Human Autoantibodies Reveal Titin as a Chromosomal Protein

doi:10.1083/jcb.141.2.321

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© The Rockefeller University Press, 0021-9525/1998//321 $5.00
The Journal of Cell Biology, Volume 141, Number 2, , 1998 321-333

Articles

Human Autoantibodies Reveal Titin as a Chromosomal Protein

Cristina Machado^*^,, Claudio E. Sunkel^,, and Deborah J. Andrew^*

^* Department of Cell Biology and Anatomy, The Johns Hopkins University School of Medicine, Baltimore, Maryland 21205-2196; Laboratório de Genética Molecular, Instituto de Biologia Molecular e Celular, 4150 Porto, Portugal; and Departamento de Biologia Molecular, Instituto de Ciências Biomédicas Abel Salazar, Universidade do Porto, 4050 Porto, Portugal

Assembly of the higher-order structure of mitotic chromosomesis a prerequisite for proper chromosome condensation, segregationand integrity. Understanding the details of this process hasbeen limited because very few proteins involved in the assemblyof chromosome structure have been discovered. Using a humanautoimmune scleroderma serum that identifies a chromosomalprotein in human cells and Drosophila embryos, we cloned thecorresponding Drosophila gene that encodes the homologue ofvertebrate titin based on protein size, sequence similarity,developmental expression and subcellular localization. Titinis a giant sarcomeric protein responsible for the elasticityof striated muscle that may also function as a molecular scaffoldfor myofibrillar assembly. Molecular analysis and immunostainingwith antibodies to multiple titin epitopes indicates that thechromosomal and muscle forms of titin may vary in their NH₂termini. The identification of titin as a chromosomal componentprovides a molecular basis for chromosome structure and elasticity.

Abbreviations used in this paper: E, glutamic acid; FN3, fibronectin type III; K, lysine; MG, myasthenia gravis; MIR, major immunogenic region; ORF, open reading frame; P, proline; V, valine.

AUTOIMMUNE diseases are characterized by the presence of multipleautoantibodies that react with components of nuclear, cytoplasmic,or surface origin (for review see Nakamura and Tan, 1992; Fritzler, 1997).In clinical medicine, autoantibodies have been used to establishdiagnosis, estimate prognosis, follow the progression of a specificautoimmune disease, and, finally, increase our knowledge ofthe pathophysiology of autoimmunity. In cell biology, autoantibodieshave been extremely useful as probes for the identificationof novel proteins and isolation of their corresponding genes.Human autoimmune sera have been particularly useful in the study of the eukaryotic nucleus where they have identified a widerange of nuclear antigens, including both single- and double-strandedDNA, RNA, histones, small nuclear RNA-binding proteins, transcriptionfactors, nuclear lamins, heterochromatin-associated proteins,topoisomerase I and II, and centromere proteins (Tan, 1989,1991; Earnshaw and Rattner, 1991; Fritzler, 1997).

Scleroderma (systemic sclerosis) is a multisystem connectivetissue autoimmune disease of unknown etiology in which vascularlesions and tissue fibrosis are prominent features. Even thoughautoantibody production may be an epiphenomenon of autoimmunediseases, autoantibody targets in scleroderma are very specific(White, 1996). The autoantigens to which scleroderma sera typicallyreact include topoisomerase I, centromere proteins, RNA polymerases,fibrillarin, and several other nucleolar antigens (LeRoy, 1996).However, autoantibodies of rare occurrence have been reportedthat react with antigens localized to metaphase chromosomesand to the centrosome (Jeppesen and Nicol, 1986; Nakamura and Tan, 1992).

Here, we report on the isolation of a Drosophila gene usinga scleroderma serum that recognized an epitope on condensedmitotic chromosomes from both human cultured cells and earlyDrosophila embryos. Using this serum to screen a Drosophilaexpression library, we isolated the gene that encodes the chromosomalprotein that proved to be the Drosophila homologue of vertebratetitin (D-Titin). Titin is a sarcomeric protein responsiblefor the elasticity of striated muscle and may also functionas a molecular scaffold for the assembly of myofibrils (forreview see Keller, 1995; Labeit and Kolmerer, 1995; Trinick, 1996; Labeit et al., 1997; Maruyama, 1997; Squire, 1997). We showthat D-Titin is expressed early and continuously in striatedmuscle and that antibodies directed against two different,nonoverlapping domains of Drosophila TITIN label the Z-disksof Drosophila sarcomeres. The D-TITIN antibodies also staincondensed human and Drosophila mitotic chromosomes, consistentwith the staining observed with the original scleroderma serum.Immunofluorescence with monoclonal and polyclonal antibodiesagainst multiple epitopes of vertebrate titin further supportsits localization to condensed mitotic human chromosomes, suggestinga role for titin not only in myofibrillar assembly and muscleelasticity, but potentially in the architecture of mitoticchromosomes.

As the name implies, titin is a giant protein. Individual filamentoustitin molecules, which range in molecular mass from 2,993 to3,700 kD, span a half-sarcomere from the Z-disk to the M-line,a distance of $~$ 1.2 µm in sarcomeres of relaxed skeletalmuscle (Labeit and Kolmerer, 1995; Kolmerer et al., 1996; Sorimachi et al., 1997).Nearly 90% of titin's mass is comprised of Ig-like and fibronectin type III (FN3)¹-like repeats which are distributed throughoutmost of the protein (Labeit et al., 1990; Maruyama et al., 1993;Labeit and Kolmerer, 1995). The I-band region of vertebratetitin also contains a domain rich in proline (P), glutamicacid (E), valine (V), and lysine (K) that varies from 163 to2,200 residues, the so-called PEVK domain. The PEVK domainand the tandemly arranged Ig domains of the I-band region oftitin confer elasticity to the titin filament (Linke et al., 1996;Trombitas et al., 1998). Titin has phosphorylation sites (Sebastyén et al., 1995),recognition sites for muscle-specific calpain proteases (Sorimachi et al., 1995;Kinbara et al., 1997) and a serine/threonine kinase domain nearthe COOH terminus (Labeit et al., 1992; Takano-Ohmuro et al., 1992).

Titin may function as the scaffold upon which the sarcomeresare assembled into myofibrils (Keller, 1995; Trinick, 1996).Titin mRNA is expressed in myoblasts before fusion (Colley et al., 1990),and titin mRNA and protein are among the earliest moleculesto localize within the developing sarcomere (Fulton and Alftine, 1997;van der Ven and Fürst, 1997). Titin binds to differentproteins in each region of the sarcomere. In the Z-disk, theNH₂ terminus of titin binds to the COOH-terminal region of ${alpha}$ -actinin, an actin-binding protein that cross-links titin toactin filaments (Ohtsuka et al., 1997a,b; Sorimachi et al., 1997;Turnacioglu et al., 1997). In cardiac muscle, the NH₂ terminus of titin binds to actin in the Z-disk near the Z/I-band junction(Linke et al., 1997; Trombitas and Granzier, 1997; Trombitas et al., 1997).The A-band region of titin provides a molecular template forthe regular assemblies of thick filament proteins such as myosin,MyBP-C, and MyBP-H (C- and H-protein; Itoh et al., 1988; Fürst et al., 1989;Soteriou et al., 1993; Houmeida et al., 1995; Freiburg and Gautel, 1996;Trombitas et al., 1997). Titin may also bind to myosin II (Eilertsen et al., 1994).In the M-line, titin binds to M-protein and phosphorylatedmyomesin, two myosin-binding proteins that cross-link titinto myosin filaments (Eppenberger et al., 1981; Obermann et al., 1996,1997). Functional evidence that titin acts as a myofibrillarscaffold derives from experiments where an NH₂-terminal fragmentof titin was fused to green fluorescent protein. This fusionprotein, which localizes to the Z-disk, causes myofibrillardisassembly when overexpressed (Turnacioglu et al., 1997). Theidentification of titin, a gigantic protein important in boththe structure and elasticity of muscle, as a chromosomal componenthas significant ramifications for understanding chromosome condensation and chromosome integrity during mitosis.

Materials and Methods

Top
Abstract
Materials and Methods
Results
Discussion
References

Staining of HEp-2 cells
Fixed HEp-2 cells (Kallestad, Chaska, MN) were blocked for 30min at RT in PBS plus 0.1% Triton X-100 and 3% BSA (PBSTB),incubated for 1 h at room temperature in primary antibody,washed 3x for 5 min in PBSTB, incubated for 1 h with fluorescentlylabeled secondary antibody and washed 3x for 5 min in PBSTB.Cells were then incubated for 5 min at room temperature in1.25 µg/ml propidium iodide (Sigma Chemical Co., St.Louis, MO) and washed twice in PBS. RNaseA (100 µg/ml;Sigma Chemical Co.) was included during antibody incubations.Images were collected on a confocal microscope (Noran Instrument,Middleton, WI). Forty scleroderma sera, provided by D. Isenberg(King's College, London, UK) were tested at a range of dilutionsfrom 1:25 to 1:5,000 in the initial screen. The chosen sclerodermaserum was used at a 1:200 dilution for subsequent experiments.Vertebrate titin polyclonal and monoclonal antibodies were usedat dilutions of 1:25 and 1:100, respectively (provided by S.Labeit, EMBL, Heidelberg, Germany and J. Trinick, Bristol University, Bristol, UK). All fluorescently labeled secondary antibodieswere used at a dilution of 1:200 (Vector Laboratories Inc.,Burlingame, CA). Several fixative procedures (acetone/MeOH,acetone, formaldehyde based), with and without prior TritonX-100 permeabilization, were tested and produced the same stainingpatterns.

Antibody Production
The ${alpha}$ -LG polyclonal antiserum was made by immunizing rabbitswith 450 µg of β-gal:D-TITIN fusion protein administeredsubcutaneously. The ${alpha}$ -LG antiserum was affinity-purified asdescribed (Earnshaw and Rattner, 1991) and used at a dilutionof 1:4. To produce the ${alpha}$ -KZ antiserum, an XhoI/EcoRI fragmentof the most 5' cDNA (see Fig. 2) encoding 636 residues wasligated in-frame to the pTrcHisA expression vector (InvitrogenCorp., Carlsbad, CA) and transformed into BL21 (DE3) cells.Protein was purified from inclusion bodies 3 h after inductionwith 0.1 mM IPTG (Rio et al., 1986). Rat polyclonal antibodieswere raised (Covance Inc., Denver, PA) against 1 mg of renaturedinclusion body protein. The ${alpha}$ -KZ antiserum was used at 1:5,000dilution for embryo immunostaining in Fig. 3 and at 1:500 forall other experiments. Equivalent dilutions of preimmune ${alpha}$ -LGand ${alpha}$ -KZ sera were used as controls, as well as secondary antibodiesalone.

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Figure 2 The chromosome-associated protein is Drosophila TITIN. (A) Restriction map of the genomic region of the D-Titin gene. The genomic phage clones were either isolated directly (phage clone 5) using the LG genomic DNA expression clone as a probe, or were isolated using DNA flanking two nearby P-element insertions. Phage clones 1–4 and 6–8 were isolated with DNA flanking the v(3)ET1 and v(3)ET2 insertions, respectively. Three different D-Titin cDNA fragments were isolated from multiple independent screens of seven available cDNA libraries. The 5' KZ cDNA was isolated from a 9–12 h embryonic cDNA library (Zinn et al., 1988). We infer that the KZ cDNA encodes an NH₂ terminus based on the presence of a putative initiator methionine codon followed by an ORF encoding 882 AA. The ORF is flanked at the 5' end by 389 nt of noncoding sequence. The NB cDNA was isolated from a 12–24 h embryonic cDNA library (Brown and Kafatos, 1988). Within the unprocessed NB cDNA, there is a 1-kb ORF flanked at its 5' end by a 3' splice acceptor site and at its 3' end by a 5' splice donor site (Mount, 1982; Mount et al., 1992). Several small ( $<=$ 312 nt) cDNAs were isolated from a 0–24 h embryonic cDNA library (Tamkun et al., 1991). The largest cDNA isolated from the Tamkum library is indicated as JT cDNA. Multiple unsuccessful attempts were made to connect the genomic DNA from phage clone 5 to the surrounding phage containing DNA from this region. Nonetheless, all of the genomic phage clones (1–7) and all of the cDNA clones colocalize to the same site on polytene chromosomes from wild-type larvae, cytological region 62C1-2. Furthermore, genomic phage clones 1–5 and all the D-Titin cDNAs map to an interval for which only a single complementation group has been identified, based on genomic Southern mapping and in situ hybridization to polytene chromosomes from larvae carrying local deficiencies. An asterisk indicates genomic fragments that revealed somatic and visceral muscle RNA accumulation in whole-mount embryos by in situ hybridization. (B) Protein sequence alignment among the corresponding ORFs from two D-Titin cDNAs (KZ and NB), chicken skeletal titin and human cardiac titin. Identities among all three proteins are indicated by an asterisk and conserved residues shared among all three proteins are indicated by period. (C) Sequence of the PEVK-rich ORF originally isolated with the scleroderma autoimmune serum (LG clone) and the sequence from the largest cDNA isolated from the Tamkun library (JT cDNA). 63% of the residues in the LG clone are either proline (P), glutamic acid (E), valine (V), or lysine (K). 56.4% of the residues encoded by the JT cDNA are either P, E, V, or K. The PEVK-rich domain of vertebrate titin, which provides muscle elasticity, is $~$ 70% P, E, V, K. These sequence data are available from GenBank/EMBL/DDJB under accession numbers AF045775, AF045776, AF045777, and AF045778.

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Figure 3 D-Titin is expressed in all the somatic and visceral musculature during embryogenesis. Pairs of embryos at the same developmental stage and view are shown with in situ hybridization to detect RNA on the left (dark blue) and immunostaining to detect protein on the right (brown). All embryos are oriented with anterior to the left. For embryos shown in lateral view, dorsal is up. Stages and structures are as described (Campos-Ortega and Hartenstein, 1985). (A/A') Embryonic stages 10/11, lateral view. D-Titin transcript and protein were first detectable in fully germ band extended embryos in the somatic and visceral mesoderm. (B/B') Embryonic stage 13, lateral view. In germ band shortened embryos, D-Titin RNA and protein could be detected in the pharyngeal, somatic and visceral musculature. (C/C') Embryonic stage 15, lateral view. High level accumulation of both transcript and protein were observed in both somatic and pharyngeal muscles. (D/D') Embryonic stage 17, lateral view. RNA and protein can be detected in the fully developed larval muscle pattern. (E/E') Embryonic stage 13, dorsal/ventral view. RNA and protein accumulation is evident in the pharynx and both visceral and somatic muscles. (F/F') Embryonic stage 14, dorsal/ventral view. D-Titin expression was observed throughout the visceral and somatic musculature, both of which are striated in Drosophila. (G/G') Embryonic stage 15, dorsal view. At this stage, individual muscle fibers are beginning to form. (H/H') Embryonic stage 16, dorsal/ventral view. Expression of D-Titin persists in the pharyngeal, somatic, and visceral muscles. ph, pharynx/pharyngeal; sm, somatic mesoderm/musculature; vm, visceral mesoderm/musculature.

Drosophila Immunostaining and In Situ Hybridization
Embryo fixation and antibody staining were performed as described(Reuter et al., 1990). In situ hybridizations to whole-mountembryos were carried out as described (Tautz and Pfeifle, 1989),except formaldehyde was used in place of paraformaldehyde andlevamisole was omitted from the staining reaction. Images werecollected on an Axiophot microscope (Carl Zeiss, Inc., Thornwood,NY). Adult thoracic muscle and larval gut muscle were preparedfor immunostaining and stained as described (Saide et al., 1989;Lakey et al., 1993). Texas red–phalloidin was used ata concentration of 0.1 U/ml (Molecular Probes, Inc., Eugene,OR). Images were collected on a Noran confocal microscope.

Immunoblot Preparation
Samples were homogenized in 2x Laemmli sample buffer and electrophoresedon 2.5–7.5% SDS-PAGE gradient gels (Laemmli, 1970); the stacking gel was 0.6% agarose in 0.1% SDS, 0.125 M Tris-glycine,pH 6.8. Proteins were transferred to nitrocellulose filters(Schleicher & Schuell, Inc., Keene, NH) for 2 h at 900mA as described (Wang et al., 1989). Samples from each extractwere run on the same gel, transferred to nitrocellulose andcut into strips for antibody incubations. Immunoblots were incubatedfor 1 h at room temperature with blocking solution (5% nonfat dried milk in 0.1% Triton X-100 in PBS [PBT]), incubated withprimary antibody for 2.5 h at room temperature (1:200 dilutionof ${alpha}$ -LG and 1:500 dilution of ${alpha}$ -KZ), and washed 3x for 10 minin blocking solution. Filters were incubated in either a 1:4,000dilution of HRP-conjugated anti-rabbit IgG ( ${alpha}$ -LG and LG preimmune;Amersham Pharmacia Biotechnology Inc., Piscataway, NJ) or a1:300 dilution of HRP-conjugated anti-rat F(ab)₂IgG ( ${alpha}$ -KZ andKZ preimmune; Amersham Pharmacia Biotechnology Inc.), washed3x for 10 min in blocking solution and 2x for 5 min in PBS.Immunoreactive bands were visualized by chemiluminescence (PierceChemical Co., Rockford, IL).

Results

Top
Abstract
Materials and Methods
Results
Discussion
References

Human Scleroderma Serum Stains Mitotic Chromosomes
To identify novel nuclear components and to isolate and characterizethe corresponding genes in Drosophila, we screened for humanautoimmune sera that recognized nuclear components with cellcycle–dependent distribution in both human cells andearly Drosophila embryos. Sera from 40 patients diagnosed withthe autoimmune disease scleroderma were studied and only oneserum was identified that gave chromosomal staining on bothhuman epithelial HEp-2 cells and Drosophila 0–2 h embryos(Fig. 1 A). During interphase, when chromosomes are decondensed,low level staining was visible throughout the nucleus, withthe exception of the nucleoli. During prophase, staining withthis serum colocalized with the condensing chromosomes. Frommetaphase through telophase, chromosomes were stained uniformly.

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Figure 1 Human scleroderma serum identifies a chromosome-associated protein in human epithelial cells and Drosophila early embryos. (A) Chromosomal staining pattern recognized by the human autoimmune serum on HEp-2 cells (left panels) and Drosophila early embryos (right panels). HEp-2 cells and Drosophila 0–2 h embryos were double-stained with the scleroderma serum (green) and propidium iodide to detect DNA (red). The merged image is on the right (yellow in region of overlap). (B) Chromosomal staining pattern on HEp-2 cells (left panels) and Drosophila 0–2 h embryos (right panels) recognized by an affinity-purified polyclonal antibody ( ${alpha}$ -LG) raised against the PEVK-rich repeats of the Drosophila protein identified by expression cloning with the human autoimmune scleroderma serum. Top and bottom panels show metaphase and anaphase nuclei, respectively, stained with ${alpha}$ -LG (green) and propidium iodide (red). The merged image is on the right (yellow). (C) Immunofluorescence of HEp-2 cells (left panels) and Drosophila 0–2 embryos (right panels) using a polyclonal serum ( ${alpha}$ -KZ) raised against an NH₂-terminal peptide encoded by the KZ cDNA (green) and a DNA dye, propidium iodide (red). The merged image is on the right (yellow). Bar, 5 µm.

Cloning of Drosophila Titin
To isolate the corresponding gene in Drosophila, the human autoimmunescleroderma serum was used to screen a Drosophila genomic expressionlibrary (Goldstein et al., 1986). Out of 5 x 10⁶ plaque-formingunits screened, five independent, overlapping genomic cloneswere isolated, each encoding several copies of a 71–aminoacid repeat rich in proline, valine, glutamic acid, and lysineresidues (Fig. 2 C). The largest clone (designated LG) wasexpressed in Escherichia coli, and the corresponding fusion protein was purified and used to immunize rabbits. ${alpha}$ -LG affinity-purifiedantibodies gave the same chromosomal staining pattern on bothhuman HEp-2 cells and Drosophila 0–2 h embryos in allstages of the cell cycle as was initially observed with thehuman serum (Fig. 1 B). We subsequently isolated additionalexons from this Drosophila gene (see below) and used a differentdomain of the protein to raise a second polyclonal antiserumin rat (designated ${alpha}$ -KZ). The ${alpha}$ -KZ antiserum reproduced the staining pattern observed with the human autoimmune serum andthe ${alpha}$ -LG antibody, that is, nuclear staining during interphase(not shown) and staining of condensed chromosomes during mitosis(Fig. 1 C).

Attempts to clone the entire genomic region corresponding tothe chromosome-associated protein gene were unsuccessful mostlikely because of its repetitive structure. The isolation ofcDNAs was similarly difficult due in part to the repetitivestructure of the gene but also because of the predicted largesize of the corresponding mRNA (see below). Nonetheless, cDNAsmapping to several discrete regions of the gene, encoding atotal of 1,608 amino acids, were isolated and characterized(Fig. 2). The partial cDNAs, designated KZ, NB, and JT, werenamed according to the libraries in which they were found.See Fig. 2 legend for the details of cloning. All of the cDNA clones and genomic phage clones 1–5 map to cytological position 62C1-2 in a region known to contain only a single gene.

Notably, every open reading frame (ORF) identified from thechromosome-associated protein gene shows significant similarityto vertebrate titins (Fig. 2 B). Using the conceptual translationof the KZ cDNA to do a BLAST search, the two proteins withgreatest similarity are chicken skeletal titin (P = 2.7e^–99)and human cardiac titin (P = 1.2e^–80). The ORF withinthe unprocessed NB cDNA also shows significant similarity tovertebrate titins. An alignment between the ORFs derived fromthe KZ and NB cDNAs and the chicken skeletal and human cardiactitins is shown in Fig. 2 B. In the region of overlap, the ORF encoded by the KZ cDNA shows 28.6% identity/ 58.3% similarityto chicken skeletal titin, and 27.4% identity/56.8% similarityto human cardiac titin. The ORF encoded by the NB cDNA shows18.4% identity/48.9% similarity to chicken skeletal titin, and17.2% identity/47.7% similarity to human cardiac titin in theregion of overlap. The sequence conservation among the ORFsfrom the LG and JT clones and vertebrate titins is not as great;however, in these clones, the frequency of P, E, V, and K residues(63% for LG, 56.4% for JT) strongly suggests that these ORFscorrespond to the elastic PEVK domain of vertebrate titin,which is 70% P, E, V, K (Fig. 2 C). Thus, starting with a humanautoimmune scleroderma serum, we have cloned a Drosophila geneencoding a nuclear protein that localizes to chromosomes andis homologous to vertebrate titins.

D-Titin in Striated Muscles and Their Precursors
To determine whether the gene that encodes the nuclear, chromosome-associatedform of titin also encodes the muscle form of titin, we examinedboth transcript and protein accumulation in embryos, and determinedthe subcellular localization of the protein in muscle. Analysisof RNA expression by in situ hybridization to whole-mount Drosophila embryos revealed RNA accumulation as early as thegerm band extended stage in both somatic and visceral muscleprecursors (Fig. 3 A). Protein was initially detected duringlate stage 11 in the precursors of both somatic and visceralmuscles (Fig. 3 A'), before myoblast fusion (stage 13; Hartenstein, 1993).This early accumulation of protein in Drosophila muscle precursorsparallels vertebrate titin accumulation in early myoblasts(Colley et al., 1990). Expression of both RNA and protein inall visceral and somatic muscles persisted throughout embryogenesis(Fig. 3, B–H'). These muscles include the somatic or bodywall muscles, the pharyngeal muscles, and the visceral musculaturewhich surrounds the digestive system. We did not detect RNAor protein in embryonic cardiac muscle or cardiac muscle precursors.

To determine if the protein localizes to specific regions inthe sarcomere, we immunostained adult thoracic muscle withantibodies directed against two different domains of the protein( ${alpha}$ -KZ and ${alpha}$ -LG; Fig. 2) and with the original human autoimmunescleroderma serum. The ${alpha}$ -KZ antiserum stained the Z-disks ofeach sarcomere, which can be identified as the phase-dark bandson myofibrils (Fig. 4 A). A double-stained image of a myofibrilstained with ${alpha}$ -KZ and Texas red–phalloidin, which stainsthe filamentous actin of the I-band, supports this localization(Fig. 4 B). Double staining with the ${alpha}$ -KZ antiserum and eitherthe human autoimmune scleroderma serum (Fig. 4 C) or the ${alpha}$ -LGaffinity-purified antibodies (Fig. 4 D) also revealed Z-diskstaining. Both the ${alpha}$ -LG antibodies and the scleroderma serumalso stained the M-line suggesting potential cross-reactivityto other antigens. The scleroderma serum, but not the ${alpha}$ -LG antibodies,also stained along the length of the myofibril (Fig. 4 C),suggesting the presence of additional, nontitin antibodies inthe serum. Two antibodies against vertebrate titin recognizedepitopes on Drosophila myofibrils: serum from a patient withmyasthenia gravis, which recognizes the major immunogenic region(MIR) epitope in the I-band near the I/A-band junction (Fig.4 E; Gautel et al., 1993), and anti-Zr5/Zr6, a polyclonal antiserumthat was raised to the expressed ${alpha}$ -actinin binding Z-repeatmotifs Zr5/Zr6 (Fig. 4 F; Sorimachi et al., 1997). The nearlycomplete overlap of the signals with ${alpha}$ -KZ and the MIR serumsuggests that the resolution of confocal microscopy was insufficientto allow visual separation of Z-disk staining from I/A-bandstaining in nonstretched Drosophila myofibrils. We also foundthat the ${alpha}$ -KZ and ${alpha}$ -LG antibodies stained the Z-disks of visceralmuscles from third instar larvae (Fig. 4 G). Drosophila visceral muscle, unlike vertebrate smooth muscle, is striated.

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Figure 4 Antibodies to Drosophila TITIN stain specific regions of the sarcomeres from Drosophila adult thoracic myofibrils and larval gut muscle. (A) The top panel shows a phase image of a myofibril from adult thoracic muscle, which has been immunostained with the ${alpha}$ -KZ antiserum (lower panel). Arrows in upper panel indicate Z-disks. (B) Adult thoracic myofibril double-stained with ${alpha}$ -KZ (green) and Texas red–phalloidin. (C) Double-staining of an adult thoracic myofibril with ${alpha}$ -KZ (green) and the human autoimmune scleroderma serum (red); the lower panel shows the merged image (yellow in region of overlap). (D) Double-staining of an adult thoracic myofibril with ${alpha}$ -KZ (green) and affinity-purified ${alpha}$ -LG (red); the lower panel shows the merged image. (E) Double-staining of an adult thoracic myofibril with ${alpha}$ -KZ (green) and the human serum MIR (red) that in vertebrate sarcomeres recognizes an epitope in the I-band near the I/A-band junction; the lower panel shows the merged image. (F) Double-staining of an adult thoracic myofibril with ${alpha}$ -KZ (green) and with the anti-Zr5/Zr6 polyclonal serum (red) that was raised against the rabbit titin Z-repeats that bind to ${alpha}$ -actinin; the lower panel shows the merged image. (G) Third instar larval gut muscle stained ${alpha}$ -KZ antiserum (green). The fluorescent staining overlaps the phase-dark bands (not shown) that correspond to the Z-disks of the gut muscles. No staining was observed with the ${alpha}$ -KZ preimmune serum nor with any of the secondary antibodies. However, a regular pattern of accumulation on myofibrils was detected with the LG preimmune serum. Bar, 3 µm.

We have named the gene isolated with the human autoimmune sclerodermaserum D-Titin for Drosophila Titin. This name is based on thehigh level of similarity to vertebrate titins, the expressionpattern of this gene during embryogenesis (Fig. 3), the localizationof two different domains of the protein to the Z-disks in sarcomeresby immunofluorescence (Fig. 4) and the size of the protein on immunoblots (Fig. 5; see below).

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Figure 5 D-TITIN migrates in the megadalton size range and is detected in nonmuscle cells. Total protein extracts from (a) Drosophila 8–24 h embryos (after myogenesis), (b) Drosophila 0–2 h embryos (several hours before myogenesis), and (c) HeLa cells were separated on SDS-PAGE 2.5–7.5% gradient gels. Lanes 1, Coomassie blue-stained SDS-gels. Lanes 2–5, immunoblots incubated with ${alpha}$ -LG, LG preimmune serum, ${alpha}$ -KZ, and KZ preimmune serum, respectively. Lane 6 in a is a shorter exposure of an immunoblot from 8–24 h embryos incubated with the ${alpha}$ -KZ antiserum that reveals the ladder-like array of titin degradation products. The protein size markers (cross-linked phosphorylase b; Sigma Chemical Co.), were visualized by Coomassie blue staining.

D-TITIN Migrates in the Megadalton Size Range
Vertebrate muscle titin isoforms range in molecular mass from2,993 to 3,700 kD (Labeit and Kolmerer, 1995; Kolmerer et al., 1996;Sorimachi et al., 1997). Because the mini-titins identifiedin Drosophila are smaller (500–1,200 kD; Ayme-Southgate et al., 1991,1995; Fyrberg et al., 1992; Lakey et al., 1993), they are unlikelyto span a half-sarcomere from the Z-disk to the M-line. Mutationalanalysis further suggests that these proteins do not providethe elasticity and proposed scaffolding functions of vertebrate titin. Our data shows that NH₂-terminal regions of D-TITIN localize to the Z-disk, that D-TITIN has significant homologyto vertebrate titins, and that D-TITIN is expressed early andcontinuously in striated muscles in Drosophila. These characteristicsmake D-TITIN a good candidate for the Drosophila homologueof vertebrate muscle titin. If it is indeed the homologue,D-TITIN should be in the 2–4-MD size range. To test thisprediction, total protein extracts from 8–24 h embryoswere prepared (in muscle precursors, D-TITIN is first detectedat $~$ 7 h by immunostaining of embryos), proteins were separatedon denaturing polyacrylamide gradient gels (2.5–7.5%),and were transferred to nitrocellulose filters. Immunoblotsincubated with both ${alpha}$ -LG and ${alpha}$ -KZ detected a discrete band inthe megadalton size range, consistent with vertebrate titin (Fig. 5 a, lanes 2 and 4). ${alpha}$ -LG and ${alpha}$ -KZ preimmune sera revealedno cross-reacting polypeptides (Fig. 5 a, lanes 3 and 5). Thus,D-TITIN is likely to be the Drosophila homologue of vertebratesarcomeric titin based on size, sequence similarity, developmentalexpression and subcellular localization.

To determine the size of chromosome-associated D-TITIN in nonmusclecells, total protein extracts were prepared from both 0–2h Drosophila embryos (myogenesis does not begin until severalhours later) and from HeLa cells (epithelial cells). In the0–2 h embryonic extracts, we detected a discrete highmolecular mass polypeptide of identical size on immunoblotswith both ${alpha}$ -LG (Fig. 5 b, lane 2) and ${alpha}$ -KZ (Fig. 5 b, lane 4).No cross-reacting polypeptides were detected with either ${alpha}$ -LGor ${alpha}$ -KZ preimmune sera (Fig. 5 b, lanes 3 and 5). Using totalcell extracts from HeLa cells, we also detected a megadaltonpolypeptide with both ${alpha}$ -LG and ${alpha}$ -KZ antisera (Fig. 5 c, lanes2 and 4), with no staining with the preimmune sera (Fig. 5c, lanes 3 and 5). Thus, antibodies to D-TITIN detected a veryhigh molecular mass polypeptide in nonmuscle cells from Drosophilaand in human epithelial cells. Since, by immunofluorescence,the only detectable staining with these antibodies on Drosophila0–2 h embryos and HEp-2 cells is chromosomal, we concludedthat the chromosomal form of D-TITIN migrates in the megadaltonsize range and is approximately as large as the muscle form.

Antibodies to Vertebrate Muscle Titin Stain Human Chromosomes
Given that Drosophila TITIN localized to condensed Drosophilamitotic chromosomes and that antibodies directed against thisprotein also stained human chromosomes, we were curious whetherantibodies to vertebrate muscle titin also stained condensedchromosomes. We used a panel of eight antibodies directed againstdifferent epitopes of vertebrate titin to immunostain HEp-2cells. Six of the eight antibodies directed against vertebratetitin stained the condensed chromosomes in a pattern indistinguishablefrom that observed with the original scleroderma serum and theantibodies to the D-TITIN protein (Fig. 6, A and B). The antibodiesthat gave chromosomal localization include three mouse monoclonals,two of which recognize distinct epitopes in the A-band (BD6and CE12; Whiting et al., 1989) and one of which recognizes the PEVK domain in the I-band (9D10; data not shown; Wang et al., 1991).We also observed chromosomal staining with two rabbit polyclonalantibodies to vertebrate titin: N2A, which recognizes an I-bandepitope in skeletal titin, and A168, which recognizes an M-lineepitope (Linke et al., 1996). Finally, the MIR human autoimmuneserum, which recognizes an I/A-band epitope (Gautel et al., 1993), also stained condensed mitotic chromosomes of HEp-2 cellsalthough additional staining of the mitotic apparatus was visiblewith this serum (Fig. 6 A). The two vertebrate titin antibodiesthat did not recognize titin on HEp-2 chromosomes, anti-Zr5/Zr6and T12, are directed against NH₂-terminal regions of titinthat either map to the Z-disk and bind to ${alpha}$ -actinin (anti-Zr5/Zr6;Sorimachi et al., 1997) or map to the Z-disk/I-band junction(T12; Fürst et al., 1988). The NH₂-terminal region ofthe D-Titin isoform encoded by the KZ cDNA does not containregions homologous to the ${alpha}$ -actinin–binding regions ofvertebrate titin. It is likely that cDNAs encoding the NH₂terminus of the muscle D-TITIN isoform will reveal homologiesto the ${alpha}$ -actinin– binding regions since (a) the COOH-terminalsequence of ${alpha}$ -actinin from Drosophila is highly homologous tothe COOH terminus of human ${alpha}$ -actinin (Fyrberg et al., 1990) and (b) the anti-Zr5/Zr6 antiserum stains Drosophila myofibrilsbut not chromosomes. Thus, titin localizes to chromosomes inboth Drosophila embryos and human cells although the chromosomaland muscle forms of titin may vary in their NH₂ termini.

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Figure 6 Titin localizes to condensed mitotic chromosomes. HEp-2 cells double-stained with antibodies to vertebrate titin (green) and propidium iodide (red). The merged image is on the right (yellow in region of overlap). From top to bottom: N2A, MIR, BD6, CE12, and A168. Antibodies directed against the most NH₂-terminal regions of vertebrate titin, anti-Zr5/Zr6 and T12, did not detect titin on chromosomes. Antibodies directed against the I-band regions of titin, N2A and 9D10 (not shown) showed weak chromosomal staining. The MIR serum (I/A-band junction) showed stronger chromosomal staining, as well as staining of the mitotic apparatus. Titin antibodies directed against A-band epitopes (BD6 and CE12) and the M-line epitope (A168) showed very strong staining of condensed chromosomes. Bar, 5 µm.

	Discussion

Top Abstract Materials and Methods Results Discussion References

Proposed Function for Titin in Chromosome Structure
The uniform distribution of titin along condensed chromosomessuggests a structural role for titin in chromosome condensation,a role similar to the one titin plays as a scaffolding elementin the sarcomeres (Trinick, 1994, 1996). Chromosome condensationduring mitosis is essential for proper segregation and forcompacting chromosomes so that they are no longer at the cleavagefurrow during cytokinesis (for review see Hirano, 1995; Koshland and Strunnikov, 1996).Chromosome condensation is thought to occur by a deterministicprocess based on the fixed length and banding patterns of individualchromosomes in a given cell-type, the invariant position ofspecific sequences within a chromosome, and the fixed axialdiameter of mitotic chromosomes (Koshland and Strunnikov, 1996).The invariant axial diameter of condensed mitotic chromosomessuggests the involvement of a protein that functions in partas a "molecular ruler", a function that has already been ascribedto titin in muscles (Trinick, 1994, 1996). Thus, we can envisionthe chromosomal form of titin functioning in the assembly ofthe higher-order structure observed in condensed mitotic chromosomes,perhaps determining the length and/or axial diameter of condensed chromosomes.

Titin is the elastic component of sarcomeres where it actsas a molecular spring that prevents sarcomere disruption whenmuscles are overstretched. Likewise, the chromosomal form oftitin could provide elasticity to chromosomes and resistanceto chromosome breakage during mitosis. The elastic propertiesof purified titin (Kellermayer et al., 1997; Rief et al., 1997;Tskhovrebova et al., 1997) correspond well to the recentlydescribed elastic properties of chromosomes in living cells(Houchmandzadeh et al., 1997). Studies on vertebrate myofibrilshave shown that the PEVK domain and the Ig/FN3 repeats constitutea two-spring system acting in series to confer reversible extensibilityto titin (Linke et al., 1996; Trombitas et al., 1998). Underphysiological stretching conditions, the Ig/FN3 domains straightenand the PEVK domain reversibly unfolds. Under more extreme nonphysiologicalstretching conditions, the Ig and FN3 domains also unfold. However,refolding of the Ig and FN3 repeats is slow and occurs onlyin the absence of stretch force. Similarly, metaphase chromosomesfrom living cells also show two levels of extensibility (Houchmandzadeh et al., 1997). Metaphase chromosomes from cultured newt lung cells can bestretched up to 10 times their normal length and return to theirnative shape. Further nonphysiological extensions of chromosomesfrom 10 to 100-fold are irreversible. The discovery of titinon chromosomes integrates the mechanical properties of muscletitin with the elastic properties of eukaryotic chromosomes.

Does titin remain associated with chromosomes during interphase?Although we detected titin in the nucleus during interphasewith both the Drosophila titin antibodies and the antibodiesdirected against vertebrate titin, the resolution of confocalmicroscopy does not allow us to directly ask if titin remainsbound to chromosomes. However, we have looked at the accumulationof D-TITIN on salivary gland polytene chromosomes from Drosophila third instar larvae using the ${alpha}$ -KZ antiserum. Based on geneactivity and chromatin ultrastructure, polytene chromosomesare functionally similar to diploid interphase chromosomes(Tissièrres et al., 1974; Elgin and Boyd, 1975; Bonner and Pardue, 1976;Woodcock et al., 1976). Low level D-TITIN staining was observedthroughout the chromosomes with several discrete sites of higheraccumulation (data not shown). These results suggest that titinremains associated with relatively decondensed interphase chromosomes,consistent with the chromosome core structure being templatedduring interphase (Andreasson et al., 1997). Measurements madeat different stages in the cell cycle indicate that chromosomeflexibility increases during the transition from interphaseto metaphase (Houchmandzadeh et al., 1997). Regulated phosphorylationof titin may control the assembly of interphase chromosomes into the higher-order structure of metaphase chromosomes andindirectly alter chromosome flexibility.

Chromosomal and Muscle Forms of Titin
The chromosomal and muscle forms of titin are unlikely to beidentical. Although both forms of D-TITIN appeared to comigrate,the resolution of the gradient gels used to detect both themuscle and chromosomal forms of D-TITIN may be insufficientto resolve the respective molecular mass differences. The most5' D-Titin cDNA isolated in this work, which encodes an NH₂terminus, does not contain the most 5' sequences found in vertebratemuscle titin, the so-called Z-repeats that bind to ${alpha}$ -actininin the Z-disk (Turnacioglu et al., 1996; Ohtsuka et al., 1997a,b; Sorimachi et al., 1997). Antibodies directed against the ${alpha}$ -actinin–bindingregion of vertebrate titin did not recognize titin on humanchromosomes, although antibodies directed to more COOH-terminalepitopes were reactive (Fig. 6). Furthermore, the most 5' cDNAcontains a unique 81–amino acid sequence at the NH₂terminus.Titin mRNA and protein have been detected in BHK (Jäckel et al., 1997).Moreover, in a subline derived from the BHK cells, the titingene contained deletions in the Z-disk region. Titin mRNA wasstill detected in the mutant cell line. Altogether, these resultssuggest that muscle titin and chromosomal titin vary at leastin their most NH₂-terminal regions. Our results with D-TITINsuggest that the muscle and chromosomal forms of titin areencoded by splice variants of the same gene, and that we havenot cloned the exons encoding the most NH₂-terminal regionsof muscle titin. Polytene chromosome in situ hybridizationand genomic southern analysis revealed that D-Titin is a single-copygene (unpublished results). Determination of whether vertebratechromosomal and muscle titins are also splice variants of thesame gene or, instead, are encoded by two closely related genesawaits further investigation of vertebrate titin.

The previously known components of condensed chromatin includeDNA, histones, topoisomerase II, the SMC family of proteins(for review see Chuang et al., 1994; Earnshaw and Mackay, 1994;Hirano and Mitchison, 1994; Peterson, 1994; Hirano, 1995; Saitoh et al., 1995;Strunnikov et al., 1995; Holt and May, 1996; Koshland and Strunnikov, 1996;Warburton and Earnshaw, 1997), the condensins, three recentlyidentified proteins that form a complex with SMC family members(Hirano et al., 1997), and the cohesins, proteins that linkcondensation and sister chromatid cohesion (Guacci et al., 1997;Michaelis et al., 1997). Topo II and SMC were identified asthe two most abundant chromosomal "scaffold" proteins, whichby definition, comprise an insoluble fraction purified fromisolated mitotic chromosomes. These scaffold proteins are proposedto determine the characteristic shape of mitotic chromosomes.Both genetic and in vitro depletion studies confirm that topoII and SMC proteins are indeed required for chromosome condensationand subsequent chromosome segregation; whether their rolesin chromosome condensation are structural or entirely enzymatic, however, remains to be determined (see previously cited reviewsand Kimura and Hirano, 1997; Sutani and Yanagida, 1997). Iftitin is part of the chromosomal scaffold, why was titin notidentified in the initial biochemical analyses of scaffoldproteins? The simplest explanation is based on the size oftitin. Almost all of the protein gels used to identify topoII, SMC and other scaffold proteins were 12.5% polyacrylamidegels and did not resolve proteins of molecular mass >200kD. Indeed, in almost every published photograph of a proteingel of purified scaffold components, there is a high molecularmass component that fails to enter the gel (Adolph et al., 1977;Paulson and Laemmli, 1977; Laemmli et al., 1978; Lewis and Laemmli, 1982; Earnshaw and Laemmli, 1983). We demonstrated that chromosomallyassociated titin from HEp-2 cells and early Drosophila embryosmigrates in the megadalton size range. Although a protein ofthis size can be resolved in 2.5–7.5% gradient gels,titin would not enter the 12.5% gels typically used in chromosomescaffold studies.

Titin as an Autoantigen
As an alternative to a biochemical approach, autoimmune serahave been successfully used as probes in the isolation of novelchromosomal proteins and for expression cloning of the correspondinggenes (for review see Earnshaw and Rattner, 1991; Tan, 1989,1991; Fritzler, 1997). Even though the prevalence for autoantibodiesagainst nuclear components appears to be higher, the spectrumof autoantibodies identified in sera from patients with autoimmune diseases is much broader, and includes numerous cytoplasmicantigens as well as several extracellular matrix proteins (Fritzler, 1997).Many autoantigens are proteins very well conserved throughoutevolution, ranging from species as distant as man, fish, amphibia,Drosophila, yeast, and plants (Snyder and Davis, 1988; Tan et al., 1987;Mole- Bajer et al., 1990; Brunet et al., 1993; Shibata et al., 1993; Rendon et al., 1994; Bejarano and Valdivia, 1996). The workpresented here is the first to identify titin autoantibodiesin scleroderma sera, the first to reveal titin as a chromosomalcomponent and, to our knowledge, the first successful cloningof a Drosophila gene using a human autoimmune serum.

The identification of autoantibodies against titin until nowhas been restricted to a subset of patients with myastheniagravis (MG) who have also developed thymus neoplasia (Aarli et al., 1990;Gautel et al., 1993). However, the stimulus for the autoimmuneresponse to titin may be due to molecular mimicry. This immunoreactivityis directed exclusively to a single epitope of titin, the MIRepitope. This epitope is shared with neurofilaments that areoverexpressed in these thymomas (Marx et al., 1996). Since titin MIR autoantibodies can be detected in 97% of sera fromMG-thymoma patients, the MIR epitope of titin is a sensitivemarker for evaluating the presence of thymoma in MG patients(Gautel et al., 1993). The isolation of the D-Titin gene inDrosophila using a scleroderma autoimmune serum raises the inevitablequestion of whether titin may represent a new, unidentifiedautoantigen in scleroderma.

D-Titin represents the third Drosophila member of the titingene family. The other two family members, both of which arereferred to as mini-titins (Vibert et al., 1996), include KETTINand PROJECTIN. KETTIN is a 500-kD family member with low homologyto vertebrate titin. KETTIN has been proposed to be one ofthe structural components of Z-disks; however, mutations inthe corresponding gene have not yet been described (Lakey et al., 1993).PROJECTIN is a highly homologous $~$ 1,200-kD titin family membermost closely related to TWITCHIN (Ayme-Southgate et al., 1991,1995; Fyrberg et al., 1992), a Caenorhabditis elegans mini-titinthat binds to myosin filaments in body wall muscles. TWITCHINhas the Ig and FN3 repeats and a myosin light chain kinasedomain near the COOH terminus, but does not have an obviousPEVK region (Benian et al., 1989; Benian et al., 1996). TWITCHIN is thought to regulate myosin activity because mutations in twitchin (unc-22) cannot develop or sustain muscle contractions(Waterston et al., 1980; Moerman et al., 1988). Furthermore,mutations in twitchin can be suppressed by mutations in themyosin heavy chain gene. Lethal alleles of Drosophila PROJECTINexist as mutations in the bent locus. Homozygous bent mutantanimals die as late embryos but, unlike twitchin mutant worms,have apparently normal muscle contractions (Fyrberg et al., 1992;Ayme-Southgate et al., 1995), suggesting normal sarcomere organization.The identification of a true titin homologue in a geneticallytractable organism will greatly facilitate the analysis oftitin function both in sarcomeres and in chromosome structureand flexibility. Indeed, we have mapped the D-Titin gene toa cytological interval known to contain only a single gene.A thorough characterization of D-Titin mutations is currentlyunderway.

Acknowledgments

We thank D. Isenberg for providing scleroderma sera from patientsat the Immunology Unit, King's College (London, UK). We thankS. Labeit and J. Trinick for vertebrate titin antibodies. Wethank J. Mason and A. Spradling for fly stocks. We thank M.Delannoy and K.D. Henderson for assistance with the NORAN confocalmicroscope. We thank P. Tuma for advice with the protein gradientgels. We thank D. Barrick, J.D. Castle, K.D. Henderson, A.Hubbard, C. Machamer, and K. Wilson for their critical commentson the manuscript. We also thank F. Domingues for assistance during the expression screen and all the members of the Andrewlaboratory for their help and patience during the final stagesof this study.

Submitted: 11 December 1997

Revised: 2 February 1998

C. Machado was supported by a Ph.D. fellowship from Junta Nacional de Investigação Cientifica e Tecnológica(JNICT) and, in part, by grants from FundaçãoLuso-Americana para o Desenvolvimento and Fundação Calouste Gulbenkian. This work was supported by a grant fromthe Council for Tobacco Research to D.J. Andrew and a grantfrom JNICT to C.E. Sunkel.

Address all correspondence to Deborah J. Andrew, Departmentof Cell Biology and Anatomy, The Johns Hopkins University Schoolof Medicine, 725 N. Wolfe Street, Baltimore, Maryland 21205-2196.Tel.: (410) 614-2722. Fax: (410) 955-4129. E-mail: debbie_andrew{at}qmail.bs.jhu.edu

References

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