Apoptotic Cleavage of Cytoplasmic Dynein Intermediate Chain and P150GluedStops Dynein-Dependent Membrane Motility

doi:10.1083/jcb.153.7.1415

Published online 25 June 2001. doi:10.1083/jcb.153.7.1415

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© The Rockefeller University Press, 0021-9525/2001//1415 $5.00
The Journal of Cell Biology, Volume 153, Number 7, , 2001 1415-1426

Original Article

Apoptotic Cleavage of Cytoplasmic Dynein Intermediate Chain and P150^GluedStops Dynein-Dependent Membrane Motility

Jon D. Lane^a, Maïlys A.S. Vergnolle^a, Philip G. Woodman^a, and Victoria J. Allan^a

^a School of Biological Sciences, University of Manchester, Manchester M13 9PT, United Kingdom
School of Biological Sciences, University of Manchester, 2.205 Stopford Building, Oxford Road, Manchester M13 9PT, UK.(44) 161-275-5082(44) 161-275-5646

viki.allan{at}man.ac.uk

Cytoplasmic dynein is the major minus end–directed microtubulemotor in animal cells, and associates with many of its cargoesin conjunction with the dynactin complex. Interaction betweencytoplasmic dynein and dynactin is mediated by the binding ofcytoplasmic dynein intermediate chains (CD-IC) to the dynactinsubunit, p150^Glued. We have found that both CD-IC and p150^Gluedare cleaved by caspases during apoptosis in cultured mammaliancells and in Xenopus egg extracts. Xenopus CD-IC is rapidlycleaved at a conserved aspartic acid residue adjacent to itsNH₂-terminal p150^Glued binding domain, resulting in loss ofthe otherwise intact cytoplasmic dynein complex from membranes.Cleavage of CD-IC and p150^Glued in apoptotic Xenopus egg extractscauses the cessation of cytoplasmic dynein–driven endoplasmicreticulum movement. Motility of apoptotic membranes is restoredby recruitment of intact cytoplasmic dynein and dynactin fromcontrol cytosol, or from apoptotic cytosol supplemented withpurified cytoplasmic dynein–dynactin, demonstrating thedynamic nature of the association of cytoplasmic dynein anddynactin with their membrane cargo.

Key Words: microtubule • motor • apoptosis • trafficking • caspase

Introduction

Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References

Apoptosis, or programmed cell death, is accompanied by the activationof a family of apoptosis-specific cysteine proteases calledcaspases (Cohen 1997). Both the signaling pathways that mediatecaspase activation, and the substrates for caspases, are highlyconserved. The so-called execution phase of apoptosis involvesa characteristic series of morphological changes that in manycases are directly coupled to caspase-dependent cleavage ofkey substrates. These events ultimately lead to the recognitionand engulfment of dying cells by their neighbors. The natureof the phagocytic signal generated by the apoptotic cell isnot known, but is likely to be complex. This is perhaps bestillustrated by the finding that "professional" and "nonprofessional"phagocytic cells clear apoptotic cells at different rates, withthe latter recognizing apoptotic cells only after the executionphase has run its full course (Parnaik et al. 2000).

The exposure of phosphatidyl serine on the surface of apoptoticcells is thought to be a key phagocytic signal (Martin et al. 1995; Fadok et al. 2000; Hamon et al. 2000), but other markersare clearly important (Savill et al. 1990; Ren et al. 1995;Platt et al. 1996; Devitt et al. 1998). Indeed, since such widelyrecognized phagocytic signals must be generic, it is probablethat general alterations in the protein composition of the plasmamembrane, or in the glycosylation of proteins or lipids, arealso involved. Such changes could be brought about by alteringthe specificity or efficiency of membrane traffic pathways.In support of this hypothesis, there is evidence that both thesecretory and endocytic pathways are affected in apoptotic cells.There are profound changes in membrane structure (Wyllie et al. 1980), including fragmentation of the Golgi complex (Mancini et al. 2000) and inhibition of the secretory pathway (Whyte et al. 1993). In addition, homotypic endosome fusion is inhibitedin apoptotic cell extracts via the caspase 3–dependentcleavage of Rabaptin 5 (Cosulich et al. 1997; Swanton et al. 1999a).

The secretory and endocytic pathways rely in numerous ways onthe function of cytoplasmic dynein and its regulator dynactin.They are required for ER-to-Golgi region traffic (Presley et al. 1997), for maintaining Golgi apparatus organization andposition (Burkhardt et al. 1997; Harada et al. 1998; Quintyne et al. 1999; Roghi and Allan 1999), and for moving endocyticorganelles and facilitating traffic between them (Blocker et al. 1997; Harada et al. 1998; Valetti et al. 1999). The ER itselfis a cargo for cytoplasmic dynein in extracts of Xenopus eggsand early embryos (Allan 1995; Lane and Allan 1999). In additionto these roles in trafficking, cytoplasmic dynein, and dynactinare also needed for maintaining microtubule organization ininterphase, as well as for correct spindle assembly, positioning,and chromosome attachment during cell division (for review seeKarki and Holzbaur 1999).

The central importance of cytoplasmic dynein in maintainingcellular architecture makes it an attractive target for inactivationduring apoptosis. Cytoplasmic dynein is a large molecule ( $~$ 1.2MDa) which consists of two heavy chains (CD-HC), two or threeintermediate chains (CD-IC), four light intermediate chains(CD-LIC), and a variety of light chains (for review see Susalka et al. 2000). More than one gene exists for the heavy, intermediate,and light intermediate chains, and in addition, the CD-ICs andthe CD-LICs undergo tissue-specific alternate splicing (Susalka et al. 2000). Whether different subsets of these chains associateto give cytoplasmic dynein molecules with distinct functionis not clear, but seems likely (Susalka et al. 2000).

Cytoplasmic dynein function generally requires dynactin, firstidentified as an activator of cytoplasmic dynein–drivenvesicle movement (Gill et al. 1991). Dynactin also consistsof multiple subunits, including two p150^Glued chains which extendout from a short filament of actin-related protein 1 which associateswith a variety of other subunits, including several dynamitinmolecules (Schafer et al. 1994; Quintyne et al. 1999). Geneticand biochemical studies have confirmed that the two complexesmust interact for virtually all cytoplasmic dynein functions(for review see Allan 1996; Schroer 1996; Karki and Holzbaur 1999). Dynactin is thought to link cytoplasmic dynein to itscargoes (for review see Allan 1996; Schroer 1996; Karki and Holzbaur 1999) and to enhance cytoplasmic dynein's processivity(King and Schroer 1999). How dynactin attaches to cargoes isnot clear, but it might bind directly to membrane lipids, orinteract with proteins such as beta spectrin on the Golgi apparatusor ZW10 on the kinetochore (Karki and Holzbaur 1999; Muresan et al. 2001). Cytoplasmic dynein then binds to dynactin viaan interaction between p150^Glued and the NH₂-terminal domainof CD-IC (Karki and Holzbaur 1995; Vaughan and Vallee 1995).

A convenient system for studying cytoplasmic dynein functionduring apoptosis is provided by Xenopus egg extracts, whichsupport active cytoplasmic dynein–driven ER movement (Allan 1995; Niclas et al. 1996; Lane and Allan 1999) and canreadily be made apoptotic (Kluck et al. 1997). Here, we showthat CD-IC and p150^Glued are cleaved by caspases both in apoptoticegg extracts and during apoptosis in vivo. The implicationsof these cleavage events for cytoplasmic dynein–dynactinfunction are described.

Materials and Methods

Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References

Chemicals and Antibodies
Unless otherwise stated, chemicals were obtained from Sigma-Aldrich.Stock solutions were stored at –20°C: anisomycin (5mg/ml in DMSO), etoposide (50 mM in DMSO), and caspase inhibitors(Ac-DEVD.CHO at 100 µM and zVAD.FMK at 50 µM, bothin DMSO; Calbiochem-Novabiochem). Protease inhibitors (leupeptin,chymostatin, pepstatin, and aprotinin) were used at 10 µg/mlfinal concentration.

For immunoblotting, we used the following monoclonal antibodies:anti–CD-IC (70.1, Sigma-Aldrich; 1618, Chemicon International),anti-p150^Glued (Transduction Labs), antifodrin (ICN Biomedicals),antitubulin (B-5-1-2), antiribophorin (CEL5C, from Birgit Lane,University of Dundee, Dundee, UK), antikinesin II (K 2.4, fromJohn Scholey, University of California at Davis, Davis, CA),and anti-p50 dynamitin (from Richard Vallee, University of Massachusetts,Worcester, MA); and the following polyclonal antibodies: anti-ratCD-IC (from Richard Vallee; Vaughan and Vallee 1995), anti-XenopusCD-LIC (Addinall et al. 2001), anti–CD-IC NH₂ terminus(Xenopus-specific; Lane and Allan 1999), anti-Xenopus CD-ICpeptide antibody (raised and affinity purified against the sequenceNRSNKRTPVQRTPLS; underlined in Fig. 3), anti–poly-ADP-ribosepolymerase (PARP; Calbiochem), antikinesin heavy chain (KHC;from Ron Vale, University of California at San Francisco, SanFrancisco, CA), anti–β-COP (D1; from Thomas Kreis,University of Geneva, Geneva, Switzerland), and anti–Arp-1(centractin; from David Meyer, University of California at LosAngeles, Los Angeles, CA). Secondary antibodies (conjugatedto alkaline phosphatase or horse radish peroxidase) were fromJackson ImmunoResearch Laboratories.

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Figure 3 Amino acid sequence of Xenopus laevis (Xl) CD-IC aligned with the NH₂ terminus of rat (Rn) CD-IC1, 2A, 2B, and 2C. The locations of several potential caspase cleavage motifs are highlighted. In each of these, the crucial aspartic acid residue at position P₁ (P₄P₃P₂P₁) of Xenopus CD-IC was altered by site-directed mutagenesis. The peptide sequence used for polyclonal antibody production is underlined.

Extract Preparation and Analysis
HL60 cells were grown in RPMI 1640 plus 10% foetal bovine serumand penicillin/streptomycin. To analyze apoptosis in vivo, cellswere treated with 5 µg/ml anisomycin or 50 µM etoposide,with or without a 30 min preincubation with 50 µM zVAD-FMK.Cells were washed three times in PBS, then broken by passing20 times through a cell cracker (Balch et al. 1984) in acetate/sucrosebuffer (100 mM K-acetate, 3 mM Mg-acetate, 5 mM EGTA, 10 mMHepes, pH 7.4, 150 mM sucrose) containing protease inhibitors.Postnuclear supernatants were prepared and stored at –80°C.

Interphase Xenopus egg extracts were prepared as described (Murray 1991). Apoptotic or control extracts were generated bythe addition of cytochrome c (to 10 µM) ± the caspaseinhibitor, Ac-DEVD-CHO (2 µM), followed by incubationfor 8 h at 25°C. Cytosol and membranes were prepared fromcontrol and apoptotic extracts, and membranes were further purifiedby flotation (Lane and Allan 1999). For biochemical analysisof rebinding to membrane, isolated membranes (10 µl 5mg/ml protein) were incubated in 90 µl control or apoptoticcytosol at 25°C for 60 min. The mixture was then centrifugedin a rotor (TLA100; Beckman Coulter) for 15 min at 40,000 g_avat 4°C through a 150-µl cushion of 0.75 M sucrosein acetate buffer. The pelleted membranes were analyzed by immunoblotting.

Biochemical Analysis of Motor Complexes
Cytoplasmic dynein and dynactin were isolated from 400 µlcontrol or apoptotic cytosols by microtubule affinity and sucrosedensity gradient centrifugation as described (Niclas et al. 1996). 50-µl fractions were collected and run on 4–15%gradient acrylamide gels then analyzed by silver staining andimmunoblotting. Immunoprecipitation experiments were performedas described (Roghi and Allan 1999). In brief, 20 µl ofcontrol or apoptotic egg cytosol was diluted to 500 µlin immunoprecipitation buffer then incubated with protein GSepharose beads (Zymed Laboratories) prebound with anti–CD-IC(1618) or anti–CD-LIC antibodies.

Motility Assays and Data Collection
Motility assays were performed using video-enhanced differentialinterference contrast (VE-DIC) microscopy using a light microscope(BX60; Olympus) (Allan 1998). To compensate for differencesin microtubule assembly between control and apoptotic cytosols,a uniform field of stable microtubules was assembled. Flow cellswere perfused with diluted control egg cytosol (1:20 in acetate/sucrose)for 5 min. After two washes with 10 µl acetate/sucrose,taxol-stabilized microtubule seeds (Allan and Vale 1991) wereadded. After 10 min, soluble tubulin (5 mg/ml) plus 1 mM GTPwas introduced, and microtubules were allowed to grow for 15min. Microtubules were stabilized by flowing through 20 µMtaxol in acetate/sucrose, washed once with acetate/sucrose,and then a mix of cytosol and membranes was added. Over time,ER networks assemble on the coverslip surface in a cytoplasmicdynein–dependent fashion. Network formation was quantitatedafter 45 min by counting the number of three way junctions in20 random fields, which correlate directly with the quantityof cytoplasmic dynein–based movement (Allan 1995). Motilityexperiments were carried out in the presence of 2 µM Ac-DEVD-CHOto prevent further caspase action.

PCR and Cloning of Xenopus CD-IC
The first 288 bases of Xenopus CD-IC were obtained from a frogoocyte cDNA library (Nicolás et al. 1997) by degeneratePCR using the following primers: forward, GGGGATCCATGTC(I)GA(CT)AA(AG)AG-(CT)GA(I)(CT)T(I)AA;reverse, GGAATTC(AG)TC(CT)TG(AG)C-T(I)CC(I)GC(AG)CT(I)GG. ThePCR product was cloned into pBluescript (pBSIIsk+; Stratagene),and was used to prepare a probe to screen the oocyte cDNA libraryto obtain a full-length Xenopus CD-IC clone. A single clonewas isolated, the sequence of which was most similar to CD-IC2B(these sequence data are available from EMBL/GenBank/DDBJ underaccession nos. AF319780 and AF319781). The clone lacked thefirst 90 bases from the 5' end, so to obtain a full-length constructit was joined to the original PCR product using a conservedNsiI site within the overlapping region. Site-directed mutagenesiswas performed using the QuikChange kit (Stratagene). All mutationswere confirmed by sequencing.

In Vitro Transcription/Translation
The full-length Xenopus CD-IC construct was subcloned into theexpression vector, pCDNA3.1 (Invitrogen). [³⁵S]methionine-labeledprotein was produced using a coupled transcription/translationkit (Promega). Translations were analyzed by autoradiography.Translated Xenopus CD-IC appeared as several 60–85-kDbands (data not shown), which were probably derived from randominitiation events, so CD-IC was routinely immunoprecipitatedusing an NH₂-terminal anti–CD-IC antibody (1618). Theimmunecomplex was then used in caspase cleavage assays. RecombinantPARP and caspase 2 were prepared as described (Swanton et al. 1999b).

Caspase Cleavage Assays
Assays using recombinant caspases 2, 3, and 7 (Alexis Biochemicals;and from Don Nicholson and Sophie Roy [Merk Frosst Centre forTherapeutic Research, Quebec, Canada]) were performed in caspasebuffer (for caspases 3 and 7; 50 mM Hepes-KOH, pH 7.0, 2 mMEGTA, 0.1% Chaps, 10% sucrose, 5 mM DTT; for caspase 2, 50 mMNa-citrate, pH 5.5 replaced the Hepes-KOH). Fractions enrichedin native Xenopus or pig brain cytoplasmic dynein–dynactinwere incubated with caspases for 3 h at 37°C and analyzedby silver staining and immunoblotting.

Cleavage of in vitro–translated, immunoprecipitated, [³⁵S]methionine-labeledXenopus CD-IC was carried out either by incubating beads incontrol or apoptotic egg cytosol for 6 h at 25°C, or byincubating beads in the presence of recombinant caspases for2 h at 30°C. Radiolabeled products were detected by autoradiography.For some experiments the caspase 3 and 7 inhibitor, Casputin^TM(Biomol Research Laboratories, Inc.; 80 µg/ml final) wasincluded.

Results

Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References

CD-IC and p150^Glued Are Targets for Caspases during Apoptosis
To investigate whether the inactivation of microtuble motorsmight contribute to the changes in cell morphology associatedwith apoptosis, we assessed the stability of a variety of moleculesafter activation of caspases in intact cells. We used a numberof cell lines (including human HL60, jurkat and A431, and ratNRK) treated with a selection of drugs (anisomycin, etoposide,staurosporine, or camptothecin). Most molecules tested (namelyKHC, kinesin II, p50 dynamitin, β-COP, and tubulin [Fig. 1 A]) were not altered during apoptosis. However, loss of immunoreactivityof both CD-IC and the p150^Glued component of the dynactin complexwas seen in apoptotic cells (Fig. 1A and Fig. B). In HL60 cellsundergoing apoptosis in response to 5 µg/ml anisomycinor 50 µM etoposide (Fig. 1 B), CD-IC rapidly became undetectableat about the same rate that the characterized caspase substratePARP was cleaved. This suggests that CD-IC may be an early targetfor caspases. The reduction in p150^Glued signal was more gradual,mirroring the loss of full-length fodrin immunoreactivity (Fig. 1 B). In each case, loss of immunoreactivity was greatly reducedby the cell permeable caspase inhibitor zVAD-FMK.

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Figure 1 CD-IC and p150^Glued are cleaved during apoptosis. (A) Cytosols were made from untreated human HL60 cells (C), cells treated with anisomycin (A; 5 µg/ml) for 4 h, and cells treated with anisomycin and the cell-permeable capsase inhibitor zVAD.FMK (Z). Equal amounts of protein were analyzed by silver staining (left) and immunoblotting. The positions of full-length β-COP and p50 are shown (<). (B) HL60 cells were treated with 5 µg/ml anisomycin or 50 µM etoposide. Cell extracts prepared at the indicated times were immunoblotted using the antibodies shown. Samples treated for the maximum times with each agent in the presence of zVAD.FMK are also shown (Z). (C) A Xenopus egg extract was incubated with 10 µM cytochrome c ± the caspase inhibitor Ac-DEVD-CHO for the times indicated. Extracts were then analyzed by immunoblotting. In all panels, the anti–CD-IC antibody used was 70.1.

To study how caspase-dependent cleavage of CD-IC and p150^Gluedaffect the function of the cytoplasmic dynein–dynactincomplex, we examined the cleavage of both proteins in vitrousing Xenopus egg extracts, since they are well-suited for studyingmotor proteins (Allan and Vale 1991) and apoptosis (Newmeyer et al. 1994). Apoptosis can be triggered in cell-free extractsby the addition of cytochrome c (Liu et al. 1996; Kluck et al. 1997), whereupon effector caspases are activated (e.g., Swanton et al. 1999b). A clear reduction in recognition of CD-IC byNH₂-terminal monoclonal antibodies was seen upon addition ofcytochrome c to Xenopus egg extracts, but no cleavage productswere detected (Fig. 1 C). This loss of signal occurred overa similar time scale to the cleavage of other caspase substratesin Xenopus extracts (Newmeyer et al. 1994; Cosulich et al. 1996)and was prevented by the caspase inhibitor Ac-DEVD-CHO (Fig. 1 C). In contrast, the monoclonal antibody to p150^Glued detecteda cleavage product in apoptotic egg extracts, $~$ 10–20 kDsmaller than the native molecule (Fig. 1 C); no such productwas seen in HL60 extracts, although the p150^Glued antibody reactivitywas lost with time (Fig. 1A and Fig. B). We do not yet knowwhy the pattern of p150^Glued cleavage differs in these two systems.

CD-IC Is Cleaved within Its NH₂-terminal p150^Glued Binding Domain
To drive the movement of a variety of cargoes towards the minusends of microtubules, cytoplasmic dynein interacts with dynactinthrough binding of the NH₂ terminus of CD-IC to p150^Glued (Fig. 2A and Fig. B; Karki and Holzbaur 1995; Vaughan and Vallee 1995).This region of CD-IC is recognized by both monoclonal antibodies70.1 and 1618 (data not shown). Since neither antibody recognizedcleavage products in apoptotic cells and extracts (Fig. 1),this suggested that caspase-dependent cleavage occurs withinthis region. To test this hypothesis, we used a polyclonal antiserumraised against full-length rat CD-IC (Vaughan and Vallee 1995),and a peptide antibody raised against a sequence towards theCOOH-terminus of CD-IC (see Materials and Methods; Fig. 3).In immunoblots of apoptotic Xenopus egg extracts, these antibodiesrevealed a cleavage product $~$ 12 kD smaller than the molecularmass of the full-length molecule (Fig. 2 C). These data suggestthat CD-IC is cleaved by caspases within its NH₂-terminal p150^Gluedbinding domain.

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Figure 2 Cleavage of CD-IC takes place within its NH₂-terminal p150^Glued binding region. (A) Schematic diagram of cytoplasmic dynein and dynactin, showing the interaction between the NH₂ terminus of CD-IC and p150^Glued. (B) Representation of CD-IC showing the regions that interact with other components of the cytoplasmic dynein and dynactin complexes. (C) Immunoblot of a Xenopus egg extract that had been treated for the times indicated (in hours) with cytochrome c ± Ac-DEVD-CHO using monoclonal (70.1) and polyclonal antibodies to CD-IC. The positions of molecular weight markers are also shown.

Comparison of multiple CD-IC sequences revealed several conservedaspartic acids towards the NH₂ terminus of the molecule (Fig. 3). To identify the caspase cleavage site, we used site-directedmutagenesis to alter these aspartic acids to alanine, and examinedthe cleavage of in vitro–translated, [³⁵S]methionine-labeledprotein when added to apoptotic egg cytosol. Two cleaved productswere generated from in vitro–translated wild-type XenopusCD-IC (Fig. 4 A): one at $~$ 74 kD (C₁) and one at $~$ 66 kD (C₂). C₁matches the size of the product seen in immunoblots of apoptoticegg extracts using the polyclonal anti–CD-IC (Fig. 2 C),whereas we have never observed a band of the size of C₂, perhapsbecause the C₂ cleavage site is inaccessible when CD-IC is inthe native cytoplasmic dynein complex. Mutating the putativesite DSGD⁹⁹G (D $->$ A) resulted in the loss of the upper cleavageproduct (C₁) (Fig. 4 A). None of the other mutations alteredthe pattern of cleavage of Xenopus CD-IC (data not shown).

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Figure 4 Cleavage of Xenopus CD-IC in vitro occurs at DSGD⁹⁹ and at another, unidentified site. (A) Immunoprecipitated [³⁵S]methionine-labeled wild-type or mutated (DSGA⁹⁹) CD-IC was incubated in apoptotic Xenopus egg cytosol for the times shown, with or without Ac-DEVD-CHO or the caspase 3 and 7 inhibitor, Casputin^TM. Two cleavage products, C₁ and C₂, are indicated. Note that appearance of C₁ is prevented by Casputin^TM and does not occur using CD-IC (DSGA⁹⁹). (B–D) Immunoprecipitated [³⁵S]methionine-labeled wild-type or mutated (DSGA⁹⁹) CD-IC was incubated for 2 h at 30°C with recombinant caspases 2 (B), 3 (C), and 7 (D). Caspase 2 activity was confirmed by assessing cleavage of in vitro–translated caspase 2, whilst caspases 3 and 7 were tested using in vitro–translated PARP. (E) Native Xenopus egg cytoplasmic dynein–dynactin was incubated with recombinant caspase 2 (50 nM) or caspase 3 (20 nM), ± Ac-DEVD-CHO for 3 h at 37°C. Proteins were analyzed after SDS-PAGE by immunoblotting (CD-IC was detected using polyclonal antiserum).

Since DSGD⁹⁹G fits with consensus sites for caspase 3 (DXXDmotif), we tested the effects of the selective caspase 3 and7 inhibitor, Casputin^TM. This inhibitor prevented cleavage ofin vitro–translated wild-type CD-IC to C₁ (Fig. 4 A),suggesting that this product is generated by caspase 3 or caspase7 in apoptotic egg extracts. We then tested the ability of recombinantcaspases 2, 3, and 7 to cleave in vitro–translated, immunoprecipitatedCD-IC (Fig. 4, B–D). These caspases were shown to be activeby incubating them with known substrates. All three caspasescleaved CD-IC to generate C₁, to varying degrees, with caspase3 being most effective. From these data, caspase 3 is the bestcandidate for cleaving CD-IC at DSGD⁹⁹G.

To confirm that CD-IC within native cytoplasmic dynein couldbe cleaved by caspase 3, we carried out in vitro cleavage assaysusing recombinant caspases 2 and 3, and cytoplasmic dynein–dynactinfractions prepared from Xenopus eggs (Fig. 4 E). Using immunoblotting,we demonstrated that endogenous Xenopus CD-IC was degraded invitro by caspase 3, but much less so by caspase 2 (Fig. 4 E).Caspase 3, but not 2, also cleaved some of the p150^Glued presentwithin the same fraction (Fig. 4 E). The inclusion of Ac-DEVD-CHOin these assays prevented caspase-mediated CD-IC and p150^Gluedcleavage. Identical results were obtained using pig brain cytoplasmicdynein–dynactin (data not shown).

Biochemical Analysis of the Cytoplasmic Dynein and Dynactin Complexes during Apoptosis
Cytoplasmic dynein and dynactin sediment as separate complexesof $~$ 20S. To test if caspase cleavage of CD-IC and p150^Glued affectedthe stability of the complexes, we compared their sedimentationproperties when isolated from control and apoptotic egg cytosol.Motors bind statically to microtubules in the absence of ATP,so cytoplasmic dynein can be enriched from cytosol relativelysimply. Dynactin copurifies with cytoplasmic dynein, since thep150^Glued subunit also possesses a microtubule binding domain(between amino acids 39–150; Waterman-Storer et al. 1995).Silver staining and immunoblotting of sucrose gradients of cytoplasmicdynein–dynactin-enriched fractions from control egg cytosolrevealed that CD-HC, CD-IC, and CD-LIC cosedimented at 20S (infractions 5 and 6; Fig. 5 A). In fractions enriched from apoptoticcytosol, CD-HC and CD-LIC were still found at 20S, even thoughfull-length CD-IC could not be detected using 70.1 (Fig. 5 A).Hence, cleavage of CD-IC does not appear to destabilize CD-HCand CD-LIC interactions.

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Figure 5 The fate of cytoplasmic dynein and dynactin complexes in apoptotic extracts. (A) Microtubule motors were isolated from control or apoptotic Xenopus egg cytosol by microtubule affinity, then separated on sucrose density gradients and analyzed by silver staining and immunoblotting (CD-IC was detected using 70.1). CD-HC was not seen in fraction 1 of the apoptotic gradient: the silver staining in that lane is artefactual. (B) The cytoplasmic dynein complex was immunoprecipitated from control (C) and apoptotic (A) egg cytosols using anti–CD-LIC antibody, and immunoblotted with polyclonal anti–CD-IC peptide antibody to detect cleaved (<<) and intact (<) CD-IC. (C) Control (C; lane 1) and apoptotic (A; lane 2) egg cytosols were depleted of any cytoplasmic dynein complex containing uncleaved CD-IC by three rounds of depletion using the monoclonal antibody, 1618, against the NH₂-terminus of CD-IC (beads from only rounds 1 and 3 are shown; lanes 3–6). The depleted cytosols (lanes 7 and 8) were then subjected to a further immunoprecipitation with anti–CD-LIC beads (lanes 9 and 10). All fractions were examined by silver stain for DHC (top) and immunoblotted with anti–CD-IC peptide antibody to detect cleaved (<<) and uncleaved (<) CD-IC (bottom).

We next asked whether the large COOH-terminal CD-IC fragmentalso remained in the complex using an immunoprecipitation approach(Fig. 5B and Fig. C). In many apoptotic egg extracts, cleavageof CD-IC is only $~$ 60–70% efficient (Fig. 5 B, lanes 1 and2). When we immunoprecipitated using anti–CD-LIC antibodies,we found that the CD-IC cleavage product, intact CD-IC (Fig. 5 B, lane 4), and CD-HC (not shown) coprecipitated efficiently.We wanted to know whether dynein complexes existed which onlycontained the cleaved CD-IC, and to address this we first depleteddynein containing intact CD-IC by three rounds of immunoprecipitationwith an NH₂-terminal monoclonal antibody (1618), which doesnot recognize cleaved CD-IC (Fig. 5 C). Interestingly, cleavedCD-IC did not coprecipitate with intact CD-IC (Fig. 5 C, lanes3–6), but remained in the unbound fraction (Fig. 5 C,lanes 7 and 8). Moreover, when we used anti–CD-LIC beadsto immunoprecipitate the remaining dynein from full-length CD-IC–depletedapoptotic cytosol, the immune complexes contained the cleavedform of CD-IC along with CD-HC (Fig. 5 C, lane 10). These experimentssuggest that, in Xenopus egg cytosol, cleavage of CD-IC chainsdoes not cause the dynein components to disassociate. Strikingly,the dynein complexes contain either all intact or all cleavedCD-ICs.

Sucrose density gradient analysis also provided informationon the dynactin complex. Using the monoclonal anti-p150^Gluedantibody, we found that in control cytosol p150^Glued sedimentedat 20S as expected (Fig. 5 A). In apoptotic cytosol, we detectedsome full-length p150^Glued at 20S (Fig. 5 A), since cleavageof p150^Glued is incomplete (Fig. 1 C). Although some cleavedp150^Glued also migrated to this position (Fig. 5 A), the majoritywas detected at the top of the gradient, suggesting that ithad dissociated from the dynactin complex (Fig. 5 A). The methodfor isolating cleaved (and intact) p150^Glued relies on microtubuleaffinity, suggesting that the truncated product contains a functionalmicrotubule binding domain (although some may be complexed withthe small amount of intact, free p150^Glued). Moreover, the monoclonalp150^Glued antibody used was raised against the NH₂-terminalmicrotubule binding domain of p150^Glued, so it seems likelythat the caspase cleavage site(s) within Xenopus p150^Glued islocated towards its COOH terminus.

Cleavage of CD-IC and p150^Glued Stops Cytoplasmic Dynein–driven Membrane Motility In Vitro
According to current models, caspase-mediated cleavage of CD-ICand p150^Glued should uncouple cytoplasmic dynein from its cargoand therefore prevent movement along microtubules. We testedthis hypothesis using two approaches. First, we determined whethercytoplasmic dynein and dynactin remained membrane-associatedin egg extracts during apoptosis, and then we looked at theconsequences of apoptotic CD-IC and p150^Glued cleavage on membranemotility using an in vitro assay. Floated Xenopus egg membranesare rich in both cytoplasmic dynein and dynactin (Fig. 6; Lane and Allan 1999). Although silver staining revealed very littledifference in the overall protein pattern in apoptotic versuscontrol cytosol or membranes (Fig. 6 A), the apoptotic membraneshad lost most of their associated CD-LIC and CD-IC (Fig. 6 B).Since the cytoplasmic dynein complex remains intact during apoptosis(Fig. 5), it is likely that the entire complex is removed frommembranes during this process.

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Figure 6 The cytoplasmic dynein complex is released from membranes during apoptosis in Xenopus egg extracts. Cytosol (Cyt) and membranes (Mem) were prepared from control or apoptotic extracts (C and A, respectively). Equal amounts of protein were loaded on SDS-PAGE gels, silver stained for total protein (A) and immunoblotted using the antibodies shown (B).

We then looked at the dynactin complex. The amount of full-lengthand cleaved p150^Glued on apoptotic membranes was greatly reduced,and p50 dynamitin also appeared to be depleted (Fig. 6 B). Membrane-associatedArp-1 was partially degraded to an $~$ 32-kD product in apoptoticegg extracts, which remained associated with membranes (no degradationwas observed in apoptotic cytosol; Fig. 6 B). We do not knowif the Arp-1 degradation product is due solely to the actionof caspases, because we always observed a similar band in immunoblotsof control membranes (Fig. 6 B). Taken together, these resultssuggest that at least part of the dynactin complex stays onapoptotic membranes. We also compared KHC and kinesin II oncontrol and apoptotic membranes (Fig. 6 B). Interestingly, whilethe amounts of kinesin II (p85 subunit) did not change, we foundthat KHC, although uncleaved (Fig. 1 A and 6 B), was lost fromapoptotic egg membranes, an observation which merits furtherinvestigation.

ER membranes present in crude frog egg extracts move exclusivelyusing cytoplasmic dynein in egg cytosol and are easily identifiedby VE-DIC microscopy (Allan 1995; Niclas et al. 1996; Lane and Allan 1999). Therefore, we used in vitro motility assays toassess cytoplasmic dynein–based membrane motility in controland apoptotic egg extracts. Extensive ER networks formed frommembranes and cytosol derived from control extracts treatedwith cytochrome c and caspase inhibitors (Fig. 7 A, left). Themotility of these networks was identical to that seen in untreatedextracts. However, upon combining membranes and cytosol fromapoptotic extracts, we saw no network formation (Fig. 7 A, right).Instead, membrane clumps rarely associated with microtubules(Fig. 7 A), and tubule extension events were never observed.We have not assessed whether ER membrane fusion is also inhibited,but this is a possibility given that homotypic endosome fusionis a target for apoptotic regulation (via caspase 3 cleavageof Rabaptin 5; Cosulich et al. 1997; Swanton et al. 1999a).

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Figure 7 Motile properties of apoptotic and nonapoptotic membranes. (A) Membranes were prepared by flotation from control and apoptotic Xenopus egg extracts, then incubated in their respective cytosols for 45 min. They were then assayed for motility using a three way junction index (see Materials and Methods). (B) Control or apoptotic cytosols and membranes were mixed as indicated, and assayed for motility as above. Values are means ± SEM for three independent experiments. In each case, Ac-DEVD-CHO was added to a final concentration of 2 µM before motility assays. Representative VE-DIC fields (27 µm across) are also shown for each assay.

These data suggest that apoptotic membranes are unable to formnetworks in apoptotic cytosol because they have lost the capacityto associate with and move along microtubules in a cytoplasmicdynein–dependent fashion. However, when apoptotic membraneswere incubated in control cytosol, they regained the abilityto move along microtubules and undergo homotypic membrane fusion(Fig. 7 B, left), generating networks which were $~$ 75% as extensiveas seen in nonapoptotic conditions. When we carried out thereciprocal experiment (control membranes in apoptotic cytosol),we found that the extent of network formation was similar (Fig. 7 B, right). All experiments were performed in the presenceof caspase inhibitor to prevent further caspase action.

When the membranes from these incubations were reisolated andimmunoblotted for cytoplasmic dynein and dynactin, we foundthat apoptotic membranes effectively recruited full-length CD-ICand CD-LIC, as well as p150^Glued, to $~$ 50% of control levels injust 1 h (Fig. 8), although under identical conditions KHC wasnot recruited (data not shown). Control membranes lost a proportionof their associated cytoplasmic dynein and dynactin when incubatedin apoptotic cytosol for 1 h (Fig. 8). This probably reflectsthe dynamic nature of cytoplasmic dynein's affinity for membranesand is not due to caspase activity, because Ac-DEVD-CHO wasincluded in these assays.

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Figure 8 Apoptotic membranes can recruit intact cytoplasmic dynein and dynactin. Membranes from control (C) or apoptotic (A) egg extracts were incubated in control or apoptotic cytosol for 1 h. Membranes were then recovered and equal protein samples were run on SDS-PAGE and immunoblotted (antiribophorin was used as a loading control).

We next asked whether membrane movement in apoptotic extractscould be restored by the addition of purified cytoplasmic dynein–dynactin.We incubated apoptotic membranes and cytosol (plus Ac-DEVD-CHO)in the presence of pig brain cytoplasmic dynein–dynactin(Fig. 9). This fraction restored the network-forming abilityof apoptotic membranes to $~$ 25% of control activity (Fig. 9 A).The addition of pig brain cytoplasmic dynein brought the amountof intact CD-IC present in the cytosol/membrane mixture to approximatelycontrol levels (Fig. 9 B). These results suggest that cytoplasmicdynein–driven ER motility is halted during apoptosis primarilythrough caspase-mediated cleavage of cytoplasmic dynein anddynactin components.

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Figure 9 Addition of purified pig brain cytoplasmic dynein–dynactin restores ER network formation. (A) Membranes were prepared by flotation from apoptotic egg extracts, and incubated for 45 min in apoptotic cytosol in the presence or absence of pig brain cytoplasmic dynein–dynactin (CD). To avoid apoptotic cleavage of the added motor components, 2 µM Ac-DEVD-CHO was included in the motility assays. Values are means ± SEM for three independent experiments. (B) Total samples from a pig brain dynein–dynactin add-back experiment were immunoblotted using the antibodies shown (C, control cytosol and membranes; A, apoptotic cytosol and membranes). Anti–CD-IC antibodies: i, 70.1; ii, anti-Xenopus CD-IC peptide antibody; iii, Xenopus-specific NH₂-terminal antibody. The position of the added pig brain motor components ( ${blacktriangleleft}$ ) and the Xenopus p150^Glued and CD-IC cleavage products (3) are shown. In contrast to Fig. 8, total samples, not re-isolated membranes, were analyzed.

	Discussion

Top Abstract Introduction Materials and Methods Results Discussion References

We have investigated the fate of cytoplasmic dynein during apoptosis,both in vivo and in vitro, as part of an ongoing study intoalterations in membrane traffic and cellular organization. Wehave used Xenopus egg extracts as a well-characterized modelsystem, as they support regulated cytoplasmic dynein–drivenER movement (Allan 1995; Niclas et al. 1996; Lane and Allan 1999) and can be driven into apoptosis by the addition of cytochromec (Kluck et al. 1997).

We have identified CD-IC as a target for caspase-dependent cleavageboth in vivo and in cell-free extracts, and have demonstratedby site-directed mutagenesis and the use of specific antibodiesthat cleavage results in the loss of the NH₂-terminal p150^Glued-bindingdomain. In contrast, CD-HC and CD-LIC are unaffected and remainas a complex containing the COOH-terminal cleavage product ofCD-IC. Interestingly, we found that dynein complexes eithercontained only full length or only cleaved CD-IC, suggestingthat once a dynein molecule is targeted by the caspase (probablycaspase 3), all the CD-IC chains are cleaved.

The p150^Glued component of dynactin is also cleaved, and mostof the cleaved form no longer migrates as part of the 20S dynactincomplex on sucrose density gradients. Since cleaved p150^Gluedseems to maintain its ability to bind to microtubules and isstill recognized by an antibody to its NH₂-terminal domain,it is likely that the cleavage occurs in its COOH-terminal domain,through which it interacts with the rest of the dynactin complex(Waterman-Storer et al. 1995). This behavior is remarkably similarto that of the COOH-terminally truncated product of the dominantGlued mutant gene in Drosophila (McGrail et al. 1995). It willclearly be of interest to map the p150^Glued cleavage site infuture studies. Since some dynamitin and Arp1 stay bound tothe membrane, this may mean that the dynactin complex minusp150^Glued is left behind. However, lack of antibodies recognizingother Xenopus dynactin components has prevented a thorough investigationof this question.

The cleavage of these two key components, CD-IC and p150^Glued,would be predicted to destroy cytoplasmic dynein's ability tobind to and therefore move cargo (Fig. 10), and we have shownthis to be the case for cytoplasmic dynein–driven ER motilityin apoptotic Xenopus egg extracts. Interestingly, apoptoticmembranes recruit intact cytoplasmic dynein and dynactin fromcontrol cytoplasm, and regain the ability to form ER networks.Moreover, the addition of a pig brain cytoplasmic dynein fraction(which also contains dynactin) to a mixture of apoptotic cytosoland membranes was sufficient to reconstitute network formationpartially. Although the amount of pig brain dynein added matchedthat present in control cytosol, motility was not fully restored.There are many possible explanations for this: first, we donot know how much of this dynein is recruited to the membrane;second, the purified dynein fraction may be partially inactive,or take time to become activated when added to cytosol; third,the concentration of dynactin may be too low; and fourth, theremay be other factors that are absent in apoptotic cytosol thatare required to restore full motility. Together, however, ourdata suggest that cytoplasmic dynein and dynactin are primarytargets for the caspase-dependent abrogation of ER tubule movementdescribed here. Any cleavage of integral membrane proteins bycaspases cannot be inhibiting cytoplasmic dynein binding inour assay, as such changes would not be reversible.

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Figure 10 Diagram showing the predicted effects of CD-IC and p150^Glued cleavage on cytoplasmic dynein–driven organelle motility. Cleavage leads to the removal of the p150^Glued-binding domain of CD-IC, rendering cytoplasmic dynein incapable of binding to, and hence moving, its cargoes. Cleavage of p150^Glued, which occurs more slowly, removes the microtubule-binding capacity of the dynactin complex, which may ensure that cargoes cannot associate with microtubules. Our results suggest that p50 dynamitin is also partially released from cargo (not shown in model).

Our results clearly demonstrate that the interaction of cytoplasmicdynein and dynactin with the membrane is dynamic, and suggeststhat there is rapid turnover, at least in the presence of apoptoticcytosol. This is in keeping with other studies in Xenopus, whichhave revealed that both cytoplasmic dynein and dynactin arerapidly released from membranes on entry into metaphase (Niclas et al. 1996; Addinall et al. 2001), or when anti–CD-ICantibodies are added to interphase extracts (Steffen et al. 1997). Similar loss of cytoplasmic dynein from membranes occurredafter the addition of anti-p150^Glued antibodies to squid axoplasm(Waterman-Storer et al. 1997) and under certain conditions incultured mammalian cells (Lin et al. 1994). In addition, overexpressionof the dynamitin subunit of dynactin causes loss of cytoplasmicdynein from kinetochores (Echeverri et al. 1996) and the Golgiapparatus (Roghi and Allan 1999), again demonstrating that cytoplasmicdynein–cargo interaction is dynamic.

What is the significance of these cleavage events to the apoptosingcell? As yet, we can only speculate, but it is clear that CD-ICin particular is an early target for cleavage, which proceedsin parallel with PARP cleavage. Given that inhibition of cytoplasmicdynein function disrupts ER-to-Golgi apparatus traffic (Presley et al. 1997) and leads to a scattering of the Golgi apparatusthroughout the cell (Burkhardt et al. 1997; Quintyne et al. 1999; Roghi and Allan 1999), it is intriguing to note that Golgiapparatus fragmentation is seen in apoptotic cells (Mancini et al. 2000). It will be of great interest to know if the lossof cytoplasmic dynein from the Golgi apparatus contributes tothis phenotype, and whether ER-to-Golgi apparatus traffic isalso inhibited due to a lack of motor.

In this study, we have investigated the effects of apoptosison membrane movement, but since cytoplasmic dynein plays manydifferent roles in the cell, it is plausible that interruptingother cytoplasmic dynein–driven motile events may alsobe important for apoptosis. Another issue is that the cleavagesite that we have identified in Xenopus CD-IC, DSGD⁹⁹G, is conservedin all rat CD-IC2 splice forms but not in rat CD-IC1. The cytoplasmicdynein intermediate chain family is encoded by two genes, ofwhich CD-IC1 is expressed only in brain and testis, while CD-IC2is found in all tissues (for review see Susalka et al. 2000).Therefore, all cells are likely to contain a cleavable CD-IC,while neurons and testis may also possess a form that lacksthis caspase cleavage site. This may provide a means of differentiallyregulating the function of distinct cytoplasmic dynein complexesduring apoptosis.

Cytoplasmic dynein has been proposed to play a direct role inan early, caspase-independent signaling event during apoptosis.The cytoplasmic dynein light chain, LC8, and the proapoptoticprotein Bim (O'Connor et al. 1998) are stably associated witheach other in healthy cells, and translocate to Bcl-2 shortlyafter triggering apoptosis (Pakthalakath et al. 1999). Hence,caspase-dependent inactivation of the cytoplasmic dynein–dynactincomplex might provide a positive feed-back loop during activationof the apoptotic cascade. However, LC8 is also a component offlagellar dynein, myosin V, I ${kappa}$ B ${alpha}$ and nitric oxide synthase (forreview see King 2000). In addition, the expression of LC8 isincreased by cyclooxygenase 2 treatment of PC12 cells, whereit is thought to protect from growth factor withdrawal-inducedapoptosis by the inhibition of nitric oxide synthesis (Chang et al. 2000). Therefore, because of the apparent promiscuousbehavior of LC8, and in the absence of definitive evidence thatBim is part of the native cytoplasmic dynein complex, it remainsunclear whether the cleavage of CD-IC that we observe here willhave any direct effects on the Bim-LC8 interaction.

Little else is known about the roles that microtubule motorsplay in apoptosis. An inhibition of the plus end–directedmicrotubule motor, kinesin, has been implicated in the clusteringof mitochondria that occurs on triggering cell death via tumornecrosis factor (De Vos et al. 1998, De Vos et al. 2000), butas a shift in mitochondrial position did not occur after otherapoptotic stimuli, it is not clear if this is a general phenomenon.Whether inactivation of kinesin is also responsible for Bax-inducedmitochondrial clustering (Desagher and Martinou 2000) remainsto be tested. Interestingly, our results show that kinesin,like dynein, was released from apoptotic membranes (Fig. 6),but it was not rerecruited from control cytosol (data not shown).Although KHC is not cleaved in apoptotic egg extracts, we donot yet know if kinesin light chains, which are thought to targetkinesin to its cargoes (Hollenbeck 2001), are affected. In addition,since caspase-induced cleavage of kinectin has been seen inapoptotic cultured cells (Machleidt et al. 1998), this raisesthe possibility that kinectin is also cleaved on apoptotic membranesin our assay system, and that this prevents rerecruitment.

The identification of cytoplasmic dynein and dynactin as targetsfor degradation adds to the list of key cytoskeletal (Brancolini et al. 1995; Caulín et al. 1997; Mills et al. 1999) andtrafficking molecules (Cosulich et al. 1997; Swanton et al. 1999a; Mancini et al. 2000) that are cleaved during the crucialprocess of apoptosis. A key issue will be to understand howthese changes together expedite the recognition and clearanceof apoptotic cells.

Acknowledgments

We thank Birgit Lane, David Meyer, Jon Scholey, Ron Vale, andRichard Vallee for supplying antibodies, and Don Nicholson andSophie Roy for caspases. We are grateful to Martin Lowe andLisa Swanton for comments and advice.

This work was supported by the Biotechnology and BiologicalSciences Research Council (34/BI11195 to V. Allan and P. Woodman),the Lister Institute for Preventive Medicine (V. Allan) andthe Medical Research Council (G117/153 to P. Woodman; and COGgrant G9722026).

Submitted: 9 November 2000

Revised: 10 May 2001

Accepted: 15 May 2001

P.G. Woodman and V.J. Allan contributed equally to this work.

Abbreviations used in this paper: CD-HC, cytoplasmic dyneinheavy chain; CD-IC, CD intermediate chain; CD-LIC, CD lightintermediate chain; KHC, kinesin heavy chain; PARP, poly-ADP-ribosepolymerase; VE-DIC, video-enhanced differential interferencecontrast.

References

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Abstract
Introduction
Materials and Methods
Results
Discussion
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