Genetics, Vol. 163, 1375-1387, April 2003, Copyright © 2003

Transvection at the End of the Truncated Chromosome in Drosophila melanogaster

Mikhail Savitskya, Tatyana Kahn1,a, Ekaterina Pomerantsevaa, and Pavel Georgieva
a Department of the Control of Genetic Processes, Institute of Gene Biology, Russian Academy of Sciences, Moscow 117334, Russia

Corresponding author: Pavel Georgiev, Russian Academy of Sciences, 34/5 Vavilov St., Moscow 117334, Russia., pgeorg{at}biogen.msk.su (E-mail)

Communicating editor: J. A. BIRCHLER


*  ABSTRACT
*TOP
 *ABSTRACT
*MATERIALS AND METHODS
 *RESULTS
 *DISCUSSION
 *LITERATURE CITED

The phenomenon of transvection is well known for the Drosophila yellow locus. Thus enhancers of a promoterless yellow locus in one homologous chromosome can activate the yellow promoter in the other chromosome where the enhancers are inactive or deleted. In this report, we examined the requirements for trans-activation of the yellow promoter at the end of the deficient chromosome. A number of truncated chromosomes ending in different areas of the yellow regulatory region were examined in combination with the promoterless y alleles. We found that trans-activation of the yellow promoter at the end of a deficient chromosome required ~6 kb of an additional upstream sequence. The nature of upstream sequences affected the strength of transvection: addition of gypsy sequences induced stronger trans-activation than addition of HeT-A or yellow sequences. Only the promoter proximal region (within -158 bp of the yellow transcription start) was essential for trans-activation; i.e., transvection did not require extensive homology in the yellow upstream region. Finally, the yellow enhancers located on the two pairing chromosomes could cooperatively activate one yellow promoter.

ENHANCERS are cis-regulatory DNA elements that can activate gene transcription irrespective of their orientation or distance relative to the transcription start site (BLACKWOOD and KADONAGA 1998 Down; DORSETT 1999 Down; DILLON and SABBATTINI 2000 Down). A fundamental question in transcriptional regulation is how enhancers find and control their target promoters over long distances. The basic models proposed to explain the distal enhancer function invoke protein-protein interactions causing DNA looping, sliding of proteins along the DNA, or generation of large chromatin domains that facilitate or prohibit gene activation (BLACKWOOD and KADONAGA 1998 Down; DORSETT 1999 Down; DILLON and SABBATTINI 2000 Down; ENGEL and TANIMOTO 2000 Down; WEST et al. 2002 Down). New insight into long-distance communication between enhancer and promoter came from the finding that in some cases a promoter on one chromosome can be activated by enhancers on the paired homolog (GEYER et al. 1990 Down; GOLDSBOROUGH and KORNBERG 1996 Down; SIPOS et al. 1998 Down; PIRROTTA 1999 Down; WU and MORRIS 1999 Down). The common term for such events—transvection—was introduced by Lewis to describe mechanisms in Drosophila that underlie the sensitivity of expression of a gene to the proximity of its homolog (LEWIS 1954 Down). Examples of transvection include events of trans enhancer-promoter interactions at the Ultrabithorax (MARTINEZ-LABORDA et al. 1992 Down), Abdominal B (SIPOS et al. 1998 Down; ZHOU et al. 1999 Down), and yellow (GEYER et al. 1990 Down) genes.

The interchromosomal enhancer-promoter interaction was most clearly shown for the yellow gene. The latter is required for larval and adult cuticle pigmentation (NASH and YARKIN 1974 Down; WALTER et al. 1991 Down). The enhancers controlling yellow expression in the wings and body cuticle are located in the upstream region of the gene, whereas the enhancer controlling yellow expression in bristles resides in the intron (GEYER and CORCES 1987 Down; BIESSMANN and MASON 1988 Down; MARTIN et al. 1989 Down). The wing and body enhancers of one allele can trans-activate the yellow promoter on the paired homologous chromosome (GEYER et al. 1990 Down; MORRIS et al. 1999B Down). However, the cis-preference of enhancers for their own promoter precludes their action in trans (MORRIS et al. 1999B Down). These observations indicate that the yellow regulatory region is an excellent system to study the mechanisms of long-distance interaction between enhancer and promoter.

Recent studies demonstrate that yellow transvection can occur at multiple genomic locations and indicate that the Drosophila genome is generally permissive to enhancer action in trans (CHEN et al. 2002 Down). However, the features of the yellow gene required for transvection have not been fully assessed. The yellow gene is located close to the X chromosome telomere, which may play a role in chromosome pairing. It is obscure whether the yellow sequences located upstream of its promoter are required for transvection.

Here we used the yellow terminal deficiencies to examine the role of telomere sequences and the requirement of homologous sequences in the upstream yellow region. Several y alleles are known to complement y2, which laid a basis for transvection studies of the yellow gene (GEYER et al. 1990 Down; MORRIS et al. 1998 Down, MORRIS et al. 1999A Down). In the y2 mutation (Fig 1A), the gypsy retrotransposon is inserted between the enhancers controlling yellow expression in the wings and body cuticle and the yellow promoter (GEYER et al. 1986 Down). Gypsy contains the best-characterized insulator, which does not allow activation or repression to reach a promoter (PARKHURST and CORCES 1986 Down; GEYER 1997 Down; CORCES and FELSENFELD 2000 Down; BELL et al. 2001 Down). This insulator has binding sites for the Su(Hw) protein required for enhancer blocking (DORSETT 1990 Down; SPANA and CORCES 1990 Down; SCOTT et al. 1999 Down). After gypsy insertion, enhancers in the body and wing are blocked by insulation, while the bristle enhancer is active (GEYER et al. 1986 Down; GEYER and CORCES 1992 Down). When y2 is heterozygous with other mutant y alleles, like y1#8 and y59b, that have lesions in the promoter (Fig 1A), there is intragenic complementation, and the wing and body pigmentation strongly increases (GEYER et al. 1990 Down; MORRIS et al. 1998 Down, MORRIS et al. 1999A Down). The y82f29 allele, generated by deletion including the wing and body enhancers (Fig 1B), in combination with the y1#8 or y59 allele produces weaker pigmentation of the wing and body cuticle (MORRIS et al. 1999A Down). This difference in the strength of trans-activation was explained by suggesting that the wing and body enhancers of the y2 allele can bypass the Su(Hw) insulator as a result of pairing between the y alleles (Fig 1A; MORRIS et al. 1998 Down).



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  		Figure 1. A model to explain complementation patterns at the yellow locus (GEYER et al. 1990 Down; MORRIS et al. 1998 Down). The yellow alleles are drawn only approximately to scale. En-w, wing enhancer; En-b, body enhancer; Su(Hw)bs, Su(Hw)-binding site. The coding yellow region is shown as a solid box. The start of yellow transcription is shown by a horizontal arrow. (A) Transvection involving trans-acting y1#8 enhancers and/or cis-acting y2 enhancers. The body and wing enhancers in the y2 allele are blocked by the Su(Hw)bs. The y1#8 allele complements y2 to give flies nearly wild-type pigmentation. The model suggests that the wing and body enhancers of y1#8 act in trans on the promoter of the y2 allele. It is possible that the y2 enhancers bypass the Su(Hw) insulator and act on the y2 promoter. (B) Transvection involving trans-action of the y1#8 wing and body enhancers.

Using terminal gene conversion (MIKHAILOVSKY et al. 1999 Down) and generating HeT-A attachments on the Su(var)2-502 mutant background (SAVITSKY et al. 2002 Down), we obtained various terminal deletions in the regulatory regions of the y2, y82f29, and y+ alleles. Previously we found that the normal functioning of the yellow enhancers located at the tip of the chromosome required ~4 kb of additional upstream sequence (MIKHAILOVSKY et al. 1999 Down). Here we show that at least 6 kb of upstream sequences is essential for strong trans-activation of the yellow promoter located at the end of the truncated chromosome. Interestingly, addition of the gypsy sequences to the end of the truncated chromosome strengthens the transvection compared with the addition of HeT-A or the upstream yellow sequences. By comparing the strength of trans-activation of the yellow promoter in a number of truncated chromosomes bearing the HeT-A attachments to different parts of the yellow regulatory region, we found that only the upstream promoter region within -158 bp is essential for transvection.


*  MATERIALS AND METHODS
*TOP
 *ABSTRACT
 *MATERIALS AND METHODS
*RESULTS
 *DISCUSSION
 *LITERATURE CITED

Drosophila mutations and genetic crosses:
The y, y2, y82f29, y1#8, and y59b alleles were described in GEYER et al. 1986 Down, GEYER et al. 1990 Down and MORRIS et al. 1998 Down, MORRIS et al. 1999A Down, MORRIS et al. 1999B Down. The genetic symbols of the yellow alleles and their origin were described elsewhere (MIKHAILOVSKY et al. 1999 Down; KAHN et al. 2000 Down; SAVITSKY et al. 2002 Down). The Df(1)w, y1w67c23; Su(var)2-502/CyO, y+ line was obtained from J. Eissenberg. All other mutant alleles and chromosomes used in this work and all balancer chromosomes are described in LINDSLEY and ZIMM 1992 Down.

To test the effect of a su(Hw) background, the su(Hw)v/su(Hw)f trans-heterozygote (HARRISON et al. 1993 Down) was combined with y alleles as described in GEORGIEV and KOZYCINA 1996 Down.

To balance the deficient chromosome terminating in the yellow regulatory region, we used the y ac chromosome. This chromosome underwent deletion of the yellow gene and the regulatory region of the achaete gene, but not of any vital genes, and thus allowed us to examine the behavior of the yellow gene on the homologous chromosome in the absence of other yellow sequences.

To induce HeT-A transpositions to the end of the yellow terminal deficiency, we used the Su(var)2-502 mutation as described in SAVITSKY et al. 2002 Down. Breaks between -1200 and -140 bp result in the y2-like phenotype with yellow-colored aristae. Addition of a HeT-A sequence restores aristal pigmentation. HeT-A attachment to the yellow sequences upstream of -1500 bp partially restores the activity of the yellow body and wing enhancers. These observations allowed us to monitor the attachment of HeT-A to the yellow terminal sequences.

Complementation tests:
All crosses were conducted at 25° on standard medium. Wing refers to wing blades, and body refers to pigmentation in the abdominal stripes, not in the interstripe abdominal cuticle or thoracic cuticle. Routinely, five females were mated with two males in vials and brooded every second day. Temperature and crowding were controlled carefully, because both affect pigmentation. Pigmentation in the wing and body cuticle was scored in 3- to 4-day-old females on a five-point scale (MORRIS et al. 1998 Down): wild-type expression was ranked 5 while the absence of yellow expression was ranked 1. Pigmentation scores were assigned by comparing the progeny of flies obtained from parallel controls. Intermediate scores were determined relative to the pigmentation levels of y1#8/y1#8, y2/y2, y82f29/y1#8, and y2/y1#8 females, which in this and previous studies (MORRIS et al. 1998 Down; CHEN et al. 2002 Down) corresponded to scores of 1, 1; 1, 1–2; 3, 3; and 4, 4 in the wing and body, respectively. Pigmentation scores were determined by two people independently and represent an analysis of 30–50 female flies from each of two independent crosses. The small variations in fly pigmentation that depended on culture condition did not exceed 0.5 point. Scores listed in Table 1 Table 2 Table 3 represent the most common phenotype observed.


 
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  		Table 1. Complementation data for terminally deficient derivatives of the y82f29 allele


 
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  		Table 2. Complementation data for the terminally truncated derivatives of the y2 allele


 
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  		Table 3. Complementation data for the yTDH alleles

Molecular methods:
DNA from adult flies was isolated using the protocol described in ASHBURNER 1989 Down. The genomic DNA was digested with restriction enzymes according to the supplier's instructions and separated in standard agarose gels (SAMBROOK et al. 1989 Down). The DNA was transferred to Hybond N+ membranes and probed according to the supplier's instructions (Amersham, Piscataway, NJ). Subcloning and purification of the plasmid DNA and mapping of restriction sites were performed by standard techniques (SAMBROOK et al. 1989 Down).

The junctions between newly transposed mobile elements and the DNA terminus were cloned by DNA amplification with two oligonucleotide primers. The primers in the yellow gene were:

  • y1, 5' act tcc act tac cat cac gcc ag 3' (+421; +399);

  • y2, 5' aag acg gcg tca cca agg tga ct 3' (+229; +207);

  • y3, 5' gta acg act ggt ggc cat aat atg 3' (+9; -15);

  • y4, 5' cag gag gct cgt gca tag aat gc 3' (-439; -461);

  • y5, 5' att gga ttt cga ttg ggc gtc ac 3' (-744; -767);

  • y6, 5' gct cta atg acc atc gcc gca ag 3' (-978; -1100);

  • y7, 5' gtt caa ctt gat ccc ttg ccc gc 3' (-1382; -1404);

  • y8, 5' caa cat cag cgg agc gcg cta a 3' (-1814; -1835);

  • y9, 5' tcc agg aca aag ggt gga tcc 3' (+176; +196).

The nucleotide map positions relative to the yellow transcription start site (GEYER et al. 1986 Down) are given in parentheses.

The primers in the HeT-A element were:

  • h1, 5' tgt tgc aag tgg cgc gca tcc 3' (456–434);

  • h2, 5' ggt gct tcc gta ctt ctg gcg g 3' (359–338);

  • h3, 5' ccc aaa ctc acc cca tcc aat g 3' (141–120).

The nucleotide map positions according to the sequence of the HeT-A element (BIESSMANN et al. 1992 Down) are given in parentheses.

The amplification products were fractionated by electrophoresis in 0.8% agarose gels in TAE. The successfully amplified products were cloned in a Bluescript plasmid (Stratagene, La Jolla, CA) and sequenced using a sequence kit (Amersham).

The DNA attachment in the yTDF allele was cloned by an invert-PCR technique. DNA isolated from yTDF flies was cleaved with BamHI; 2.4 to 3.0-kb DNA fragments were isolated from the gel, purified, and ligated. The required DNA fragment was amplified between primers y4 and y9 and cloned into the pSK vector.


*  RESULTS
*TOP
 *ABSTRACT
 *MATERIALS AND METHODS
 *RESULTS
*DISCUSSION
 *LITERATURE CITED

Trans-activation of the yellow promoter at the tip of the deficient chromosome requires ~6 kb between the promoter and the end of the terminal deficiency:
To assess whether the yellow promoter located at the end of the deficient chromosome could be trans-activated by the yellow enhancer located on the homologous chromosome, we selected five lines with the chromosome terminating in the region from 400 to 800 bp upstream of the yellow transcription start site. The chromosomes carrying yellow terminal deficiencies (abbreviated as yTD) were balanced over the y ac w chromosomes bearing a deficiency of the yellow-achaete region. The yTD/y ac w females displayed a y2-like phenotype: yellow wing and body cuticle and pigmented bristles.

To test the intragenic complementation, the yTD alleles were placed in trans to y1#8 or y59b. For the complementation tests, two alleles were considered to complement each other if the scores in the wings or body for a trans-heterozygote were at least one point darker on the pigmentation scale than those for females heterozygous in either allele and in y ac. All trans-heterozygous females obtained had pigmentation scores of 1 in wing and body tissue as control yTD/y ac w females (data not shown). Thus, the body and wing enhancers located on the y1#8 or y59b chromosome failed to trans-activate the yellow promoter if it was located close to the end of the deficient chromosome.

To determine the distance between the end of the deficient chromosome and the yellow promoter that is required for trans-activation, we used the method of terminal chromosome elongation by gene conversion, which allows different combinations of the regulatory elements to be generated at the same genomic position (MIKHAILOVSKY et al. 1999 Down). As a template for terminal gene conversion, we used the y82f29 allele with a 4.1-kb deletion removing the wing and body enhancers (Fig 3A; MORRIS et al. 1998 Down). Flies of the y82f29/y1#8 or /y59b genotypes had pigmentation scores of 3 in both wing and body, suggesting trans-activation of the y82f29 promoter by the enhancer located on the homologous chromosome (MORRIS et al. 1998 Down).



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  		Figure 2. Schemes used to obtain terminal DNA elongation. (A) The genetic scheme to obtain deficient chromosomes ending in different regions of the y82f29 allele. (B) The genetic scheme to obtain deficient chromosomes ending in different regions of the y2 allele. (C) The genetic scheme for isolation of individual stable lines bearing terminally truncated chromosomes with new HeT-A attachment. yTD* indicates the y allele with new phenotype (new HeT-A attachment).



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  		Figure 3. Structure of the y82f29 derivatives. (A) Schematic presentation of terminal yellow deficiencies. The y82f29 allele is generated by a 4.1-kb deletion, which is indicated. Each vertical arrow marks the approximate region of the end of the deficient chromosome in the particular case. B, BamHI; C, ClaI; G, BglII; H, HindIII; K, KpnI; E, EcoRV; P, PstI; S, SpeI. The genomic DNA fragment PstI-ClaI used for Southern blot analysis is indicated by the thick line. Other designations are as in Fig 1. (B) Southern blot analysis of DNAs prepared from y82f29 flies and flies with derivative yTD82f alleles. The DNAs were digested with BamHI or KpnI. The filters were hybridized with the PstI-ClaI probe.

By Southern blot analysis, we selected the yTD+100 line with a deficient chromosome terminating ~100 bp downstream of the yellow transcription start site. The yTD+100 flies had a y-null phenotype because of deletion of the yellow promoter. To induce terminal gene conversion, the yTD+100 wa chromosome was paired with the y82f29w chromosome (Fig 2A). The yTD+100wa/y82f29w females were crossed to y82f29w males for three subsequent generations. To select the derivative yTD alleles with terminal DNA addition, yTD+100wa/y82f29w females were crossed to y ac w males. yTD*wa/y ac w females displaying y2-like phenotype were selected and individually crossed with y ac males. In the next generation, yTD*wa/y ac females were crossed with y ac males. The size of terminal DNA elongation in the derivative yTD lines was examined by Southern blot analysis (Fig 3B). As a result, we selected nine derivative lines with the deficient chromosome extended to reach between -1700 and -6100 bp relative to the yellow transcription start site. Since the y82f29 allele was used for terminal DNA elongation, we named all newly obtained terminally deficient alleles as yTD82f. Flies bearing any yTD82f in trans to y ac were fully mutant in wings and body, with scores of 1 for both tissues (Table 1). If the distance between the yellow promoter and the end of the deficient chromosome was <=4000 bp, flies bearing such yTD82f in trans to y1#8 or y59b showed no pigmentation in the body and wing (Table 1). The yTD82f-8 allele, which had the end of the truncated chromosome at -4800 bp, complemented weakly only with y1#8 but not with y59b (Table 1). The yTD82f-9 allele produced better complementation with y1#8 or y59b; it had ~6000 bp between the yellow promoter and the end of truncated chromosome (Fig 3), suggesting that this distance is essential for transvection.

Gypsy facilitates trans-activation of the yellow promoter at the end of the truncated chromosome:
Next, we examined how gypsy sequences at the end of the deficient chromosome would influence the strength of transvection. For this purpose, we generated a number of lines with the chromosomes ending at different parts of gypsy inserted in the y2 allele (Fig 2B).

By Southern blot analysis, two yTDw lines were selected carrying deficient chromosomes terminating ~400 bp downstream of the yellow transcription start site. To select a proper combination of the y alleles, we used the z mutation as a marker. To induce terminal gene conversion, the yTDw chromosomes were paired with the y2z homologs containing the y2 allele as a template for terminal gene conversion (Fig 2B). In the next generation, yTDw/y2z females were crossed to y2z males. The yTDw/y2z females had red eyes, while homozygous y2z/y2z females had yellow eyes. After three generations, in which terminal DNA elongation could occur, yTDw/y2z females were individually crossed to y59bz males to select yTDw/y59bz females with darker wing and body pigmentation (partial or complete complementation). In the next generation, we selected six independent yTDw/y59bz females (red eyes) that had pigmented wing and body cuticle. Flies with the same yTD alleles balanced over y ac w had pigmentation scores 1, 1 in body and wings (Table 2), suggesting that pairing with the y59b allele is required for wing and body pigmentation. Since the y2 allele was used as a template for the terminal DNA elongation, the terminally deficient alleles obtained were named yTD2.

To determine the end of the deficient chromosome, DNA samples isolated from yTD2 lines were studied by Southern blot analysis (Fig 4C). The yTD2-3, yTD2-4, and yTD2-5 had the end of the truncated chromosome between -4200 and -3800 bp relative to the yellow transcription start site. Flies of genotypes yTD2-3, yTD2-4, or yTD2-5 vs. y1#8 or y59b had pigmentation scores of 2–3 in body and 3 in wings (Table 2), suggesting that ~4000 bp from the yellow promoter is enough for trans-activation of the yellow promoter in this case. However, flies with yTD2-1 or yTD2-2 in trans to y1#8 or y59b had the maximum pigmentation scores of 4 in both wing and body, as did y2/y1#8 flies (Table 2). This result shows that strong transvection can be reproduced at the end of a deficient chromosome, and the telomere sequences are not permanently required for the pairing between the y alleles. The yTD2-1 and yTD2-2 alleles had the ends of the truncated chromosomes at -10,000 and -6000 bp, respectively (Fig 4A and Fig C). Thus, an ~6000-bp distance between the promoter and the end of the truncated chromosome is required for strong transvection.



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  		Figure 4. Structure of the y2 derivatives. (A) Schematic presentation of terminal yellow deficiencies ending in the gypsy or distal yellow enhancers. Vertical arrowheads approximately mark the end of the truncated chromosome in each particular case. The genomic DNA fragment HindIII-BamHI used for Southern blot analysis is indicated by the thick line. B, BamHI; C, ClaI; H, HindIII; K, KpnI; E, EcoRV; S, SpeI; N, NcoI; O, XhoI; X, XbaI; V, PvuII. Other designations are as in Fig 1. (B) Schematic presentation of the yTDF allele and its derivatives. The primers used to clone the F-element attachment are indicated by arrowheads. Shown below is the junction between the F element and gypsy in the yTDF allele. The F element is attached at 1003 bp of the gypsy sequence (MARLOR et al. 1986 Down). Frames mark the Su(Hw)-binding sites. Lowercase letters indicate the new sequence, including the ClaI site at the F-gypsy junction. (C) Southern blot analysis of DNAs prepared from the yTD2 alleles. The DNAs were digested with BamHI. The filters were hybridized with the HindIII-BamHI probe. The unmarked lanes correspond to the short DNA attachments that we did not use in the transvection experiments. (D) Southern blot analysis of DNAs prepared from the yTDF alleles. To determine the structure and size of new DNA attachment in yTDF, the DNAs of y2 and yTDF flies were digested with BamHI and PvuII, with BamHI, with BamH and XbaI, with BamHI and XhoI, with BamHI and NcoI, with BamHI and ClaI, or with SpeI. The filters were hybridized with the HindIII-BamHI probe. To map the end of the deficient chromosome in the yTDF derivatives, DNAs were digested with EcoRV. To verify the origin of the yTDF derivatives, DNAs were digested with BamHI and ClaI. The ClaI site is located at the junction between the F element and gypsy.

As found previously (BIESSMANN and MASON 1988 Down, BIESSMANN and MASON 1997 Down), chromosomes lose DNA sequences from the broken end at the same rate of 70–80 bp/generation. After maintaining yTD25/y1#8 flies for several months, we found females with less pigmented or nonpigmented wing and body cuticle. Southern blot analysis showed that in the new yTD25 derivatives truncated chromosomes ended in the region between -2800 bp (yTD26) and -1300 bp (yTD29) relative to the yellow transcription start site (Fig 4A and Fig C; Table 2). Thus, there is no trans-activation if the distance between the promoter and the end of the truncated chromosome is <3 kb.

One of the yTD2 alleles had a large DNA addition with a restriction map unrelated to the gypsy or yellow sequences (Fig 4D). Southern blot analysis showed that the new DNA is attached to the 5' LTR of gypsy: the XhoI and XbaI restriction sites located in the LTR were retained, while the NcoI site following the Su(Hw)-binding site was removed (Fig 4D). To elucidate the nature of the new DNA attachment, the DNA fragment adjacent to the gypsy LTR was cloned by the inverse PCR technique with the y4 and y9 primers shown in Fig 4B. Sequencing of the cloned DNA showed that the newly added DNA sequence was derived from an F element attached to the twelfth Su(Hw)-binding site of gypsy (Fig 4B). Hence this yTD2 allele was renamed as yTDF. Flies of the genotype yTDF/y1#8 or yTDF/y59b had scores of 4 in both wing and body (Table 2). Upon observing the yTDF/y1#8 line for several generations, two females were isolated that had no pigmentation (score 1) in the body and wings. By Southern blot analysis, the ends of the truncated chromosomes in these yTDF derivatives were mapped at ~-2400 bp (yTDF-1) and -3100 bp (yTDF-2) relative to the yellow transcription start site (Fig 4B and Fig D). Thus, these results again show that the distance between the yellow promoter and the end of the deficient chromosome has to be >3.5 kb to provide any transvection.

The yTD2 and yTDF alleles have the Su(Hw) insulator that might be responsible for the effective transvection. The Su(Hw) protein binds to the Su(Hw) insulator and is responsible for its activity (DORSETT 1990 Down; SPANA and CORCES 1990 Down; HOLDRIDGE and DORSETT 1991 Down; SCOTT et al. 1999 Down). To find out the role of the Su(Hw) insulator in transvection between the y alleles, we obtained the yTDF/y1#8 and yTD2-2/y1#8 trans-heterozygotes on the su(Hw)- background, which proved to have no effect on fly pigmentation (data not shown). Thus, the Su(Hw) insulator is not required to facilitate trans-activation of the yellow promoter at the end of the truncated chromosome.

Role of the yellow upstream regulatory sequences in transvection between the yellow alleles:
The existence of transvection at the end of the truncated chromosome offers an opportunity to assess the role of the upstream yellow sequences in trans-activation of the yellow promoter. SAVITSKY et al. 2002 Down described a number of truncated chromosomes carrying HeT-A attachments to the yellow regulatory region. For the complementation test, we selected the yTD alleles that had HeT-A attachments >7 kb (Fig 5B). To distinguish the yTD alleles generated by attachment of HeT-A to the yellow 5' regulatory region, we named them yTDH.



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  		Figure 5. Structure of the yTDH alleles. (A) Schematic presentation of terminal yellow deficiencies associated with different y phenotypes. The locations of promoter (TATA) and start of translation (ATG) are indicated. Other designations are as in Fig 3. The thin horizontal lines cover the regions of yellow sequence in which the termini of the yTD line that correspond to the same class of the yTDH alleles have been mapped. The points of HeT-A attachment are shown by vertical arrowheads with positions relative to the yellow transcription start site. For the A, B, and C classes of the yTDH alleles, only the HeT-A attachments delimiting the boundary of the class are indicated. The KpnI-EcoRV genomic fragment used as a probe for Southern blot analysis is indicated by the thick line. (B) Example of the Southern blot analysis to determine the size of the HeT-A attachments. DNAs were digested with EcoRV. The filter was hybridized with the KpnI-EcoRV probe. Only the HeT-A attachments >7 kb are indicated. Asterisks indicate DNA attachments with the site for EcoRV, as the same DNA samples were digested with SpeI-produced fragments >7 kb (data not shown). The unmarked lanes correspond to the short DNA attachments that we did not use in the transvection experiments.

We also obtained additional HeT-A attachments by crossing the yTD alleles with the Su(var)2-502 mutation that strongly induced HeT-A transposition to the chromosome end (Fig 2C). Eight yTD/y ac; If/CyO lines carrying deficiencies ending at -2800 to -300 bp were selected with the aid of Southern blot hybridization. The yTD/y ac; If/CyO females were crossed to y ac; Su(var)2-502/CyO males as shown in Fig 2C. In the offspring, yTD/y ac; Su(var)2-502/CyO females were crossed to y ac; Su(var)2-502/CyO males for three to seven generations to determine the appearance of flies with the new y phenotype. To establish stable yTDH lines, the Su(var)2-502 mutation was crossed out from the individual yTDH/y ac; Su(var)2-502/CyO females. As a result, new HeT-A additions were selected in the yTDH/y ac; If/CyO progeny.

To find out the precise site of HeT-A attachments to the yellow sequences, the junctions between terminal yellow sequences and new DNA attachments were cloned by PCR and sequenced (Fig 5A; Table 3). The PCR primers were located in the yellow gene and in the conserved regions from the 3' ends of HeT-A. A number of new HeT-A attachments were obtained in the region of the wing and body enhancers. As shown previously (MIKHAILOVSKY et al. 1999 Down), the wing and body enhancers are inactive at the end of the deficient chromosome. Large HeT-A attachments restored activation of the yellow promoter by the enhancers (Table 3, classes D and E).

The ability of each yTDH allele to support transvection was assessed in combination with y1#8 or y59b. The complementation tests defined five classes of the yTDH alleles. No transvection was determined in the yTDH alleles that have HeT-A attachments in the region between -80 and +165 bp around the yellow transcription start site (Table 3, class A). The promoter located at the 3' end of the HeT-A element (DANILEVSKAYA et al. 1997 Down) can substitute for the deleted yellow promoter and drive yellow expression in bristles (BIESSMANN et al. 1990B Down; KAHN et al. 2000 Down). However, lack of complementation suggests that the yellow enhancers are not able to trans-activate the HeT-A or yellow promoter in the absence of upstream yellow sequences.

In class B, flies of genotype yTDH/y1#8 or yTDH/y59b had pigmentation scores of 1–2 for the wing and 1 for the body. These yTDH alleles had HeT-A attachments in the small region between -98 and -116 bp. In class C, flies of genotype yTDH/y1#8 or yTDH/y59b had pigmentation scores of 2 or 2–3 for the wing and 1–2 or 2 for the body. Class C includes the yTDH alleles with the HeT-A attachments in the region between -158 and -1142 bp. All the yTDH alleles of classes A, B, and C in heterozygous yTDH/y ac flies had pigmentation scores of 1 for both the wing and the body cuticle (Table 3). These results suggest that the promoter proximal region between the TATA box and -158 bp is essential for trans-activation of the yellow promoter by the wing and body enhancers located on the homologous chromosome, whereas the yellow upstream region between -158 and -1142 bp has no effect on transvection efficiency.

Cooperation between enhancers located on the pairing chromosomes in activation of the yellow promoter:
In class D, flies of genotype yTDH/y ac displayed different levels of yellow activation in the wing and body (Table 3). The addition of the sequences corresponding to the body and wing enhancers gradually increased the level of pigmentation. The yTDH-1491/y ac flies had pigmentation scores of 1 for the wing and 2 for the body, while the yTDH-2097/y ac flies had scores of 2–3 for the wing and 5 for the body. Other yTDH/y ac flies of class D displayed the pigmentation level of intermediate scores. The yTDH-2491/y ac and yTDH-2576/y ac flies produced a wild-type level of pigmentation, suggesting that both body and wing enhancers are localized downstream of -2491 bp (class E). The complementation analysis with each of the class D yTDH alleles showed that yTDH/y1#8 or y59b flies had scores 1 or 2 points higher than yTDH/y ac flies. This result may be explained by coactivation of the yellow promoter in the yTDH/y1#8 or y59b flies by the enhancers located on the paired chromosomes.

To further study the cooperation between the yellow enhancers located on the homologous chromosomes, we used y2. In this y allele the Su(Hw) insulator blocks the wing and body enhancers (GEYER et al. 1986 Down). Flies of the y82f29/y2 genotype have pigmentation scores of 1 and 1–2 for wing and body tissues, respectively (MORRIS et al. 1998 Down, MORRIS et al. 1999A Down). Thus, the wing and body enhancers located on the y2 chromosome fail to activate the yellow promoter on the pairing y82f29 chromosome. The same results were obtained in intragenic complementation tests between class C yTDH alleles and y2 (Table 3). These observations can be explained assuming that the Su(Hw) insulator blocks cis and trans interactions between the yellow enhancers and promoter. However, the yTDH alleles of class D complement with y2. Flies of the yTDH(D)/y2 genotype had darker pigmentation of the wing and body cuticle than yTDH(D)/y ac flies (Table 3). To exclude the role of the y2 promoter in the complementation, we used the yvsA3 allele that was generated by deletion of the -146 to -70 bp upstream promoter sequences in y2 (BELENKAYA et al. 1998 Down). This deletion strongly diminishes yellow expression because of inactivation of the promoter. The yTDH(D)/yvsA3 flies had wing and body pigmentation similar to that of yTDH(D)/y2 flies (Table 3), suggesting that the y2 promoter is not involved in yellow activation. Hence, again the cooperation in the promoter activation between the yellow enhancers located on the y2 and yTDH(D) paired chromosomes can explain the complementation between y2 or yvsA3 and yTDH alleles.

To confirm the role of pairing between y alleles in this complementation, we made use of the previous observation that insertion of another gypsy into the neighboring scute locus (scD1 mutation) partially hinders transvection between y2 and y59b or y1#8, presumably because of the disruption of proper chromosomal synapsis between the yellow alleles (GEYER et al. 1990 Down; GAUSE and GEORGIEV 2000 Down). It is also possible that the interaction between the Su(Hw) insulators located in the yellow (y2) and scute (scD1) loci partially blocks the ability of the wing and body enhancers to activate the yellow promoter in trans (GAUSE and GEORGIEV 2000 Down). In this study we used the y2scD1waG line and the derivative line y1u1scD1waG. The null y1u1 allele was generated by insertion of the retrotransposon Stalker into the coding yellow region of the y2 allele (GEORGIEV et al. 1990 Down). Flies of genotype yTDH(D)/y2scD1 or yTDH(D)/y1u1scD1 had scores intermediate between yTDH(D)/y ac and yTDH(D)/y2 flies (Table 3). Thus, the inability of the yellow enhancers to efficiently act in trans in the presence of scD1 partially suppresses the complementation between the y2 and yTDH(D) alleles. This result supports the assumption that the y2 enhancers are involved in activation of the yTDH promoter in trans-heterozygous flies.


*  DISCUSSION
*TOP
 *ABSTRACT
 *MATERIALS AND METHODS
 *RESULTS
 *DISCUSSION
*LITERATURE CITED

Transvection can occur at the end of the truncated chromosome:
Telomeres in Drosophila melanogaster are very different from those in other eukaryotes (BIESSMANN and MASON 1997 Down; PARDUE and DEBARYSHE 1999 Down, PARDUE and DEBARYSHE 2000 Down). They consist of a terminal array of HeT-A and TART retrotransposons, which perform the elongation function that is performed by telomerase in other eukaryotes, and of a relatively short subtelomeric satellite, called TAS (MASON et al. 2000 Down). Corepression of the transposons inserted in TAS of different telomeres suggests interaction between telomeres in Drosophila (GOLUBOVSKY et al. 2001 Down). The yellow gene resides ~100 kb from the X chromosome telomere (ADAMS et al. 2000 Down). Thus, the presence of a telomere may be important for establishing the allele proximity necessary for trans-regulatory interactions.

Terminal deletions in Drosophila have been obtained (BIESSMANN and MASON 1988 Down; TRAVERSE and PARDUE 1988 Down; LEVIS 1989 Down; BIESSMANN et al. 1990A Down; MIKHAILOVSKY et al. 1999 Down; GOLUBOVSKY et al. 2001 Down). Drosophila broken chromosomes behave as capped ones: they are stably transmitted through many generations (LEVIS 1989 Down; BIESSMANN et al. 1990A Down). One protein that is required for capping is HP1, which binds to the telomere and terminal deficiencies (FANTI et al. 1998 Down).

Our previous results indicate that the yellow enhancers do not function properly when located very near the chromosome end (MIKHAILOVSKY et al. 1999 Down). However, further addition of upstream yellow sequences gradually increased the level of pigmentation, and wild-type levels were established when a sequence of ~4 kb distal to the yellow enhancers was added. Here we found that the yellow enhancers are not able to trans-activate the yellow promoter if the latter is located close to the end of the deficient chromosome. To explain these results, we propose that the hypothetical end-binding complex occupies ~4–6 kb of terminal DNA and interferes with long-distance communication between the yellow enhancers and promoter.

Addition of HeT-A or the upstream yellow sequences only partially restored the transvection as compared with the y82f29 allele generated by deletion of the upstream yellow enhancers. This observation supports the significance of the telomere sequences deleted from the terminally truncated chromosome for chromosome pairing that is required for trans-activation of the yellow promoter. However, the presence of gypsy sequences at the end of the truncated chromosome restores efficient transvection. Interestingly, the Su(Hw) protein, the major functional component of the insulator, is apparently not required to facilitate transvection. The gypsy sequences, but not the Su(Hw) insulator, negatively influence yellow transcription (BELENKAYA et al. 1998 Down), excluding the possibility of direct positive action of the gypsy sequences on the yellow promoter. The presence of the gypsy sequences only in the terminally deficient chromosome argues against the possibility that the pairing between gypsy sequences facilitates transvection. The possible explanation of the gypsy activity comes from the recent finding that gypsy is frequently located at the nuclear envelope (GERASIMOVA et al. 2000 Down). Thus, the gypsy sequences may stabilize interaction between the end of the terminally truncated chromosome and the nuclear envelope. It was shown that the yeast telomeres are positioned in clusters adjacent to the nuclear envelope (HEDIGER and GASSER 2002 Down). The interaction between the regulatory elements located on the different Drosophila telomeres suggests that telomeres interact with each other to assess their integrity (GOLUBOVSKY et al. 2001 Down). This interaction might stabilize pairing between homologous chromosomes that reinforces the transvection.

Trans-interaction between the yellow enhancers and promoter:
Here we found that only ~130 bp upstream of TATA is significant for trans-activation of the yellow promoter (Fig 6A and Fig B). Interestingly, the upstream yellow sequences distal to -158 bp do not substantially influence the efficiency of trans-activation of the yellow promoter. Thus, no extensive homology upstream to the yellow promoter is required for the transvection.



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  		Figure 6. Models. The yellow alleles are drawn only approximately to scale. En-w, wing enhancer; En-b, body enhancer; Su(Hw)bs, Su(Hw)-binding site. The coding yellow region is shown as a solid box. The start of yellow transcription is shown by a horizontal arrow. The upstream promoter region required for transvection is shown as an open bar.

Our results suggest that the yellow enhancers located on the two pairing chromosomes can cooperatively activate one yellow promoter (Fig 6C). Previous studies (GEYER and CORCES 1987 Down; MARTIN et al. 1989 Down; MORRIS et al. 1998 Down) and our unpublished results (M. SAVITSKY, O. KRAVCHUK and P. GEORGIEV) suggest that the wing and body enhancers spreading over a 2-kb region consist of many separate modules, which cooperatively activate the yellow promoter. Hence it is not surprising that the enhancer modules can cooperate in trans in the case of pairing between y alleles located on the homologous chromosomes. Alternatively, the increase of yellow expression might be explained by the suggestion that the yellow promoter is activated by the enhancers located in cis in some cells and by the enhancers located in trans in other cells. Therefore the presence of the additional enhancers in trans increases the probability of yellow activation.

The complementation between the yTDH (class D) alleles and y2 (Fig 6D and Fig E) may also be explained by the interaction between the y2 and yTDH yellow enhancers that helps to bypass the gypsy insulator. However, the complementation between these alleles can also be explained by the model of MORRIS et al. 1998 Down, on the basis of the striking complementation between y2 and y3c3 alleles. The y3c3 allele, in which a deletion removes the body enhancer and promoter, complements y2 for both wing and body expression, demonstrating that the body enhancer in y2 is not insulated by Su(Hw). The simplest interpretation is that homologous chromosome pairing forces gypsy and other unpaired sequences out in a loop, thereby bringing the body enhancer in physical proximity to the promoter. Complementation between the yTDH (class D) alleles and y2 may also be explained by the suggestion that pairing between the yellow sequences extending from -700 bp, the site of gypsy insertion in y2, to the HeT-A attachment helps in looping out the gypsy, which facilitates the trans-interaction between the y2 enhancers and the yTDH promoter. We think that the last mechanism is unlikely, because it implies strong pairing between relatively short yellow sequences. However, at this moment it is impossible to discriminate between these two models.


*  FOOTNOTES

1 Present address: Department of Zoology, University of Geneva, CH1211 Geneva, Switzerland. Back


*  ACKNOWLEDGMENTS

This work was supported by the Russian State Program "Frontiers in Genetics," the Russian Foundation for Basic Research; by an International Research Scholar award from the Howard Hughes Medical Institute to P.G.; and by the Volkswagen-Stiftung Foundation, Federal Republic of Germany.

Manuscript received September 13, 2002; Accepted for publication January 6, 2003.


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