS Lett 544:99–102
Kim UJ, Birren B, Slepak T, Mancino V, Boysen C, Kang HL, Simon M, Shizuya H (1994) Construction and characterization of a human bacterial artificial chromosome library. Genomics 34:213–218
Koizuka N, Imai R, Fujimoto H, Hayakawa T, Kimura Y, Kohno-Murase J, Sakai T, Kawasaki S, Imamura J (2003) Genetic characterization of a pentatricopeptide repeat protein gene, orf687, that restores fertility in the cytoplasmic male-sterile Kosena radish. Plant J 34:407–415
Komori T, Ohta S, Murai N, Takakura Y, Kuraya Y, Suzuki S, Hiei Y, Imaseki H, Nitta N (2004) Map-based cloning of a fertility restorer gene, Rf-1, in rice (Oryza sativa L.). Plant J 37:315–325
Kubo T, Nishizawa S, Sugawara A, Itchoda N, Estiati A, Mikami T (2000) The complete nucleotide sequence of the mitochondrial genome of sugar beet (Beta vulgaris L.) reveals a novel gene for tRNACys (GCA). Nucleic Acids Res 28:2571–2576
Liu YG, Whittier RF (1994) Rapid preparation of megabase plant DNA from nuclei in agarose plugs and microbeads. Nucleic Acids Res 22:2168–2169
Liu YG, Whittier RF (1995) Thermal asymmetric interlaced PCR: automatable amplification and sequencing of insert end fragments from P1 and YAC clones for chromosome walking. Genomics 25:674–681
McGrath JM, Shaw RS, de los Reyes BG, Weiland JJ (2004) Construction of a sugar beet BAC library from a hybrid with diverse traits. Plant Mol Biol Rep 22:23–28
Owen FV (1945) Cytoplasmically inherited male-sterility in sugar beets. J Agric Res 71:423–440
Riley J, Butler R, Ogilvie D, Finniear R, Jenner D, Powell S, Anand R, Smith JC, Markham AF (1990) A novel, rapid method for the isolation of terminal sequence from YAC clones. Nucleic Acids Res 18:2887–2890
Sambrook J, Fritsh EF, Maniatis T (1989) Molecular cloning: a laboratory manual, 2nd edn. Cold Spring Harbor Laboratory, Cold Spring Harbor, New York
Schnable PS, Wise RP (1998) The molecular basis of cytoplasmic male sterility and fertility restoration. Trends Plant Sci 3:175–180
Strong S, Ohta Y, Litman G, Amemiya C (1997) Marked improvement of PAC and BAC cloning is achieved using electroelution of pulsed-field gel-separated partial digests of genomic DNA. Nucleic Acids Res 25:3959–3961
Vos P, Hogers R, Bleeker M, Reijans M, Van Der Lee T, Hornes M, Frijters A, Pot J, Peleman J, Kuiper M, Zabeau M (1995) AFLP: a new technique for DNA fingerprinting. Nucleic Acids Res 23:4407–4414
Woo SS, Jiang J, Gill B, Paterson A, Wing R (1994) Construction and characterization of a bacterial artificial chromosome library of Sorghum bicolor. Nucleic Acids Res 22:4922–4931
Yamamoto MP, Kubo T, Mikami T (2005) The 5′-leader sequence of sugar beet mitochondrial atp6 encodes a novel polypeptide that is characteristic of Owen cytoplasmic male sterility. Mol Gen Genomics 273:342–349
Acknowledgments
The authors wish to thank Drs. M. Watanabe, M. Itoh and S. Nakamura for valuable suggestions and technical advice about BAC library construction and handling. This work was done in part at the Research Center for Molecular Genetics, Hokkaido University, and was supported in part by Grants in Aid for Scientific Research from the Ministry of Education, Culture, Sports, Science and Technology, Japan, and in part by a grant from the Ministry of Agriculture, Forestry and Fisheries, Japan, (Research Project for Utilizing Advanced Technologies in Agriculture, Forestry and Fisheries No. 1423). E.H. was, and H.M. is, a recipient of the JSPS Fellowship for Japanese Junior Scientists.
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The first two authors contributed equally to this work.
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Hagihara, E., Matsuhira, H., Ueda, M. et al. Sugar beet BAC library construction and assembly of a contig spanning Rf1, a restorer-of-fertility gene for Owen cytoplasmic male sterility. Mol Genet Genomics 274, 316–323 (2005). https://doi.org/10.1007/s00438-005-0024-5
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DOI: https://doi.org/10.1007/s00438-005-0024-5