AlternativeTranscriptionInitiationSite

Alternative Transcription Initiation Sites and Polyadenylation Sites Are Recruited During Mu Suppression at the rf2a Locus of Maize

http://www.100md.com 《基因杂志》2003年第2期

     ^a Interdepartmental Genetics Program, United States Department of Agriculture-Agricultural Research Servicej&wl, 百拇医药

    ^b Department of Zoology and Genetics, United States Department of Agriculture-Agricultural Research Servicej&wl, 百拇医药

    ^c Department of Agronomy, United States Department of Agriculture-Agricultural Research Servicej&wl, 百拇医药

    ^d Department of Mathematics, United States Department of Agriculture-Agricultural Research Servicej&wl, 百拇医药

    ^e Corn Insects and Crop Genetics Research, United States Department of Agriculture-Agricultural Research Servicej&wl, 百拇医药

    ^f Department of Plant Pathology, Iowa State University, Ames, Iowa 50011j&wl, 百拇医药

    ^g Center for Plant Genomics, Iowa State University, Ames, Iowa 50011j&wl, 百拇医药

    ABSTRACTj&wl, 百拇医药

    Even in the absence of excisional loss of the associated Mutransposons, some Mu-induced mutant alleles of maize can losetheir capacity to condition a mutant phenotype. Three of fiveMu-derived rf2a alleles are susceptible to such Mu suppression.The suppressible rf2a-m9437 allele has a novel Mu transposoninsertion (Mu10) in its 5' untranslated region (UTR). The suppressiblerf2a-m9390 allele has a Mu1 insertion in its 5' UTR. Duringsuppression, alternative transcription initiation sites flankingthe Mu1 transposon yield functional transcripts. The suppressiblerf2a-m8110 allele has an rcy/Mu7 insertion in its 3' UTR. Suppressionof this allele occurs via a previously unreported mechanism;sequences in the terminal inverted repeats of rcy/Mu7 functionas alternative polyadenylation sites such that the suppressedrf2a-m8110 allele yields functional rf2a transcripts. No significantdifferences were observed in the nucleotide compositions ofthese alternative polyadenylation sites as compared with 94other polyadenylation sites from maize genes.

    THERE are two broad categories of DNA transposons, autonomousand nonautonomous. Autonomous transposons encode all nonhostfactors required for their own transposition. In contrast, thetransposition of nonautonomous transposons is dependent uponfactors encoded by autonomous transposons of the same family.Hence, only in the presence of factors encoded by the autonomousSpm/En, Ac, and MuDR maize transposons can the nonautonomousdSpm/I, Ds, and Mu transposons undergo excision and transposition(reviewed by MASSON et al. 1991 ; BENNETZEN et al. 1993 ;BENNETZEN 1996 ; KUNZE 1996 ; FEDOROFF 1999 ). However, bothautonomous and nonautonomous transposons can cause mutationswhen they insert into genes. The Mutator (MuDR/Mu) transposonfamily (ROBERTSON 1978 ) has been widely used for gene mutagenesisand cloning (BENNETZEN et al. 1993 ; BENNETZEN 1996 ). Its4.9-kb autonomous member, MuDR, mediates the transposition ofthe nonautonomous transposons, Mu1–Mu8 (SCHNABLE and PETERSON1986 ; ROBERTSON and STINARD 1989 ; CHOMET et al. 1991 ; HERSHBERGER et al. 1991 ; QIN et al. 1991 ; HSIA and SCHNABLE1996 ). MuDR contains two open reading frames (ORFs), mudrAand mudrB (HERSHBERGER et al. 1991 ; JAMES et al. 1993 ). ThemudrA gene encodes a DNA-binding protein with a region of sequencesimilarity to bacterial transposases (EISEN et al. 1994 ; BENITOand WALBOT 1997 ). The mudrA gene is necessary and sufficientfor somatic excision of Mu transposons (LISCH et al. 1999 ;RAIZADA and WALBOT 2000 ). The mudrB gene may be involved insuppression (DONLIN et al. 1995 ; LISCH et al. 1999 ).

    Many transposon-induced mutants exhibit unstable phenotypesas a result of DNA rearrangements such as excision. In addition,some transposon-induced alleles also exhibit instabilities thatoccur in the absence of DNA rearrangements (MCCLINTOCK 1964, MCCLINTOCK 1967 ; MARTIENSSEN et al. 1989 ). The mechanismsunderlining these phenomena are not well understood.4p8e, 百拇医药

    The loss of a Mu-induced allele's capacity to condition a mutantphenotype is termed Mu suppression. Mu suppression was firstreported at the hcf106::Mu1 mutant allele, which has a Mu1 insertionin its 5' untranslated region (UTR; MARTIENSSEN et al. 1989). In the presence of active MuDR transposons, this allele conditionsa pale-green seedling. In the absence of MuDR, the hcf106::Mu1 allele can condition a nonmutant phenotype that consistsof dark-green "normal" leaf tissue (MARTIENSSEN et al. 1989, MARTIENSSEN et al. 1990 ). In this suppressed state, alternativetranscription initiation sites generate functional hcf106 transcriptsthat are not present in plants that carry active MuDR. Thesealternative transcription initiation sites are in the 5' terminalinverted repeat (TIR) of Mu1 and in regions of the 5' UTR ofthe hcf106 genes that are 3' of the Mu1 insertion site (BARKANand MARTIENSSEN 1991 ).

    Mu suppression has been observed in several other Mu-inducedmutants. Two suppressible Knotted1 (Kn1) alleles arose via Mu1and Mu8 insertions in the junction region of the Kn1-0 repeats.This junction region contains the promoter region of the downstreamcopy of Kn1-0 (LOWE et al. 1992 ). Two other suppressible Kn1alleles, Kn1-mum2 and Kn1-mum7, have Mu8 and Mu1 insertionsin the third intron of the Kn1 locus (GREENE et al. 1994 ).Mu suppression has also been observed with the Les22-7 mutantallele, which has a Mu1 insertion in its 5' UTR (HU et al. 1998), and with the a1-mum2 allele, which carries a Mu1 insertion81 bp upstream of the transcription initiation site (CHOMETet al. 1991 ). Some Lg3 and Rs1 alleles, which have Mu insertionsin 5' UTRs (Lg3-Or422, Lg3-Or102, and Lg3-Or331) or introns(Lg3-Or211 and Rs1-Or11) also exhibit suppression (GIRARD andFREELING 2000 ). Hence, Mu insertions in promoter regions, 5'UTRs, and introns can all generate suppressible alleles.k^@3, 百拇医药

    The hcf106::Mu1 mutation and the genetically unlinked Mu-inducedsuppressible mutation Les28 exhibit coordinated suppressionand reactivation. The suppression of both mutant phenotypesis well correlated with hypermethylation of Mu transposons throughoutthe entire genome and also with hypermethylation of the regionof the hcf106 locus flanking the Mu1 insertion (MARTIENSSENand BARON 1994 ). As is true for hcf106:: Mu1 and Les28, Musuppression of the four Kn1 alleles is correlated with genomewidehypermethylation of Mu transposons (LOWE et al. 1992 ; GREENEet al. 1994 . At least two of these Kn1 alleles (Kn1-mum2 andKn1-mum7) can be reactivated by crossing to Mu-active lines(GREENE et al. 1994 ). Because loss of Mu activity is correlatedwith hypermethylation of Mu transposons (reviewed by CHANDLERand HARDEMAN 1992 ; BENNETZEN et al. 1993 ) and the presenceof MuDR (CHOMET et al. 1991 ), and because expression of the823 amino acids of MURA in transgenic plants is sufficient toresult in demethylation (RAIZADA and WALBOT 2000 ), it is likelythat Mu suppression is caused by an absence of MURA.

    Mu suppression has the potential to complicate efforts to clonegenes via transposon tagging, because a critical step in sucha project is to identify the particular Mu-containing restrictionfragment length polymorphism or PCR fragment responsible fora Mu-induced mutation. This step is generally accomplished byidentifying Mu-containing DNA fragments that cosegregate withthe mutant phenotype through meioses. Because suppressed plantsexhibit a wild-type phenotype even though they carry a Mu transposonin the target gene, suppression can mask the cosegregation betweenthe mutant phenotype and the Mu-containing DNA fragment. Musuppression can also lead to the loss of mutant phenotypes duringbackcrossing programs, which are becoming increasingly importantwith the adoption of new technologies such as RNA profilingand proteomics. These problems can be avoided if these analysesare conducted in an active Mu stock but this restriction limitsthe available genetic backgrounds.], http://www.100md.com

    Mu suppression also impacts technologies, such as Trait UtilitySystem for Corn (BENSEN et al. 1995 ) and Mu rescue (WALBOT1999 ), which are important components of maize functional genomicsprojects. Each of these projects utilizes Mu transposon sequenceas bait to obtain Mu-insertion mutants through reverse geneticsfor functional analysis. This selection strategy does not excludesuppressible mutants, which can condition either mutant or normalphenotypes and thereby complicate the functional analysis oftarget genes. This is a particular concern because Mu transposonsappear to exhibit a strong preference for insertion within the5' UTRs of at least one gene (DIETRICH et al. 2002 ). On theother hand, Mu suppression during somatic development can produceclonal sectors on an unsuppressed background. Such chimericplants provide a unique environment for analyzing mutants (FOWLERet al. 1996 ).

    Therefore, understanding the frequency and mechanisms of Musuppression is critical to using Mu transposons to understandmaize biology. Here we report the identification and characterizationof three Mu-suppressible rf2a alleles. We found that Mu suppressioncan occur not only at alleles caused by Mu insertions in a 5'UTR via the recruitment of alternative transcription initiationsites as reported previously, but also at an allele caused bya Mu insertion in the 3' UTR. Polyadenylation sites within theTIRs of the inserted Mu transposon are recruited during Mu suppressionof this new class of Mu-suppressible alleles. In addition, thesestudies establish that insertions of two additional classesof Mu transposons can generate suppressible alleles.[0an, http://www.100md.com

    MATERIALS AND METHODS[0an, http://www.100md.com

    Alleles of the rf2a gene:[0an, http://www.100md.com

    The rf2a gene (previously designated rf2; SKIBBE et al. 2002) is one of the two complementary restorers of T-cytoplasm malesterility (reviewed by SCHNABLE and WISE 1998 ; WISE et al.1999 ), which encodes a mitochondrial aldehyde dehydrogenase(CUI et al. 1996 ; LIU et al. 2001 ). Plants that carry T cytoplasmand that are homozygous for mutant allels of either rf1 orrf2a are male sterile. All lines used in this study carry Rf1and Rf2a alleles unless otherwise indicated. The reference allele,rf2a-R213, is a spontaneous mutant carried by the inbred linesWf9 and R213. All other described rf2a mutant alleles were isolatedvia transposon tagging experiments (SCHNABLE and WISE 1994 ).Mutant alleles rf2a-m8110, rf2a-m8122, rf2a-m9323, rf2a-m9390,rf2a-m9385, and rf2a-m9437 were all obtained from a Mu-containingpopulation. The wild-type progenitor of rf2a-m8110 and rf2a-m9390is Rf2a-Q67. The progenitor of rf2a-m8122 and rf2a-m9323 isRf2a-Q66. The progenitor of rf2a-m9437 is Rf2a-B79 (CUI et al.1996 ). Each of the rf2a-m alleles used in these experimentswas backcrossed to the inbred line Ky21 for at least three generations.The rf2a-m9385 allele was not included in this study becausean adequate number of backcrosses had not been completed. Therf2a-m8904 allele was isolated from an Spm/En population. Theinbred line B73 has the genotype rf1Rf2a.

    Backcrosses of the rf2a-m alleles:u, 百拇医药

    Plants heterozygous for each rf2a-m allele (rf2a-m/Rf2a) carryingT cytoplasm were crossed as females by the inbred line Ky21.Progeny that carried the rf2a-m alleles were identified by DNAgel blot or PCR analyses. The 1.2-kb partial or 2.2-kb full-lengthrf2a cDNA was used as a hybridization probe against EcoRV- (forrf2a-m9437) or HindIII- (for the rest of the rf2a-m alleles)digested genomic DNA in DNA gel blot analyses. Genotypes ofplants in families segregating for rf2a-m alleles were oftenconfirmed via testcrosses: (T) rf2a-R213/rf2a-R213 x rf2a-m/Rf2a-Ky21(or Rf2a-Ky21/Rf2a-Ky21). Segregation of male-sterile and male-fertileplants (1:1) in the resulting progeny confirmed the presenceof a nonsuppressed rf2a-m allele in a particular male parent.u, 百拇医药

    Male-fertility ratings:u, 百拇医药

    Phenotypes were scored in the morning during the period of pollenshedding for several days according to the rating system ofSCHNABLE and WISE 1994 . Plants were scored as male fertile(F), full fertile, with >90% of the anthers exerted; semifertile("F"), with <90% but more than half of the anthers exerted;semisterile ("S"), with <50% of the anthers exerted (usuallyonly a few percent of anthers exerted); or male sterile (S),completely male sterile with no anthers exerted.

    Mu-active lines:{x, 百拇医药

    Mu-active lines were derived either from the stocks used togenerate the rf2a-m alleles (SCHNABLE and WISE 1994 ) or fromvery similar crosses that also involved Mu stocks and the inbredR213.{x, 百拇医药

    Rf2a genomic clones:{x, 百拇医药

    Two overlapping rf2a-hybridizing genomic clones were obtainedby screening B73 libraries. Both libraries were constructedusing the {lambda} DASHII (Stratagene, La Jolla, CA) vector and wereprepared by Pam Close and John Tossberg, respectively. Libraryscreening conditions were as described by XU et al. 1997 .Phage inserts were subcloned into pBluescript SK or KS (Stratagene)vectors for further analysis or sequencing. Some of these fragmentswere sequenced by utilizing the TN1000 transposon system (GoldBiotechnology, St. Louis, adapted from STRATHMANN et al. 1991). Both DNA strands were completely sequenced unless otherwiseindicated.{x, 百拇医药

    Clone rf2-DNA1 was obtained using a 900-bp probe (DD1, see 1C of CUI et al. 1996 ) that includes the last two introns(9 and 10) and exons (10 and 11) of the rf2a gene. An alignmentof the sequence of the entire 20,072-bp insert of rf2-DNA1 withthe full-length rf2a cDNA (GenBank accession no. ) revealedthat 353 bp from the 5' end of the cDNA clone were not includedin clone rf2-DNA1. Hence, another rf2a genomic clone (rf2-DNA2-65)was isolated from the second B73 genomic library using the full-lengthrf2a cDNA as probe. Sequencing and restriction mapping experimentsrevealed that the two rf2a genomic clones differ in the region5' of exon 2 but not in the region defined by exons 2 and 11.Furthermore, data from PCR amplification of B73 genomic DNAusing various primer pair combinations and genomic mapping viaDNA gel blot analyses indicate that the structure of rf2-DNA2-65,but not of rf2-DNA1, reflects the structure of the Rf2a-B73allele. On the basis of these results we propose that clonerf2-DNA1 is chimeric and contains the region 3' of intron 1derived from the rf2a gene, while the region 5' of intron 1is of unknown origin. Hence, to generate the complete genomicsequence of the Rf2a-B73 allele, 5.2 kb of sequence from the5' end of clone rf2-DNA2-65 was combined with 12.6 kb of sequencefrom the 3' end of clone rf2-DNA1 and deposited in GenBank (accessionno. ).

    fig.ommitteed|vnv6, 百拇医药

    Figure 1. The structure of the rf2a gene (GenBank accession no. ). Solid and open boxes represent coding regions and 5' or 3' UTRs, respectively. Hatched box represents a copia-like retrotransposon, DON QUIXOTE. The positions of the transposon insertions responsible for the indicated alleles are indicated by triangles (not to scale). Solid triangles represent Mu insertions responsible for suppressible alleles. The arrows inside the triangles indicate the orientations of the transposon sequences in GenBank. The position of probe rf2-5m within exon 1 is shown as a bar underneath the 5' UTR. The positions of PCR primers are indicated by arrows. Bm, BamHI; Bg, BglII; Xb, XbaI.|vnv6, 百拇医药

    Mapping transposon insertion sites and identifying Mu transposons:|vnv6, 百拇医药

    The transposon insertion site in the rf2a-m8122 allele was establishedduring the cloning of the rf2a gene (CUI et al. 1996 ). Genomicrestriction mapping was conducted on rf2a-m8110, rf2a-m9323,rf2a-m9390, and rf2a-m9437 alleles using a variety of restrictionenzymes. These DNA gel blots were hybridized with the rf2a-specificprobes rf2-5m, C4-C6, B461-xq, and C1-C2 (see below). Usingthis method, it was possible to map the Mu insertions in threeof the four alleles analyzed (rf2a-m8110, rf2a-m9390, and rf2a-m9437)to specific regions of the rf2a gene.

    PCR reactions were also conducted on DNA from plants homozygousfor each of the rf2a-m alleles to map and to identify Mu transposons.Each PCR reaction included a Mu-TIR primer and one of many primersspecific to the exons of rf2a. Due to the large introns of thisgene, most of these PCR reactions did not yield rf2a-specificproducts. After some of the transposon insertion sites weremapped via genomic restriction mapping, appropriate rf2a-specificprimers were used (RF2C6 for rf2a-m9390 and rf2a-m9437 and RF2C1for rf2a-m8110) to amplify these rf2a-m alleles (1). Inthese instances the transposon insertion sites were physicallymapped via sequence comparisons between the resulting PCR productsand the sequence of the rf2a gene (GenBank accession no. ).The junction between the rf2a and Mu-TIR sequences in thesePCR products defines the Mu insertion site. Because the TIRsof each class of Mu transposon contain diagnostic polymorphisms,it was possible to determine the identities of the Mu transposonsinserted in rf2a-m alleles by comparing the Mu-TIR sequencecontained in the allele-specific PCR products to the TIRs ofall known Mu transposons. In addition, because the sequencesof the two TIRs of most Mu transposons have one or more polymorphismsrelative to each other, the orientations of the Mu insertionsin rf2a-m alleles could also be determined.

    To confirm the identity of the transposon inserted into therf2a-m9390 allele, genomic DNA samples from plants homozygousfor rf2a-m9390 and its progenitor Q67 were digested with EcoRV,HindIII, XbaI, EcoRV + HindIII, EcoRV + XbaI, and HindIII +XbaI and then hybridized with the rf2a-specific probe, rf2-5m.The same filter was stripped (AUSUBEL et al. 1999 ) and hybridizedwith a Mu1-specific probe. In each restriction digest the rf2a-hybridizingfragments were the same size as the Mu1-hybridizing fragments,which provided further support for the conclusion that the transposoninserted into rf2a-m9390 is Mu1.#1z%', http://www.100md.com

    The identity of the rcy/Mu7 transposon in rf2a-m8110 was confirmedsimilarly with the rf2a-specific probe C1-C2 and a rcy/Mu7-specificprobe. To further confirm the identity and orientation of thercy/Mu7 transposon insertion in rf2a-m8110, an rf2a-specificprimer, RF2C2, which is ~ 0.1 kb 3' of the rcy/Mu7 insertion sitein this allele, and an rcy/Mu7 internal primer, Mu7-R, wereused to amplify a 1.7-kb fragment from the 5' end (i.e., therightmost end in 1) of the rcy/Mu7 transposon in rf2a-m8110.This PCR product was subcloned into a pGEM-T vector (Promega,Madison, WI) and >80% was sequenced. Sequence comparisons betweenthis PCR product and rcy/Mu7 (GenBank accession no. )identified only a few nucleotide polymorphisms.

    The transposon insertion in the rf2a-m8904 allele was identifiedby PCR amplification using primers rf2a-3320 and RF2C5UTRR,which flank the transposon insertion. Based on its sequence,this transposon is Ds1 (GenBank accession no. ).xh|fd), 百拇医药

    Probes:xh|fd), 百拇医药

    DNA fragments used as probes in this study were obtained asfollows. The 2.2-kb full-length rf2a cDNA fragment was obtainedfrom plasmid prf273-11 with the restriction enzymes XhoI andEcoRI. The 1.2-kb partial rf2a cDNA was obtained from plasmidprf2a-1.2 with the restriction enzyme EcoRI. Plasmids prf273-11and prf2a-1.2 contain the 1.2-kb and 2.2-kb rf2a cDNAs as describedin CUI et al. 1996 . The rf2a 5' 0.15-kb probe, rf2-5m, wasPCR amplified from plasmid prf273-11 using primers RF2C6 andRF2C8 (1). Another rf2a 5' probe, C4-C6, was PCR amplifiedfrom plasmid prf273-11 using primers RF2C4 and RF2C6. ProbesB461-xq (from 461 to 927 bp in GenBank accession no. )and C1-C2 (from 1374 to 2029 bp in GenBank accession no. )were PCR amplified from plasmid prf273-11 using primers rf2-B461and rf2-xq or primers RF2C1 and RF2C2 (1). A 0.96-kb Mu1-specificfragment was isolated from plasmid pRB1 (ROBERTSON et al. 1988) using the restriction enzyme MluI. The 0.16-kb rcy/Mu7 probewas isolated from plasmid pSB9-in (SCHNABLE et al. 1989 ) usingrestriction enzymes BamHI and EcoRI. Maize GAPDH cDNA (GenBankaccession no. ) was isolated from pGAPDH with the restrictionenzymes EcoRI and HindIII. All probes were labeled with dCTP³²using a random primer labeling protocol (AUSUBEL et al. 1999).

    Genotyping rf2a-m alleles via PCR:w2x), 百拇医药

    To determine which plants in a segregating family carry an rf2a-mallele, PCR amplifications were conducted using a Mu-TIR primerin combination with an appropriate rf2a-specific primer. Variousprimers that anneal to Mu-TIRs, such as XX153, were used inthese PCR reactions. The rf2a-specific primers used for genotypingrf2a-m alleles include RF2C1 (for rf2a-m8110 and rf2a-m8122)and RF2C6 (for rf2a-m9390 and rf2a-m9437; 1). PCR reactionswere performed for 34 cycles as follows: denature at 94°for 40 sec; anneal primers for 40 sec at 55°–58°(depends upon the Mu-TIR primer used); extend at 72° for2 min in the presence of 2.5 units of Taq polymerase (Promega)per reaction.w2x), 百拇医药

    Primer sequences:w2x), 百拇医药

    Mu7-R: 5' TTCTCCGCCGTTGCCATCTC 3^'w2x), 百拇医药

    RF2C1: 5' GCGTCGTTGGTGATCCGTTC3'w2x), 百拇医药

    RF2C2: 5' CCAGGCTAGGGCAAATCTTAT 3'

    RF2C4: 5' AGCGGGAGACGAGCGAGGAC3'n|g62g!, 百拇医药

    RF2C5: 5' ATGCTGCGATTCCGTTTGGTG 3'n|g62g!, 百拇医药

    RF2C6: 5' TCCTCACTCCCACACCAACC3'n|g62g!, 百拇医药

    RF2C8: 5' GCAGCAGGAGAAGCGGCAGGCAG 3'n|g62g!, 百拇医药

    RF2C9: 5' GTGATGGGCTCCTCTACT3'n|g62g!, 百拇医药

    XX153: 5' CGCCTCCATTTCGTCGAATCC 3'n|g62g!, 百拇医药

    rf2-B461: 5' ACAGATCTAAAGCTCCTCATTAAT3'n|g62g!, 百拇医药

    rf2-xq: 5' CCAACTTTCCAGGCATACATCA 3'n|g62g!, 百拇医药

    rf2a-3320: 5' GAGGAACCAGTAGCGGAGGC3'n|g62g!, 百拇医药

    RF2C5UTRR: 5' GCTCCCGTTCGCAGTCG 3'n|g62g!, 百拇医药

    DNA and RNA gel blot analyses:n|g62g!, 百拇医药

    Maize genomic DNA was isolated using a 1x CTAB procedure (SAGHAI-MAROOFet al. 1984 ). About 10 µg of DNA was digested with theindicated restricted enzyme in a 30-µl reaction volumefor >3 hr and then separated via electrophoresis through a 0.8%agarose gel. DNA was transferred to nylon filters (MSI, Westboro,MA) and hybridized with probes labeled with dCTP³² (AUSUBELet al. 1999 ).

    Total RNA from immature tassels (still in the whorl) was isolatedaccording to DEAN et al. 1985 . Approximately 10 µg oftotal RNA was subjected to electrophoresis using a MOPS buffersystem (AUSUBEL et al. 1999 ) and transferred onto Gene-Screenfilters (NEN Research Products, Boston). The filters were hybridizedwith probes labeled with dCTP³² (AUSUBEL et al. 1999 ). Thehybridization density of each band was quantified using a GS-710densitometer (Bio-Rad Laboratories, Hercules, CA).e, 百拇医药

    3' and 5' rapid amplification of cDNA ends:e, 百拇医药

    RNA was isolated from immature tassels (still in the whorl)using the Trizol reagent (GIBCO BRL, Rockville, MD) and treatedwith PCR-grade DNaseI (GIBCO BRL) according to the manufacturer'sinstructions. A total of 5 µg and 100 ng of RNA were usedfor 3' and 5' rapid amplification of cDNA ends (RACE) experiments,respectively, using kits obtained from GIBCO BRL. The rf2a-specificprimers RF2C5 and RF2C9 (1) were used for 3' and 5' RACE,respectively. The position of RF2C9 in exon 2 allows the inadvertentamplification of genomic DNA to be detected. Primer RF2C 4 wasused as a nested primer for the 5' RACE experiments. RACE productswere subcloned into the pGEM-T vector (Promega) and sequenced.

    Analysis of polyadenylation sites:c/, http://www.100md.com

    All GenBank records for which the organism was Zea mays (excludingchloroplast and mitochondrial genes) that had the feature of"polyA_site" were downloaded on March 22, 2000. This data setwas then parsed for the feature of polyadenylation site. Thefew records that lacked sequence data downstream of the reportedpoly(A) site or that had only "A" bases downstream of this sitewere excluded. Only the most recent GenBank submission was usedin those instances of multiple submissions of the same gene.Chi-square homogeneity tests were performed according to STEELand TORRIE 1980 .c/, http://www.100md.com

    RESULTSc/, http://www.100md.com

    Structure of the rf2a gene:c/, http://www.100md.com

    The rf2a cDNA encodes a mitochondrially localized aldehyde dehydrogenase(CUI et al. 1996 ; LIU et al. 2001 ). Two overlapping genomicclones (rf2-DNA1 and rf2-DNA2-65) were obtained by screeningB73 genomic libraries (MATERIALS AND METHODS). Sequence comparisonsof 17.8 kb derived from these genomic clones (GenBank accessionno. ) and the full-length rf2a cDNA clone (GenBankaccession no. ) defined 11 exons and 10 introns (1).The extreme 5' end of the genomic sequence (base positions102–740) is 81.5 and 80.7% identical to the 3' long terminalrepeat (LTR; GenBank accession no. ) and the 5' LTR(GenBank accession no. ) of the maize Milt retrotransposon.In addition, a member of a newly defined class of retrotransposons,DON QUIXOTE, which is present in intron 5 (base positions 6763–13,927of GenBank accession no. ), contains a characteristicnucleic acid binding site that serves as the primer site forreverse transcription and an uninterrupted ORF of ~ 4 kb (positions8335–12,129) that encodes predicted proteins with highdegrees of sequence similarity to the reverse transcriptase,protease, integrase, and endonuclease typical of copia-likeretrotransposons (KONIECZNY et al. 1991 ). A 0.6-kb region thatis ~ 140 bp 5' of exon 2 in rf2-DNA2-65 exhibits 91% sequenceidentity to the LTR of Grande1-4 retrotransposon (GenBank accessionno. ). Two other regions of the rf2a gene (base positions2065–3096, 5' of the transcription initiation site andpositions 4875–5270 in intron 1) exhibit ~ 88 and 85% sequencesimilarity, respectively, to the noncoding regions of variousmaize genes (GenBank accession nos. and These regions of sequence similarity have not beenassigned any putative functions and do not exhibit characteristicsof DNA transposons or retrotransposons.

    Positions of transposons in rf2a-m alleles:g;23, http://www.100md.com

    The positions of transposon insertions responsible for fourof the five Mu-derived rf2a-m alleles (rf2a-m8110, rf2a-m8122,rf2a-m9390, and rf2a-m9437) were mapped via genomic restrictionmapping and sequence comparisons between PCR products obtainedusing rf2a-m DNA templates in conjunction with Mu-TIR- and rf2a-specificprimer pairs and the sequence of the rf2a gene (1). Thespecific class of Mu transposon responsible for each mutantand its orientation were determined via sequence analysis ofthe Mu-TIRs obtained from these PCR products. The rf2a-m9390allele has a Mu1 transposon inserted into its 5' UTR, 105 bp5' of the translation start codon. The identity of this Mu1transposon was confirmed by DNA gel blot analysis (MATERIALSAND METHODS). The rf2a-m9437 allele contains a novel Mu transposoninsertion in its 5' UTR, 35 bp 5' of the translation start codon.The TIR of this transposon differs from all other describedMu transposons. Therefore, this Mu transposon has been designatedMu10 (GenBank accession no. . The rf2a-m8110 allelearose via an rcy/Mu7 insertion in the 3' UTR, 30 bp 3' of thetranslation stop codon. The identity of this rcy/Mu7 transposonwas confirmed by sequence analysis of a 1.7-kb fragment of itand DNA gel blot analyses. The rf2a-m8122 allele has a Mu1 insertionin exon 9 (CUI et al. 1996 ). It has not yet been possible toidentify the molecular lesions associated with the rf2a-m9323and rf2a-m9385 alleles. The rf2a-m8904 allele contains a Ds1transposon a few base pairs downstream of the translation startcodon. This 395-bp Ds1 has three single nucleotide polymorphismsrelative to the Ds1 sequence in GenBank (accession no).

    Reanalysis of data from Schnable and Wise 1994 :&\p%, 百拇医药

    Although one-half of the progeny from the testcross, (T) rf2a-m8110/Rf2ax rf2a-R213/rf2a-R213, would be expected to be male sterile,Schnable and Wise found only 4 of 26 progeny from this crossto be male sterile. A high rate of nonconcordance between themale sterile phenotype and a nearby marker (wx1) was also obtainedfrom a similar testcross but involving rf2a-m9390 allele (SCHNABLEand WISE 1994 ). After the rf2a gene was cloned and the positionsof the Mu insertions responsible for these alleles were determined,genomic DNA samples from these testcross families were genotypedvia PCR (MATERIALS AND METHODS). The results of these analysesare presented in 1. Families segregating for rf2a-m8110(92 2123) and rf2a-m9390 (92 2148) contain three and six male-fertileplants, respectively, with the genotype of rf2a-m/rf2a-R213.Hence, in these families, these two alleles display only 70and 40% penetrance, respectively. In contrast, a similar familybut segregating for the rf2a-m8122 allele, which has a Mu1 insertionin the coding region, exhibited 100% penetrance (family 92 2126in 1). The rf2a-m9323 allele was not included in thesegenotyping experiments, but it has not exhibited low penetrancein the backcrossing program. Another allele, rf2a-m9437 (family92 2153), with a Mu10 insertion in the 5' UTR, also exhibited100% penetrance in this generation. However, after three generationsof backcrossing to the inbred line Ky21, the rf2a-m9437 allelealso began to show evidence of low penetrance (data not shown).These genotyping results establish that the low penetrance observedby SCHNABLE and WISE 1994 does not involve excisional lossof the Mu transposons. Because the rf2a-m8122 allele (whichhas a Mu1 insertion in the coding region) did not exhibit lowpenetrance in otherwise identical crosses (e.g., family 92 2126,1), it is not likely that the low penetrance of thesealleles is conditioned by genetic suppressors (PRELICH 1999) of rf2a carried by the inbred line Ky21.

    fig.ommitteed5, 百拇医药

    Table 1. Comparison of the penetrance of suppressible and nonsuppressible rf2a-m alleles5, 百拇医药

    Reactivation of rf2a-m alleles:5, 百拇医药

    Because these three alleles (rf2a-m8110, rf2a-m9390, and rf2a-m9437)all have a transposon insertion in an UTR, this low penetrancecould reflect Mu suppression, which occurs when a genome lacksMu activity (MARTIENSSEN et al. 1989 ). One of the hallmarksof Mu suppression is the possibility of reactivation, wherebysuppressed Mu-induced alleles are reactivated by the reintroductionof Mu activity via genetic crosses. To determine whether rf2a-m8110and/or rf2a-m9390 can be reactivated (and thereby again conditionmutant phenotypes), stocks carrying suppressed versions of thesealleles were crossed to Mu-active lines. To minimize the confoundingeffects of genetic backgrounds, the Mu-active lines used inthese crosses were closely related to the lines used for generatingthe rf2a-m alleles (SCHNABLE and WISE 1994 ). As a control,some male-fertile plants that carried suppressed versions ofthese two alleles were self-pollinated. No male-sterile plantsappeared in the resulting progenies (96g 6104-05 and 98 6336in 2). In contrast, various rates of reactivation (asdetermined by the frequency of male-sterile progeny) were obtainedin the crosses with Mu stocks (2). Hence these rf2a-malleles can be reactivated via crosses to active Mu lines. Thisresult is consistent with the hypothesis that the low penetranceof these alleles is due to Mu suppression.

    fig.ommitteedxf.{l, 百拇医药

    Table 2. Reactivation of suppressed rf2a-m allelesxf.{l, 百拇医药

    The stability of the reactivation of rf2a-m8110 was tested bycrossing a reactivated (i.e., male sterile) heterozygous plant,(T) rf2a-m8110/rf2a-R213, by (N) rf2a-m8904/rf2a-m8904. Therf2a-m8904 allele was used for this cross instead of rf2a-R213because unlike rf2a-R213 it does not accumulate a detectableamount of rf2a mRNA (CUI et al. 1996 ). About 100 of the resultingprogeny were scored for male fertility (data not shown). Mostwere male sterile. Of 16 randomly selected male-sterile plants,7 carried the rf2a-m8110 allele. Hence, rf2a-m8110 can be transmittedthrough meiosis in the reactivated state.xf.{l, 百拇医药

    Because the rf2a-m9390 allele became suppressed early in thebackcrossing program, male-sterile plants homozygous for rf2a-m9390were not initially available for mRNA accumulation analyses.To generate unsuppressed stocks homozygous for this allele,some unsuppressed heterozygous plants, (T) rf2a-m9390/rf2a-R213from an early generation, were crossed by suppressed (i.e.,male fertile) plants with the genotype (T) rf2a-m9390/rf2a-m9390.About 300 progeny were screened for male-sterile (i.e., unsuppressed)plants. Only 19 were obtained. When these 19 plants were genotyped,it was found that they all had the genotype rf2a-m9390/rf2a-R213;i.e., no male-sterile rf2a-m9390 homozygous plants were obtained.The reason for this unbalanced result is not known.

    Methylation and Mu suppression of rf2a-m9390:a:, http://www.100md.com

    There is a good correlation between the methylation of Mu-TIRsand Mu activity (reviewed by BENNETZEN 1996 ). In previouslyreported studies of Mu suppression, hypermethylation of Mu transposonsthroughout the genome was generally correlated with Mu suppression,although exceptions were found (MARTIENSSEN et al. 1990 ; LOWEet al. 1992 ). To further test whether the low penetrance ofrf2a-m9390 is due to Mu suppression, the methylation statusof Mu1 elements in the genome was determined via DNA gel blothybridization following HinfI digestion (2C; CHANDLER andWALBOT 1986 ). Mu1 elements with hypomethylated HinfI sites(which are therefore susceptible to restriction digestion) intheir TIRs will yield Mu1-hybridizing fragments of 1.34 kb.In contrast, Mu1 elements with methylated HinfI sites will yieldlarger hybridizing fragments (2C). Although the Mu1 probecan also cross-hybridize with Mu2 transposons, there were fewMu2 transposons in the families analyzed in this study. Theresults obtained using genomic DNA isolated from young leavesof plants carrying rf2a-m9390 are summarized in 3. Allmale-sterile (i.e., not suppressed) and semisterile ("S," partiallysuppressed) plants in families segregating for recently reactivatedrf2a-m9390 (families 96 2209, 96 2214, and 96 2218) from thereactivation experiment contained mostly hypomethylated Mu1elements (3). Of the 13 analyzed fertile (i.e., suppressed)plants, 11 contained completely or mostly methylated Mu1 elements;the two exceptions contained both methylated and hypomethylatedelements. Examples of these analyses are shown in 2A. Generally,fertile (i.e., suppressed) plants exhibited a higher degreeof methylation than did sterile (i.e., not suppressed) plants.A chi-square homogeneity test showed that the ratios of 0 methylated:4hypomethylated male-sterile plants vs. the 11 methylated:2 hypomethylatedfertile plants are significantly different ({chi} ² = 9.59). Thisresult is consistent with the hypothesis that the low penetranceof rf2a-m9390 is due to Mu suppression. Interestingly, plantsfrom a family (family 92 2148) that had just begun to show suppressionafter outcrossing to inbred lines exhibited a higher level ofMu methylation in general (3) than did plants from thereactivated families.

    fig.ommitteed7iw4r, http://www.100md.com

    Figure 2. Methylation status in suppressed and nonsuppressed plants with the genotype rf2a-m9390/rf2a-R213. DNA isolated from young leaves of plants from families 96 2209 and 96 2214 was digested with HinfI. (A) DNA gel blot was hybridized with the Mu1-specific probe illustrated in C. (B) The same blot was stripped and hybridized with the rf2a-specific probe rf2-5m (C). (C) The Mu1 insertion and HinfI sites in the rf2a-m9390 allele. All plants carry T cytoplasm and their phenotypes are indicated as F, fully male fertile, and S, completely male sterile with no anthers exerted. H, HinfI; distances between restriction sites are indicated in kilobases.7iw4r, http://www.100md.com

    fig.ommitteed7iw4r, http://www.100md.com

    Table 3. Correlation between male fertility of rf2a-m9390/rf2a-R213 plants and the methylation status of Mu1 transposons within their genomes and within rf2a-m93907iw4r, http://www.100md.com

    MARTIENSSEN et al. 1990 reported that suppression is alsocorrelated with hypermethylation of the Mu1 transposon insertedin the hcf106::Mu1 allele. To detect the methylation statusof the Mu1 insertion in rf2a-m9390, an rf2a probe (rf2-5m),was hybridized to HinfI-digested genomic DNA from the segregatingprogenies (the results are shown in 3). This probe hybridizesto a 1.1-kb fragment bounded by the HinfI site 5' of the probein the rf2a promoter region and by the HinfI site in the 3'TIR (i.e., leftmost end in 2C) of the Mu1 transposon. Themethylation status of the Mu1 inserted in rf2a-m9390 was scoredby determining the signal strength of the 1.1-kb rf2a-hybridizingfragment relative to the 2.4- and 2.8-kb rf2a-hybridizing fragments.If the 3' HinfI site in the Mu1 transposon is susceptible toHinfI digestion (i.e., if it is hypomethylated), a 1.1-kb rf2a-hybridizingfragment will be detected (e.g., the lanes of "S" in 2B).If this site is not susceptible to HinfI digestion (i.e., ifit is methylated), either the 2.4-kb (the 5' HinfI site in theMu1 transposon is digested) or the 2.8-kb (neither of the twoHinfI sites in the Mu1 transposon is digested) rf2a-hybridizingfragment will be detected (e.g., the "F" category in 2B).A strong correlation was observed between the methylation statusof the Mu1 transposon in rf2a-m9390 and the methylation statusof other Mu1 transposons in the genome (compare A and B in 2).

    Accumulation of rf2a mRNA in plants homozygous for suppressed rf2a-m alleles:l:4}j], 百拇医药

    Prior RNA gel blot analysis identified a plant homozygous forrf2a-m9390 that accumulated rf2a mRNA at the same level as wild-typeplants (CUI et al. 1996 ). Because the entire young tassel ofthis plant had been collected for RNA in that study, the malefertility status of this plant could not be determined. To overcomethis problem in subsequent experiments, only a few branchesof each young tassel were collected from plants homozygous forthe rf2a-m9390 or rf2a-m8110 alleles. An RNA gel blot analysisof these individuals is shown in 3. Hybridization witha full-length rf2a cDNA detected an mRNA that accumulated tothe same or only slightly lower levels in fertile plants (i.e.,suppressed) that were homozygous for either rf2a-m8110 or rf2a-m9390as accumulated in wild-type controls. In addition, at the levelof resolution provided by RNA gel blot analyses, these mRNAswere indistinguishable in size from those that accumulated inthe wild-type controls.

    fig.ommitteedqmz, 百拇医药

    Figure 3. The accumulation of rf2a mRNA in many suppressed plants is as high as or only slightly lower than that in wild type. An RNA gel blot containing RNA isolated from young tassels of the indicated genotypes was hybridized with a full-length rf2a cDNA probe (A) and the loading control maize GAPDH (B). The density of each band was quantified using a GS-710 densitometer (Bio-Rad Laboratories). The density ratio of each band in A to its corresponding band in B is listed below B. All plants were homozygous for the indicated rf2a alleles unless otherwise noted. The inbred line Q67 is homozygous for the wild-type progenitor (Rf2a-Q67) of rf2a-m8110 and rf2a-m9390. (T), T cytoplasm; (N), N cytoplasm. The male fertility phenotypes were denoted unless unavailable. F, fertile; "F," semifertile.qmz, 百拇医药

    Native transcription initiation sites are not used in suppressed rf2a-m9390 plants:qmz, 百拇医药

    Because the rf2a-m9390 allele contains a Mu1 insertion in its5' UTR, the rf2a transcripts that accumulate in the suppressedrf2a-m9390 plants (3) could be derived from alternativetranscription initiation sites downstream of the native sites(i.e., in Mu1 and/or in its flanking region) as has been reportedfor hcf106::Mu1 (BARKAN and MARTIENSSEN 1991 ). Alternatively,these transcripts could arise via readthrough transcriptionof the Mu1 transposon followed by the splicing of the Mu1 fromthe transcripts. To distinguish between these two possibilities,a probe (rf2-5m) upstream of the Mu1 transposon (1) washybridized to RNA from suppressed plants homozygous for rf2a-m9390.The results of this experiment are shown in 4. Becauserf2a-m9390 transcripts could not be detected with the rf2-5mprobe (4B), it can be concluded that transcription initiationin suppressed rf2a-m9390 does not occur from the native transcriptioninitiation sites of rf2a. Instead, transcription of this allele(4A) must initiate downstream of the position of probe rf2-5m(1), likely from the 5' TIR (i.e., the rightmost TIR in1) of Mu1 and/or of an rf2a flanking region.

    fig.ommitteedmx0, 百拇医药

    Figure 4. RNA gel blot analysis reveals that the suppressed rf2a-m9390 allele does not utilize native transcription initiation sites. About 10 µg of RNA from young tassels was loaded in each lane. Full-length rf2a cDNA (A) and rf2-5m, a 5' fragment (see 1) of the rf2a gene (B), were used as hybridization probes. All plants were homozygous for the indicated alleles.mx0, 百拇医药

    Transcription initiation sites in rf2a-m9390:mx0, 百拇医药

    Initially 5' RACE experiments were conducted on RNA extractedfrom the inbred line Q67, which is homozygous for the wild-typeprogenitor of rf2a-m9390 (CUI et al. 1996 ). The primer (RF2C9)used for the first-strand synthesis was located at position+182 relative to the start of translation and the nested primer(RF2C4) was located at position +37. DNA gel blot analysis revealedthat the resulting RACE products were ~ 290 bp, a result thatis consistent with the size of the longest rf2a cDNA clone isolatedto date (prf273-11), which begins at position -253. Cloned 5'RACE products obtained using RNA extracted from a plant homozygousfor suppressed rf2a-m9390 were considerably smaller than thoseobtained from the inbred line Q67. Sequence analysis of nineof the RACE products from rf2a-m9390 revealed multiple transcriptioninitiation sites, all of which were located between the positionof the Mu1 insertion (-105) and the translation start codon(5). This result is similar to what has been observed duringsuppression of hcf106::Mu1 (BARKAN and MARTIENSSEN 1991 ).

    fig.ommitteed7g@+, 百拇医药

    Figure 5. Alternative transcription initiation sites in the suppressed rf2a-m9390 allele. The open and solid boxes indicate the 5' UTR and coding regions of exons 1 and 2, respectively. Horizontal arrows indicate the primers used for the 5' RACE experiments. Sequence is provided for the rf2a 5' UTR and the beginning of the coding region. The translation start codon is boxed. The triangles indicate the position of the Mu1 insertion in rf2a-m9390. The vertical arrows indicate the transcription initiation sites revealed by 5' RACE using tassel RNA from a male-fertile plant homozygous for the rf2a-m9390 allele. The number of clones (if there are multiple clones) isolated with each initiation site is indicated above the arrows. Alternative transcription initiation sites are designated by roman numerals.7g@+, 百拇医药

    Alternative polyadenylation sites in the TIR of rcy/Mu7 are used during suppression of rf2a-m8110:7g@+, 百拇医药

    The rf2a-m8110 allele contains an rcy/Mu7 insertion in its 3'UTR. As is true for rf2a-m9390, suppressed plants homozygousfor rf2a-m8110 accumulate rf2a mRNA that is indistinguishablefrom wild type by RNA gel blot analyses (3). On the basisof the analysis of cDNA clones, two Rf2a alleles (Rf2a-B73 andRf2a-W22) use polyadenylation sites >140 bp 3' of the site ofthe rcy/Mu7 insertion in the rf2a-m8110 allele (6). In addition,3' RACE experiments have established that this is also truefor the Rf2a-Q67 allele, which is the wild-type progenitor ofrf2a-m8110 (6). These results indicate that the rf2a-m8110allele either uses the native polyadenylation sites but withthe rcy/Mu7 transposon subsequently spliced out or uses alternativepolyadenylation sites. 3' RACE was used to identify the polyadenylationsites used by suppressed rf2a-m8110 and to thereby distinguishbetween these two possibilities. As shown in 6, five alternativepolyadenylation sites were detected in two independent 3' RACEexperiments. Some sites were recovered in both experiments.All identified sites are within the 3' TIR (i.e., leftmost TIRin 6) of the rcy/Mu7 transposon insertion in rf2a-m8110.

    fig.ommitteed6, http://www.100md.com

    Figure 6. Polyadenylation sites used in suppressed rf2a-m8110 plants and in wild-type Rf2a plants. The solid and open boxes indicate the translated and 3' UTR regions of the last exon of the rf2a gene, respectively. The triangle represents the rcy/Mu7 transposon insertion responsible for the rf2a-m8110 mutation. The two hatched boxes containing horizontal arrows represent the TIRs of the rcy/Mu7 transposon. The vertical arrows above the TIRs indicate the polyadenylation sites used in the suppressed plants as revealed by 3' RACE experiments. Each arrow represents one event unless otherwise indicated. The solid and dashed arrows indicate the events revealed in the first and the second 3' RACE experiments, respectively. The primer used in the 3' RACE experiment is indicated as a horizontal arrow labeled as RF2C5. The rcy/Mu7 TIR sequence in which the polyadenylation sites were revealed is shown above the transposon. The 3' UTR sequence of Rf2a-B73 is shown below. The arrows below the gene structure represent the polyadenylation sites used by the Rf2a-B73 (solid arrows), Rf2a-W22 (shaded arrowhead), and Rf2a-Q67 (dashed arrows) alleles as determined by sequence analysis of cDNA clones (B73 and W22) or 3' RACE (Q67). Polyadenylation sites are designated by roman numerals. The translation stop codon, TAG, is boxed. The AAUAAA-like PE elements are shaded. U-rich regions flanking polyadenylation sites are underlined.

    Polyadenylation sites are preferentially located at the 3' endof a YA (i.e., UA, CA, or GA) sequence in at least some eukaryotes(reviewed by ROTHNIE 1996 ; WAHLE and RUEGSEGGER 1999 ). Todetermine whether this pattern holds for maize, the polyadenylationsites associated with Z. mays records in GenBank were examined.Fifty-eight records with a total of 94 polyadenylation siteswere obtained. Of these 94 sites, 73 fit the YA rule (4).Similarly, 6 of the 7 polyadenylation sites within the 3'UTR of the rf2a gene are YA. In contrast, only 2 of the 5 alternativepolyadenylation sites within rcy/Mu7 (GA, GA, UC, AC, and CC)fit this pattern. A ² homogeneity test (² = 3.67) indicatedthat the rate of YA polyadenylation sites in rcy/Mu7 at the95% confidence level is not significantly different from thatin other maize genes.08s][h5, http://www.100md.com

    fig.ommitteed08s][h5, http://www.100md.com

    Table 4. Summary of 94 polyadenylation sites from 58 maize genes in GenBank08s][h5, http://www.100md.com

    DISCUSSION1!yd, 百拇医药

    Mu suppression occurs at a high frequency:1!yd, 百拇医药

    Mu transposons are widely used for the functional analysis ofthe maize genome, including gene tagging, gene discovery, andreverse genetics. It has been known for over a decade that inthe absence of Mu activity, some Mu-insertion alleles lose thecapacity to condition a mutant phenotype (MARTIENSSEN et al.1989). This phenomenon, Mu suppression, has important implicationsfor the use of Mu transposons in understanding maize biology.1!yd, 百拇医药

    Of the thousands of mutant alleles derived from Mu stocks, only12 have been described as suppressible (MARTIENSSEN et al. 1990; CHOMET et al. 1991; GREENE et al. 1994 ; HU et al. 1998; GIRARD and FREELING 2000 ). These suppressible alleles arosevia Mu insertion into promoters (3 alleles), 5' UTRs (5), andintrons (4). The low rate at which suppressible alleles havebeen described probably underestimates the rate at which theyarise. This is because many suppressible alleles are likelyto have been incorrectly characterized as not transmissible/heritableand were therefore not further analyzed. Consistent with thishypothesis, we found that 65 of 75 Mu insertions in the glossy8gene were in the promoter or in the 5' UTR and are thereforepotentially suppressible (DIETRICH et al. 2002 ).

    In this study a collection of five Mu-derived rf2a mutant allelesoriginally obtained via a phenotypic screen was backcrossedto a non-Mu inbred line (Ky21) for at least three generations.Two alleles (rf2a-m9390 and rf2a-m8110) with Mu insertions innoncoding regions exhibited low penetrance early in this backcrossingprogram. A third allele, rf2a-m9437, exhibited low penetrancein later generations (data not shown). The low penetrance ofthese three alleles is not the result of DNA rearrangementsand at least rf2a-m8110 and rf2a-m9390 can be reactivated bythe introduction of Mu activity. The Mu1 transposon in rf2a-m9390is methylated in fertile plants, further confirming the relationshipbetween the low penetrance and the absence of Mu activity. Furthermore,on the basis of its low penetrance and Mu insertion site, rf2a-m9437is also likely to be a suppressible allele. Thus three of thefive Mu-insertion alleles analyzed appear to be Mu suppressible.Hence, it is clear that Mu-suppressible alleles arise frequentlyenough to seriously impact the outcome of genetic experiments.In retrospect, suppression probably accounts for our lack ofsuccess in identifying a Mu-containing DNA fragment that cosegregatedwith any of the five Mu-induced rf2a alleles except rf2a-m8122(CUI et al. 1996 ). An even greater proportion of suppressiblealleles are likely to be recovered by reverse genetic screens(e.g., DIETRICH et al. 2002 ), because such alleles would nothave been prescreened by phenotypic selection as was true forthis collection of rf2a-m alleles.

    It has previously been established that the insertion of Mutransposons into promoter regions, 5' UTRs, and introns cangenerate suppressible alleles. By determining the structureof the Rf2a-B73 allele and the insertion sites of the Mu transposonsresponsible for four of five rf2a-m alleles, this study notonly identified two suppressible alleles with Mu insertionsin the 5' UTR of the rf2a gene (rf2a-m9390 and rf2a-m9437),but also for the first time demonstrated that a Mu insertioninto a 3' UTR can result in a suppressible allele (rf2a-m8110).Only the apparently nonsuppressible rf2a-m8122 allele arosevia a Mu insertion in an exon..', 百拇医药

    The Rf2a-B73 allele spans >17 kb (1) and contains many smallexons and introns as well as two large introns (the largestof which is >7 kb). It is worth noting that if a reverse geneticscreen that depends upon PCR-based detection of Mu insertions(BENSEN et al. 1995 ) were to be conducted on the rf2a gene,it is likely that most of the rf2a-m alleles described in thisreport would have been missed. This is because as a result ofthe presence of two large introns, only rf2a primers from asmall portion of the gene can amplify the rf2a-m alleles. Forexample, Mu- and rf2a-specific (such as RF2C6, 1) primersfrom the 5' end of the rf2a gene fail to amplify DNA templatesfrom plants that carry rf2a-m8122 or rf2a-m8110 (data not shown).Similarly, under all PCR conditions tested, Mu and rf2a primersfrom the 3' end of the gene fail to amplify DNA from plantsthat carry rf2a-m9390 and rf2a-m9437. Instead, such a reversegenetic screen would most likely identify Mu insertions in intronsthat would be unlikely to confer a mutant phenotype. These resultspoint to the importance of having a gene structure availablebefore performing reverse genetics and/or using a large numberof primer pairs when conducting reverse genetic screens in speciessuch as maize, which may have large introns.

    Suppressible alleles described previously arose via the insertionof a variety of Mu transposons: Mu1, Mu3, Mu8, and MuDR deletionderivatives (BARKAN and MARTIENSSEN 1991 ; LOWE et al. 1992; GREENE et al. 1994 ; HU et al. 1998 ; GIRARD and FREELING2000 ). Three rf2a-m-suppressible alleles, rf2a-m9390, rf2a-m8110,and rf2a-m9437, are Mu1-, rcy/Mu7-, and Mu10-induced, respectively.These results indicate that insertions of at least six differentclasses of Mu transposons can generate suppressible alleles.n-m/ao, http://www.100md.com

    Mu suppression occurs to alleles that have a Mu insertion in the 5' UTR:n-m/ao, http://www.100md.com

    Three mutant alleles that arose via Mu transposon insertionsin 5' UTRs recruit alternative transcription initiation sitesduring suppression. The hcf106::Mu1, Lg3-Or422, and rf2a-m9390alleles have Mu1, Mu3, and Mu1 insertions at positions -34 (BARKANand MARTIENSSEN 1991 ), -238 (GIRARD and FREELING 2000 ), and-105 relative to the presumed translation start codons, respectively.The alternative transcription sites recruited during suppressionof hcf106::Mu1 and rf2a-m9390 exhibit a significant differencein relation to their Mu1 insertions. In the suppressed hcf106::Mu1allele, alternative transcription sites are recruited both fromthe downstream TIR of the inserted Mu1 transposon and from theregion of the 5' UTR that is 3' of this Mu1 insertion. In contrast,all of the transcription initiation sites recruited during suppressionof rf2a-m9390 are located 3' of the Mu1 insertion; i.e., thereis no evidence that this allele recruits transcription initiationsites from within Mu1. This difference is not due to the orientationof the transposons; the Mu1 transposons responsible for thehcf106::Mu1 allele and the rf2a-m9390 allele are inserted inthe same relative orientation. However, the positions of allthese alternative transcription initiation sites are similarrelative to the presumed translation start sites: hcf106::Mu1uses positions -7 to -80 and rf2a-m9390 uses positions -6 to-91. This observation suggests that there may be a downstreamcis-acting signal that interacts with the promoter to determinethe locations of transcription initiation sites.

    The rf2a-m9437 allele also arose via a Mu insertion in the 5'UTR. Unlike rf2a-m9390, which exhibited evidence of suppressionvery early in the backcrossing program, rf2a-m9437 did not beginto exhibit evidence of suppression until after three generationsof backcrossing to the inbred line Ky21 (1 and data notshown). Interestingly, the position of the Mu10 insertion responsiblefor rf2a-m9437 (base pair -35 relative to the presumed translationstart codon) precludes the use of all but one of the alternativetranscription initiation sites used by rf2a-m9390.m, http://www.100md.com

    Mu suppression affects an allele that has a Mu insertion in its 3' UTR:m, http://www.100md.com

    Analysis of rf2a-m8110 revealed a novel mechanism of Mu suppression.This allele has an rcy/Mu7 transposon insertion 30 bp downstreamof the stop codon in the 3' UTR. Sequence analysis of cloned3' RACE products revealed that during suppression the rf2a-m8110allele recruits novel polyadenylation sites from within theTIR of the rcy/Mu7 transposon. This is the first report thatrcy/Mu7 contains polyadenylation sites. Because the TIRs ofthe 10 classes of Mu transposons are well conserved, analysisof the rf2a-m8110 allele suggests that the recruitment of alternativepolyadenylation sites might be a general mechanism by whichmutants containing other classes of Mu insertions in their 3'UTRs could be suppressed. This is similar to the finding thatthe long terminal repeats of retroviruses can provide polyadenylationsites for human cellular transcripts (MAGER et al. 1999 ; BAUSTet al. 2000 ). Thus, the TIRs of Mu transposon may serve aspolyadenylation sites for maize genes and thereby contributeto the generation of genetic diversity.

    Polyadenylation sites in Mu1 were identified previously followingthe analysis of truncated transcripts produced by the adh1-s3034allele, which contains a Mu1 insertion in its first intron (ORTIZand STROMMER 1990 ). However, these alternative polyadenylationsites differ from those in the current report in that they arelocated in the central (i.e., non-TIR) region and the 3' TIRof the Mu1 transposon.#)%., http://www.100md.com

    In eukaryotes, polyadenylation occurs following the cleavageof the hnRNA, which produces a 3' -OH. The positions at whichcleavage, and hence polyadenylation, occur are controlled bycis-acting elements that are usually located between the stopcodon and the cleavage site. In mammals, the polyadenylationsignals consist of the AAUAAA positioning element (PE) and theU- or UG-rich downstream element (DE; WAHLE and RUEGSEGGER1999 ; ZHAO et al. 1999 ). Plant and yeast genes contain AAUAAA-likePEs and U- or UG-rich upstream elements (UEs), which resemblethe DEs of mammals (reviewed by ROTHNIE 1996 ; HUNT and MESSING1998 ; WAHLE and RUEGSEGGER 1999 ). In addition, the polyadenylationsites of rice and Arabidopsis genes are often located in U-richregions (GRABER et al. 999 ).

    Seven polyadenylation sites were detected in Rf2a alleles (VI–XIIin 6). Each of these sites is 20–50 bases downstreamof an AAUAAA-like PE and in the vicinity of a U-rich flankingregion (each ~ 50% U). No obvious UE was detected in the rf2agene. Similarly, all five polyadenylation sites in the TIR ofrcy/Mu7 (I–V in 6) are located in the vicinity ofU-rich regions and 20–50 bp downstream of one of the threeAAUAAA-like PE elements that exist in this TIR.0c$h:9-, 百拇医药

    The fact that only the TIR polyadenylation sites are used insuppressed rf2a-m8110 plants indicates either that transcriptiondoes not proceed through the rcy/Mu7 transposon to the nativepolyadenylation sites or that the TIR sites are preferred overthe native sites by the polyadenylation machinery. One hypothesisto explain such a preference would be the presence of an as-yet-unidentifiedpolyadenylation signal upstream of the position of the rcy/Mu7insertion. The spatial separation between this upstream signaland the native sites caused by the 2.2-kb rcy/Mu7 insertionin the rf2a-m8110 allele might cause such an upstream signalto interact more efficiently with the nearby TIR sites thanwith the native sites.

    In vitro and in vivo polyadenylation experiments demonstratedthat cleavage occurs preferentially at the 3' end of a YA (i.e.,UA, CA, or GA) sequence (reviewed by ROTHNIE 1996 ; WAHLEand RUEGSEGGER 1999 ). In mammals, this YA consensus was observedin ~ 70 of 100 polyadenylation sites (SHEETS et al. 1990 ). YAwas also found to be the most frequent sequence at the polyadenylationsites in the yeast cyc1 gene (GUO and SHERMAN 1995 ) and severalplant genes (WU et al. 1995 ). Our analysis of 94 polyadenylationsites from 58 maize genes confirmed that this rule also holdsfor maize; 73 of 94 polyadenylation sites fit the YA pattern(4). In contrast, only 2 of 5 polyadenylation sites inthe TIR of the rcy/Mu7 transposon inserted into rf2a-m8110 followthis rule. In mammals, the preferred bases at the first positionof the YA consensus are C >> U > G, where C accounts for ~ 60%of sites (SHEETS et al. 1990 ). In contrast, UA is most common(45%) among maize polyadenylation sites.e\(, 百拇医药

    ACKNOWLEDGMENTS

    We thank Ms. Weijun Chen for assistance in sequencing the rf2-DNA1genomic clone; Steve Briggs, who, while at Pioneer Hi-Bred International,provided the two B73 genomic libraries; and Alfons Gierl (TechnischeUniversitat, Munchen, Germany) for the GAPDH clone. This researchwas partially supported by a USDA/NRI grant (9600804) to P.S.S.and R.P.W., USDA/NRI grants (98001805, 0001478, 0201414) toP.S.S., a Human Frontiers in Science program grant (RG0067)to Cris Kuhlemeier (Institute of Plant Physiology, Universityof Berne, Switzerland) and P.S.S., a National Science Foundationgrant (DBI-9975868) to P.S.S. and D.A., and Hatch Act and Stateof Iowa funds. This is journal paper no. J-18707 of the IowaAgriculture and Home Economics Experiment Station (Ames, IA);project numbers are 3368, 3390, 3485, and 3554.wow6#l, 百拇医药

    Manuscript received March 1, 2002; Accepted for publication November 4, 2002.wow6#l, 百拇医药

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