A Novel Chromodomain Protein, Pdd3p, Associates with Internal Eliminated Sequences during Macronuclear Development in Tetrahymena thermophila

doi:10.1128/MCB.20.11.4128-4134.2000

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Molecular and Cellular Biology, June 2000, p. 4128-4134, Vol. 20, No. 11
0270-7306/00/$04.00+0
Copyright © 2000, American Society for Microbiology. All rights reserved.

A Novel Chromodomain Protein, Pdd3p, Associates with Internal Eliminated Sequences during Macronuclear Development in Tetrahymena thermophila

Mikhail A. Nikiforov, Martin A. Gorovsky, and C. David Allis^*

Department of Biology, University of Rochester, Rochester, New York 14627

Received 1 December 1999/Returned for modification 3 January 2000/Accepted 3 March 2000

	ABSTRACT

Top Abstract Introduction Materials and Methods Results Discussion References

Conversion of the germ line micronuclear genome into the genome of a somatic macronucleus in Tetrahymena thermophila requiresseveral DNA rearrangement processes. These include (i) excisionand subsequent elimination of several thousand internal eliminatedsequences (IESs) scattered throughout the micronuclear genomeand (ii) breakage of the micronuclear chromosomes into hundredsof DNA fragments, followed by de novo telomere addition to theirends. Chromosome breakage sequences (Cbs) that determine the sitesof breakage and short regions of DNA adjacent to them are alsoeliminated. Both processes occur concomitantly in the developingmacronucleus. Two stage-specific protein factors involved in germline DNA elimination have been described previously. Pdd1p andPdd2p (for programmed DNA degradation) physically associate withinternal eliminated sequences in transient electron-dense structuresin the developing macronucleus. Here, we report the purification,sequence analysis, and characterization of Pdd3p, a novel developmentallyregulated, chromodomain-containing polypeptide. Pdd3p colocalizeswith Pdd1p in the peripheral regions of DNA elimination structures,but is also found more internally. DNA cross-linked and immunoprecipitatedwith Pdd1p- or Pdd3p-specific antibodies is enriched in IESs,but not Cbs, suggesting that different protein factors are involvedin elimination of these two groups ofsequences.

	INTRODUCTION

Top Abstract Introduction Materials and Methods Results Discussion References

Developmentally programmed excision and subsequent degradation of specific germ line DNA sequences have been reported to occurin a variety of species, including humans (4). In some organisms,programmed DNA rearrangements are essential steps in somatic developmentand differentiation of certain cell types. Examples include rearrangementsin immunoglobulin and T-cell receptor genes (reviewed in reference11), surface antigen variation in trypanosomes (27), and switchingof mating type in yeast (1).

Partial elimination of the germ line genome is an important process in somatic nuclear differentiation in ciliated protozoa(6, 25). Like most ciliates, Tetrahymena thermophila containstwo types of nuclei: a diploid, transcriptionally inert germ linemicronucleus, responsible for storage and transmission of thegenetic information, and a polyploid, transcriptionally activesomatic macronucleus whose function is to express the geneticinformation (reviewed in reference 13). The sequence complexityof macronuclear DNA is 15 to 20% lower than that of micronuclearDNA, owing to the loss of micronucleus-specific germ line DNAsequences that occurs in the developing macronuclei during conjugation(31). Conjugation is a sexual pathway during which two cellsmate and exchange gametic micronuclei, which then fuse to forma zygotic nucleus that divides twice (22). Products of thisdivision differentiate into two micronuclei and two developingmacronuclei, often referred to as anlagen (24). Two major DNArearrangement events occur in developing anlagen, resulting inloss of germ line sequences: (i) excision and elimination of internaleliminated sequences (IESs) (31) and (ii) processing of themicronuclear chromosomes (n = 5) into 200 to 300 macronuclearchromosomes (33). There are approximately 6,000 IESs dispersedthroughout the micronuclear genome, consisting of both single-copyand repetitive sequences ranging in size from hundreds to severalthousands of base pairs (reviewed in reference 6). AlthoughIES excision occurs with high precision, no consensus excisionsignals have been identified at or near IES boundaries (35).In contrast, breakage, the first step of chromosome processing,requires chromosome breakage sequences (Cbs), a highly conservedmotif of 15 bp (34). Telomeres are added to the DNA fragmentscreated by chromosome breakage (36), while Cbs and about 40bp of DNA adjacent to them are eliminated (33). Eliminationof both IESs and Cbs occurs during a very short period of time,and it remains unclear whether the same trans-acting factors areinvolved. At approximately the same time, the old parental macronucleusis degraded through mechanisms resembling apoptotic DNA degradation(8).

To date, two polypeptides have been associated with DNA elimination events in Tetrahymena: Pdd1p and Pdd2p (for programmedDNA degradation). Both proteins are found in the degrading oldmacronucleus as well as in the new macronucleus, where they colocalizein specialized electron-dense structures that also contain IESs(20, 29). Both Pddps have been shown to associate with IESsin chromatin immunoprecipitation assays (29). Pdd1p possessesthree chromodomains, suggestive of its association with the germline DNA packaged in a specialized heterochromatin form (20).No conserved domains or other homology was detected between Pdd2pand other known proteins (29). Interestingly, expression ofPdd1p and Pdd2p begins early in development, well ahead of anlagenformation and DNA elimination, raising the possibility that thesepolypeptides have other, yet unidentified, function(s). Consistentwith this possibility, inhibition of pre-anlagen expression ofPdd1p and Pdd2p by disrupting their genes in the somatic macronucleusleads to impairment of the DNA rearrangements in anlagen, resultingin lethality (7, 23).

In this study, we describe the properties of a new developmentally regulated protein, Pdd3p. The derived sequence of the geneencoding this polypeptide predicts that it is a chromodomain-containingprotein. Immunoblotting experiments demonstrated that expressionof Pdd3p differs from that of Pdd1p and Pdd2p inasmuch as it isrestricted to the anlagen stage of Tetrahymena development, peakingat the time when DNA rearrangements are known to occur (3).Immunofluorescence analysis showed that Pdd3p initially colocalizeswith Pdd1p in the old macronucleus and in anlagen. At later stages,in addition to colocalization with Pdd1p at the periphery of thespecialized DNA elimination structures, Pdd3p is detected in thecentral area of these structures. These data suggest that Pdd3phas a unique function in the DNA degradation process. Analysisof anlagen DNA coimmunoprecipitated with either Pdd3p- or Pdd1p-specificantibodies demonstrated that it was enriched in IESs but not Cbs,suggesting that different trans-factors are involved in thesemajor DNA eliminationprocesses.

	MATERIALS AND METHODS

Top Abstract Introduction Materials and Methods Results Discussion References

Strains and cell culture. T. thermophila CU428 [mpr1-1/mpr1-1 (MPR1, mp-s, VII)] and CU427 [chx-1/chx-1 (CHX1, cy-s, VI)] were kindly provided by P.J. Bruns (Cornell University, Ithaca, N.Y.). Cells were grownin 1× SPP medium containing 1% Proteose Peptone (12). For conjugation,cells of different mating types were washed, starved (16 to 24h, 30°C), and mated in 10 mM Tris-HCl (pH 7.5), as described inreference 2. Pairing efficiency was estimated by counting pairsat 2 h postmixing and was at least 85%. Labeling of conjugatingcells with [³H]lysine at 1 µCi/ml of cell culture was performed between 9 and10 hpostmixing.

Preparation of nuclei. Macronuclei, micronuclei, and anlagen were isolated from Tetrahymena at 10 h postmixing as described in reference 12, exceptthat the nucleus isolation buffer contained 1 mM iodoacetamide,1 mM phenylmethylsulfonyl fluoride (PMSF), and 10 mM sodium butyrate,but not spermidine. Purification of nuclei by sedimentation atunit gravity was performed according to the method of Allis andDennison (2).

Purification of p32 and peptide sequencing. Purified anlagen were resuspended in 2 M sodium perchlorate at a concentration of 2 × 10⁶ nuclei/ml, sonicated (Sonifier Cell Disruptor 200; Branson) onice with five 10-s bursts at an output of 3 and a duty cycle of30%, and extracted for 1 h at 4°C. After centrifugation at 12,000× g for 20 min, the supernatant was loaded onto a butylsilane-bondedsilica gel solid-phase extraction cartridge (J. T. Baker), andproteins were eluted with 60% acetonitrile containing 0.1% trifluoroaceticacid (TFA) and fractionated by high-performance liquid chromatography(HPLC) on an octylsilane-bonded silica column with a linear gradientof 25 to 55% acetonitrile in 0.1% TFA over a period of 60 min.HPLC fractions were resolved on 12% sodium dodecyl sulfate (SDS)-polyacrylamidegel, and bands corresponding to p32, previously identified asa major newly synthesized anlagen protein (19), were localizedby fluorography and excised from the gel. Approximately 100 pmolof p32 was digested by Lys-C protease at 35°C for 24 h. Peptideswere extracted by sonication, fractionated on a Pharmacia SMARTHPLC system, and sequenced with an Applied Biosystems model 477Asequencer.

Cloning of the PDD3 gene. First-strand cDNA was synthesized by a standard reverse transcription procedure with oligonucleotide LT [5'-GGTCAGAGCTAGGCCTCAAAGCTTCTCGAGGGATCCGAGTC(T)₁₈-3']and total RNA (1 µg) extracted from mating cells 10 h postmixing.This cDNA was used in the first round of PCR with primers Pep1(5'-AGAGGWGGWATYCCYTTYGGYATG-3') and ST (5'-GGTCAGAGCTAGGCCTCA-3').PCR products were diluted 1:100 and used in the second round ofPCR with primers Pep2 (5'-TGGGAACCYGAATGGAAT-3') and IT (5'-AAGCTTCTCGAGGGATCCGAGTC-3').The sequence of the Pep1 and Pep2 primers was derived from thesequence of p32-specific peptides. In both cases, PCR consistedof 30 cycles. Each cycle was composed of a melting step at 94°Cfor 45 s, an annealing step at 52°C for 1 min, and an elongationstep at 72°C for 1 min. To obtain information about the 5' endof the p32 gene cDNA, we used inverse PCR (16). Briefly, first-strandcDNA obtained as indicated above was incubated with T4 RNA ligase(New England Biolabs) according to the manufacturer's instructionsto obtain single-stranded circular DNA molecules. After phenol-chloroformextraction and ethanol precipitation, ligation products were usedin PCR with the following oligonucleotides: ECAR (5'-TGGGAACCTGAATGGAATC-3')and RACE (5'-GTATTTAAATGATCTGCATAGCCTTTCC-3'). PCR products werediluted 1: 100 and used in the second round of PCR with primersSEQ1 (5'-TAGTGAAGTATCTGATG-3') and RACE1 (5'-GAGTTAATCATCATACTTAGTC-3').In both cases, PCR consisted of 35 cycles. Each cycle was composedof a melting step at 94°C for 45 s, an annealing step at 52°Cfor 1 min, and an elongation step at 72°C for 1 min. Productsobtained in the secondary PCR were sequenced with a sequencingkit from U.S.Biochemicals.

Codon alteration and expression of recombinant p32. To convert all TAG and TAA codons in the p32 gene to the conventional CAG and CAA codons, respectively, we performed single-strandedDNA mutagenesis (15) on the P32 cDNA cloned in pRSET-B expressionvector (Invitrogen) in frame with a N-terminal polyhistidine (6xHis)tag. pRSET-B vector containing modified p32 cDNA (pRSET-B-P32-M)was introduced into the BL21 strain of Escherichia coli. Expressionof the fusion protein from pRSET-B-P32-M was induced by adding1 mM isopropyl $beta$ -D-thiogalactopyranoside (IPTG) to the bacterialculture at an optical density at 600 nm of $approx$ 0.5 for 4 h. Purificationof the fusion 6xHis::p32 protein was carried out according tothe manufacturer'sinstructions.

Generation of antibodies. Two Pdd3p-specific peptides, peptide F (Y₃₆LVKWKGYADHLNTWEPEWNL₅₆-C) and peptide E (T₁₀₆NKRKNDENSVSTRRSNK₁₂₃-C), were synthesizedcontaining an artificial cysteine on the C terminus. Peptideswere conjugated to keyhole limpet hemocyanin via cysteine by standardprotocols (Pierce). Rabbits were then immunized with injectionsof 1 mg of conjugated peptide of 1 mg of recombinant p32 (fordetails, see reference 18).

Electrophoresis and immunoblotting. SDS-polyacrylamide gel electrophoresis (PAGE) and immunoblotting analyses were performed as described previously (18). Whenwhole-cell SDS lysates were used, aliquots of 10⁶ cells were removed from a mating cell culture and processed asdescribed previously (14). Rabbit polyclonal antibodies againstPdd1p were used as described previously (29).

Chromatin immunoprecipitation. Conjugating Tetrahymena cells were collected by centrifugation at 14 h postmixing followed by isolation of nuclei. Chromatincross-linking was carried out according to the method of Smotherset al. (29). Briefly, 5 × 10⁶ to 10 × 10⁶ anlagen were cross-linked by incubation for 1 h on ice in buffercontaining 1% formaldehyde, 0.25 M sucrose, 10 mM HEPES (pH 7.5),3 mM CaCl₂, 1 mM MgCl₂, 1 mM iodoacetamide, 10 mM butyric acid,and 1 mM PMSF. After fixation, nuclei were washed twice in theabove buffer lacking formaldehyde, dispersed in buffer A (50 mMTris-HCl [pH 8.6], 0.2% SDS, 5 mM EDTA), and sonicated on icewith five 10-s bursts with an output of 3 and a duty cycle of30%. Sonicated material was cleared by centrifugation, and solubilizedchromatin was diluted 10× in buffer B (1% Triton X-100, 0.15 Msodium chloride, 2 mM EDTA, 20 mM Tris-HCl [pH 8.6]) and incubatedwith antibodies overnight at 4°C. Antibodies were precipitatedwith protein A-Sepharose (Amersham Pharmacia Biotech AB) accordingto the manufacturer's instructions. Precipitated material waseluted from antibodies in a solution containing 100 mM sodiumbicarbonate and 1% SDS, and cross-linking was reversed in thesame buffer by incubation for 4 h at 65°C. DNA was then purifiedby phenol-chloroform extraction and precipitated with ethanol.DNA samples were quantitated by spectrophotometry and slot blottedto a Nylon membrane (Millipore). Fragments a and c obtained byHaeIII restriction digestion of the insert from plasmid pTt2512(a gift from Meng-Chao Yao, Fred Hutchinson Cancer Center, Seattle,Wash.) were used as a probe for Tetrahymena IES DNA. For a loadingcontrol, we used a BTU-1 ( $beta$ -tubulin) gene (10). All probes werelabeled with [ $alpha$ -³²P] dATP by random priming (26). Oligonucleotide CBS1 (5'TAAAGAAAGAGGTTGGTTTA-3')(33) was used as a probe for Cbs. CBS1 was labeled with [ $gamma$ -³²P]ATP and hybridized as described previously (33). Autoradiographswere scanned and imported into Adobe Photoshop TM (version 4.0),and densitometric analysis was performed with the NIH Imageprogram.

Indirect immunofluorescence analysis. Conjugating cells were fixed and processed for indirect immunofluorescence as described previously (28). Cells were stainedwith the DNA-specific dye diamidinophenolindole (DAPI) at 0.3µg/ml in Tris-buffered saline. Mouse polyclonal Pdd1p-specificantibodies were used as described previously (29).

Fluorescent and confocal microscopy. Fluorescent microscopy was performed with an Olympus BH-2 microscope. Confocal images were obtained with a Leica TCS NT microscope,and digital images were processed with Adobe Photoshop (AdobeSystems, Inc., San Jose, Calif.).

Nucleotide sequence accession number. The GenBank accession number for the PDD3 gene is AF226856.

	RESULTS

Top Abstract Introduction Materials and Methods Results Discussion References

p32 is a chromodomain-containing protein. With a metabolic labeling protocol, several anlagen-specific polypeptides were detected (19) whose expression peaks duringstages of conjugation when DNA rearrangements occur (macronucleardevelopment II [MAC II] stage). Shown in Fig. 1A is a typicalfluorograph of a 12% SDS gel of total nuclear protein extractedfrom purified micronuclei, old macronuclei, and new macronucleior anlagen (An) isolated from mating cells pulse-labeled with[³H]lysine at the MAC II stage. Four polypeptides with apparentmasses of 90, 65, 43, and 32 kDa are strongly labeled and selectivelydeposited into anlagen. Two of these proteins, Pdd1p and Pdd2p(Fig. 1A), were recently isolated and characterized (20, 29).Another polypeptide, with an apparent molecular mass of 32 kDa(p32), is also actively synthesized and deposited in anlagen atthis stage. To isolate and characterize p32, total anlagen proteinwas extracted with 2 M sodium perchlorate and subjected to fractionationby reverse-phase HPLC, followed by separation from contaminatingproteins on a 12% SDS gel (see Materials and Methods for details).p32 identified by incorporation of [³H]lysine (Fig. 1B) was excised from the gel and digested withLys-C protease, and three HPLC-purified peptides were subjectedto microsequence analysis. This analysis provided us with sufficientsequence to synthesize degenerate oligonucleotide primers. Byusing a combination of reverse transcription PCR and 5'- and 3'-rapidamplification of cDNA ends PCR, we isolated a P32 cDNA.

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FIG. 1. Polypeptides synthesized and targeted to different nuclei during late stages of Tetrahymena development. (A) Conjugating cells (schematically represented on the top of the figure) were pulse-labeled with [³H]lysine from 9 to 10 h postmixing. Nuclei were purified by sedimentation at 1 U of gravity (2). Total protein from different types of nuclei was resolved on a 12% SDS-polyacrylamide gel and analyzed by fluorography. Approximately 10⁷ micronuclei (Mic), 10⁶ old macronuclei (OM), and 3 × 10⁶ anlagen (An) were used. Previously identified Tetrahymena polypeptides and protein molecular mass standards (kilodaltons) are shown. (B) p32 recovered from reverse-phase HPLC fractionation of proteins extracted from purified anlagen and resolved on 12% SDS-polyacrylamide gel. Proteins were visualized by staining with Coomassie blue, followed by fluorography to verify the position of p32 (shown on the right). An, total anlagen protein before the extraction; Fr, HPLC fraction containing p32. Protein molecular mass standards (kilodaltons) are designated on the left.

The predicted amino acid sequence corresponding to the longest open reading frame of the gene encoding p32 is shown in Fig.2A. Several observations suggest that this sequence is correct.First, all three sequenced peptides are found in the predictedprotein (Fig. 2A). Second, the calculated molecular mass of thededuced translation product open reading frame ( $approx$ 26 kDa) is closeto the apparent molecular mass of p32 on SDS gel (32 kDa). Finally,the predicted isoelectric point of p32 (9.1) is in a good agreementwith that determined for p32 earlier (approximately 9.0) (19).

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FIG. 2. Analysis of p32 cDNA and amino acid sequence. (A) Nucleotide sequence of p32 cDNA. Nucleotides from the longest open reading frame are indicated by capital letters. The positions of oligonucleotides used in PCR are indicated by arrows (see Materials and Methods for details). (B) Derived amino acid sequence of the longest open reading frame of P32 cDNA. Underlined are peptides used for microsequencing. Shown in boldface is the chromodomain. Shown in brackets and designated by E and F are sequences of peptides used for antibody generation. (C) Alignment of the Pdd3p chromodomain with chromodomain from other proteins. Amino acid residues common with Pdd3p are shown in boldface. Horizontal bars define the type of secondary structure ( $beta$ -sheet or $alpha$ -helix) of the mouse MoMOD 1 protein (5). Note that Pdd1p and Pdd3p chromodomains share homology in the least-conserved $alpha$ -helical region.

Comparison of the deduced amino acid sequence of p32 with those in the protein databases suggests that p32 contains a chromodomain(from chromatin organizing modifier) (Fig. 2C), a group of aminoacids found predominantly in heterochromatin-associated proteins(17). Interestingly, the highest degree of homology to the p32chromodomain is found in one of the three chromodomains of Pdd1p,a protein implicated in DNA elimination in Tetrahymena (describedabove). In both cases, the chromodomains are at the N-terminalend of thepolypeptides.

p32 localizes to the DNA elimination structures in anlagen. To determine the expression pattern and intranuclear localization of p32, we generated a set of p32-specific polyclonal antisera.First, two peptides (Fig. 2A) were synthesized based on the derivedp32 sequence and were used to immunize rabbits. Second, the entirep32 fused with a histidine tag (30) was expressed in E. coliafter changing TAG and TAA codons encoding glutamine in Tetrahymenato the conventional glutamine codons CAG and CAA, respectively(see Materials and Methods). Recombinant p32, when resolved onSDS gel, migrated more slowly than the original p32 (data notshown), probably because of the polyhistidine tag. Recombinantp32 was used to generate polyclonal antiserum inrabbits.

All three sera demonstrated high specificity toward p32 on Western blots containing total protein extracted from purifiedanlagen (Fig. 3A). Immunoblotting analysis of total protein fromcells collected at different stages of conjugation and imunofluorescencedata (not shown) revealed that, unlike Pdd1p (20) and Pdd2p(29), p32 is expressed only during later stages of conjugation,after anlagen are formed (roughly at 6 h [see dotted line in Fig.3B]). The highest level of p32 is detected during stages of Tetrahymenadevelopment when DNA rearrangements were reported to occur (3),and the termination of its expression (as in case with Pdd1p andPdd2p [19, 20, 29]) corresponds to the end of this process.These results were confirmed with several p32-specific antisera.

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FIG. 3. p32 is a developmentally regulated polypeptide. (A) Equal amounts of total anlagen protein from 14-h conjugating cells were loaded on 10% SDS-polyacrylamide gel. One part of the gel was stained with Coomassie blue, while the others were analyzed by Western blotting with antibodies generated against peptide F, peptide E, and recombinant p32 (designated by F, E, and R, respectively). (B) Total proteins from conjugating Tetrahymena cells at different times postmixing (indicated at the top in hours) were extracted and resolved on a 12% SDS-polyacrylamide gel, and distinct sections of the gel were probed in Western blots with serum against recombinant p32 and with previously obtained Pdd1p antibodies. Note the difference in the timing of expression of p32 and Pdd1p.

To determine the nuclear localization of p32 during macronuclear development, we performed indirect immunofluorescence analysesof Tetrahymena cells during conjugation by using antibodies againstrecombinant p32 (lane "R" in Fig. 3). As shown in Fig. 4A, p32is uniformly distributed in new macronuclei as well as in thedegenerating old macronucleus at 10 h postmixing. However, atabout 12 h of conjugation the staining becomes uneven, culminatingin clustering into characteristic circle-like intranuclear structuresapproximately 2 h later. Previous reports demonstrated that thesestructures contain micronucleus-specific DNA destined for elimination(20). Immunofluorescence experiments with Pdd1p and Pdd2p antibodiesrevealed that these proteins localize mostly at the peripheryof these structures, resulting in characteristic "doughnut-like"images (19). It is noteworthy that the pattern of p32 distributionin anlagen coincides well with that of Pdd1p during most of macronucleardevelopment, as evidenced by the double staining of anlagen withp32 rabbit and Pdd1p mouse polyclonal antibodies (Fig. 4A). However,as shown in Fig. 4B, the concentration of p32 inside DNA eliminationstructures is considerably higher than that of Pdd1p, suggestingthat p32 plays a different role in the process of DNA degradation.Close association of p32 with DNA degradation structures motivatedus to change its name to Pdd3p (for programmed DNA degradation).

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FIG. 4. Intranuclear localization of p32. (A) Confocal sections of Tetrahymena cells fixed at the indicated time points and stained simultaneously with DAPI and with (i) mouse Pdd1p and fluorescein isothiocyanate-conjugated secondary antibodies and (ii) rabbit recombinant p32 (R) (lane R in Fig. 3) and rhodamine-conjugated secondary antibodies as shown. White arrows indicate anlagen, stained with DAPI. Shown above is a schematic representation of the late stages of conjugation: macronuclear development II (MAC II) and macronuclear development III (MAC III). Mi, An, and OM, micronucleus, anlagen, and old macronucleus (black circle), respectively. Only one of two paired cells is shown. Bar, 4 µm. Note that in approximately 30% of conjugations, we completely failed to detect p32 in nuclei at the time corresponding to the formation of DNA elimination structures, while Pdd1p in these cells was still readily detectable. Interestingly, p32 in these conjugations colocalizes with Pdd1p at earlier stages, and the amounts of p32 in anlagen purified from either type of conjugation as well as the duration of p32 expression in either case were similar, as evidenced by Western blotting (data not shown). Therefore, we attributed the absence of p32-specific staining to the inaccessibility of p32 to antibodies, which most likely is a result of its localization inside DNA degradation structures. (B) Consecutive confocal images (numbered 1 to 3; 0.4 µm apart) of a Tetrahymena cell at the MAC III stage, fixed, and stained as in panel A. White arrowheads indicate donut-like DNA degradation structures. Note the difference in the intranuclear distributions of Pdd1p and p32. Bar, 1 µm.

Pdd3p and Pdd1p associate with IES-specific, but not Cbs-specific, DNA. Localization of Pdd3p inside DNA degradation structures prompted us to analyze what DNA sequences might be physically associatedwith it. To this end, we obtained a nuclear fraction from 14-hconjugating Tetrahymena cells highly enriched in anlagen. At thistime, anlagen contain multiple DNA elimination structures. Nucleiwere then cross-linked with 1% paraformaldehyde and sonicated,and solubilized nuclear material was subjected to immunoprecipitationwith various antibodies. Following cross-link reversal, immunoprecipitatedDNA was purified, quantitated, slot blotted to the Nylon membrane,and probed sequentially with various sequences, stripping themembrane after each hybridization. To detect IES DNA, a fragmentof pTt2512 was used that contains a sequence homologous to highlydispersed micronucleus-limited sequences that are repeated about200 times in the micronuclear genome (32). To detect Cbs, a20-bp oligonucleotide, CBS-1, that contains a consensus for Cbssequences (33) was used. A PCR fragment of the Tetrahymena BTU-1gene (10) was used as a control forloading.

The results of these hybridization analyses are shown in Fig. 5A and summarized in Fig. 5B. Chromatin immunoprecipitated withantibodies selective for Pdd3p or Pdd1p is clearly enriched withDNA hybridizing to the pTt2512 plasmid. In contrast, no enrichmentover input DNA was observed in the same samples hybridized withthe probe for Cbs or BTU. As expected, no enrichment for any probewas detected in DNA precipitated with histone H4 antibodies. Thus,we conclude that Pdd1p and Pdd3p associate with IES, but not Cbs,sequences in the anlagen genome at this stage of development.

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FIG. 5. Pdd3p associates with Pdd1p and with DNA enriched in IES, but not Cbs. (A) DNA samples obtained by chromatin immunoprecipitation with the antibodies shown on the left, as well as DNA isolated from solubilized, cross-linked chromatin before immunoprecipitation (input), were quantitated, slot blotted onto a Nylon membrane, and sequentially probed with the DNA sequences designated on the top of each section. The numbers above each column indicate the amount of loaded DNA in nanograms. (B) Relative densitometric signals for samples shown in panel A. Error bars indicate the standard deviation from average reading of signals in two groups: 150 and 75 ng. (C) Material immunoprecipitated with the antibodies designated on the top from either cross-linked (Formaldehyde +) or untreated (Formaldehyde $-$ ) solubilized chromatin from 14-h anlagen was resolved on the 12% SDS gel and probed by Western blotting with the antibodies shown on the left. $alpha$ -prePdd1p and $alpha$ -prePdd3p, preimmune Pdd1p and Pdd3p sera, respectively. Inp., input.

	DISCUSSION

Top Abstract Introduction Materials and Methods Results Discussion References

In the present study, we report the purification and characterization of a new chromodomain-containing polypeptide, referredto as Pdd3p. Several lines of evidence suggest its involvementin the DNA elimination process in Tetrahymena. First, Pdd3p expressionpeaks during a short period corresponding to the major DNA rearrangementprocesses in the new macronucleus. Second, immunofluorescencedata demonstrate that Pdd3p is uniquely localized throughout structuresknown to be associated with sequences undergoing elimination inanlagen. Finally, Pdd3p physically associates with at least onerandomly selected family of micronucleus-specific DNA sequencesdestined forelimination.

There are several structural and biological similarities between Pdd3p and the founding member of this small family of proteins $---$ Pdd1p.Pdd1p has three chromodomains (20), one of which shares especiallyhigh homology with the chromodomain of Pdd3p. Interestingly, thearea of homology between these two proteins includes an $alpha$ -helicalregion, which normally is one of the least conserved regions throughoutchromodomains (Fig. 2C). Chromodomain proteins were shown to takepart in transcriptional regulation (both activation and repression)and in maintenance of genomic stability (reviewed in references5 and 17). The chromodomain is detected in proteins in conjunctionwith other domains, such as helicase, transposase, and Zn fingerdomains (17). Although the function of chromodomains has notyet been determined, it is generally believed that they are responsiblefor targeting proteins to specialized chromatin sites via protein-proteininteractions (5). Since both Pdd1p and Pdd3p colocalize inthe degenerating old macronucleus and in anlagen and are targetedto the same subnuclear structures in anlagen, it is likely thatthere is a shared mechanism of their recruitment to the eliminatingDNA sequences. Our immunofluorescence and coimmunoprecipitationdata suggest that both Pdd proteins exist in a complex with eliminatedDNA, although the nature of our analysis does not allow us toconclude whether these proteins coimmunoprecipitate only whenbound to IESelements.

On the other hand, several features of Pdd3p distinguish it from other members of the Pdd group. First, expression of Pdd3p,unlike that of Pdd1p and Pdd2p, has not been detected in the pre-anlagenstage of Tetrahymena development, suggesting that is not requiredfor processes preceding anlagen differentiation. The precise linkbetween these processes and DNA elimination in anlagen has notbeen established; however, pre-anlagen expression of Pdd1p andPdd2p is essential for DNA elimination and nuclear differentiation(7, 23). Second, our immunofluorescence data suggest thatthe relative concentration of Pdd3p in the center of the DNA eliminationstructures is higher than that of other Pdd proteins. These resultswere obtained by using several previously characterized Pdd1p-and Pdd2p-specific antisera (19, 29) and polyclonal antiseraagainst recombinant Pdd3p (R in Fig. 3) obtained from tworabbits.

Since the micronucleus-limited DNA sequences also localize to these regions, our data suggest that Pdd3p may be more directlyin contact with eliminating DNA sequences than other Pddproteins.

From the abundant nature of Pddps and the presence of chromodomains in two of them, we favor the view that chromatin structureand nucleostructural organization in addition to sequence specificityare responsible for directing excision of micronucleus-specificDNA $---$ the first step in DNA elimination. This view is consistentwith the observation that no consensual signals for IES excisionhave been identified yet. Also in accord with this hypothesisis the recent report that chromatin modifications are essentialfor another DNA rearrangement process: VDJ recombination in Band T cells (21).

IES excision and chromosome breakage, which includes excision and elimination of Cbs and adjacent regions, are two major DNArearrangements occurring in anlagen during a short interval. Thisobservation gave rise to the hypothesis that the same chromatinfactors might be involved in both processes. Our experiments demonstratethat, unlike some IES, Cbs sequences are not enriched in DNA cross-linkedto either Pdd1p or Pdd3p. These data are further supported bythe finding that somatic disruption of the PDD1 gene impairs IESexcision, but does not affect chromosome processing and telomereaddition (7). The simplest interpretation of our data is thatdifferent sets of proteins are involved in two DNA rearrangementprocesses in the developingmacronucleus.

	ACKNOWLEDGMENTS

We are grateful to Jim Smothers and Craig Mizzen for their technical help, Richard Cook for protein sequencing, and ThomasDoak for his help in protein sequence analysis. We thank NataliyaShulga for help with confocal microscopy, Jody Bowen for criticalreading of the manuscript, and Jianxin Zhou for constant encouragementand suggestions throughout thework.

M.A.N. was a recipient of an Oncology Research Faculty Development Program Fellowship, NCI, NIH. This research was supportedby grants from the National Institutes of Health to C.D.A. andM.A.G.

	FOOTNOTES

^* Corresponding author. Present address: Department of Biochemistry and Molecular Genetics, University of Virginia, Charlottesville,VA 22908. Phone: (804) 243-6048. Fax: (804) 924-5069. E-mail:allis{at}virginia.edu.

Present address: Department of Molecular Biology, Lewis Thomas Lab, Princeton University, Princeton, NJ08544.

REFERENCES

Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References

1. Abraham, J., K. A. Nasmyth, J. N. Strathern, A. J. S. Klar, and J. B. Hicks. 1984. Regulation of mating type information in yeasts. Negative control requiring sequences both 5' and 3' to the regulated regions. J. Mol. Biol. 176:307-311[CrossRef][Medline].

2. Allis, C. D., and D. K. Dennison. 1982. Identification and purification of young macronuclear anlagen from conjugating cells of Tetrahymena thermophila. Dev. Biol. 93:519-533[CrossRef][Medline].

3. Austerberry, C. F., C. D. Allis, and M. C. Yao. 1984. Specific DNA rearrangements in synchronously developing nuclei of Tetrahymena. Proc. Natl. Acad. Sci. USA 81:7383-7387[Abstract/Free Full Text].

4. Bassnett, S., and D. Mataic. 1997. Chromatin degradation in differentiating fiber cells of the eye lens. J. Cell Biol. 137:37-49[Abstract/Free Full Text].

5. Cavalli, G., and R. Paro. 1998. Chromo-domain proteins: linking chromatin structure to epigenetic regulation. Curr. Opin. Cell Biol. 10:354-360[CrossRef][Medline].

6. Coyne, R. S., D. L. Chalker, and M. C. Yao. 1996. Genome downsizing during ciliate development: nuclear division of labor through chromosome restructuring. Annu. Rev. Genet. 30:557-578[CrossRef][Medline].

7. Coyne, R. S., M. A. Nikiforov, J. F. Smothers, C. D. Allis, and M.-C. Yao. 1999. Parental expression of the chromodomain protein Pdd1p is required for completion of programmed DNA elimination and nuclear differentiation. Mol. Cell 4:865-872[CrossRef][Medline].

8. Davis, M. C., J. G. Ward, G. Herrick, and C. D. Allis. 1992. Programmed nuclear death: apoptotic-like degradation of specific nuclei in conjugating Tetrahymena. Dev. Biol. 154:419-432[CrossRef][Medline].

9. Frohman, M. A. 1993. Rapid amplification of complementary DNA ends for generation of full-length complementary DNAs: thermal RACE. Methods Enzymol. 218:340-356[Medline].

10. Gaertig, J., L. Gu, B. Hai, and M. A. Gorovsky. 1994. High frequency vector-mediated transformation and gene replacement in Tetrahymena. Nucleic Acids Res. 22:5391-5398[Abstract/Free Full Text].

11. Gelert, M. 1992. V(D)J recombination gets a break. Trends Genet. 8:408-412[CrossRef][Medline].

12. Gorovsky, M. A., M. C. Yao, J. B. Keevert, and G. L. Pleger. 1975. Isolation of micro- and macronuclei of Tetrahymena pyriformis. Methods Cell Biol. 9:311-327[Medline].

13. Gorovsky, M. A. 1980. Genome organization and reorganization in Tetrahymena. Annu. Rev. Genet. 14:203-239[CrossRef][Medline].

14. Guttman, S. D., C. V. Glover, C. D. Allis, and M. A. Gorovsky. 1980. Heat shock, deciliation and release from anoxia induce the synthesis of the same set of polypeptides in starved T. pyriformis. Cell 22:299-307[CrossRef][Medline].

15. Hill, D. E. 1988. Mutagenesis of cloned DNA, p. 8.0.1-8.5.9. In F. M. Ausubel, R. Brent, R. E. Kingston, D. D. Moore, J. G. Seidman, J. A. Smith, and K. Struhl (ed.), Current protocols in molecular biology, vol. 1. Wiley Interscience, New York, N.Y.

16. Huang, S. H. 1994. Inverse polymerase chain reaction. An efficient approach to cloning cDNA ends. Mol. Biotechnol. 2:15-22[Medline].

17. Koonin, E. V., S. Zhou, and J. C. Lucchesi. 1995. The chromo superfamily: new members, duplication of the chromo domain and possible role in delivering transcription regulators to chromatin. Nucleic Acids Res. 23:4229-4233[Abstract/Free Full Text].

18. Lin, R., J. W. Leone, R. G. Cook, and C. D. Allis. 1989. Antibodies specific to acetylated histones document the existence of deposition- and transcription-related histone acetylation in Tetrahymena. J. Cell Biol. 108:1577-1588[Abstract/Free Full Text].

19. Madireddi, M. T., M. C. Davis, and C. D. Allis. 1994. Identification of a novel polypeptide involved in the formation of DNA-containing vesicles during macronuclear development in Tetrahymena. Dev. Biol. 165:418-431[CrossRef][Medline].

20. Madireddi, M. T., R. S. Coyne, J. F. Smothers, K. M. Mickey, M. C. Yao, and C. D. Allis. 1996. Pdd1p, a novel chromodomain-containing protein, links heterochromatin assembly and DNA elimination in Tetrahymena. Cell 87:75-84[CrossRef][Medline].

21. McMurry, M. T., and M. S. Krangel. 2000. A role for histone acetylation in the developmental regulation of V(D)J recombination. Science 287:495-498[Abstract/Free Full Text].

22. Nanney, D. L. 1986. Introduction, p. 1-21. In J. G. Gall (ed.), Molecular biology of ciliated protozoa. Academic Press, Orlando, Fla.

23. Nikiforov, M. A., J. F. Smothers, M. A. Gorovsky, and C. D. Allis. 1999. Excision of micronuclear-specific DNA requires parental expression of Pdd2p and occurs independently from DNA replication in Tetrahymena thermophila. Genes Dev. 13:2852-2862[Abstract/Free Full Text].

24. Orias, E. 1986. Ciliate conjugation, p. 45-84. In J. G. Gall (ed.), Molecular biology of ciliated protozoa. Academic Press, Orlando, Fla.

25. Prescott, D. M. 1994. The DNA of ciliated protozoa. Microbiol. Rev. 58:233-267[Abstract/Free Full Text].

26. Richards, E. J. 1988. Preparation and analysis of DNA, p. 2.0.1.-2.12.5.. In F. M. Ausubel, R. Brent, R. E. Kingston, D. D. Moore, J. G. Seidman, J. A. Smith, and K. Struhl (ed.), Current protocols in molecular biology, vol. 1. Wiley Interscience, New York, N.Y.

27. Robertson, B. D., and T. F. Meyer. 1992. Genetic variation in pathogenic bacteria. Trends Genet. 8:422-427[Medline].

28. Smothers, J. F., M. T. Madireddi, F. D. Warner, and C. D. Allis. 1997. Programmed DNA degradation and nucleolar biogenesis occur in distinct organelles during macronuclear development in Tetrahymena. J. Eukaryot. Microbiol. 44:79-88[Medline].

29. Smothers, J. F., C. A. Mizzen, M. M. Tubbert, R. G. Cook, and C. D. Allis. 1997. Pdd1p associates with germline-restricted chromatin and a second novel anlagen-enriched protein in developmentally programmed DNA elimination structures. Development 124:4537-4545[Abstract].

30. Tabor, S. 1988. Protein expression, p. 16.0.5-16.5.4. In F. M. Ausubel, R. Brent, R. E. Kingston, D. D. Moore, J. G. Seidman, J. A. Smith, and K. Struhl (ed.), Current protocols in molecular biology, vol. 1. Wiley Interscience, New York, N.Y.

31. Yao, M. C., and M. A. Gorovsky. 1974. Comparison of the sequences of macro- and micronuclear DNA of Tetrahymena pyriformis. Chromosoma 48:1-18[Medline].

32. Yao, M. C. 1982. Elimination of specific DNA sequences from the somatic nucleus of the ciliate Tetrahymena. J. Cell Biol. 92:783-789[Abstract/Free Full Text].

33. Yao, M. C., K. Zheng, and C. H. Yao. 1987. A conserved nucleotide sequence at the sites of developmentally regulated chromosomal breakage in Tetrahymena. Cell 48:779-788[CrossRef][Medline].

34. Yao, M. C., C. H. Yao, and B. Monks. 1990. The controlling sequence for site-specific chromosome breakage in Tetrahymena. Cell 63:763-772[CrossRef][Medline].

35. Yao, M. C. 1996. Programmed DNA deletions in Tetrahymena: mechanisms and implications. Trends Genet. 12:26-30[CrossRef][Medline].

36. Yu, G. L., and E. H. Blackburn. 1991. Developmentally programmed healing of chromosomes by telomerase in Tetrahymena. Cell 67:823-832[CrossRef][Medline].

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1.	Abraham, J., K. A. Nasmyth, J. N. Strathern, A. J. S. Klar, and J. B. Hicks. 1984. Regulation of mating type information in yeasts. Negative control requiring sequences both 5' and 3' to the regulated regions. J. Mol. Biol. 176:307-311[CrossRef][Medline].
2.	Allis, C. D., and D. K. Dennison. 1982. Identification and purification of young macronuclear anlagen from conjugating cells of Tetrahymena thermophila. Dev. Biol. 93:519-533[CrossRef][Medline].
3.	Austerberry, C. F., C. D. Allis, and M. C. Yao. 1984. Specific DNA rearrangements in synchronously developing nuclei of Tetrahymena. Proc. Natl. Acad. Sci. USA 81:7383-7387[Abstract/Free Full Text].
4.	Bassnett, S., and D. Mataic. 1997. Chromatin degradation in differentiating fiber cells of the eye lens. J. Cell Biol. 137:37-49[Abstract/Free Full Text].
5.	Cavalli, G., and R. Paro. 1998. Chromo-domain proteins: linking chromatin structure to epigenetic regulation. Curr. Opin. Cell Biol. 10:354-360[CrossRef][Medline].
6.	Coyne, R. S., D. L. Chalker, and M. C. Yao. 1996. Genome downsizing during ciliate development: nuclear division of labor through chromosome restructuring. Annu. Rev. Genet. 30:557-578[CrossRef][Medline].
7.	Coyne, R. S., M. A. Nikiforov, J. F. Smothers, C. D. Allis, and M.-C. Yao. 1999. Parental expression of the chromodomain protein Pdd1p is required for completion of programmed DNA elimination and nuclear differentiation. Mol. Cell 4:865-872[CrossRef][Medline].
8.	Davis, M. C., J. G. Ward, G. Herrick, and C. D. Allis. 1992. Programmed nuclear death: apoptotic-like degradation of specific nuclei in conjugating Tetrahymena. Dev. Biol. 154:419-432[CrossRef][Medline].
9.	Frohman, M. A. 1993. Rapid amplification of complementary DNA ends for generation of full-length complementary DNAs: thermal RACE. Methods Enzymol. 218:340-356[Medline].
10.	Gaertig, J., L. Gu, B. Hai, and M. A. Gorovsky. 1994. High frequency vector-mediated transformation and gene replacement in Tetrahymena. Nucleic Acids Res. 22:5391-5398[Abstract/Free Full Text].
11.	Gelert, M. 1992. V(D)J recombination gets a break. Trends Genet. 8:408-412[CrossRef][Medline].
12.	Gorovsky, M. A., M. C. Yao, J. B. Keevert, and G. L. Pleger. 1975. Isolation of micro- and macronuclei of Tetrahymena pyriformis. Methods Cell Biol. 9:311-327[Medline].
13.	Gorovsky, M. A. 1980. Genome organization and reorganization in Tetrahymena. Annu. Rev. Genet. 14:203-239[CrossRef][Medline].
14.	Guttman, S. D., C. V. Glover, C. D. Allis, and M. A. Gorovsky. 1980. Heat shock, deciliation and release from anoxia induce the synthesis of the same set of polypeptides in starved T. pyriformis. Cell 22:299-307[CrossRef][Medline].
15.	Hill, D. E. 1988. Mutagenesis of cloned DNA, p. 8.0.1-8.5.9. In F. M. Ausubel, R. Brent, R. E. Kingston, D. D. Moore, J. G. Seidman, J. A. Smith, and K. Struhl (ed.), Current protocols in molecular biology, vol. 1. Wiley Interscience, New York, N.Y.
16.	Huang, S. H. 1994. Inverse polymerase chain reaction. An efficient approach to cloning cDNA ends. Mol. Biotechnol. 2:15-22[Medline].
17.	Koonin, E. V., S. Zhou, and J. C. Lucchesi. 1995. The chromo superfamily: new members, duplication of the chromo domain and possible role in delivering transcription regulators to chromatin. Nucleic Acids Res. 23:4229-4233[Abstract/Free Full Text].
18.	Lin, R., J. W. Leone, R. G. Cook, and C. D. Allis. 1989. Antibodies specific to acetylated histones document the existence of deposition- and transcription-related histone acetylation in Tetrahymena. J. Cell Biol. 108:1577-1588[Abstract/Free Full Text].
19.	Madireddi, M. T., M. C. Davis, and C. D. Allis. 1994. Identification of a novel polypeptide involved in the formation of DNA-containing vesicles during macronuclear development in Tetrahymena. Dev. Biol. 165:418-431[CrossRef][Medline].
20.	Madireddi, M. T., R. S. Coyne, J. F. Smothers, K. M. Mickey, M. C. Yao, and C. D. Allis. 1996. Pdd1p, a novel chromodomain-containing protein, links heterochromatin assembly and DNA elimination in Tetrahymena. Cell 87:75-84[CrossRef][Medline].
21.	McMurry, M. T., and M. S. Krangel. 2000. A role for histone acetylation in the developmental regulation of V(D)J recombination. Science 287:495-498[Abstract/Free Full Text].
22.	Nanney, D. L. 1986. Introduction, p. 1-21. In J. G. Gall (ed.), Molecular biology of ciliated protozoa. Academic Press, Orlando, Fla.
23.	Nikiforov, M. A., J. F. Smothers, M. A. Gorovsky, and C. D. Allis. 1999. Excision of micronuclear-specific DNA requires parental expression of Pdd2p and occurs independently from DNA replication in Tetrahymena thermophila. Genes Dev. 13:2852-2862[Abstract/Free Full Text].
24.	Orias, E. 1986. Ciliate conjugation, p. 45-84. In J. G. Gall (ed.), Molecular biology of ciliated protozoa. Academic Press, Orlando, Fla.
25.	Prescott, D. M. 1994. The DNA of ciliated protozoa. Microbiol. Rev. 58:233-267[Abstract/Free Full Text].
26.	Richards, E. J. 1988. Preparation and analysis of DNA, p. 2.0.1.-2.12.5.. In F. M. Ausubel, R. Brent, R. E. Kingston, D. D. Moore, J. G. Seidman, J. A. Smith, and K. Struhl (ed.), Current protocols in molecular biology, vol. 1. Wiley Interscience, New York, N.Y.
27.	Robertson, B. D., and T. F. Meyer. 1992. Genetic variation in pathogenic bacteria. Trends Genet. 8:422-427[Medline].
28.	Smothers, J. F., M. T. Madireddi, F. D. Warner, and C. D. Allis. 1997. Programmed DNA degradation and nucleolar biogenesis occur in distinct organelles during macronuclear development in Tetrahymena. J. Eukaryot. Microbiol. 44:79-88[Medline].
29.	Smothers, J. F., C. A. Mizzen, M. M. Tubbert, R. G. Cook, and C. D. Allis. 1997. Pdd1p associates with germline-restricted chromatin and a second novel anlagen-enriched protein in developmentally programmed DNA elimination structures. Development 124:4537-4545[Abstract].
30.	Tabor, S. 1988. Protein expression, p. 16.0.5-16.5.4. In F. M. Ausubel, R. Brent, R. E. Kingston, D. D. Moore, J. G. Seidman, J. A. Smith, and K. Struhl (ed.), Current protocols in molecular biology, vol. 1. Wiley Interscience, New York, N.Y.
31.	Yao, M. C., and M. A. Gorovsky. 1974. Comparison of the sequences of macro- and micronuclear DNA of Tetrahymena pyriformis. Chromosoma 48:1-18[Medline].
32.	Yao, M. C. 1982. Elimination of specific DNA sequences from the somatic nucleus of the ciliate Tetrahymena. J. Cell Biol. 92:783-789[Abstract/Free Full Text].
33.	Yao, M. C., K. Zheng, and C. H. Yao. 1987. A conserved nucleotide sequence at the sites of developmentally regulated chromosomal breakage in Tetrahymena. Cell 48:779-788[CrossRef][Medline].
34.	Yao, M. C., C. H. Yao, and B. Monks. 1990. The controlling sequence for site-specific chromosome breakage in Tetrahymena. Cell 63:763-772[CrossRef][Medline].
35.	Yao, M. C. 1996. Programmed DNA deletions in Tetrahymena: mechanisms and implications. Trends Genet. 12:26-30[CrossRef][Medline].
36.	Yu, G. L., and E. H. Blackburn. 1991. Developmentally programmed healing of chromosomes by telomerase in Tetrahymena. Cell 67:823-832[CrossRef][Medline].