| HOME | HELP | FEEDBACK | SUBSCRIPTIONS | ARCHIVE | SEARCH | TABLE OF CONTENTS |
|
|
|
|||||||
|
|||||||||
|
First published online September 26, 2002; 10.1105/tpc.005959 American Society of Plant Biologists Severe Developmental Defects, Hypersensitivity to DNA-Damaging Agents, and Lengthened Telomeres in Arabidopsis MRE11 MutantsInstitute for Molecular Plant Sciences, Wassenaarseweg 64, 2333 AL, Leiden, The Netherlands 1 To whom correspondence should be addressed. E-mail bundock{at}rulbim.leidenuniv.nl; fax 00-31-(0)715274999
The Mre11 protein is essential for the long-term genetic stability of the cell and acts to ensure the efficient repair of DNA damage. Vertebrate cells lacking Mre11 function are not viable. However, we report here that this is not the case in the model plant Arabidopsis. We have isolated two different Arabidopsis lines containing a T-DNA copy integrated at a different point in the MRE11 gene (AtMRE11). Both mutant plant lines were hypersensitive to DNA-damaging treatments but exhibited strikingly different developmental phenotypes. Furthermore, we also observed lengthened telomeres in these plant lines, showing that AtMre11 is involved in telomere maintenance. Thus, the lines we have isolated are unique tools with which to study in detail the role of AtMre11 in the mature plant.
An organism's genetic material is damaged frequently by external agents, such as ionizing or solar radiation, aggressive metabolites, or during the process of DNA replication. DNA damage can be catastrophic to the cell, and its accurate repair is essential for the cell and its descendants to maintain genetic stability. Breaks in both strands of a duplex DNA molecule, a double-strand break (DSB), are among the most threatening for the cell. Two independent pathways have evolved for the repair of DSBs. The homologous recombination (HR) pathway for DSB repair is conservative and uses homologous sequences on the sister chromatid or elsewhere in the genome as a template to repair the DSB. The second pathway, nonhomologous end joining (NHEJ), rejoins the two ends of a DSB without using a homologous template. NHEJ can be mutagenic, because nucleotides can be lost or added at the repair site. The predominant DNA repair pathway (HR or NHEJ) varies in different cell types. Generally, HR is the major pathway in single-celled organisms such as bacteria and yeast, but NHEJ is the dominant DNA repair mechanism in most cell types of higher eukaryotes. However, there are exceptions, such as in the ES and DT40 cell lines of vertebrates and cells of the moss Physcomitrella patens, which use the HR pathway efficiently.
Cells have evolved an array of powerful enzymatic tools that are able to recognize DSBs, repair the DNA lesion, and prevent cell cycle progression until this is accomplished. In the yeast Saccharomyces cerevisiae, genes in the RAD52 epistasis group, which includes the MRE11 gene, are required. The Mre11 protein forms a complex with the Rad50 and Xrs2 proteins (the MRX complex), as shown in a yeast two-hybrid assay (Johzuka and Ogawa, 1995
An insight into the possible biochemical role of Mre11 in the cell came from the observation that the Escherichia coli SbcC protein and the SbcD nuclease are homologous with the Rad50 and Mre11 proteins, respectively (Sharples and Leach, 1995
The Mre11 protein is also essential during meiosis. During sexual reproduction, cells undergoing meiosis reduce their diploid chromosome content by half. To ensure the correct segregation of chromosomes to the respective gametes, chromosome sorting is followed by crossover recombination between homologous chromosomes. This, in collaboration with sister chromatid cohesion, allows the establishment of temporary connections between homologs, which allows them to orient toward the opposite poles of the meiosis I spindle (Moore and Orr-Weaver, 1998
In yeast, Mre11, along with other NHEJ proteins such as the Ku heterodimer, also is necessary for the maintenance of telomere length. Mutations in any of these components result in shortened telomeres (Porter et al., 1996
The kinetics of MRX complex formation in response to DNA damage also has been studied. The MRX complex forms foci at DSBs induced by ionizing radiation or those associated with the process of V(D)J rearrangement during B and T cell development (Carney et al., 1998
Studying the role of MRE11 in multicellular organisms is difficult, given that it is essential in mammalian cells (Xiao and Weaver, 1997
The MRE11 gene has been identified in the genomes of all of the eukaryotes sequenced to date. Recently, the sequencing of the genome of Arabidopsis allowed the identification of a plant MRE11 ortholog (Hartung and Puchta, 1999  ). A comparison of the Arabidopsis Mre11 protein (AtMre11) with Mre11 proteins from several other organisms is shown in Figure 1
. The homology between the different Mre11 orthologs is strongest in the four conserved phosphoesterase domains but is less pronounced in the C terminus of the proteins. We screened the Arabidopsis Knockout Facility (Krysan et al., 1999) to identify Arabidopsis lines containing T-DNA insertions in AtMRE11. After several rounds of screening, we were able to isolate two Arabidopsis lines that contain such insertions and named them AtMRE11-1 and AtMRE11-2.
Isolation and Characterization of the AtMRE11-1 Mutant A reverse genetics approach was taken to identify Arabidopsis lines containing mutations in AtMRE11. The gene-specific primer TS1 in combination with a T-DNA–specific primer (JL-202) were used to screen DNA pools from a collection of T-DNA–transformed Arabidopsis plant lines. A 1.7-kb PCR product was amplified using these primers. Sequencing of this product revealed that a plant line was present in the collection containing a T-DNA copy inserted into exon 9 of the AtMRE11 gene. After several further PCR rounds on smaller DNA pools, we eventually isolated a single plant containing this T-DNA insertion and named the line AtMRE11-1. The single original plant of the AtMRE11-1 line we isolated appeared normal and produced seeds. On a DNA gel blot, this plant was heterozygous for the T-DNA insertion in AtMRE11 (Figure 2C , lane 3). Seeds from this original plant were germinated on medium containing kanamycin. The seedlings segregated 3:1 for kanamycin resistance:sensitivity (203 resistant:69 sensitive), indicating that this line contained a single T-DNA locus. This finding was confirmed by DNA gel blot analysis using a NPTII probe to detect the T-DNA (data not shown). Six days after germination, approximately one-third (64) of the kanamycin-resistant seedlings started to show a dwarf phenotype (Figure 3A) . DNA from a pool of these small seedlings (60 in total) was isolated and analyzed on a DNA gel blot (Figure 2C, lane 2). All of these dwarf plants were homozygous for the T-DNA insertion, as demonstrated by the absence of a characteristic 5.6-kb EcoRI fragment. Furthermore, this result shows that the dwarf phenotype was linked to the T-DNA insertion.
To establish the effect of this T-DNA insertion on plant development, a detailed phenotypic analysis of the AtMRE11-1 line was performed. Because the dwarf seedlings homozygous for the AtMRE11-1 mutation (AtMRE11-1-/-) grew so slowly, we left them to grow on half-strength Murashige and Skoog (1962) (MS) medium for up to 6 weeks. After this period, it was apparent that these plants had severe developmental abnormalities, but the severity of the phenotypes varied between different seedlings (Figures 3D to 3G). In all of these seedlings, the hypocotyls were thickened, the roots became agravitropic, and the plants had an altered leaf morphology and an obvious defect in radial symmetry. The cotyledons also showed early necrosis. This often began as a brown spot (Figure 3E), which then spread to the entire cotyledon. This process often was very fast, with the first signs of necrosis to complete cotyledon necrosis occurring within 24 to 36 h. The necrosis occurred earlier in smaller seedlings with the more severe developmental phenotypes. Cotyledons and leaves from plants showing the mild phenotypes were cleared and studied using dark-field microscopy. Every leaf studied had an altered morphology and defects in the vasculature (Figure 3L). In a detailed analysis of the leaf epidermis, we also often observed clustering of stomata (Figure 3K). Examination of the root meristems also revealed some severe defects. As a control, root meristems from AtMRE11-1+/- plants were examined (Figure 3H). These showed the distinctive precise organization of cell files characteristic of the Arabidopsis root meristem. By contrast, the root meristem of 6-week-old AtMRE11-1-/- seedlings had lost all organization and were composed of large cells (Figure 3I). Development of lateral roots seemed to begin normally, but this broke down completely as the lateral roots matured (Figure 3J).
Only the fittest AtMRE11-1-/- seedlings (Figure 3D) survived in soil to form mature plants (Figure 3B). In fact, the most severely affected seedlings eventually died on the half-strength MS medium after approximately 8 weeks. Plants with the milder phenotype that grew into mature plants in soil often showed fasciation in the stems or in the floral organs and had very few small, thin leaves (Figure 3C). The components of the MRX complex are essential for gametogenesis (Ajimura et al., 1993 When we germinated seed from AtMRE11-1+/- plants on medium, we observed a 3:1 segregation of the dwarf phenotype, suggesting that the AtMRE11-1 mutation was recessive. When AtMRE11-1+/- seedlings were germinated on half-strength MS medium and then transferred to soil, they appeared normal. However, when seed from AtMRE11-1+/- plants was sown directly in soil, the plants that were heterozygous for the AtMRE11-1 mutation presented several phenotypes, such as fasciation and altered leaf morphology characteristic of the mature AtMRE11-1-/- plants (data not shown). This finding suggested that the AtMRE11-1 mutation can, under certain stress conditions, act in a semidominant manner. In these experiments, we never observed mature AtMRE11-1-/- plants, suggesting that they are unable to develop directly in soil. We attempted to complement the developmental phenotypes of the AtMRE11-1 line by expressing the AtMRE11 cDNA under the control of the constitutive 35S promoter. T2 AtMRE11-1-/- and AtMRE11-1+/- seedlings from several independent lines expressing the AtMRE11 cDNA were checked for developmental phenotypes. The complemented AtMRE11-1-/- seedlings were intermediate in size and developed normally (data not shown). However, the fertility of such plants was reduced compared with that of complemented AtMRE11-1+/- plants, which produced wild-type amounts of seed. The siliques were small and contained only a few viable seeds. Therefore, in the AtMRE11-1 line, we were able to complement the fasciation phenotypes, but the sterility and growth defects of AtMRE11-1-/- were complemented only partially. This finding is not surprising, given the semidominant nature of the AtMRE11-1 mutation.
Isolation and Characterization of the AtMRE11-2 Mutant The AtMRE11-2-/- plants developed normally and showed none of the developmental defects observed in AtMRE11-1-/- plants (Figure 3B). Unexpectedly, AtMRE11-2-/- plants also were fertile. AtMRE11-2-/- plants were grown for six generations to test any possible effect of the mutation on reproductive capacity. No difference in the phenotype of plants or the number of seeds they produced was observed between plants from the first or later generations. Therefore, we propose that the missing 191 amino acids from the C terminus of the AtMre11 protein are not necessary for gametogenesis in Arabidopsis.
Expression Analysis
AtMRE11-2-/- Plants Are Hypersensitive to DNA-Damaging Treatments
Lengthened Telomeres in the AtMRE11-1 and AtMRE11-2 Mutants In other organisms, mutations in components of the NHEJ pathway shorten the telomeres. To investigate this possibility in plants, and in view of the observed developmental abnormalities in the AtMRE11-1 line, we determined the length of the telomeres in AtMRE11-1-/-, AtMRE11-1+/-, and AtMRE11-2-/- plants. Because the AtMRE11-2-/- plants are fertile, we also were able to determine whether the telomere length changed during six successive generations. We isolated DNA from seedlings from each generation and performed DNA gel blot analysis using a telomere-repeat probe to detect the characteristic telomere smears. To our surprise, in all of the mutant plants analyzed, the telomeres were longer than those in the wild-type plant (Figure 5) . In the AtMRE11-2-/- plants, the telomeres also were maintained at this longer size during all six generations tested (data not shown). In addition, we found that the AtMRE11-1 mutation is dominant for increased telomere length, because the AtMRE11-1+/- plants also showed lengthened telomeres, although in this case the telomeres were not lengthened to the extent seen in AtMRE11-2-/- plants. These results show that although the MRE11 genes are conserved in many organisms, in plants it functions to maintain shortened telomeres, and the C terminus of the protein is essential for this process. Recently, we and others have isolated a plant line containing a mutation in the Arabidopsis KU70 (AtKU70) gene. In line with the data presented here, plants homozygous for this mutation also show lengthened telomeres, but in this case, their length is increased to greater than  30 kb (Bundock et al., 2002; Riha et al., 2002). Thus, although plants contain orthologs of the MRE11 and KU70 genes, these proteins have a different effect on telomere length than that observed in yeast and animals.
Previous studies have revealed that Mre11, as part of a complex with the Rad50 and Xrs2/Nbs1 proteins, functions in many diverse mechanisms of DNA repair and metabolism. Here, we report the isolation and characterization of two Arabidopsis lines containing mutations in the AtMRE11 gene. The differences between the two lines are striking. Although AtMRE11-1-/- plants are dwarf, sterile, and show numerous developmental defects, AtMRE11-2-/- plants are normal and fertile. The developmental, sensitivity to DNA-damaging agents, and telomere length phenotypes of the AtMRE11-1 mutation demonstrate that it is semidominant. Expression analysis showed that the mutant plant lines express AtMRE11 mRNA to wild-type levels; however, because of the T-DNA insertions, we were unable to detect the full-length AtMre11 proteins. The antibody also recognized other proteins, present in all samples analyzed, that were identical in size to the predicted truncated proteins in the AtMRE11-1-/- and AtMRE11-2-/- plants. Therefore, we were unable to detect such truncated proteins, although given the semidominant nature of the AtMRE11-1 mutation, we would expect a truncated protein to be produced in this line. A truncated AtMre11 protein in AtMRE11-/- plants may function in a dominant manner by titrating out cellular components involved in development, MMS resistance, and telomere length maintenance. This truncated protein may prevent the formation of AtMre11 homodimers or the interaction with AtRad50 or with other unidentified proteins. Similarly, the phenotypes of AtMRE11-2-/- plants could be attributable to altered protein–protein interactions. It will be interesting to perform coimmunoprecipitation experiments with extracts from the mutant plants to identify proteins that copurify with any truncated forms of AtMre11 produced in the mutant lines. Such experiments also would allow us to map the interaction domains of AtMre11 with itself and with AtRad50. Alternatively, the developmental phenotypes may be characteristic of an accumulation of inaccurately repaired DNA breaks during cell growth. However, if this were the case, such phenotypes would be apparent in AtMRE11-2-/- plants, which also are affected in DNA repair, as shown by the hypersensitivity to MMS.
The data presented here indicate that AtMre11 influences the length of plant telomeres. Telomeres are specialized structures at the ends of chromosomes that are essential for genomic stability. Telomeres are made up of short G-rich repeats that conform to the consensus sequence Tx(A)Gy. The length of the telomeres varies by organism and cell type. In Arabidopsis, telomeres are 2 to 4 kb in length and consist of repeats of the sequence TTTAGGGn. During mitosis, the DNA replication machinery is unable to replicate the ends of chromosomes, leading to a progressive shortening of chromosomes during successive cell divisions. This had led to speculation that telomere shortening may be linked to cellular senescence. This end replication problem is overcome by the activity of the reverse transcriptase telomerase, which is able to add telomere sequences to the ends of chromosomes. In mammals, telomerase is regulated developmentally in different cell types and shows high expression in reproductive tissues but is inactivated in somatic tissues. The telomerase activity in different plant tissues also has been measured. The highest activity is found in proliferating tissues, such as meristems, but telomerase activity is low or undetectable in nonmeristematic tissues, such as leaves (Rhia et al., 1998
Recently published reports (Riha et al., 2001
Several hypotheses may explain this result. In the cell, telomere length is thought to be governed by a homeostasis mechanism that operates via the influence of positive and negative factors on the enzyme telomerase. One possible role of AtMre11 at Arabidopsis telomeres may be its action on proteins that inhibit telomere elongation. In mammalian cells, the telomere binding proteins TRF1 and TRF2 have been identified. Cells expressing truncated dominant-negative forms of these proteins have lengthened telomeres (van Steensel and de Lange, 1997
Our data are in contrast to recent data reporting that no change in telomere length was seen in plants lacking AtRad50. In addition, cultured cell lines lacking AtRad50 showed a progressive shortening of telomeres (Gallego and White, 2001
It is important to stress the differences found in this study between the proposed functional domains of the Mre11 proteins of S. cerevisiae and Arabidopsis. Many studies have attempted to map the regions of the S. cerevisiae Mre11 protein that are required for meiosis. Many mutations in the conserved phosphoesterase motifs (e.g., P84S, T188I, H213Y, and H125N), in addition to deletion of the C terminus of Mre11, cause defects in meiosis (Nairz and Klein, 1997 In conclusion, we have demonstrated that AtMRE11 plays a role in DNA repair, plant development, and telomere maintenance in Arabidopsis. Plants seem to be able to tolerate mutations in nonhomologous end joining (NHEJ) genes much more readily than mammalian cells. This makes plants an ideal system in which to investigate the roles of NHR genes in multicellular organisms by studying lines that have multiple mutations in NHR genes, as has been done previously in yeast.
Constructs The Arabidopsis thaliana MRE11 cDNA was amplified from a pool of seedling cDNA and inserted into pGEM-T Easy (Promega) to generate pSDM2011. A NcoI-SpeI fragment then was cloned into pCAMBIA3301 cut with NcoI-NheI to form pSDM2012, which was electroporated to Agrobacterium tumefaciens strain LBA1115. Plants were transformed using the floral dip method (Clough and Bent, 1998 ). Seeds from these plants were collected and surface-sterilized. Transformants were selected on half-strength Murashige and Skoog (1962) (MS) medium containing glufosinate-ammonium (20 mg/L) and timentin (100 mg/L).
Isolation and Characterization of the Plant Lines
Hypersensitivity to Methyl Methane Sulfonate and X-Rays
Reverse Transcriptase–Mediated PCR Upon request, all novel materials described in this article will be made available in a timely manner for noncommercial research purposes. No restrictions or conditions will be placed on the use of any materials described in this article that would limit their use for noncommercial research purposes.
Accession Number
We thank Hildo Offenberg for the kind gift of the anti-AtMre11 antibody, Haico van Attikum for our many useful discussions, and Peter Hock for his work on the figures. This work was supported by the Stichting Binair Vector Systeem and Framework V European Union project Plantrec (QLRT-2000-01397).
Article, publication date, and citation information can be found at www.plantcell.org/cgi/doi/10.1105/tpc.005959. Received May 30, 2002; accepted July 26, 2002.
Ajimura, M., Leem, S.H., and Ogawa, H. (1993). Identification of new genes required for meiotic recombination in Saccharomyces cerevisiae. Genetics 133, 51–66.[Abstract] Boulton, S.J., and Jackson, S.P. (1998). Components of the Ku-dependent non-homologous end-joining pathway are involved in telomeric length maintenance and telomeric silencing. EMBO J. 17, 1819–1828.[CrossRef][ISI][Medline]
Bressan, D.A., Olivares, H.A., Nelms, B.E., and Petrini, J.H.J. (1998). Alteration of N-terminal phosphoesterase signature motifs inactivates Saccharomyces cerevisiae Mre11. Genetics 150, 591–600.
Bundock, P., van Attikum, H., and Hooykaas, P. (2002). Increased telomere length and hypersensitivity to DNA damaging agents in an Arabidopsis KU70 mutant. Nucleic Acids Res. 30, 1–6. Carney, J.P., Maser, R.S., Olivares, H., Davies, E.M., Le Beau, M., Yates, J.R., Hays, L., Morgan, J.F., and Petrini, J.H. (1998). The hMre11/hRad50 protein complex and Nijmegen breakage syndrome: Linkage of double-strand break repair to the cellular DNA damage response. Cell 93, 477–486.[CrossRef][ISI][Medline]
Chen, C.M., Wang, C.T., and Ho, C.H. (2001a). A plant gene encoding a Myb-like protein that binds telomeric GGTTTAG repeats in vitro. J. Biol. Chem. 276, 16511–16519.
Chen, H.T., et al. (2000). Response to RAG-mediated V(D)J cleavage by NBS1 and Chen, L., Trujillo, K., Ramos, W., Sung, P., and Tomkinson, A.E. (2001b). Promotion of Dnl4-catalyzed DNA end-joining by the Rad50/ Mre11/Xrs2 and Hdf1/Hdf2 complexes. Mol. Cell 8, 1105–1115.[CrossRef][ISI][Medline]
Chin, G.M., and Villeneuve, A.M. (2001). C. elegans mre-11 is required for meiotic recombination and DNA repair but is dispensable for the meiotic G2 DNA damage checkpoint. Genes Dev. 15, 522–534. Clough, S.J., and Bent, A.F. (1998). Floral dip: A simplified method for Agrobacterium-mediated transformation of Arabidopsis thaliana. Plant J. 16, 735–743.[CrossRef][ISI][Medline] D'Adda di Fagagna, F., Hande, M.P., Tong, W.-M., Roth, D., Lansdorp, P.M., Wang, Z.-Q., and Jackson, S.P. (2001). Effects of DNA nonhomologous end-joining factors on telomere length and chromosomal stability in mammalian cells. Curr. Biol. 11, 1192–1196.[CrossRef][ISI][Medline] Daoudal-Cotterell, S., Gallego, M.E., and White, C.I. (2002). The plant Rad50-Mre11 protein complex. FEMS Lett. 516, 164–166.[CrossRef][ISI][Medline] de Jager, M., van Noort, J., van Gent, D.C., Dekker, C., Kanaar, R., and Wyman, C. (2001). Human Rad50/Mre11 is a flexible complex that can tether DNA ends. Mol. Cell 8, 1129–1135.[CrossRef][ISI][Medline] Dolganov, G.M., Maser, R.S., Novikov, A., Tosto, L., Chong, S., Bressan, D.A., and Petrini, J.H.J. (1996). Human Rad50 is physically associated with human Mre11: Identification of a conserved multiprotein complex implicated in recombinational DNA repair. Mol. Cell. Biol. 16, 4832–4841.[Abstract]
Fitzgerald, M.S., Riha, K., Gao, F., Ren, S., McKnight, T.D., and Shippen, D.E. (1999). Disruption of the telomerase catalytic subunit gene from Arabidopsis inactivates telomerase and leads to a slow loss of telomeric DNA. Proc. Natl. Acad. Sci. USA 96, 14813–14818. Furuse, M., Nagase, Y., Tsubouchi, H., Murakami-Murofushi, K., Shibata, T., and Ohta, K. (1998). Distinct roles of two separable in vitro activities of yeast Mre11 in mitotic and meiotic recombination. EMBO J. 17, 6412–6425.[CrossRef][ISI][Medline] Gallego, M.E., Jeanneau, M., Granier, F., Bouchez, D., Bechtold, N., and White, C.I. (2001). Disruption of the Arabidopsis RAD50 gene leads to plant sterility and MMS sensitivity. Plant J. 25, 31–41.[CrossRef][ISI][Medline]
Gallego, M.E., and White, C.I. (2001). RAD50 function is essential for telomere maintenance in Arabidopsis. Proc. Natl. Acad. Sci. USA 98, 1711–1716. Goedecke, W., Eijpe, M., Offenberg, H.H., van Aalderen, M., and Heyting, C. (1999). Mre11 and Ku70 interact in somatic cells, but are differentially expressed in early meiosis. Nat. Genet. 23, 194–198.[CrossRef][ISI][Medline] Haber, J.E. (1998). The many interfaces of Mre11. Cell 95, 583–586.[CrossRef][ISI][Medline] Hartung, F., and Puchta, H. (1999). Isolation of the complete cDNA of the Mre11 homologue of Arabidopsis (accession No. AJ243822) indicates conservation of DNA recombination mechanisms between plants and other eukaryotes. Plant Physiol. 121, 312. Johzuka, K., and Ogawa, H. (1995). Interaction of Mre11 and Rad50: Two proteins required for DNA repair and meiosis-specific double-strand break formation in Saccharomyces cerevisiae. Genetics 139, 1521–1532.[Abstract]
Krysan, P.J., Young, J.C., and Sussman, M.R. (1999). T-DNA as an insertional mutagen in Arabidopsis. Plant Cell 11, 2283–2290.
Maser, R.S., Mirzoeva, O.K., Wells, J., Olivares, H., Williams, B., Zinkel, R.A., Farnham, P.J., and Petrini, J.H. (2001). Mre11 complex and DNA replication: Linkage to E2F and sites of DNA synthesis. Mol. Cell. Biol. 21, 6006–6016. Milne, G.T., Jin, S., Shannon, K.B., and Weaver, D.T. (1996). Mutations in two Ku homologs define a DNA end-joining repair pathway in Saccharomyces cerevisiae. Mol. Cell. Biol. 16, 4189–4198.[Abstract] Moore, D.P., and Orr-Weaver, T.L. (1998). Chromosome segregation during meiosis: Building an unambivalent bivalent. Curr. Top. Dev. Biol. 37, 263–299.[ISI][Medline] Moore, J.K., and Haber, J.E. (1996). Cell cycle and genetic requirements for two pathways of nonhomologous end-joining repair of double-strand breaks in Saccharomyces cerevisiae. Mol. Cell. Biol. 16, 2164–2173.[Abstract]
Moreau, S., Ferguson, J.R., and Symington, L.S. (1999). The nuclease activity of Mre11 is required for meiosis but not for mating type switching, end joining, or telomere maintenance. Mol. Cell. Biol. 19, 556–566. Murashige, T., and Skoog, F. (1962). A revised medium for rapid growth and bioassays with tobacco tissue cultures. Physiol. Plant. 15, 473–497.[CrossRef]
Nairz, K., and Klein, F. (1997). mre11S: A yeast mutation that blocks double-strand-break processing and permits nonhomologous synapsis. Genes Dev. 11, 2272–2290. Nugent, C.I., Bosco, G., Ross, L.O., Evans, S.K., Salinger, A.P., Moore, J.K., Haber, J.E., and Lundblad, V. (1998). Telomere maintenance is dependent on activities required for and repair of double-strand breaks. Curr. Biol. 8, 657–660.[CrossRef][ISI][Medline]
Ohta, K., Nicolas, A., Furuse, M., Nabetani, A., Ogawa, H., and Shibata, T. (1998). Mutations in the MRE11, RAD50, XRS2 and MRE2 genes alter chromatin configuration at meiotic DNA double-stranded break sites in premeiotic and meiotic cells. Proc. Natl. Acad. Sci. USA 95, 646–651. Paull, T.T., and Gellert, M. (1998). The 3' to 5' exonuclease activity of Mre11 facilitates repair of DNA double strand breaks. Mol. Cell 1, 969–980.[CrossRef][ISI][Medline]
Paull, T.T., and Gellert, M. (1999). Nbs1 potentiates ATP-driven DNA unwinding and endonuclease cleavage by the Mre11/Rad50 complex. Genes Dev. 13, 1276–1288.
Porter, S.E., Greenwell, P.W., Ritchie, K.B., and Petes, T.D. (1996). The DNA-binding protein Hdfp1 (a putative Ku homologue) is required for maintaining normal telomere length in Saccharomyces cerevisiae. Nucleic Acids Res. 24, 582–585.
Rhia, K., Fajkus, J., Siroky, J., and Vyskot, B. (1998). Developmental control of telomere lengths and telomerase activity in plants. Plant Cell 10, 1691–1698.
Riha, K., McKnight, T.D., Griffing, L.R., and Shippen, D.E. (2001). Living with genome instability: Plant responses to telomere dysfunction. Science 291, 1797–1800. Riha, K., Watson, J.M., Parkey, J., and Shippen, D.E. (2002). Telomere length deregulation and enhanced sensitivity to genotoxic stress in Arabidopsis mutants deficient in Ku70. EMBO J. 21, 2819–2826.[CrossRef][ISI][Medline] Sharples, G.J., and Leach, D.R. (1995). Structural and functional similarities between the SbcCD proteins of Escherichia coli and the RAD50 and MRE11 (RAD32) recombination and repair proteins of yeast. Mol. Microbiol. 17, 1215–1217.[CrossRef][ISI][Medline]
Smogorzewska, A., van Steensel, B., Bianchi, A., Oelmann, S., Schaefer, M.R., Schnapp, G., and de Lange, T. (2000). Control of human telomere length by TRF1 and TRF2. Mol. Cell. Biol. 20, 1659–1668. Stewart, G.S., Maser, R.S., Stankovic, T., Bressan, D.A., Kaplan, M.I., Jaspers, N.G., Raams, A., Byrd, P.J., Petrini, J.H., and Taylor, A.M. (1999). The DNA double-strand break repair gene hMRE11 is mutated in individuals with an ataxia-telangiectasia-like disorder. Cell 99, 577–587.[CrossRef][ISI][Medline]
Tavassoli, M., Shayeghi, M., Nasim, A., and Watts, F.Z. (1995). Cloning and characterization of the Schizosaccharomyces pombe rad32 gene: A gene required for repair of double strand breaks and recombination. Nucleic Acids Res. 23, 383–388.
Trujillo, K.M., Yuan, S.S., Lee, E.Y., and Sung, P. (1998). Nuclease activities in a complex of human recombination and DNA repair factors Rad50, Mre11 and p95. J. Biol. Chem. 273, 21447–21450.
Tsubouchi, H., and Ogawa, H. (1998). A novel mre11 mutation impairs processing of double strand breaks of DNA during both mitosis and meiosis. Mol. Cell. Biol. 18, 260–268. Usui, T., Ohta, T., Oshiumi, H., Tomizawa, J., Ogawa, H., and Ogawa, T. (1998). Complex formation and functional versatility of Mre11 of budding yeast in recombination. Cell 95, 705–716.[CrossRef][ISI][Medline] van Steensel, B., and de Lange, T. (1997). Control of telomere length by the human telomeric protein TRF1. Nature 385, 740–742.[CrossRef][Medline] Varon, R., et al. (1998). Nibrin, a novel DNA double-strand break repair protein, is mutated in Nijmegen breakage syndrome. Cell 93, 467–476.[CrossRef][ISI][Medline]
Weijers, D., Franke-van Dijk, M., Vencken, R.-J., Quint, A., Hooykaas, P., and Offringa, R. (2001). An Arabidopsis Minute-like phenotype caused by a semi-dominant mutation in a RIBOSOMAL PROTEIN S5 gene. Development 128, 4289–4299.
Wilson, S., Warr, N., Taylor, D.L., and Watts, F.Z. (1999). The role of Schizosaccharomyces pombe Rad32, the Mre11 homologue, and other DNA damage response proteins in non-homologous end joining and telomere length maintenance. Nucleic Acids Res. 27, 2655–2661.
Xiao, Y., and Weaver, D.T. (1997). Conditional gene targeted deletion by Cre recombinase demonstrates the requirement for the double-strand break repair Mre11 protein in murine embryonic stem cells. Nucleic Acids Res. 25, 2985–2991. Yamaguchi-Iwai, Y., Sonoda, E., Sasaki, M.S., Morrison, C., Haraguchi, T., Hiraoka, Y., Yamashita, Y.M., Yagi, T., Takata, M., Price, C., Kakazu, N., and Takeda, S. (1999). Mre11 is essential for the maintenance of chromosomal DNA in vertebrate cells. EMBO J. 18, 6619–6629.[CrossRef][ISI][Medline] Zhu, X.-D., Kuster, B., Mann, M., Petrini, J.H.J., and de Lange, T. (2000). Cell-cycle-regulated association of RAD50/MRE11/NBS1 with TRF2 and human telomeres. Nat. Genet. 25, 347–352.[CrossRef][ISI][Medline] This article has been cited by other articles:
| |||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||
TOP
Abstract
INTRODUCTION
-glucuronidase (GUS) transcription cassettes are shown. The primers JL-202 and XR2 also are shown. LB, left border; RB, right border.
-H2AX. Science 290, 1962–1965.
