Caenorhabditis elegans Kettin, a Large Immunoglobulin-like Repeat Protein, Binds to Filamentous Actin and Provides Mechanical Stability to the Contractile Apparatuses in Body Wall Muscle

Kanako Ono, Robinson Yu, Kurato Mohri^*, and Shoichiro Ono

Department of Pathology, Emory University, Atlanta, GA 30322

Submitted February 7, 2006; Revised March 9, 2006; Accepted March 23, 2006
Monitoring Editor: Thomas Pollard

ABSTRACT

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Kettin is a large actin-binding protein with immunoglobulin-like(Ig) repeats, which is associated with the thin filaments inarthropod muscles. Here, we report identification and functionalcharacterization of kettin in the nematode Caenorhabditis elegans.We found that one of the monoclonal antibodies that were raisedagainst C. elegans muscle proteins specifically reacts withkettin (Ce-kettin). We determined the entire cDNA sequence ofCe-kettin that encodes a protein of 472 kDa with 31 Ig repeats.Arthropod kettins are splice variants of much larger connectin/titin-relatedproteins. However, the gene for Ce-kettin is independent ofother connectin/titin-related genes. Ce-kettin localizes tothe thin filaments near the dense bodies in both striated andnonstriated muscles. The C-terminal four Ig repeats and theadjacent non-Ig region synergistically bind to actin filamentsin vitro. RNA interference of Ce-kettin caused weak disorganizationof the actin filaments in body wall muscle. This phenotype wassuppressed by inhibiting muscle contraction by a myosin mutation,but it was enhanced by tetramisole-induced hypercontraction.Furthermore, Ce-kettin was involved in organizing the cytoplasmicportion of the dense bodies in cooperation with ${alpha}$ -actinin. Theseresults suggest that kettin is an important regulator of myofibrillarorganization and provides mechanical stability to the myofibrilsduring contraction.

INTRODUCTION

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

In muscle cells, the actin cytoskeleton is highly differentiatedto form the myofibrils that are specialized for producing contractileforces. In addition to actin and myosin as the essential contractilecomponents, regulatory components for the contractile activityare integrated into the structure (Squire, 1997). Despite thefact that many myofibrillar components have been identified,little is known about how these components functionally interactto assemble and maintain the myofibrils in living cells (Littlefieldand Fowler, 1998; Gregorio and Antin, 2000; Clark et al., 2002).In particular, the assembly process of actin filaments is complex.During development, actin-monomer binding proteins, includingprofilin, and actin depolymerizing factor/cofilin regulate actinfilament dynamics (Obinata, 1993; Obinata et al., 1997; Ono,2003a, b). However, in mature myofibrils, these proteins areno longer major components of the thin filaments, and filamentbinding proteins, such as tropomyosin and ${alpha}$ -actinin, and end-cappingproteins, such as CapZ and tropomodulin, become the major actin-associatedproteins. However, the list of actin binding proteins in muscleis still growing and cellular functions of many of these proteinsare not clearly understood.

Kettin is a large protein of 500-700 kDa found in the Z-discsand the I-bands of arthropod muscles (Bullard et al., 2000;Bullard et al., 2002, 2006). Kettin directly binds to actinfilaments with high-affinity (Lakey et al., 1993; Maki et al.,1995; van Straaten et al., 1999). Proteolytic removal of kettinby calpain from the Z-discs causes disintegration of the Z-discs(Lakey et al., 1993) and decrease in stiffness of the myofibrils(Kulke et al., 2001b). Kettin is one of the first proteins tocolocalize with actin during the early stages of myofibrillogenesis(Ayme-Southgate et al., 2004), and genetic analysis has shownthat it is essential for myofibril assembly in the fruit fly(Hakeda et al., 2000). The sequence of kettin contains 35 immunoglobulin-like(Ig) repeats separated by short linker sequences (Hakeda etal., 2000; Kolmerer et al., 2000) and is related to the connectin/titinfamily of giant elastic proteins (Maruyama, 1997; Gautel etal., 1999; Gregorio et al., 1999; Maruyama and Kimura, 2000;Granzier et al., 2002). However, kettin does not have fibronectin-like,elastic PEVK, or kinase domains, and seems to be a uniquelyevolved member of the connectin/titin family of proteins. Importantly,recent molecular genetic studies have shown that kettin is asplice variant of connectin/titin in Drosophila (Machado andAndrew, 2000; Zhang et al., 2000) and crayfish (Fukuzawa etal., 2001). Therefore, the previously reported phenotype ofthe Drosophila kettin mutants (Hakeda et al., 2000) may be partlydue to a defect in the D-titin gene.

Based on sequence homology, a gene coding for a kettin-likeprotein has been found in the nematode Caenorhabditis elegans(Hakeda et al., 2000; Kolmerer et al., 2000). Transcripts ofthis gene are expressed in various muscle cells, and a monoclonalantibody (mAb) against insect kettin reacts with the dense bodiesin obliquely striated body wall muscle (Kolmerer et al., 2000),which is equivalent to the Z-lines in cross-striated muscle.However, the product of the C. elegans kettin-like gene hasnot been extensively studied at the protein level. In this study,we show that the antigen of MH44, one of monoclonal antibodiesraised against C. elegans muscle proteins, is kettin (Francisand Waterston, 1985; Ono et al., 2006). Unlike arthropods, theC. elegans kettin gene is independent of other connectin/titin-relatedgenes, and genetic manipulation of kettin can be applied withoutaffecting them. Our functional analysis of C. elegans kettinsuggests that kettin is an important regulator of actin organizationand myofibril stability in muscle cells.

MATERIALS AND METHODS

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Nematode Strains
Wild-type C. elegans strain N2; an RNA interference (RNAi)-sensitivestrain, NL2099 rrf-3(pk1426) (Simmer et al., 2002); and a myosinheavy chain mutant unc-54(s95) (Moerman et al., 1982) were obtainedfrom the Caenorhabditis Genetics Center (Minneapolis, MN). An ${alpha}$ -actinin mutant, atn-1(ok84), was provided by Drs. Gary Moulderand Robert Barstead (Oklahoma Medical Research Foundation, OklahomaCity, OK). Nematodes were grown under standard conditions at20°C (Brenner, 1974).

Immunoprecipitation and Microsequencing
During the process of purifying actin from C. elegans (Ono,1999), high salt/ATP extracts that are enriched with the thinfilament proteins were saved and used for immunoprecipitation.Briefly, frozen nematodes were thawed in a homogenizing buffer(50 mM NaCl, 1 mM EDTA, 20 mM Tris-HCl, 1 mM dithiothreitol,and 1 mM phenylmethylsulfonyl fluoride [PMSF], pH 8.0) and homogenizedby passing twice through a French pressure cell at 360-580 kg/cm².The homogenate was centrifuged at 10,000 x g for 10 min, andthe pellet was washed twice with the homogenizing buffer. Thewashed pellet was extracted twice with 1 volume of a high salt/ATPbuffer (0.6 M KCl, 5 mM ATP, 5 mM MgCl₂, 20 mM Tris-HCl, 0.2mM EGTA, 1 mM dithiothreitol, and 1 mM PMSF, pH 8.0) and centrifugedat 10,000 x g for 10 min. The supernatant (1 ml) was dialyzedagainst phosphate-buffered saline (PBS) overnight at 4°C.The extract was cleared by centrifugation at 20,000 x g for10 min, mixed with 50 µl of 10% Triton X-100 and 5 µlof the mAb MH44 (Francis and Waterston, 1985) (provided by PamelaHoppe, Western Michigan University, Kalamazoo, MI) in ascitesfluid, and incubated on ice for 2 h. Then, 30 µl of proteinG-agarose beads (Pierce Chemical, Rockford, IL) that had beenwashed with PBS was added and incubated for 90 min at 4°Cwith gentle mixing. The beads were recovered by brief centrifugationat 5000 x g and washed three times with 1 ml each of PBS containing0.5% Triton X-100 and twice with 1 ml each of PBS. The boundproteins were eluted with 50 µl of SDS-lysis buffer (2%SDS, 80 mM Tris-HCl, 5% $beta$ -mercaptoethanol. 15% glycerol, and0.05% bromophenol blue, pH 6.8) at 97°C for 2 min.

The immunoprecipitates were resolved by sodium dodecyl sulfate-polyacrylamidegel electrophoresis (SDS-PAGE) and analyzed by silver staining(Figure 1) or Coomassie blue staining for microsequencing. The60- to 62-kDa bands were excised together from the gel and submittedto ProtTech (Fairview Village, PA) for identification of theprotein following their standard procedure. Briefly, the proteinin the gel piece was digested with trypsin in 50 mM ammoniumbicarbonate at pH 8.5, and the peptides were extracted by 3–5volumes of acetonitrile, dried, and dissolved in 0.5% aceticacid. The peptides were analyzed by liquid chromatography coupledwith tandem mass spectrometry (LC-MS/MS). The MS/MS data weresubjected to homology search against the protein database andmanually analyzed for the quality of the results.

cDNA Cloning and Sequencing
Total C. elegans RNA was prepared from N2 using a TRI reagent(Sigma-Aldrich, St. Louis, MO). Fragments (1-2 kb) of the Ce-kettincDNA were amplified with reverse transcriptase (RT)-PCR usinga SuperScript III one-step RT-PCR with Platinum Taq DNA polymerase(Invitrogen, Carlsbad, CA) with primers listed in SupplementalTable 1. Nematode mRNAs often have the SL1 trans-spliced leadersequence at their 5' ends. Therefore, the 5' end of the Ce-kettinmRNA was amplified by PCR using SL1 as a forward primer (Fr-1in Supplemental Table 1). They were cloned into a pCR-II plasmidvector using a TOPO-TA cloning kit (Invitrogen), and the sequenceswere determined by DNA sequencing. The sequences were manuallyassembled into a contiguous full-length cDNA sequence.

Fluorescence Microscopy
For immunofluorescent staining of adult body wall muscle inFigure 3, adult worms were cut in halves near the vulva by needleson poly-lysine–coated slides and permeabilized by a freeze-crackmethod (Epstein et al., 1993). The gonads were dissected bycutting adult hermaphrodites at the level of pharynx on poly-lysine–coatedslides as described previously (Rose et al., 1997). Worm embryoswere obtained by cutting gravid adults on poly-lysine–coatedslides and permeabilized by a freeze-crack method. These sampleswere fixed by an optimal method and stained with antibodiesas listed in Table 1. Immunofluorescent staining of adult bodywall muscle in Figure 8 was performed by a whole-mount stainingprocedure as described previously (Finney and Ruvkun, 1990).When the host animals of the primary antibodies were different,they were mixed and reacted with the samples simultaneously,and followed by treatments with appropriate fluorescently labeledsecondary antibodies (Table 1). We also succeeded in differentiallylabeling two mouse monoclonal antibodies by using secondaryantibodies that distinguish IgG isotypes. MH44 is IgG2a, andmouse monoclonal antibodies of the IgG1 isotype were used forsimultaneous staining with MH44. The samples were first treatedwith mixture of mouse IgG1 antibody and rabbit or guinea pigantibody, and then with secondary antibodies (nonspecific forIgG isotypes). They were washed with PBS and blocked with 0.1mg/ml mouse IgG (Rockland, Gilbertsville, PA) in 1% bovine serumalbumin in PBS for 10 min and reacted with MH44. Then, MH44was visualized by Zenon Alexa Fluor mouse IgG2a labeling reagents(Invitrogen) (Table 1).

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Table 1. Fixation methods and antibodies for immunofluorescent staining

Guinea pig anti-tropomyosin (CeTM) antibody was described previously(Ono and Ono, 2002

). Rabbit polyclonal anti-actin antibody (AAN01)was purchased from Cytoskeleton (Denver, CO). Mouse monoclonalanti-actin antibody (C4) was purchased from MP Biomedicals (Irvine,CA). Mouse monoclonal anti-myoA antibody (clone 5-6) (Milleret al., 1983

) was provided by Henry Epstein (University of TexasMedical Branch at Galveston, Galveston, TX). Mouse monoclonalanti-vinculin antibody (MH24) and mouse monoclonal anti- ${alpha}$ -actininantibody (MH40) (Francis and Waterston, 1985

) was provided byPamela Hoppe.

Samples were viewed by epifluorescence using a Nikon EclipseTE2000 inverted microscope with a 40 or 60x CFI Plan Fluor objective.Images were captured by a SPOT RT monochrome charge-coupleddevice camera (Diagnostic Instruments, Sterling Heights, MI)and processed by the IPLab imaging software (Scanalytics, Rockville,MD) and Adobe Photoshop 6.0 (Adobe Systems, Mountain View, CA).

Preparation of Recombinant Ce-Kettin Fragments
To construct an expression vector for KETN-CT1, a cDNA fragmentencoding residues 3830-4250 was amplified by PCR using primers5'-GATCGGATCCCAAGCTCCACCGACAATCTCCC and 5'-GATCGGTACCCTAGCGACTGAGTGTGAGCTTGthat have added BamHI and KpnI restriction sites (underlined),respectively. The PCR product was digested by BamHI and KpnIand ligated with pQE-30 (QIAGEN, Valencia, CA) at BamHI–KpnIcloning sites. Expression of a 6xHis-tagged protein from thisvector was not successful. Therefore, the cDNA fragment wasexcised from the vector by BamHI and SmaI and ligated with pGEX-2T(GE Healthcare, Little Chalfont, Buckinghamshire, United Kingdom)at BamHI–SmaI cloning sites. The cDNA insert was entirelysequenced to verify that there were no PCR-induced mutations.

To construct an expression vector for KETN-CT2, two cDNA fragmentsCT2-1 and CT2-2 that overlap by 22 base pairs were amplifiedby RT-PCR. Primers for CT2-1 were 5'-GGTTCCGCGTGGATCCAGACAGACCAAGTTGAGACCGGCand 5'-GGGAGATTGTCGGTGGAGCTTG. Primers for CT2-2 were 5'-CAAGCTCCACCGACAATCTCCCand 5'-TCACGATGAATTCCCCTAGCGACTGAGTGTGAGCTTG. Fifteen or 16base pairs of overlapping sequences with pGEX-2T were designedat the 5' and 3' ends of CT2-1 and CT2-2 (underlined), respectively.CT2-1, CT2-2, and pGEX-2T that had been cut by BamHI and SmaIwere fused at their homologous ends by an In-fusion PCR cloningkit (Clontech). The cDNA insert was entirely sequenced to verifythat there were no PCR-induced mutations.

To construct an expression vector for KETN-CT3, a cDNA fragmentencoding residues 3554-3831 was amplified from pGEX-KETN-CT2by PCR using primers 5'-GGTTCCGCGTGGATCCAGACAGACCAAGTTGAGACCGGCand 5'-TCACGATGAATTCCCTCAAGCTTGCTTAGATTGCCCGATCTTTG. Fifteenor 16 base pairs of overlapping sequences with pGEX-2T wereadded at the 5' and 3' ends (underlined). The PCR product andpGEX-2T that had been cut by BamHI and SmaI were fused at theirhomologous ends by an In-fusion PCR cloning kit (Clontech).The cDNA insert was entirely sequenced to verify that therewere no PCR-induced mutations.

KETN-CT1, KETN-CT2, and KETN-CT3 were expressed in Escherichiacoli as glutathione S-transferase (GST)-fusion proteins andpurified by the same method. The E. coli strain BL21 (DE3) wastransformed with the expression vector and cultured in M9ZBmedium containing 50 µg/ml ampicillin at 37°C untilabsorbance at 600 nm reached 0.6 cm^–1. Then, the culturewas cooled to room temperature, and protein expression was inducedby adding 0.1 mM isopropyl $beta$ -D-thiogalactopyranoside for 3 hat room temperature. The cells were harvested by centrifugationat 5000 x g for 10 min and disrupted by a French pressure cellat 360-580 kg/cm² in PBS containing 0.2 mM dithiothreitol and0.4 mM PMSF. The homogenates were centrifuged at 20,000 x gfor 15 min, and the supernatants were applied to a glutathione-Uniflowcolumn (bed volume of 1 ml) (Clontech). The columns were washedby 10 column volumes of PBS and bound proteins were eluted with10 mM glutathione, 20 mM Tris-HCl, 0.2 mM dithiothreitol, pH8.0. Fractions containing the GST-fusion proteins were dialyzedagainst 0.1 M KCl, 20 mM MES-KOH, and 0.2 mM dithiothreitol,pH 6.0, and purified further with Mono S column chromatography.The proteins were eluted from the Mono S column with a linearKCl gradient of 0.1–0.5 M and dialyzed overnight against0.1 M KCl, 2 mM MgCl₂, 20 mM HEPES-NaOH, and 0.2 mM dithiothreitol,pH 7.5. Protein concentrations were determined by a BCA ProteinAssay kit (Pierce Chemical).

Actin Binding Assay
Rabbit muscle actin was prepared as described previously (Pardeeand Spudich, 1982), and its binding with the kettin fragmentswas examined by a copelleting assay as described previously(Mohri and Ono, 2003; Mohri et al., 2004) with modifications.GST-KETN-CT1, GST-KETN-CT2, or GST-KETN-CT3 (all 0-30 µM0was incubated with or without 5 µM F-actin in a buffercontaining 0.1 M KCl, 2 mM MgCl₂, 1 mM dithiothreitol, and 20mM HEPES-NaOH, pH 7.5, for 30 min at room temperature and ultracentrifugedat 80,000 rpm for 20 min in a Beckman TLA-100 rotor. The supernatantsand pellets were adjusted to the same volumes and analyzed bySDS-PAGE. Gels were stained with Coomassie brilliant blue R-250(National Diagnostics, Atlanta, GA), scanned by a UMAX PowerlookIII scanner at 300 dpi, and the band intensity was quantifiedby Scion Image Beta 4.02 (Scion, Frederick, MD). To quantifythe amounts of the kettin fragments that bound to actin, theamounts of nonspecific sedimentation of the kettin fragmentswere determined from control experiments without F-actin andsubtracted from the data of the assays with actin.

RNA Interference Experiments
Nematodes were treated with RNAi for ketn-1 by feeding E. coliexpressing double-stranded RNA under the conditions as describedpreviously (Ono and Ono, 2002). The RNAi clone for ketn-1 (V-2F01)was obtained from the C. elegans RNAi library from Geneservice(Cambridge, United Kingdom) (Kamath et al., 2003). Control experimentswere performed with the E. coli strain HT115 (DE3) that wastransformed with an empty RNAi vector L4440 (Timmons and Fire,1998; Timmons et al., 2001). Phenotypes were analyzed in theirF1 generation. Staining of worms with tetramethylrhodamine-phalloidinwas performed as described previously (Ono, 2001). For tetramisoletreatment, worms were harvested by M9 buffer, washed once withM9 buffer, and incubated in 10 ml M9 buffer with or without0.01% tetramisole (MP Biomedicals) for 1 h at room temperatureon a nutator. To determine brood size, F1 RNAi-treated wormswere isolated at the L4 larval stage in individual plates, andthe number of progeny was counted by removing the progeny fromthe plates until the worms cease producing progeny.

Protein Electrophoresis and Western Blot
Fifty adult worms were lysed in 20 µl of SDS-lysis buffer(2% SDS, 80 mM Tris-HCl, 5% $beta$ -mercaptoethanol, 15% glycerol,and 0.05% bromophenol blue, pH 6.8), heated at 97°C for2 min, homogenized by brief sonication, and heated again at97°C for 2 min. The samples were resolved by SDS-PAGE usinga 4 or 5% acrylamide gel and transferred onto a polyvinylidenedifluoride membrane (Immobilon-P; Millipore, Billerica, MA)using a Genie Blotter (Idea Scientific, Minneapolis, MN). Themembrane was blocked in 5% nonfat milk in PBS containing 0.1%Tween 20 for 30 min and incubated with MH44 (1/2000-dilutedascites fluid) for 1 h followed by treatment with peroxidase-labeledgoat anti-mouse IgG (Pierce Chemical). The reactivity was detectedwith a SuperSignal chemiluminescence reagent (Pierce Chemical).The membrane was treated with a buffer containing 2% SDS, 100mM $beta$ -mercaptoethanol, and 62.5 mM Tris-HCl, pH 6.8, at 50°Cfor 30 min to remove bound probes, and reprobed with mouse monoclonalanti-myoA antibody (5-6) as a loading control.

RESULTS

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Identification of the Antigen for the Monoclonal Antibody MH44 as C. elegans Kettin
Francis and Waterston (1985) generated the mAb MH44 and reportedthat its antigen was a 400- to 440-kDa protein and localizedto the I-bands in C. elegans body wall muscle. We confirmedby Western blot that MH44 specifically reacted with this high-molecular-weightprotein with very weak reactivity with smaller proteins thatcould be proteolytic products or unknown splice variants ofthe major band (Ono et al., 2006). Although MH44 has been usedas a marker for the I-bands, the MH44 antigen had not been molecularlyidentified. To determine the molecular nature of the MH44 antigen,we isolated this protein from the crude thin filament fractionby immunoprecipitation (Figure 1). In three independent experiments,no high-molecular-weight proteins of 400-440 kDa were recovered.Instead, two 60- to 62-kDa proteins were reproducibly precipitatedby MH44 (Figure 1, lane 1). We determined partial peptide sequenceof these proteins by LC-MS/MS analysis and identified 27 trypticpeptides (Supplemental Table 2) that corresponded to the sequenceof a putative C. elegans protein F54E2.3 (GenBank/European MolecularBiology Laboratory [EMBL]/DNA Data Bank of Japan [DDBJ] accessionno. AAC78200) with a predicted M_r of 500 K, suggesting thatthe isolated proteins were proteolytic fragments of this largeprotein.

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Figure 1. Immunoprecipitation of the MH44 antigen. Immunoprecipitates with MH44 (lane 1) and control precipitates in the absence of MH44 (lane 2) were analyzed by SDS-PAGE (5% acrylamide gel) and silver staining. There were no specific bands around 400-500 kDa, Instead, two bands of 60-62 kDa (arrows) were detected in the precipitates with MH44. These bands were subjected to microsequencing. Molecular mass markers in kilodaltons (lane M) are indicated on the left of the gel.

Two previous studies have reported that F54E2.3 is an orthologueof Drosophila kettin, a large Ig-repeat protein in striatedmuscle (Hakeda et al., 2000

; Kolmerer et al., 2000

). However,its gene products have been deduced from computer-predictedexon–intron structures and only partial cDNA sequencesnear the 3' end of the gene have been analyzed by the ExpressedSequence Tag project. Therefore, we determined the full-lengthcDNA sequence (13.6 kb) of the F54E2.3 gene product from eightcontiguous cDNA fragments (Supplemental Table 1) and found thatthis gene indeed encodes a kettin-like protein that consistsof 4250 amino acids with calculated molecular weight of 471,704(GenBank/EMBL/DDBJ accession no. AY819766).

Ce-kettin is composed of 31 Ig-repeats (Figure 2, gray region)and a unique kettin-specific sequence that is located betweenthe 27th and 28th repeats (Figure 2). All the Ig-repeats havebeen accurately predicted by Kolmerer et al., (2000), and theyare separated by weakly conserved linker sequences. Previousgenome-wide analyses of Ig-repeat proteins in C. elegans didnot annotate the Ce-kettin gene correctly (Teichmann and Chothia,2000; Vogel et al., 2003) due to lack of information on thecDNA sequence. In addition, this gene has been predicted togenerate a protein with a prion-like-Q/N-rich (PQN) domain atthe N terminus and designated as pqn-43 in the WormBase (Chenet al., 2005) and the sequence database (GenBank/EMBL/DDBJ accessionno. NP_503758). However, our cDNA sequence does not containthe PQN sequence in the open reading frame. Therefore, we proposethat ketn-1 is an appropriate designation for the Ce-kettingene.

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Figure 2. Domain structure of Ce-kettin. Ig domains are shown in gray. The C-terminal fragments KETN-CT1, KETN-CT2, and KETN-CT3 were bacterially produced as fusion proteins with GST and used in in vitro assays in Figure 6. These Ce-kettin fragments were also tested for reactivity with MH44 on Western blot. The reactivity (+ or –) is shown on the right.

We found that MH44 strongly reacted with bacterially expressedC-terminal fragments of this protein, KETN-CT1 (residues 3830-4250)and KETN-CT2 (residues 3554-4250) but not with KETN-CT3 (residues3554-3831) on Western blot (Figure 2), indicating that the epitopeof MH44 is present within the four C-terminal Ig-repeats. Insupport of these data, the tryptic peptides of the MH44 precipitatescorrespond to the C-terminal region of this sequence (SupplementalTable 2).

Localization of Ce-Kettin to the Thin Filaments in Striated and Nonstriated Muscle
MH44 was previously shown to label the entire I-bands in bodywall muscle (Francis and Waterston, 1985). We reexamined intracellularlocalization of Ce-kettin by double or triple staining withother cytoskeletal markers and found that it localized to aportion, not the entire length, of the I-bands (Figure 3). Triplestaining of body wall muscle for actin (thin filaments), Ce-kettin(MH44), and myosin heavy chain (thick filaments) confirmed thatCe-kettin is associated with the thin filaments (Figure 3, A,D, G, and J). However, Ce-kettin localized to a ladder-likepattern and its localization was limited to a narrow regionin the middle of the bands of actin (Figure 3, compare D–Ffor Ce-kettin with A–C for actin). Triple staining foractin, Ce-kettin, and vinculin (dense bodies) showed that Ce-kettinhas some overlap with vinculin, but the center of the densebodies was devoid of Ce-kettin (Figure 3, B, E, H, and K). Inaddition, comparison with the location of tropomyosin showedthat tropomyosin localized to the outer region on the thin filamentswith minimal overlap with Ce-kettin (Figure 3, C, F, I, andL). These results indicate that Ce-kettin is associated witha portion of the thin filaments near the dense bodies.

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Figure 3. Localization of Ce-kettin in adult body wall muscle. Adult body wall muscle was stained for actin (A–C), Ce-kettin (D–F), and myoA myosin heavy chain (G), vinculin (H), or tropomyosin (I). Merged images of actin (red), Ce-kettin (green), and myoA, vinculin, or tropomyosin (blue) are shown in J–L. Bar, 10 µm.

Our results on the Ce-kettin localization differ from the reportby Kolmerer et al. (2000)

, which demonstrated that an antibodyagainst insect kettin stained the dense bodies. Therefore, wereevaluated the specificity of the mAb MAC155 (provided by BelindaBullard, EMBL, Heidelberg, Germany) against insect kettin thatwas used in Kolmerer et al. (2000)

. By Western blot of totalC. elegans extracts, we found that MAC155 reacted with a 200-kDaprotein but not with proteins of 400-500 kDa that were recognizedby MH44 (our unpublished data). This result suggests that MAC155has other reactivities with an unknown component of the densebodies other than kettin.

In addition, Ce-kettin was expressed in nonstriated muscles,including the pharynx, the vulva, and the myoepithelial sheathof the proximal ovary (Figure 4). In particular, Ce-kettin wasassociated with the actin filaments in spots adjacent to thedense bodies (Figure 4, A–D) in the ovarian myoepithelialsheath that expresses the same myosin heavy chain isoform asthe body wall muscle (Ardizzi and Epstein, 1987) and uses tropomyosinand troponin for regulation of contraction (Ono and Ono, 2004).Differential localization of tropomyosin and Ce-kettin on theactin filaments was more clearly observed in this nonstriatedmuscle (Figure 4, E–H). Tropomyosin was associated withthe entire length of the actin filaments (Figure 4G), whereasCe-kettin localized to spots that are associated with the actinfilaments (Figure 4F). Observation at a higher magnificationrevealed that tropomyosin is not detected where Ce-kettin islocated (Figure 4, I–L, arrows). These localization patternssuggest that tropomyosin and Ce-kettin bind to actin in a mutuallyexclusive manner.

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Figure 4. Localization of Ce-kettin in ovarian nonstriated muscle. Myoepithelial sheath of the proximal ovary was stained for actin (A, E, and I), Ce-kettin (B, F, and J), and vinculin (C) or tropomyosin (G and K). Merged images of actin (red), Ce-kettin (green), and vinculin or tropomyosin (blue) are shown in D, H, and L. High-magnification images in I–L show a representative area where differential localization of Ce-kettin and tropomyosin is clearly observed (arrows). Bars, 10 µm (A–H) and 5 µm (I–L).

During development, expression of Ce-kettin in body wall musclewas detected as early as the comma stage (290 min after thefirst cleavage) (Figure 5A), and it colocalized with actin atthe early stage of myofibril assembly (Figure 5, B and C). Atthe twofold stage (430 min), in addition to the expression inthe body wall muscle (Figure 5, D–F), strong expressionof Ce-kettin in the pharynx was detected (Figure 5G) beforerobust assembly of actin was initiated (Figure 5, G–I).At the threefold stage (520 min), expression of Ce-kettin inthe body wall muscle (Figure 5, J–L) and the pharynx (Figure 5,M–O) became stronger, and its localization to the contractileapparatuses was more remarkable. These results indicate thatCe-kettin is one of the earliest proteins to be assembled intothe myofibrils.

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Figure 5. Localization of Ce-kettin in embryos. Embryos at the comma (A–C), twofold (D–I), and threefold (J–O) stages were stained for Ce-kettin (A, D, G, J, and M) and actin (B, E, H, K, and N). Merged images of Ce-kettin (green) and actin (red) are shown in C, F, I, L, and O. Focus was adjusted for the body wall muscle in D–F and J–L or the pharynx in G–I and M–O. Actin-rich structure in H (asterisk) is the nerve ring. Bar, 10 µm.

Binding of the C-Terminal Kettin-specific and Ig Domains to Filamentous Actin
We reasoned that an actin binding site is present in the C terminusof Ce-kettin, because a C-terminal fragment of Ce-kettin wasfractionated in the crude thin filament preparation (Figure 1).To test actin binding activity of the Ce-kettin C-terminal domains,we purified bacterially expressed C-terminal fragments of Ce-kettinand examined their ability to interact with filamentous actin.We prepared three Ce-kettin fragments as fusion proteins withGST. KETN-CT1 corresponds to residues 3830-4250 containing thefour C-terminal Ig-repeats (repeats 28-31). KETN-CT2 (residues3554-4250) has the kettin-specific sequence with unknown functionin addition to Ig-repeats 28-31. KETN-CT3 (residues 3554-3831)has only the kettin-specific sequence (Figure 2).

KETN-CT1, KETN-CT2, and KETN-CT3 bound to F-actin with differentaffinity and stoichiometry (Figure 6). In cosedimentation assays,significant portions of GST-KETN-CT1, GST-KETN-CT2, or GST-KETN-CT3,cosedimented with F-actin (Figure 6, A–C). GST alone didnot cosediment with actin under the same conditions, and nonspecifictrapping of GST in the pellets was very minor (Figure 6D) (Mohriet al., 2004). Quantitative analysis of the data showed thatKETN-CT2 bound to F-actin with higher affinity (K_d = 0.68 ±0.062 µM) than KETN-CT1 (K_d = 0.93 ± 0.36 µM)or KETN-CT3 (K_d = 5.5 µM ± 1.2 µM). Alsointerestingly, binding was saturated for KETN-CT2 or KETN-CT3at higher stoichiometry (mol KETN-CT2/mol actin = 0.34 ±0.0080 or $~$ 3:1; mol KETN-CT3/mol actin = 0.42 ± 0.029or $~$ 2.4:1) than for KETN-CT1 (mol KETN-CT1/mol actin = 0.15 ±0.016 or $~$ 6.7:1) (Figure 6E). These results suggest that thekettin-specific region augments the actin binding activity ofthe Ig-repeats.

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Figure 6. Binding of the C-terminal fragments of Ce-kettin with actin filaments in vitro. Various concentrations of GST-KETN-CT1 (A), GST-KETN-CT2 (B), GST-KETN-CT3 (C), or GST (D) were incubated with or without 5 µM F-actin, and their interactions were examined by copelleting assays. The samples were fractionated into supernatants (s) and pellets (p) and analyzed by SDS-PAGE. Positions of actin (A), Ce-kettin fragments (K), and GST (G) are indicated on the right of the gels. The data were quantified by densitometric analysis (E).

RNA Interference of Ce-Kettin Causes Disorganization of Actin Filaments in a Contraction-dependent Manner
To examine the in vivo function of Ce-kettin, Ce-kettin wasknocked down by RNAi and the resultant phenotype examined. RNAiof Ce-kettin [ketn-1(RNAi)] by the feeding method effectivelyreduced Ce-kettin to undetectable levels on Western blot inwild-type background (Figure 7A). The ketn-1(RNAi)–treatedworms moved slightly slower than control worms (our unpublisheddata), suggesting that ketn-1(RNAi) caused a defect in bodywall muscle contractility. Staining of the muscle actin filamentswith fluorescently labeled phalloidin revealed that the ketn-1(RNAi)–treatedworms had alterations in the actin filaments in the body wallmuscle (Figure 7, C–F). Small round actin aggregates orunusual accumulations of actin were detected in 23% (n = 100)of the ketn-1(RNAi)–treated worms (Figure 7D, arrows),whereas no worms exhibited these phenotypes in control experiments(n = 100) (Figure 7, B and C). Some genes are not efficientlyaffected by RNAi in wild-type background but are susceptibleto RNAi in an rrf-3 mutant background (Simmer et al., 2002

,2003

). However, in the rrf-3 background, the phenotypes wereonly slightly enhanced. The rrf-3; ketn-1(RNAi) worms also hadsmall round actin aggregates or unusual accumulations of actinin the body wall muscle in 30% of treated animals (n = 100)(Figure 7, B and F), whereas no control rrf-3 worms exhibitedthese phenotypes (n = 100) (Figure 7, B and E). Therefore, thelow penetrance of the ketn-1(RNAi) phenotype is not simply dueto the efficiency of RNAi. Actin organization in the pharynxand ovarian nonstriated muscle was not significantly alteredby the RNAi treatments (our unpublished data). However, broodsize was reduced by ketn-1(RNAi) in the rrf-3 background [83.4± 18 in control RNAi and 47.2 ± 6.8 in ketn-1(RNAi),n = 5], but not in wild-type background [280 ± 30 incontrol RNAi and 281 ± 28 in ketn-1(RNAi), n = 5], suggestingthat the reproductive system, in particular the activity ofthe ovarian myoepithelial sheath, uterine muscle, or vulvalmuscle, might be partially impaired. In the control experiments,rrf-3 mutants produced fewer progeny than wild type, suggestingthat rrf-3 is less tolerant to functional alterations in thereproductive system. These results strongly suggest that Ce-kettinis involved in assembly and/or maintenance of actin filamentsin muscle cells.

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Figure 7. Disorganization of actin filaments in adult body wall muscle by RNA interference of Ce-kettin. (A) Protein levels of Ce-kettin in control or ketn-1 (RNAi) worms (50 worms per lane) in wild-type or rrf-3 background were examined by Western blot with MH44. The same membrane was reprobed with anti-myoA antibody to confirm equal loading of the proteins. (B) Frequency of formation of actin aggregates. Worms were stained with tetramethylrhodamine-phalloidin, and percentages of adult worms (n = 100) with actin aggregates in the body wall muscle were determined. (C–H) Actin organization in the body wall muscle of control RNAi (C, E, G, I, and K) or ketn-1 (RNAi) (D, F, H, J, and L) worms in wild-type (C, D, and I–L), rrf-3 (E and F), or unc-54 (G and H) backgrounds was examined by staining with tetramethylrhodamine-phalloidin. Worms in I–L were incubated in M9 buffer for 1 h in the absence (I and J) or presence (K and L) of 0.01% tetramisole before fixation. In ketn-1 (RNAi) worms, small round aggregates and unusual actin accumulations at the edges of muscle cells (arrows in D, F, and J) were detected, and this phenotype was enhanced by tetramisole-induced hypercontraction (L). Bar, 50 µm.

Although disorganized actin filaments after ketn-1(RNAi) weredetected at low penetrance, we found that this phenotype issensitive to the state of muscle contraction. unc-54(s95) isa mutation in the head domain of the UNC-54 myosin heavy chainthat reduces muscle contraction without affecting overall structureof the myofibrils (Moerman et al., 1982

). In the unc-54(s95)homozygous background, ketn-1(RNAi) did not cause formationof actin aggregates (Figure 7, B and H), suggesting that reducedmuscle contraction suppressed disruption of actin filaments.In contrast, when hypercontraction was induced by tetramisole,an agonist of acetylcholine receptors, larger actin aggregateswere formed more frequently at the cell periphery in 94% (n= 100) of the ketn-1(RNAi) worms (Figure 7B and compare Figure 7,J and L). These results suggest that disorganization of actinfilaments in the ketn-1(RNAi) worms is caused by mechanicaldisruption of the actin filaments during contraction and thatCe-kettin provides stability to the myofibrils.

Ce-Kettin Regulates Localization of Tropomyosin and ${alpha}$ -Actinin
In vitro studies have shown that insect kettin binds to ${alpha}$ -actinin,whereas it competes with tropomyosin for binding to actin (Lakeyet al., 1993; van Straaten et al., 1999), but their functionalrelationship in vivo is not understood. We examined how Ce-kettininteracts with tropomyosin and ${alpha}$ -actinin in the C. elegans bodywall muscle. As shown in Figure 3, tropomyosin is normally localizedto the outer region on the thin filaments. In worms treatedwith control RNAi, the normal localization of tropomyosin asdouble lines was observed (Figure 8A, a). However, in ketn-1(RNAi)worms, tropomyosin also localized to regions where Ce-kettinnormally localizes, resulting in the ladder-like localization(Figure 8A, d). This result strongly suggests that Ce-kettinand tropomyosin compete for binding to actin in vivo.

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Figure 8. Functional interaction between Ce-kettin and ${alpha}$ -actinin in the body wall muscle. (A) Tropomyosin (a and d), ${alpha}$ -actinin (g and j), vinculin (m and p), or myoA myosin heavy chain (s and v) was double-stained with actin (b, e, h, k, n, q, t, and w) in the body wall muscle of control or ketn-1(RNAi) adult worms. Merged images are shown (c, f, i, l, o, r, u, and x). (B) Ce-kettin (a) and actin (b) were immunolocalized in the atn-1(ok84) homozygous worms. (C) Actin filaments in the body wall muscle of the atn-1(ok84) worms with control RNAi (a) or ketn-1(RNAi) (b) were stained with tetramethylrhodamine-phalloidin. Bars, 10 µm (A), 20 µm (B), and 50 µm (C).

Normal organization of ${alpha}$ -actinin was dependent on Ce-kettin. ${alpha}$ -Actinin was deposited at the dense bodies in control worms(Figure 8A, g), whereas, in ketn-1(RNAi) worms, the patternof ${alpha}$ -actinin was disturbed and the shape of the accumulationsof ${alpha}$ -actinin became highly irregular (Figure 8A, j). In contrast,the pattern of vinculin at the dense bodies was only slightlyaffected by ketn-1(RNAi) (Figure 8A, compare m and p). Vinculinis at the base of the dense bodies near the plasma membrane,whereas ${alpha}$ -actinin localizes at the cytoplasmic portion (Francisand Waterston, 1985

). Therefore, Ce-kettin is specifically involvedin the organization of the cytoplasmic region of the dense bodies.The striated pattern of the myoA myosin heavy chain was unaffectedby ketn-1(RNAi) (Figure 8A, compare s and v), supporting thespecific function of Ce-kettin in the thin filaments and thedense bodies.

The functional relationship between Ce-kettin and ${alpha}$ -actinin wasfurther examined in an ${alpha}$ -actinin mutant (Figure 8, B and C).atn-1(ok84) has a 1.1-kb deletion in the single gene for ${alpha}$ -actininatn-1 (Barstead et al., 1991), is homozygous viable, and showsonly minor alterations in the striated arrangement of actinfilaments and small aggregations of actin at the edges of thebody wall muscle cells (Moulder and Barstead, personal communication)(Figure 8B, b). Position of the atn-1(ok84) deletion suggeststhat a truncated ${alpha}$ -actinin protein containing the N-terminalactin binding domain could be expressed, but the presence ofsuch a truncated protein has not been confirmed (Moulder andBarstead, personal communication). In the ${alpha}$ -actinin mutant, Ce-kettincolocalized with actin to the striated myofibrils, but the patternof Ce-kettin was continuous (Figure 8B, a) rather than ladder-like(Figure 3). This is probably because the cytoplasmic portionof the dense bodies may not be well defined, in which ${alpha}$ -actininis the major component. Ce-kettin was not associated with theactin aggregates in the ${alpha}$ -actinin mutant (Figure 8B, a–c).Furthermore, when the ${alpha}$ -actinin mutant was treated with ketn-1(RNAi),disorganization of the actin filaments was enhanced and largeractin aggregates were often detected (Figure 8C, compare a andb). These results suggest that Ce-kettin and ${alpha}$ -actinin cooperateto organize the dense bodies and the thin filaments.

DISCUSSION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

In this study, we identified the C. elegans kettin gene andthe gene product as the antigen for the mAb MH44 that has beenused as a marker for the I-bands in the C. elegans muscle. Comparisonsof the localization pattern of Ce-kettin with that of otherthin filament proteins revealed that Ce-kettin is associatedwith the thin filaments near the dense bodies, the homologousstructures to the Z-discs in cross-striated muscles. Biochemicalanalysis showed that the four C-terminal Ig domains of Ce-kettindirectly bind to actin filaments in vitro and that the kettin-specificsequence immediately N-terminal to these Ig domains enhancesits actin binding activity. RNAi of Ce-kettin caused disorganizationof actin filaments in body wall muscle. This phenotype was suppressedby reducing muscle contraction, but enhanced by hypercontraction.RNAi of Ce-kettin also disturbed organization of ${alpha}$ -actinin atthe dense bodies and enhanced the actin disorganization phenotypein an ${alpha}$ -actinin mutant. These results suggest that Ce-kettinis important for maintaining organized architecture of the actinfilaments and dense bodies and provides mechanical stabilityto the contractile apparatuses in muscle cells.

Localization of Ce-kettin on the thin filaments was proximalto the dense bodies and was similar to that of kettins frominsects (Lakey et al., 1990, 1993; van Straaten et al., 1999)and crayfish (Maki et al., 1995; Fukuzawa et al., 2001), whichare localized to the side of the Z-discs. In addition, the Nterminus of insect kettin is located within the Z-discs (vanStraaten et al., 1999). Because MH44 recognizes the C terminusof Ce-kettin, the N terminus of Ce-kettin is likely to be embeddedin the dense bodies. This limited localization of kettin isprobably due to competition with tropomyosin for binding toactin (van Straaten et al., 1999), because Ce-tropomyosin ismore distally localized on the thin filaments (Figures 3 and4). We also found that Ce-kettin localizes to the proximal regionof the thin filaments in the ovarian nonstriated muscle (Figure 4).This is the first demonstration of kettin as a component ofnonstriated myofibrils. Although the C. elegans ovarian muscleis nonstriated, it shares some physiological properties withstriated muscle and uses the tropomyosin–troponin systemfor its contraction (Myers et al., 1996; Ono and Ono, 2004).Therefore, Ce-kettin may play common cellular roles in bothstriated and nonstriated muscles.

We showed that the four C-terminal Ig-repeats directly bindto actin filaments and that the adjacent kettin-specific regionenhances its actin binding. Previously, the full-length kettinhas been demonstrated to bind to actin filaments with high affinity(Maki et al., 1995; van Straaten et al., 1999), and the stoichiometryhas suggested that one Ig-repeat may bind one actin monomerin the filament (van Straaten et al., 1999). This was also supportedby the report that a single Ig-repeat of kettin is capable ofbinding to actin filaments (Lakey et al., 1993). However, ourresults show that the four C-terminal Ig-repeats (KETN-CT1)bind to actin at lower stoichiometry than one repeat per oneactin monomer, and, interestingly, that the adjacent non-Igregion augments both affinity and stoichiometry for bindingto actin. This suggests that the Ig-repeats and non-Ig regionof the molecule cooperatively bind to actin filaments. Similarly,a single Ig-domain of myotilin is sufficient for actin binding,but flanking non-Ig sequences also play important roles in actinbinding (von Nandelstadh et al., 2005). The full-length kettinbinds to actin with a nanomolar affinity (van Straaten et al.,1999), whereas our C-terminal fragments binds to actin witha micromolar affinity, suggesting that other Ig-repeats andnon-Ig sequence may cooperate to achieve tight binding to actinfilaments with proper stoichiometry.

The Ce-kettin gene ketn-1 is independent of genes coding forother connectin/titin-related Ig-repeat proteins. ketn-1 (RNAi)caused disorganization of actin filaments in muscle. This phenotypeis different from the defects in regulation of muscle contractionin the mutants of unc-22 coding for twitchin (Benian et al.,1993) and the defects in M-line assembly in the mutants of unc-89coding for UNC-89, a protein similar to obscurin (Benian etal., 1996; Small et al., 2004). Therefore, the RNAi phenotypestrongly suggests that Ce-kettin has specific function in assemblyand/or maintenance of actin filaments in muscle. However, thephenotype is relatively weak with low penetrance under normalculture conditions, and the extent of actin disorganizationwas not as drastic as that observed in mutants of actin depolymerizingfactor/cofilin (UNC-60B) (Ono et al., 1999, 2003), actin-interactingprotein 1 (UNC-78) (Ono, 2001), or a calponin-like protein (UNC-87)(Goetinck and Waterston, 1994a,b), or in worms that are treatedwith RNAi of tropomyosin (Ono and Ono, 2002). This suggeststhat kettin might have partially redundant function with othermuscle proteins. Ce-titins are candidates for functionally redundantproteins with Ce-kettin. The N-terminal portion of Ce-titinslocalizes to the I-bands (Flaherty et al., 2002), but mutantor RNAi phenotypes for the Ce-titin gene have not been clearlydefined. Vertebrate connectin/titin directly binds to actinfilaments (Kimura et al., 1984; Maruyama et al., 1987) via thePEVK domain in the I-band part (Kulke et al., 2001a; Yamasakiet al., 2001; Linke et al., 2002; Nagy et al., 2004) and isinvolved in maintenance of the thin filament structure (Linkeet al., 1999). Thus, vertebrate connectin/titin may have a similaractin regulatory function to kettin by using a different domainfrom kettin for binding to actin filaments.

We demonstrated that the organization of ${alpha}$ -actinin at the densebodies was disturbed by depletion of Ce-kettin. This suggeststhat Ce-kettin may directly interact with ${alpha}$ -actinin and regulateits assembly, or that Ce-kettin may organize actin filamentsnear the barbed ends, possibly by bundling, and facilitate efficientassociation with the dense bodies. ${alpha}$ -Actinin and insect kettinhave been shown to bind to actin simultaneously (van Straatenet al., 1999). Thus, these two proteins may cooperate to strengthenthe anchorage between thin filaments and dense bodies and providemechanical stability. Insect kettin also binds to myosin andis involved in stiffness of myofibrils (Kulke et al., 2001b).Although we have not examined interaction between Ce-kettinand myosin, it is also a possible mechanism to stabilize themyofibrils.

Kettin is a unique member of the connectin/titin family of Ig-repeatproteins and is found only in invertebrates (Bullard et al.,2002). However, kettin might be functionally homologous to palladin(Parast and Otey, 2000), myopalladin (Bang et al., 2001), andmyotilin (Salmikangas et al., 1999), which have two to fiveIg-repeats and localize to the Z-lines of vertebrate striatedmuscle. These proteins are critical for actin filament reorganizationin nonmuscle cells (Boukhelifa et al., 2001, 2003; Salmikangaset al., 2003; Otey et al., 2005) and myofibril assembly in musclecells (Bang et al., 2001; Salmikangas et al., 2003; Otey etal., 2005). In particular, myotilin directly binds to actinfilaments, and its mutations in the human gene are associatedwith limb girdle muscular dystrophy 1A (Salmikangas et al.,1999) and myofibrillar myopathy (Selcen and Engel, 2004), whichare termed myotilinopathies (Goebel, 2005; Olive et al., 2005).Therefore, C. elegans could be an excellent model to study functionsof actin binding proteins with Ig-repeats in muscle and theirinteraction with other myofibrillar proteins.

ACKNOWLEDGMENTS

We thank Belinda Bullard and Taylor Allen for communicatingstudies on C. elegans kettin and helpful discussion; SumikoKimura for helpful discussion; Guy Benian for comments on themanuscript; Henry Epstein for anti-myoA antibody; Gary Moulderand Robert Barstead for an ${alpha}$ -actinin mutant; and Pamela Hoppefor MH24, MH40, and MH44. Some C. elegans strains were providedby the Caenorhabditis Genetics Center, which is funded by theNational Institute of Health National Center for Research Resources.This work was supported by National Institutes of Health GrantR01 AR48615 (to S. O.).

Footnotes

This article was published online ahead of print in MBC in Press(http://www.molbiolcell.org/cgi/doi/10.1091/mbc.E05-02-0114)on April 5, 2006.

The online version of thisarticle contains supplemental material at MBC Online (http://www.molbiolcell.org).

* Present address: Department of Biophysics, Graduate Schoolof Science, Kyoto University, Kyoto 606-8502, Japan.

Address correspondence to: Shoichiro Ono ( sono{at}emory.edu)

Abbreviations used: GST, glutathione S-transferase; Ig, immunoglobulin-like; RNAi, RNA interference.

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