Two Genes Become One: The Genes Encoding Heterochromatin Protein SU(VAR)3-9 and Translation Initiation Factor Subunit eIF-2{gamma} Are Joined to a Dicistronic Unit in Holometabolic Insects

Two Genes Become One: The Genes Encoding Heterochromatin Protein SU(VAR)3-9 and Translation Initiation Factor Subunit eIF-2 ${gamma}$ Are Joined to a Dicistronic Unit in Holometabolic Insects

Veiko Krauss^a and Gunter Reuter^a
^a Institute of Genetics, Martin Luther University Halle-Wittenberg, D-06108 Halle, Germany

Corresponding author: Veiko Krauss, Department of Genetics, University of Leipzig, D-04103 Leipzig, Johannisallee 21–23, Germany., krauss{at}rz.uni-leipzig.de (E-mail)

Communicating editor: J. A. BIRCHLER

ABSTRACT

TOP
ABSTRACT
MATERIALS AND METHODS
RESULTS
DISCUSSION
LITERATURE CITED

The Drosophila suppressor of position-effect variegation Su(var)3-9encodes a heterochromatin-associated protein that is evolutionarilyconserved. In contrast to its yeast and mammalian orthologs,the Drosophila Su(var)3-9 gene is fused with the locus encodingthe ${gamma}$ subunit of translation initiation factor eIF2. Synthesisof the two unrelated proteins is resolved by alternative splicing.A similar dicistronic Su(var)3-9/eIF-2 ${gamma}$ transcription unit wasfound in Clytus arietis, Leptinotarsa decemlineata, and Scoliopterixlibatrix, representing two different orders of holometabolicinsects (Coleoptera and Lepidoptera). In all these species theN terminus of the eIF-2 ${gamma}$ , which is encoded by the first two exons,is fused to SU(VAR)3-9. In contrast to Drosophila melanogaster,RT-PCR analysis in the two coleopteran and the lepidopteranspecies demonstrated the usage of a nonconserved splice donorsite located within the 3' end of the SU(VAR)3-9 ORF, resultingin removal of the Su(var)3-9-specific stop codon from the mRNAand complete in-frame fusion of the SU(VAR)3-9 and eIF-2 ${gamma}$ ORFs.In the centipede Lithobius forficatus eIF-2 ${gamma}$ and Su(var)3-9 areunconnected. Conservation of the dicistronic Su(var)3–9/eIF-2 ${gamma}$ transcription unit in the studied insects indicates its originbefore radiation of holometabolic insects and represents a usefultool for molecular phylogenetic analysis in arthropods.

DURING recent years molecular analysis has revealed severalinteresting exceptional types of gene organization in eukaryotes(BLUMENTHAL 1998 ). These include cases where several genesare arranged into a multicistronic unit expressed from a singlepromoter. The polycistronic pre-mRNA is processed by alternativeor trans-splicing to monocistronic mRNAs. In Caenorhabditiselegans $~$ 25% of the genes are estimated to be contained in polycistronicunits (ZORIO et al. 1994 ). Dicistronic transcription unitsthat are resolved by alternative splicing were documented inC. elegans unc-17/cha-1, Drosophila ChAT/VAChT, and mammalianUOG-1/GDF-1 (LEE 1991 ; ALFONSO et al. 1994 ; KITAMOTO etal. 1998 ). A similar gene structure was found for the sesB/Ant2genes in Drosophila (ZHANG et al. 1999 ). In contrast the Adh/Adhrlocus of Drosophila melanogaster is transcribed as one dicistronicmRNA (BROGNA and ASHBURNER 1997 ).

Here we describe another dicistronic transcription unit thatevolved by the fusion of two functionally unrelated genes: thesuppressor of position-effect variegation Su(var)3-9 and thegene encoding the ${gamma}$ subunit of translation initiation factoreIF-2. The eIF-2 ${gamma}$ protein binds GTP and the initiator ^MettRNAat translation initiation (ERICKSON and HANNIG 1996 ) whereasSU(VAR)3-9 is a heterochromatin-associated protein involvedin chromatin condensation (TSCHIERSCH et al. 1994 ; SCHOTTAand REUTER 2000 ). Heterochromatin-associated proteins (HPs)were first identified by dominant modifier mutations of position-effectvariegation (PEV) in Drosophila (REUTER and SPIERER 1992 ; WEILER and WAKIMOTO 1995 ; WALLRATH 1998 ). Three differentHPs have been studied in more detail: the HP1 chromo domain(JAMES and ELGIN 1986 ; EISSENBERG et al. 1992 ), the SU(VAR)3-7zinc finger (CLEARD et al. 1997 ), and the SU(VAR)3-9 chromoand SET domain protein (TSCHIERSCH et al. 1994 ). HP1 and SU(VAR)3-9are evolutionarily conserved. Su(var)3-9 orthologs were identifiedin Schizosaccharomyces pombe (Clr4; IVANOVA et al. 1998 ) andin mice and humans (SUV39h1/SUV39H1; AAGAARD et al. 1999 ).Molecular analysis of the Su(var)3-9 genomic region in Drosophilarevealed a unique gene structure (TSCHIERSCH et al. 1994 ).The D. melanogaster SU(VAR)3-9 sequences are encoded by a specificexon within intron 2 of eIF-2 ${gamma}$ . The mRNAs of the two genes areproduced by alternative splicing. SU(VAR)3-9 becomes fused tothe N-terminal 80 amino acids of eIF-2 ${gamma}$ encoded by the firsttwo exons. This unusual gene structure is not found in fissionyeast or mammals. Human eIF–2 ${gamma}$ and SUV39H1 are both X chromosomalgenes but are located at distant regions (Xp21 and Xp11.2, respectively; GERAGHTY et al. 1993 ; EHRMANN et al. 1998 ).

Here we show that the fusion of Su(var)3-9 and eIF-2 ${gamma}$ into adicistronic transcription unit is conserved in holometabolicinsects. It is not found in the centipede Lithobius forficatus.In D. melanogaster SU(VAR)3-9 is fused to the 80 N-terminalamino acids of eIF-2 ${gamma}$ whereas in the coleopteran and lepidopteranspecies studied in addition alternative splicing at a nonconservedsplice donor site at the 3' end of the SU(VAR)3-9 open readingframe (ORF) results in a complete fusion of the SU(VAR)3-9 andeIF-2 ${gamma}$ ORFs.

MATERIALS AND METHODS

TOP
ABSTRACT
MATERIALS AND METHODS
RESULTS
DISCUSSION
LITERATURE CITED

Study specimens:
D. erecta was received from Umea European Drosophila Stock Center.Adult specimens of Leptinotarsa decemlineata and L. forficatuswere captured around Halle (Sachsen-Anhalt, Germany). AdultClytus arietis and Scoliopterix libatrix were captured nearNebra (Sachsen-Anhalt) and Ruhla (Thüringen, Germany),respectively. From each species one individual was used forRNA isolation (Trizol reagent; Life Technologies) and RT-PCRanalysis. Two other individuals from each species were usedfor independent DNA isolation and PCR analysis of genomic fragmentsto evaluate DNA polymorphisms.

Sampling DNA sequences:
Sequences of primers and their positions within the correspondinggenes can be found in Table 1 and Fig 1, respectively. Su(var)3-9-specificsequences of $~$ 1 kb length were isolated with the degeneratedprimer pair chromo800 and chromo1790 from C. arietis and S.libatrix. Partial eIF-2 ${gamma}$ cDNAs from C. arietis, S. libatrix,L. decemlineata, and L. forficatus were isolated by reversetranscriptase (RT)-PCR using degenerate primers EF120 and EF440.Thereafter, for each of the studied species, a separate sequencesampling strategy was applied: In Scoliopterix, genomic PCRfragments were generated using the primer pairs EF120/Sco4-1and Sco4-3/EF440. The genomic region including exons 1 and 2was amplified by inverse PCR using primers Sco1-5, Sco2, andSco4-3. The exon-intron structure at the 5' end of ScoliopterixeIF-2 ${gamma}$ was determined after RT-PCR using the primers Sco5-1,Sco5-2 (5' to the putative translation start point), and primerSco8-2 (inside exon 3). Similarly, the splicing of Su(var)3-9was determined by RT-PCR using the primers Sco5-1, Sco5-2, Sco1-4,and Sco4-2 for the 5' end; and Sco4-3, Sco4-4, Sco8-1, and Sco8-2at the 3' end of the Su(var)3-9-specific exon (2a). 5' rapidamplification of cDNA ends (RACE) and 3' RACE products couldnot be generated from this species.

View larger version (17K):
In this window
In a new window
Download PPT slide

Figure 1. The Su(var)3-9/eIF-2 ${gamma}$ dicistronic transcription unit of four insect species and the eIF-2 ${gamma}$ gene of the centipede Lithobius. The commonly accepted phylogenetic relationships (FORTEY and THOMAS 1998

) of the analyzed arthropod species are indicated by the tree. Dm, D. melanogaster; Sl, S. libatrix; Ca, C. arietis; Ld, L. decemlineata; Lf, L. forficatus; and pA, poly(A) tail. The nomenclature of the exon-intron structure is given at the top. Introns are in open boxes and exons are in solid boxes. The eIF-2 ${gamma}$ transcript part of L. decemlineata containing undetermined intron positions is in a shaded box. All eIF-2 ${gamma}$ exons are in yellow boxes, the chromo domain coding regions are indicated in red, the SAC domain coding regions are in green, and the SET domain coding regions are marked blue. Positions and directions of the used degenerate PCR primers are shown at the D.melanogaster gene structure. Positions of the used species-specific primers are given under each exon-intron scheme. Downstream-directed oligonucleotides are red and upstream-directed oligonucleotides are blue.

View this table:
In this window
In a new window

Table 1. Primers used for PCR analysis

In Clytus, genomic PCR fragments were amplified using the primerpairs EF120/Clyrev1 and Cly3-9-4/EF440. The sequence of theeIF-2 ${gamma}$ transcript was determined by overlapping 5' RACE (primersClyEF2 and ClyEF3) and 3' RACE (primers Cly5, ClyEF1, and ClyEF4).With the help of primer pairs ClyEF4/ClyEF8 and ClyEF5/ClyEF7,the position and sizes of introns 3, 4, 5, and 6 were determined.The exon-intron structure of Su(var)3-9 was analyzed by RT-PCRusing primer pairs Cly5/Clyrev1, Cly3-9-4/ClyEF2, and Cly3-9-5/ClyEF7.

In Leptinotarsa, the sequence of the eIF-2 ${gamma}$ -transcript was determinedwith overlapping 5' RACE (primers Lep2 and Lep7) and 3' RACE(primers Lep5, Lep1, and Lep15) experiments. The sequence ofexons 1 and 2 and of introns 1 and 2a, as well as the 5' partof the Su(var)3-9-specific exon 2a were determined using inversePCR. Circularized genomic DNA was amplified using primer Lepinvin combination with Lep8, Lepint1, Lep9, Lep10, Lep11, and Lep12.The exon-intron structure of Su(var)3-9 was determined by RT-PCRusing primer pairs Lep5/Lep13, Lep14/Lep2, and Lep17/Lep16.

For the centipede L. forficatus a 1.7-kb genomic and a 320-bpcDNA product were amplified by genomic PCR and RT-PCR usingprimer pair EF120/EF440.

Sequences were determined by direct sequencing or sequencingof two or three independent clones from different genomic PCRreactions. In addition, all transcribed regions were sequencedas RT-PCR products (directly or as a clone). Therefore, thetranscript sequences were determined from three independentspecimens of each species. PCR fragments were cloned using thepGEM-T PCR cloning kit (Promega, Madison, WI) according to themanufacturer's conditions.

5' RACE, 3' RACE, and RT-PCR:
5' RACE experiments were carried out on 1–2 µg totalRNA using the 5' RACE kit version 2 (Life Technologies) accordingto the manufacturer's instructions. 3' RACE was carried outon 1–2 µg total RNA with 200 units M-MLV reversetranscriptase (Life Technologies). For first-strand cDNA synthesisa poly(T)-primer with anchor sequences was used. After second-strandsynthesis cDNA was amplified with anchor oligo and gene-specificprimers. The 3' RACE amplification was performed with a nestedgene-specific primer. Reverse transcription of total RNA wascarried out with M-MLV reverse transcriptase (Life Technologies)and subsequent PCR was done using standard conditions.

Sequencing:
PCR products from 5' RACE, 3' RACE, and RT-PCR were gel elutedand directly sequenced using an ABI 377 sequencer. Genomic PCRfragments from D. erecta and products of inverse genomic PCRwere directly sequenced. For DNA sequence analysis, MacVector5.0 (Oxford Molecular, Palo Alto, CA) software was used. TheGenBank/EMBL numbers of the genomic and cDNA sequences are,for D. melanogaster, AJ290956; D. erecta, AJ290957; L. forficatus,AJ290958; S. libatrix, AJ290959 and AJ290960; C. arietus, AJ290961,AJ290962, and AJ290963; and L. decemlineata, AJ290964 and AJ290965.

Phylogenetic analysis:
Multiple protein sequence alignments were performed by meansof the ClustalW algorithm of the SeqPup program (D. G. Gilbert),with corrections made by eye. For phylogenetic analysis we usedthe maximum-likelihood tree reconstruction method of the PUZZLE4.0 program (STRIMMER and HAESELER 1997 ) on the basis of theJTT model of amino acid substitution (JONES et al. 1992 ). Quartetpuzzling (1000 steps) was performed to infer support valuesfor internal branches. Trees were drawn using Treeview (R. Page).The alignments were also analyzed by bootstrapping (branch-and-boundsearch method, 100 steps) with the maximum parsimony algorithmof PAUP 3.1 (SWOFFORD 1993 ). Alignments are accessible at http://www.uni-leipzig.de/~genetics/ForschVK.htm.

RESULTS

TOP
ABSTRACT
MATERIALS AND METHODS
RESULTS
DISCUSSION
LITERATURE CITED

The Su(var)3-9/eIF-2 ${gamma}$ dicistronic transcription unit of holometabolic insects:
The fusion of the two functionally unrelated Su(var)3-9 andeIF-2 ${gamma}$ genes into a dicistronic transcription unit was firstindicated in D. melanogaster (TSCHIERSCH et al. 1994 ). TheeIF-2 ${gamma}$ locus of D. melanogaster consists of five exons (Fig 1).Most of the ORF of the SU(VAR)3-9 heterochromatin protein issituated within the large intron 2 of eIF-2 ${gamma}$ . 5' RACE experimentsproved that both the Su(var)3-9 and eIF-2 ${gamma}$ mRNAs use the sametranscription initiation site 109 bp before the translationinitiation codon of both proteins (accession no. AJ290956),suggesting that the two mRNAs for the unrelated proteins aretranscribed as a single pre-mRNA, which is alternatively spliced.The two genes share a common promoter and both mRNAs containthe first two exons, resulting in an 80-amino-acid N-terminalextension of SU(VAR)3-9 in D. melanogaster.

An identical genomic organization of Su(var)3-9/eIF-2 ${gamma}$ was foundin D. erecta, which is 9–15 million years evolutionarilydistant (POWELL 1997 ). To study the evolutionary conservationof this unusual gene structure within insects, we analyzed C.arietis, L. decemlineata (both Coleoptera), and S. libatrix(Lepidoptera). Genomic and cDNA fragments of the Su(var)3-9/eIF-2 ${gamma}$ region in these species were isolated by a combination of genomicPCR using degenerated primers, inverse genomic PCR, 5' and 3'RACE, as well as RT-PCR (cf. MATERIALS AND METHODS).

Sequence analysis of these DNA fragments proved the locationof the SU(VAR)3-9 ORF within intron 2 of eIF-2 ${gamma}$ in all thesespecies (Fig 1). In 5' RACE experiments the transcription initiationsite of eIF-2 ${gamma}$ was determined in Clytus and Leptinotarsa. Sequencecomparison with Su(var)3-9-specific RT-PCR fragments showedthat exons 1 and 2 are present in both the Su(var)3-9 and theeIF-2 ${gamma}$ mRNAs.

The cDNA sequences of eIF-2 ${gamma}$ were completed with 3' RACE or RT-PCRexperiments. Surprisingly, cDNA sequences that cover exon 2a[Su(var)3-9] and exon 3 (eIF-2 ${gamma}$ ) could be amplified by RT-PCRin all studied coleopteran and lepidopteran species. Directsequencing of these RT-PCR amplificates yielded the interestingresult that in all the non-Drosophilid species the Su(var)3-9exon 2a was fused in-frame with exon 3 of eIF-2 ${gamma}$ . This was provedby RT-PCR for every species using two different primer pairs.First, the region between the SET domain-encoding sequence ofSu(var)3-9 and exon 3 of eIF-2 ${gamma}$ was amplified. Afterward, forthe two coleopteran species primer pairs were used that amplifiedthe sequence of the fusion transcript between Su(var)3-9 exon2a (Cly3-9-5 or Lep17 and ClyEF7 or Lep16, respectively) andthe 3' untranslated region of eIF-2 ${gamma}$ (cf. Fig 1). In C. arietisbeside the Su(var)3-9-eIF-2 ${gamma}$ in-frame fusion transcript, a polyadenylatedSu(var)3-9 transcript variant not fused with eIF-2 ${gamma}$ exons 3–7has been detected in 3' RACE experiments. Within Su(var)3-9exon 2a in each of the studied species a specific 5' splicesite is found (Fig 2). The in-frame fusion of the SU(VAR)3-9and eIF-2 ${gamma}$ ORFs results in small terminal deletions in the ORFof exon 2a. Furthermore, in S. libatrix two different amplificateswere isolated, indicating the usage of two alternative 5' splicesites (Fig 2). This could be proved by an RT-PCR plot usingprimers Sco4-4/Sco8-2 for PCR and a 300-bp genomic fragmentcovering exon 3 within eIF-2 ${gamma}$ for hybridization (Fig 3). Accordingto the Drosophila 5' splice site scoring table (MOUNT 1993 ),the best possible splice site between the SET domain and theconserved stop is used. In the Drosophila species studied nosplice consensus sequence is found in the corresponding regionof Su(var)3-9. Remarkably, only three single nucleotide substitutionsbetween Clytus and Leptinotarsa cause the use of a slightlydifferently positioned 5' splice site.

View larger version (26K):
In this window
In a new window
Download PPT slide

Figure 2. Splicing of intron 2b in Su(var)3-9/eIF-2 ${gamma}$ . For nomenclature see Fig 1. Specific exons of Su(var)3-9 are green; exons of eIF-2 ${gamma}$ are yellow. The out-of-frame ORF of the pink boxed eIF-2 ${gamma}$ exon 3 sequence in Scoliopterix is in parentheses. Note that exon 3 in Scoliopterix is identical in both cases, but used in different reading frames. Also in Clytus two splice variants of Su(var)3-9 exist, one with and one without exons 3–7.

View larger version (54K):
In this window
In a new window
Download PPT slide

Figure 3. RT-PCR amplification of Scoliopterix Su(var)3-9 and eIF-2 ${gamma}$ transcripts. Oligo(dT)-primed cDNA from adults was amplified by using the Su(var)3-9-specific primer pair Sco4-4 and Sco8-2 or the eIF-2 ${gamma}$ -specific primer pair Sco5-2 and Sco8-2, respectively. The amplified regions span the intron 2b of Su(var)3-9 or introns 1 and 2 of eIF-2 ${gamma}$ , respectively. Fragments of 451 and 264 bp correspond to the major and minor splice variants of Su(var)3-9. The 351-bp fragment represents the transcript of eIF-2 ${gamma}$ . The RT-PCR reaction separated on a 1% agarose gel was hybridized after blotting with the indicated eIF-2 ${gamma}$ -exon3-specific 300-bp fragment. The three additional fragments in the Su(var)3-9 lane might indicate the presence of three other transcript variants. The additional signal in the eIF-2 ${gamma}$ lane is likely due to a partial spliced transcript containing intron 1.

The dicistronic organization of Su(var)3-9/eIF-2 ${gamma}$ was found inall the holometabolic insect species studied (Fig 1). The mRNAsof Su(var)3-9 and eIF-2 ${gamma}$ in holometabolic insects are producedby alternative splicing, resulting in an N-terminal fusion ofthe SU(VAR)3-9 protein with the first 80 amino acids of eIF-2 ${gamma}$ .A further fusion of SU(VAR)3-9 at the C terminus with the eIF-2 ${gamma}$ protein appears to be caused by the usage of a 5' splice siteat the 3' end of the SU(VAR)3-9 ORF in the coleopteran and lepidopteranspecies (Fig 1 and Fig 2).

Phylogenetic analysis of SU(VAR)3-9 orthologs:
Because of high sequence conservation between all known eIF-2 ${gamma}$ genes, the first AUG used as a start codon can unambiguouslybe deduced. There is evidence for the use of the same startsite of translation in SU(VAR)3-9. The first AUG in Su(var)3-9mRNAs is in the same sequence context as in the eIF-2 ${gamma}$ transcripts.In both Leptinotarsa and Scoliopterix, in-frame stop codonsare found 5' to the first AUG codon. No other methionine codonN-terminal to the chromobox is conserved between all the studiedinsect species. Furthermore, in Clytus and Leptinotarsa no otherAUG codon is found between the putative start AUG and the chromobox.

The sequence data available allow detailed analysis of conservedand more variable regions within SU(VAR)3-9 and eIF-2 ${gamma}$ (Fig 4).No significant sequence conservation between different insectorders is found within regions II, IV, and VII, which are locatedbetween the conserved regions of SU(VAR)3-9. The highest degreeof sequence identity between all the known SU(VAR)3-9 orthologsis found in the SET domain (35%), followed by the SET-domain-associatedcysteine-rich (SAC; 16%) and chromo domains (12%). Phylogenetictrees were computed using the complete SU(VAR)3-9 sequence orindividual regions within the gene. If the SET and SAC domainsare computed together (Fig 5), all known SU(VAR)3-9 orthologsare branched together with 93% quartet puzzle and 67% bootstrapsupport excluding other similar SET domain proteins as Dm E(Z)(JONES and GELBART 1993 ), Hs G9a (MILNER and CAMPBELL 1993), and Ce R05D3.11 (accession no. P34544). Our results suggesta common origin of all SU(VAR)3-9 orthologs, independent ofthe diagnostic feature, which is the occurrence of both thechromo and SET domains within all SU(VAR)3-9 proteins.

View larger version (90K):
In this window
In a new window
Download PPT slide

Figure 4. Alignment of SU(VAR)3-9 orthologs. Above each amino acid sequence the regional subdivision and the degree of conservation are shown. Sequences of conserved regions are colored: The common region with eIF-2 ${gamma}$ is yellow boxed, the chromo domain is red, the SAC domain is green, and the SET domain is blue. A block of a weakly conserved sequence [consensus E(RL)(LV)(SQ)(EF)] immediately C-terminal to the common region with eIF-2 ${gamma}$ is gray boxed. The SAC domain (HUANG et al. 1998

) contains parts before and after the SET domain. Sequences that are black boxed at the C terminus are deleted as a result of the in-frame fusion of SU(VAR)3-9 and eIF-2 ${gamma}$ ORFs in the indicated species. Abbreviations (in addition to Fig 1): Sp Clr4p, S. pombe Clr4p (IVANOVA et al. 1998

); Dm Suv39, D. melanogaster Su(var)3-9 (TSCHIERSCH et al. 1994

); Hs SUV39H1, Homo sapiens SUV39H1 (AAGAARD et al. 1999

View larger version (12K):
In this window
In a new window
Download PPT slide

Figure 5. SAC and SET domain-based tree of SU(VAR)3-9-related protein sequences. Numbers refer to support above (quartet puzzling) and below (bootstrap) internal branches, and branch length reflects maximum-likelihood distances. Abbreviations (in addition to Fig 1 and Fig 4): Dm E(Z), D. melanogaster E(Z) (JONES and GELBART 1993

); Hs G9a, H. sapiens G9a (MILNER and CAMPBELL 1993

); Ce R05D3.11, C. elegans ORF (accession no. P34544).

Characterization of the eIF-2 ${gamma}$ gene structure in arthropods:
The eIF-2 ${gamma}$ gene was isolated from Saccharomyces cerevisiae, S.pombe, and humans (HANNIG et al. 1993 ; GASPAR et al. 1994; DORRIS et al. 1995 ). Further eIF-2 ${gamma}$ homologous sequencescould be identified by BLAST searches (ALTSCHUL et al. 1997) in Arabidopsis thaliana [two different genes, accession nos.AC002411 and AL021713, verified by overlapping expressed sequencetags (EST)] and C. elegans (genomic clone Y74C10, verified byoverlapping EST). We isolated eIF-2 ${gamma}$ homologous sequences fromfive holometabolic insects (D. melanogaster, D. erecta, S. libatrix,C. arietis, and L. decemlineata) as well as from the centipedeL. forficatus (Fig 6). In all analyzed insect species eIF-2 ${gamma}$ is associated with Su(var)3-9 within a dicistronic transcriptionunit. In contrast, in all noninsect species studied these genesare independent.

View larger version (65K):
In this window
In a new window
Download PPT slide

Figure 6. eIF-2 ${gamma}$ alignment. Above the amino acid sequence the three parts of the GTP binding domain (NARANDA et al. 1995

) are boxed in gray. The N-terminal prolongation in budding yeast is boxed. A deletion of this region is without consequences (ERICKSON et al. 1997

). In all sequences, identified locations of loss-of-function point mutations are shaded gray (DORRIS et al. 1995

; NARANDA et al. 1995

; ERICKSON and HANNIG 1996

; ERICKSON et al. 1997

). Known intron positions are boxed in black. Under the sequence of the N-terminal amino acid block a secondary structure prediction (ROST 1996

) for the eIF-2 ${gamma}$ proteins is shown. "Disturbed" indicates the prediction of secondary structure for the N-terminal eIF-2 ${gamma}$ region fused to SU(VAR)3-9. ${alpha}$ -helices and ß-sheets are minimal consensus predictions of structures for all shown insect proteins. Abbreviations (in addition to Fig 1 and Fig 4): Sc GCD11p, S. cerevisiae eIF-2 ${gamma}$ (HANNIG et al. 1993

); Ce, C. elegans.

A maximum-likelihood tree that is based on eIF-2 ${gamma}$ amino acidsequences is shown in Fig 7 and is consistent with a recentconsensus species phylogeny (MADDISON 1997 ). However, KEELINGet al. 1998 places C. elegans on different nodes in an eIF-2 ${gamma}$ gene tree. This may be due to a partially incorrect proteinsequence contained in the WORMPEP (rel. 16) database (Y39G10A246.C). We corrected this sequence with the help of overlappingESTs and improved the alignment. The resulting perfect agreementof the eIF-2 ${gamma}$ gene tree with the species tree argues for a trueorthologue relation of all compared eIF-2 ${gamma}$ sequences, irrespectiveof their quite distinct gene structure in insects, and underlinesthe usefulness of the eIF-2 ${gamma}$ sequence and gene structure as anexcellent molecular marker for phylogenetics.

View larger version (9K):
In this window
In a new window
Download PPT slide

Figure 7. Maximum-likelihood tree of eIF-2 ${gamma}$ protein sequences. Numbers refer to support above (quartet puzzling) and below (bootstrap) internal branches, and branch length reflects maximum-likelihood distances.

DISCUSSION

TOP
ABSTRACT
MATERIALS AND METHODS
RESULTS
DISCUSSION
LITERATURE CITED

In only a few cases have polycistronic transcription units inhigher eukaryotes been found where unrelated proteins are specifiedby a single pre-mRNA after alternative splicing (BLUMENTHAL1998 ). The unc-17/cha-1 dicistronic cluster, which was firstdiscovered in C. elegans (ALFONSO et al. 1994 ), is also foundin insects and mammals (BERRARD et al. 1995 ; KITAMOTO et al.1998 ), indicating an early origin during evolution as wellas a functional relevance of this structure. In contrast, ouranalysis of the Su(var)3-9/eIF-2 ${gamma}$ dicistronic transcription unitshowed that it is only found in insects. Therefore, we concludethat the fusion of these two functionally completely unrelatedgenes into a dicistronic unit arose before radiation of holometabolicinsects after the crown arthropod lines (chelicerates, crustaceans,myriapods, and hexapods) had been separated. Suggesting a monophyleticorigin of this gene arrangement, we have to place the eventbetween 280 and 545 million years ago (FORTEY and THOMAS 1998).

In contrast to already known cases of polycistronic clusters(ALFONSO et al. 1994 ; ZHANG et al. 1999 ) where the sharedexons are noncoding, the fused Su(var)3-9 and eIF-2 ${gamma}$ genes areunique in sharing N-terminally two coding exons. The insertionof Su(var)3-9 into an intron of eIF-2 ${gamma}$ could be caused by eitheran insertion of an intron-free Su(var)3-9 gene by retroinsertionor via a translocation-like process. The ancient Su(var)3-9gene has been lost because in none of the studied species hasany indication for other Su(var)3-9 or eIF-2 ${gamma}$ homologous sequencesbeen detected and it is unlikely that gene duplications exist.

In the dicistronic transcription unit SU(VAR)3-9 becomes fusedwith the 80 N-terminal amino acids of eIF-2 ${gamma}$ . Our data suggestthat the same translation start site is used for both proteins,also indicating that the original Su(var)3-9 gene was not completelyinserted into eIF-2 ${gamma}$ . Probably, the ancient promoter and at leastone exon remained at the original site. In all studied speciessuch as yeast, D. melanogaster, and mammals, the SU(VAR)3-9protein is associated with heterochromatin and is connectedwith gene silencing (TSCHIERSCH et al. 1994 ; IVANOVA et al.1998 ; AAGAARD et al. 1999 ). This functional conservationindicates that the N-terminal addition of eIF-2 ${gamma}$ amino acid sequencesto SU(VAR)3-9 in insects does not interfere with its function.This is also supported by studies with transgenic Drosophilalines expressing N-terminally truncated SU(VAR)3-9 (AAGAARDet al. 1999 ). Overexpression of both the Drosophila full-lengthas well as the N-terminally truncated protein results in enhancementof gene silencing in position-effect variegation.

In Coleopterans and Lepidopterans an in-frame fusion of theSU(VAR)3-9 and eIF-2 ${gamma}$ encoding sequences raises the questionabout possible implications for function of the deduced fusionprotein. The N-terminal $~$ 200 amino acids of eIF-2 ${gamma}$ represent theconserved G domain, involved in both GTP and ^MettRNA binding(DORRIS et al. 1995 ; ERICKSON and HANNIG 1996 ; ERICKSON etal. 1997). In the putative fusion protein, amino acids of theG domain essential for GTP and ^MettRNA binding become separatedby the inserted SU(VAR)3-9 sequence. Structure predictions (PredictProteinserver; http://www2.ebi.ac.uk/~rost/predictprotein/; ROST 1996) indicate a complete disruption of the conserved secondarystructure of the whole N-terminal region of eIF-2 ${gamma}$ within theputative SU(VAR)3-9/eIF-2 ${gamma}$ fusion protein (Fig 6). Furthermore,in the SU(VAR)3-9-specific sequence immediately following theN-terminal 80–82 amino acids of eIF-2 ${gamma}$ in all the speciesstudied, a helical structure is predicted for the first 5–10amino acids. In this region a weak sequence conservation witha consensus of E(R/K)(L/V)(S/Q)(E/F) is found (gray sequenceblock in Fig 4), which could be efficient in total disruptionof protein secondary structure within the N-terminal part ofthe eIF-2 ${gamma}$ G domain fused to SU(VAR)3-9.

Within all Su(var)3-9 genes the position of the stop codon isconserved, indicating that this position predates the evolutionof the dicistronic gene structure. In the coleopteran and lepidopteranspecies studied, where a transcript with a complete in-framefusion of the SU(VAR)3-9 and eIF-2 ${gamma}$ ORFs is found, a nonconserved5' splice donor site located at the 3' end of the Su(var)3-9ORF is used. In the putative SU(VAR)3-9/eIF-2 ${gamma}$ chimeric proteinof coleopteran and lepidopteran species $~$ 470 most highly conservedamino acid positions of eIF-2 ${gamma}$ are added C-terminally to theputative SU(VAR)3-9 proteins. Whether such a fusion proteinis stable or post-translationally processed is not yet known.However, the fusions of SU(VAR)3-9 with eIF-2 ${gamma}$ sequences mightalso have promoted modifications of SU(VAR)3-9 function.

The dicistronic Su(var)3-9/eIF-2 ${gamma}$ gene structure in holometabolicinsects represents an exceptionally useful tool for phylogeneticanalysis within arthropods. There are considerable differencesin phylogenetic concepts within this phylum (FORTEY and THOMAS1998 ). The fusion of the two conserved Su(var)3-9 and eIF-2 ${gamma}$ genes into a dicistronic transcription unit is unlikely to occurseveral times independently. This gene arrangement thereforeshould represent a synapomorphy (shared derived character) fora monophyletic group of arthropods. Both the genomic organizationas well as sequence conservation of Su(var)3-9 and eIF-2 ${gamma}$ allowa comprehensive molecular analysis of arthropod systematicsand evolution.

ACKNOWLEDGMENTS

We are grateful to Andreas Fischer for supplying specimens.We thank Dr. Michael Ashburner for critical reading of the manuscriptand helpful comments. This work was supported by grants fromthe Deutsche Forschungsgemeinschaft and the Fonds der ChemischenIndustrie (to G.R.).

Manuscript received January 25, 2000; Accepted for publication July 13, 2000.

LITERATURE CITED

TOP
ABSTRACT
MATERIALS AND METHODS
RESULTS
DISCUSSION
LITERATURE CITED

AAGAARD, L., G. LAIBLE, P. SELENKO, M. SCHMID, and R. DORN et al., 1999 Functional mammalian homologues of the Drosophila PEV-modifier Su(var)3-9 encode centromere-associated proteins that complex with the heterochromatin component M31. EMBO J. 18:1923-1938[Medline].

ALFONSO, A., K. GRUNDAHL, J. R. MCMANUS, J. M. ASBURY, and J. B. RAND, 1994 Alternative splicing leads to two cholinergic proteins in Caenorhabditis elegans.. J. Mol. Biol. 241:627-630[Medline].

ALTSCHUL, S. F., T. L. MADDEN, A. A. SCHÄFFER, J. ZHANG, and Z. ZHANG et al., 1997 Gapped BLAST and PSI-BLAST: a new generation of protein database search programs. Nucleic Acids Res. 25:3389-3402[Abstract/Free Full Text].

BERRARD, S., H. VAROQUI, R. CERVINI, M. ISRAEL, and J. MALLET et al., 1995 Coregulation of two embedded gene products, choline acetyltransferase and the vesicular acetylcholine transporter. J. Neurochem. 65:939-942[Medline].

BLUMENTHAL, T., 1998 Gene clusters and polycistronic transcription in eukaryotes. Bioessays 20:480-487[Medline].

BROGNA, S. and M. ASHBURNER, 1997 The Adh-related gene of Drosophila melanogaster is expressed as a functional dicistronic messenger RNA: multigenic transcription in higher organisms. EMBO J. 16:2023-2031[Medline].

CLEARD, F., M. DELATTRE, and P. SPIERER, 1997 SU(VAR)3-7, a Drosophila heterochromatin-associated protein and companion of HP1 in the genomic silencing of position-effect variegation. EMBO J. 17:5280-5288.

DORRIS, D. R., F. L. ERICKSON, and E. M. HANNIG, 1995 Mutations in GCD11, the structural gene for eIF-2 ${gamma}$ in yeast, alter translational regulation of GCN4 and the selection of the start site for protein synthesis. EMBO J. 14:2239-2249[Medline].

EHRMANN, I. E., P. S. ELLIS, S. MAZEYRAT, S. DUTHIE, and N. BROCKDORFF et al., 1998 Characterization of genes encoding translation initiation factor eIF-2 ${gamma}$ in mouse and human: sex chromosome localization, escape from X-inactivation and evolution. Hum. Mol. Genet. 7:1725-1737[Abstract/Free Full Text].

EISSENBERG, J. C., G. D. MORRIS, G. REUTER, and T. HARTNETT, 1992 The heterochromatin-associated protein HP-1 is an essential protein in Drosophila with dosage-dependent effects on position-effect variegation. Genetics 131:345-352[Abstract].

ERICKSON, F. L. and E. M. HANNIG, 1996 Ligand interactions with eukaryotic translation initiation factor 2: role of the ${gamma}$ -subunit. EMBO J. 15:6311-6320[Medline].

ERICKSON, F. L., L. D. HARDING, D. R. DORRIS, and E. M. HANNIG, 1997 Functional analysis of homologs of translation initiation factor 2 ${gamma}$ in yeast. Mol. Gen. Genet. 253:711-719[Medline].

FORTEY, R. A., and R. H. THOMAS, 1998 Arthropod Relationships. Chapman & Hall, London.

GASPAR, N. J., T. G. KINZY, B. J. SCHERER, M. HÜMBELIN, and J. W. B. HERSHEY et al., 1994 Translation initiation factor eIF-2: cloning and expression of the human cDNA encoding the ${gamma}$ -subunit. J. Biol. Chem. 269:3415-3422[Abstract/Free Full Text].

GERAGHTY, M. T., L. C. BRODY, L. S. MARTIN, M. MARBLE, and W. KEARNS et al., 1993 The isolation of cDNAs from OATL1 at Xp11.2 using a 480-kb YAC. Genomics 16:440-446[Medline].

HANNIG, E. M., A. M. CIGAN, B. A. FREEMAN, and T. G. KINZY, 1993 GCD11, a negative regulator of GCN4 expression, encodes the ${gamma}$ subunit of eIF-2 in Saccharomyces cerevisiae.. Mol. Cell. Biol. 13:506-520[Abstract/Free Full Text].

HUANG, N., E. V. BAUR, J.-M. GARNIER, T. LEROUGE, and J.-L. VONESCH et al., 1998 Two distinct nuclear receptor interaction domains in NSD1, a novel SET protein that exhibits characteristics of both corepressors and coactivators. EMBO J. 17:3398-3412[Medline].

IVANOVA, A. V., M. J. BONADUCE, S. V. IVANOV, and A. J. S. KLAR, 1998 The chromo and SET domains of the Clr4 protein are essential for silencing in fission yeast. Nat. Genet. 19:192-195[Medline].

JAMES, T. C. and S. C. R. ELGIN, 1986 Identification of a nonhistone chromosomal protein associated with heterochromatin in Drosophila melanogaster and its gene. Mol. Cell. Biol. 6:3862-3872[Abstract/Free Full Text].

JONES, R. S. and W. M. GELBART, 1993 The Drosophila polycomb-group gene enhancer of zeste contains a region with sequence similarity to trithorax. Mol. Cell. Biol. 13:6357-6366[Abstract/Free Full Text].

JONES, D. T., W. R. TAYLOR, and J. M. THORNTON, 1992 The rapid generation of mutation data matrices from protein sequences. Comput. Appl. Biosci. 8:275-282[Abstract/Free Full Text].

KEELING, P. J., N. M. FAST, and G. I. MCFADDEN, 1998 Evolutionary relationship between translation initiation factor eIF-2 ${gamma}$ and selenocysteine-specific elongation factor SELB: change of function in translation factors. J. Mol. Evol. 47:649-655[Medline].

KITAMOTO, T., W. WANG, and P. M. SALVATERRA, 1998 Structure and organization of the Drosophila cholinergic locus. J. Biol. Chem. 273:2706-2713[Abstract/Free Full Text].

LEE, S. J., 1991 Expression of growth/differentiation factor 1 in the nervous system: conservation of a dicistronic structure. Proc. Natl. Acad. Sci. USA 88:4250-4254[Abstract/Free Full Text].

MADDISON, D. R., 1997 The Tree of Life homepage. http://phylogeny.arizona.edu/tree

MILNER, C. M. and D. R. CAMPBELL, 1993 The G9a gene in the human major histocompatibility complex encodes a novel protein containing ankyrin-like repeats. Biochem. J. 290:811-818.

MOUNT, S. M., 1993 Messenger RNA splicing signals in Drosophila genes, pp. 333–358 in An Atlas of Drosophila Genes, edited by G. MARONI. Oxford University Press, Oxford/New York.

NARANDA, T., I. SIRANGELO, B. J. FABBRI, and J. W. B. HERSHEY, 1995 Mutations in the NKXD consensus element indicate that GTP binds to the ${gamma}$ -subunit of translation initiation factor eIF2. FEBS Lett. 372:249-252[Medline].

POWELL, J. R., 1997 Progress and Prospects in Evolutionary Biology: The Drosophila Model. Oxford University Press, Oxford/New York.

REUTER, G. and P. SPIERER, 1992 Position-effect variegation and chromatin proteins. Bioessays 14:605-612[Medline].

ROST, B., 1996 PHD: predicting one-dimensional protein structure by profile-based neural networks. Methods Enzymol. 266:525-539[Medline].

SCHOTTA, G. and G. REUTER, 2000 Controlled expression of tagged protein proteins in Drosophila using a new modular P-element vector system. Mol. Gen. Genet. 262:916-920[Medline].

STRIMMER, K., and A. V. HAESELER, 1997 PUZZLE 4.0: Maximum Likelihood Analysis for Nucleotide, Amino Acid, and Two-State Data. http://evolution.genetics.washington.edu/phylip/software.html

SWOFFORD, D. L., 1993 PAUP: Phylogenetic Analysis Using Parsimony. Illinois Natural History Survey, Champaign, IL.

TSCHIERSCH, B., A. HOFMANN, V. KRAUSS, R. DORN, and G. KORGE et al., 1994 The protein encoded by the Drosophila position-effect variegation suppressor gene Su(var)3-9 combines domains of antagonistic regulators of homeotic gene complexes. EMBO J. 13:3822-3831[Medline].

WALLRATH, L. L., 1998 Unfolding the mysteries of heterochromatin. Curr. Opin. Genet. Dev. 8:147-153[Medline].

WEILER, K. S. and B. T. WAKIMOTO, 1995 Heterochromatin and gene expression in Drosophila. Annu. Rev. Genet. 29:577-605[Medline].

ZHANG, Y. Q., J. ROOTE, S. BROGNA, A. W. DAVIS, and D. N. BARBASH et al., 1999 Stress sensitive B encodes an adenine nucleotide translocase in Drosophila melanogaster.. Genetics 153:891-903[Abstract/Free Full Text].

ZORIO, D. A. R., N. N. CHENG, T. BLUMENTHAL, and J. SPIETH, 1994 Operons as a common form of chromosomal organization in C. elegans.. Nature 372:270-272[Medline].

This article has been cited by other articles:

A. Sivakumar, C. Wilton, and L. Holm
From sequences to a functional unit
Physiol Genomics, March 13, 2006; 25(1): 1 - 8.
[Abstract] [Full Text] [PDF]

V. Krauss, M. Pecyna, K. Kurz, and H. Sass
Phylogenetic Mapping of Intron Positions: A Case Study of Translation Initiation Factor eIF2{gamma}
Mol. Biol. Evol., January 1, 2005; 22(1): 74 - 84.
[Abstract] [Full Text] [PDF]

				V. Krauss, M. Pecyna, K. Kurz, and H. Sass Phylogenetic Mapping of Intron Positions: A Case Study of Translation Initiation Factor eIF2{gamma} Mol. Biol. Evol., January 1, 2005; 22(1): 74 - 84. [Abstract] [Full Text] [PDF]

Two Genes Become One: The Genes Encoding Heterochromatin Protein SU(VAR)3-9 and Translation Initiation Factor Subunit eIF-2 Are Joined to a Dicistronic Unit in Holometabolic Insects

Two Genes Become One: The Genes Encoding Heterochromatin Protein SU(VAR)3-9 and Translation Initiation Factor Subunit eIF-2 ${gamma}$ Are Joined to a Dicistronic Unit in Holometabolic Insects