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PLoS Genet. Aug 2007; 3(8): e128.
Published online Aug 3, 2007. doi:  10.1371/journal.pgen.0030128
PMCID: PMC1937013

Dynein Modifiers in C. elegans: Light Chains Suppress Conditional Heavy Chain Mutants

Susan E Mango, Editor

Abstract

Cytoplasmic dynein is a microtubule-dependent motor protein that functions in mitotic cells during centrosome separation, metaphase chromosome congression, anaphase spindle elongation, and chromosome segregation. Dynein is also utilized during interphase for vesicle transport and organelle positioning. While numerous cellular processes require cytoplasmic dynein, the mechanisms that target and regulate this microtubule motor remain largely unknown. By screening a conditional Caenorhabditis elegans cytoplasmic dynein heavy chain mutant at a semipermissive temperature with a genome-wide RNA interference library to reduce gene functions, we have isolated and characterized twenty dynein-specific suppressor genes. When reduced in function, these genes suppress dynein mutants but not other conditionally mutant loci, and twelve of the 20 specific suppressors do not exhibit sterile or lethal phenotypes when their function is reduced in wild-type worms. Many of the suppressor proteins, including two dynein light chains, localize to subcellular sites that overlap with those reported by others for the dynein heavy chain. Furthermore, knocking down any one of four putative dynein accessory chains suppresses the conditional heavy chain mutants, suggesting that some accessory chains negatively regulate heavy chain function. We also identified 29 additional genes that, when reduced in function, suppress conditional mutations not only in dynein but also in loci required for unrelated essential processes. In conclusion, we have identified twenty genes that in many cases are not essential themselves but are conserved and when reduced in function can suppress conditionally lethal C. elegans cytoplasmic dynein heavy chain mutants. We conclude that conserved but nonessential genes contribute to dynein function during the essential process of mitosis.

Author Summary

Microtubules and microtubule-dependent motor proteins segregate chromosomes during mitosis and also promote cellular organization in nondividing cells. An essential motor protein complex called cytoplasmic dynein powers many aspects of microtubule-dependent transport, but it is currently unclear how dynein is regulated such that it can execute different processes. We have performed a genome-wide screen to isolate genes that are involved in dynein-dependent processes. We determined that 20 of the 49 genes we identified specifically influenced the viability of dynein mutant strains but not the viability of other C. elegans mutants. Many of the proteins that specifically influence dynein localized to subcellular sites where the dynein heavy chain has been reported by others to be found. Additionally, we identified four dynein components that appear to negatively regulate the force-generating dynein heavy chain. The identification and initial characterization of this group of genes represents a route to identify genes that are not themselves essential but do participate in essential processes.

Introduction

The microtubule motor called cytoplasmic dynein has roles in diverse cellular processes including meiotic and mitotic spindle assembly and function, neuronal transport, and organelle positioning [1]. Cytoplasmic dynein is composed of a dimer of heavy chains (HCs), along with several accessory chains (ACs: intermediate, light intermediate, and light chains). Other dynein-interacting proteins, such as dynactin and LIS1, are likely present at substoichiometric levels and further modulate dynein function. The HCs contain both ATPase and microtubule binding activities and are sufficient for microtubule-based motility in vitro, moving toward the minus, or slow-growing, end of microtubules [2]. The dynein ACs provide cargo docking sites and often are encoded by multigene families in any one species [reviewed in 1,3]. In C. elegans, a single gene called dhc-1 encodes a cytoplasmic dynein 1 HC, while 11 other genes encode five classes of predicted dynein ACs [3,4].

The early C. elegans embryo is an excellent system for investigating gene contributions for essential cellular processes, including cytoskeletal functions [5]. The C. elegans dynein HC DHC-1 is essential and required for multiple microtubule-dependent events during early embryogenesis [69]. Depletion of DHC-1 by RNA interference (RNAi) in early C. elegans embryos produces defects in female meiotic divisions, migration of the oocyte and sperm pronuclei after fertilization, and centrosome separation during mitotic spindle assembly [6]. Analysis of fast-acting dhc-1 temperature-sensitive (ts) mutants has further revealed that dynein is required for chromosome congression to the metaphase plate during mitosis, as well as for mitotic spindle positioning [10].

While many requirements for cytoplasmic dynein are known, our knowledge of the molecular mechanisms that target and regulate dynein remains limited. Clearly, the multiple ACs can couple the dynein HC to particular substrates [11], including vesicles, nuclei, viruses, kinetochores, and rhodopsin [see table in 1]. However, reducing the function of only four of the eleven dynein ACs in C. elegans produces lethal phenotypes [12]. Thus, it remains unclear how ACs influence the different essential requirements for dynein. Another potential route for dynein regulation involves the phosphorylation state of the different dynein chains, which in some cases confers distinctive functional properties to the motor. While many examples of dynein phosphorylation exist, and cell cycle dependent changes in phosphorylation have been described [1315], few if any studies have demonstrated a requirement for such modification during mitosis. Large-scale forward genetic screens have identified genes with requirements similar to those for dynein, but many of these encode core components of the microtubule cytoskeleton and few are known to directly influence dynein itself [12,16]. Genes that do influence dynein function might also have other essential roles, leading to pleiotropic mutant phenotypes that obscure their relationship to dynein [1719]. Moreover, redundancy within the multigene dynein subunit families, and also perhaps between the different ACs, may complicate the identification of single gene requirements that are important for dynein function. Thus far, reducing the function of individual genes has not provided substantial insight into the mechanisms that regulate and mediate the many different requirements for cytoplasmic dynein during mitosis.

To identify potential regulators of cytoplasmic dynein, we have used a sensitized genetic background to conduct a genome-wide screen for modifiers of dynein function in C. elegans. Other groups have successfully used RNAi modifier screens to identify genes that function in particular pathways [2023]; we have used RNAi to screen for genes that, when reduced in function, suppress the embryonic lethality associated with a temperature-sensitive (ts) allele of the dhc-1 dynein HC gene. Using the dhc-1ts genetic background, we found 49 genes that, when depleted, suppress the partial loss of HC function. Twenty of these genes suppress conditional dynein HC mutants but not other conditional mutants with unrelated defects. Finally, we show that some of these dynein-specific suppressors encode proteins that may overlap with the dynein HC in subcellular localization.

Results

To identify dynein suppressors, we used three different conditional and recessive dhc-1 mutants that were identified previously [7]. These ts alleles of dhc-1 (or195, or283, and or352) produce similar defects at the restrictive temperature of 26 °C, including incomplete mitotic spindle assembly in one-cell embryos and embryonic lethality [7]. We sequenced the dhc-1 locus in the three mutants. The independently isolated or195 and or283 alleles each change a conserved serine to leucine at codon 3200, within the coiled-coil region of the microtubule-binding stalk domain (Figure 1A and and1C).1C). The or352 allele replaces a conserved glycine with aspartic acid at codon 2158, in the ATP-binding walker A motif of the second AAA ATPase domain (Figure 1B and and1C).1C). As both missense mutations affect conserved residues, they may prove useful for engineering ts alleles in other organisms. The temperature versus viability curves of the dynein ts mutants feature a steep central transition zone ideal for modifier screening because subtle changes in temperature produce large changes in embryonic viability (Figure 2A).

Figure 1
Identification of Mutations in Three Recessive dhc-1ts Mutant Alleles
Figure 2
Characterization of dhc-1ts Mutants and Overview of the Suppressor RNAi Screening Strategy

To identify genes that, when reduced in function, can suppress conditional dhc-1 mutants, we developed a high-throughput RNAi-based screen (Figure 2B). To reduce gene function we used a library of 16,757 bacterial strains that each express a dsRNA corresponding to exon-rich gene sequences [17,19]. We then tested over 99% of the bacterial strains in this library for RNAi-mediated suppression of dhc-1(or195) embryonic lethality at 23 °C, after raising synchronized L1 larvae to adulthood on dsRNA-expressing bacterial lawns in 48-well agar plates. This screening procedure should work to identify nonessential and essential suppressor genes, because RNAi does not always fully reduce gene function [24,25], and even if RNAi does produce lethality, cosuppression could restore viability. Nevertheless, essential genes may be missed due to earlier requirements that produce strong larval arrest, sterile, or embryonic lethal phenotypes.

Using this screening procedure, we identified 49 bacterial clones that consistently increased embryonic viability at the semipermissive temperature. The dsRNA-producing plasmids were then sequenced to verify gene identity. Quantification of embryonic viability using dhc-1(or195) animals showed that the RNAi-mediated depletion of suppressor gene function increased viability to 5%–100%, compared to less than 2% in unsuppressed controls (Figure 3A; Table S1). The proteins encoded by the suppressor genes we identified are summarized in Figure 4.

Figure 3
dhc-1-Suppressing Genes
Figure 4
Specificity of the Dynein HC Suppressors As Assayed with Multiple ts Loci.

As a more direct assay for dynein activity in the suppressed dhc-1 embryos, we measured spindle length and cytokinesis success: dhc-1 mutant embryos have severe spindle assembly defects and subsequent cytokinesis failures [6,7,10]. We shifted dhc-1 adult hermaphrodites from 23 °C to the fully restrictive temperature of 26 °C for 3–5 hours and made time-lapse video micrographs using Nomarski optics to monitor the first embryonic cell division. This procedure results in dhc-1(or195) embryos with P0 spindles 30% the length of wild-type spindles (Figure S1). In the suppressed dhc-1(or195) backgrounds, spindle lengths ranged from 30%–83% of wild-type lengths (Figure S1). Similarly, cytokinesis failed in unsuppressed dhc-1(or195) embryos 89% of the time, but most of the suppressors rescued this phenotype (Figure S1). These results indicate that most of the suppressors influence dynein-dependent cellular processes, as expected given their ability to restore viability when reduced in function.

Specificity of Suppression

Because RNAi can reduce the function of unintended targets (so-called “off-target effects” [26,27]), we also used available mutations in some of the suppressor genes we identified to reduce their function. We constructed double mutant strains using dhc-1(or195) and viable deletion alleles for two suppressor genes, dylt-1(ok417) and ufd-2(tm1380), and examined embryonic viability (Figure 3B). The deletion alleles of dylt-1 (encoding a Tctex1-type dynein light chain), and ufd-2 (encoding a ubiquitin conjugating enzyme) both recapitulated the suppression produced by RNAi knockdown (Figure 3B). The dpy-3(e27) and dpy-10(e128) point mutation alleles [28] also suppressed embryonic lethality in double mutants (Figure 3B). Based on this small sampling, and because RNAi in C. elegans appears to be highly gene specific in the absence of close paralogs [12,19], we conclude that many of the suppressors we have identified will prove to be suppressor locus specific. The dsRNA-expressing bacterial clones we used to deplete two of the dynein suppressors (tag-300 and ZK1127.10) probably also knock down expression of one close paralog for each locus [29].

We next asked whether the suppressors are specific for dynein function or if their depletion more generally stabilizes ts proteins. We tested for specificity using two conditional mutants with cell fate patterning defects unrelated to dynein function, lit-1(or131) and spn-4(or191). The lit-1 gene encodes a MAP kinase-related protein [30], while spn-4 encodes a protein with an RNA binding motif [31]. We found that ten of the dhc-1-interacting genes significantly increased embryonic viability in both lit-1 and spn-4 mutants, while 18 others suppressed one or the other of these two conditional mutants when reduced in function using the same RNAi protocol as that used for dhc-1ts mutants (Figure 4, right two columns; Table S1). Therefore, about half of the suppressors appear to act nonspecifically on multiple ts mutants to restore embryonic viability. From here on, we will refer to the suppressors that only acted on dhc-1, and not on lit-1 and spn-4 ts mutants, as dynein-specific suppressors.

Because many ts mutations exert their effect via protein assembly or unfolding mechanisms [32], suppressor genes reduced in function by RNAi might not be expected to exhibit allele specificity with most ts mutations. To determine if the dynein suppressors are either allele or strain specific, we tested the two other conditional dhc-1 strains (containing the or283 and or352 alleles). Although the or283 allele is identical to or195, it provides a useful control for the presence of background mutations because the two strains were isolated independently. In most cases, depletion of the dynein-specific suppressors also restored viability to the other two ts dhc-1 alleles. Y40B1B.5, a putative translation initiation factor, suppressed only one conditional dhc-1 strain, and we consider this as an example of a nonspecific interaction (Figure 4, left three columns; Table S1). Two dsRNAs that do not suppress lit-1 or spn-4 mutants produced suppression in the dhc-1(or195) and dhc-1(or283) strains, but not in the dhc-1(or352) strain, perhaps indicating allele specificity or variability in the RNAi treatments. We conclude that strain background differences are relatively rare, and that the majority of the suppressors are allele-independent. To summarize, we have identified 20 genes that when reduced in function specifically suppress multiple dynein ts strains but not unrelated ts loci.

Survey of Putative Dynein Accessory Chains

We were surprised to discover that depleting two predicted dynein ACs specifically suppressed the partial loss of HC function, because most dynein accessory subunits are presumed to promote dynein function by aiding dynein complex formation or mediating cargo attachment [3,11,33]. Depletion of either dylt-1 (encoding a Tctex1-type light chain) or dyrb-1 (encoding a roadblock-type light chain) suppressed embryonic lethality in all three ts dynein HC mutant strains (Figure 4). To extend this observation, we surveyed all genes encoding predicted dynein components for suppression of the three ts dhc-1 mutants (Figure 5A; Table S2). We reasoned that some dynein subunit genes could have been missed in the primary screening and several dynein AC genes were not represented in the E. coli RNAi library. After using RNAi to reduce their function, we found that one of three Tctex1 homologs (dylt-1), one of four LC8 homologs (dlc-1), one of two light intermediate chains (dli-1), as well as the sole roadblock homolog (dyrb-1) each strongly suppressed the three conditional dynein mutants. Lower-level suppression was also seen for the second light intermediate chain, xbx-1, when its function was reduced. Thus, one gene of each of four subunit classes restores viability to the three dhc-1 mutant strains when depleted by RNAi.

Figure 5
Single Members of C. elegans Dynein Subunit Families Restore Embryonic Viability When Reduced in Function in dhc-1ts Mutants

The only subunit class not found to suppress was the intermediate chain, encoded by a single gene in C. elegans, dyci-1. When reduced in function by RNAi, dyci-1 produces a larval arrest phenotype like that observed for dhc-1(RNAi); this phenotype precludes any suppression of the conditional embryonic lethality (shown as “la” in Figure 5A). In contrast, knockdown of either dlc-1 or dli-1 suppresses embryonic lethality in the dhc-1ts mutants, even though reducing their function in otherwise wild-type embryos produces dhc-1-like defects, including embryonic lethality [12,34] (see Figure 5B and Discussion). The suppressing cytoplasmic dynein subunits and DYCI-1 are shown in a putative complex in Figure 5E.

We performed several genetic assays to better understand how the suppressor genes may be operating. First, suppression of dhc-1 lethality by reducing AC function may indicate that our dhc-1 alleles express a neomorphic and toxic DHC-1 protein: if the suppressor dynein AC subunits positively function in dynein processes, depleting them might suppress any neomorphic effects. This explanation is perhaps unlikely, because the dhc-1ts alleles are all recessive, but remained a possibility in dhc-1 homozygotes. We therefore reduced dynein function using RNAi in animals that had passed through the larval arrest points for dhc-1(RNAi) and dyci-1(RNAi). Specifically, we transferred dhc-1(or195) L4 hermaphrodites to plates with bacteria expressing dhc-1 or dyci-1 dsRNA. As control we performed dylt-1(RNAi) using the same procedure. We observed substantial suppression with dylt-1 in this assay, but we saw no suppression with the heavy or intermediate chains (Figure 5C). This suggests that the DHC-1ts protein is not toxic and that dyci-1 acts more like dhc-1 than the other suppressing ACs because it does not suppress the heavy chain mutant.

To further examine the nature of the AC suppression, we asked if depletion of the suppressor chains could bypass the requirement for dhc-1. We transferred wild-type L4 larvae to plates with bacteria expressing dsRNA corresponding to both the suppressor ACs and dhc-1. We did not observe any suppression in these double RNAi assays (Figure 5D), suggesting that dhc-1ts suppression requires the residual activity of the defective DHC-1 protein. We conclude that the dynein AC suppressors inhibit or somehow oppose the function of the DHC-1ts protein, and that the dhc-1(or195ts) mutation does not produce a toxic gene product but simply reduces DHC-1 activity to a low, but non-null, level.

Localization of the Dynein Suppressor Proteins

To further explore how the suppressor proteins function, we examined the subcellular localization of nine of them as stably expressed N-terminal GFP::S fusions. We chose to first focus on the suppressor genes that were conserved but poorly characterized in any system, or were conserved but uncharacterized during early C. elegans embryogenesis. Prior dynein immunocytochemistry-based localization studies serve as a comparison [6,10,35]. As in other species, C. elegans DHC-1 is associated with mitotic spindles, centrosomes, the nuclear envelope, the cell cortex, the midbody, and throughout the cytoplasm. Most of the suppressor proteins we examined localized to sites where DHC-1 is known to act or localize (Figure 6). However, the nearly ubiquitous distribution of DHC-1 in early embryonic cells makes colocalization likely but not necessarily meaningful, and biochemical studies are needed to conclusively address any direct or indirect physical associations.

Figure 6
Localization of GFP-Tagged Dynein Suppressor Proteins in Wild-Type Embryos

Four suppressor GFP fusion proteins localized to nuclear membranes and to spindle poles or pericentrosomal regions. The DYLT-1 and DYRB-1 dynein light chains were associated with nuclear envelopes and centrosomes, as well as meiotic and mitotic spindle poles (Figure 6A–6H; Videos S1 and S2). The potential coiled-coil protein K04F10.3 was present on the nuclear envelope and in a pericentrosomal position during mitosis, similar to endoplasmic reticulum proteins [36] (Figure 6I–6L; Video S3). K04F10.3 was also highly enriched at meiotic spindle poles (Figure 6I), which has been observed for other endoplasmic reticulum proteins [36]. The NPP-22 transmembrane nucleoporin was found at nuclear envelopes (Figure 6M–6P; Video S4), as previously reported for later stage embryos [37], and it also surrounded centrosomes during mitosis. Two splice isoforms of the pleckstrin homology domain–containing EFA-6/Y55D9A.1, an ARF guanine nucleotide exchange factor, were enriched cortically both in the anterior portion of the one-cell zygote and at the blastomere boundary in two-cell embryos (Figure 6Q–6T; Videos S5 and S6). The conserved Mo25 homolog MOP-25.2/Y53C12A.4 was found enriched in a single spot after cytokinesis that appears to correspond to the midbody (Figure 6U–6X; Video S7). F10E7.8, a highly conserved ortholog of S. cerevisiae Far11, appears nuclear (Figure 6Y–6B′ and Video S8). Finally, the nonspecific suppressor protein STAR-2, a predicted RNA binding protein, appears to be associated with P-granules (like its homolog GLD-1), where dynein is neither localized nor known to function (Figure 6C′–6F′).

DLYT-1 and DYRB-1: Dynein Light Chain Localization

The C. elegans dynein HC protein weakly localizes to spindle poles during early embryonic cell cycles [6,10], and so did DYRB-1 and DYLT-1 (Videos S9 and S10). However, ts mutant forms of the DHC-1 protein (including DHC-1 encoded by the or195 allele) strongly localize to centrosomes when shifted to the non-permissive temperature [10]. The mechanism underlying this enhanced localization is not known, but it may represent trapping of the defective protein at a normally transient location. We exploited this behavior of the mutant DHC-1 protein to determine whether redistribution of the putative DYRB-1 and DYLT-1 dynein light chains also occurred in the dhc-1(or195) background.

We found that the cellular distributions of DYRB-1 and DYLT-1 were dramatically altered in dhc-1(or195) mutant embryos. After shifting the parental worms to the restrictive temperature for 3–5 h prior to collecting embryos, these two proteins were prominently localized to centrosomes and to spindle poles that did not separate in one-cell stage embryos (Figure 7; Videos S11 and S12). The spindle pole to cytoplasmic fluorescence ratio during late anaphase was 5-fold higher in both of the dhc-1 homozygous mutant strains when compared to wild-type embryos expressing the GFP fusions. We also assayed localization of the two putative dynein light chains after short temperature shifts to the nonpermissive temperature in the dhc-1(or195) mutant background, which yields mitotic spindles with an overall wild-type appearance and function. These short temperature shifts also resulted in robust localization of these two dynein light chains to centrosomes (unpublished data). Finally, we examined the localization of GFP::DYRB-1 and GFP::DYLT-1 in embryos from dhc-1(or195) −/+ worms grown at the dhc-1(or195) permissive temperature of 15 °C. Even though embryos from mothers heterozygous for this recessive mutation are viable and develop normally, even at 26 °C [7], we observed a substantial increase in both GFP fusion proteins at the mitotic spindle poles in early embryos (Figure 7; Videos S13 and S14). Importantly, localization of DYLT-1 and DYRB-1 to centrosomes does not occur in embryos depleted for DHC-1 with RNAi (our unpublished results), indicating that these proteins require the mutant DHC-1 polypeptide for centrosomal targeting in the dhc-1(or195) embryos. In summary, the DYRB-1 and DYLT-1 proteins localize to sites where the DHC-1 HC is also found in wild-type embryos, and all three proteins respond similarly to mutational alterations in DHC-1.

Figure 7
Time-Lapse Images of GFP::DYRB-1 and GFP::DYLT-1 in Wild-Type and dhc-1(or195) Mutant Embryos

Genetic Characterization of the DYLT-1 and DYRB-1 Dynein Light Chains

We obtained putative null alleles to determine if dylt-1 and dyrb-1 function in dynein-dependent processes. DYLT-1 is 40% identical to human DYNLT3 and 38% identical to Drosophila Dlc90F (see alignment in Figure 8A). Two other C. elegans genes, dylt-2 and dylt-3, encode more divergent members of this protein family. DYRB-1 is 49% identical to both human DYNLRB1 and Drosophila Robl (see alignment in Figure 8A). There do not appear to be other Roadblock genes in the C. elegans genome [3]. Deletion alleles for both dylt-1 and dyrb-1 have been isolated (Figure 8B). The dylt-1(ok417) deletion removes the entire DYLT-1 open reading frame and does not affect adjacent coding regions. The dyrb-1(tm2645) deletion removes 69% of the dyrb-1 coding region, leaving 29 predicted N-terminal amino acids, and does not affect adjacent coding regions.

Figure 8
Characterization of Genes Encoding the dylt-1 and dyrb-1 Dynein Light Chains

Both deletions are currently annotated as homozygous viable [29]. However, we found that the dyrb-1(tm2645) strain was in fact heterozygous for the deletion and that most embryos produced by dyrb-1(tm2645) homozygous animals failed to hatch (Figure 8C). Homozygous dyrb-1(tm2645) worms also showed an egg-laying defect and produced small broods (unpublished data). To determine if the dyrb-1 deletion was responsible for the embryonic lethality, we crossed the GFP::dyrb-1 transgene into the deletion background. The presence of the transgene fully rescued the embryonic lethality (Figure 8C), but not the egg-laying defect: the transgene is driven from a germline-specific promoter and so would not be expected to rescue zygotic phenotypes. The embryonic lethality exhibited by dyrb-1(tm2645) mutants is consistent with RNAi studies performed by injection or soaking [12,38]. In contrast, homozygous dylt-1 deletion mutants did not exhibit any larval or embryonic lethality (Figure 8C).

To determine if these dynein light chain mutants exhibit dynein HC-like phenotypes, we observed the completion of meiotic polar body extrusion and the first two mitotic cell divisions in mutant embryos (Figure 8D). The dylt-1 embryos appeared wild type for completion of meiosis, pronuclear migration, and spindle assembly and function. However, the dyrb-1 embryos occasionally contained extra female pronuclei (observed in four of 12 recordings, Figure 8D), suggesting that polar body extrusion was defective, and pronuclear migration was often slow compared to wild-type embryos. Once formed, spindles appeared functional using Nomarski optics, although they were frequently positioned improperly and had large spindle poles, as has also been observed after RNAi knockdown [12]. Thus, these two genes are not strictly essential, but the DYRB-1 protein clearly is required for dynein-dependent processes.

Discussion

By using the suppressor screening method outlined in Figure 2B, we have isolated and characterized 49 genes that when reduced in function can suppress a partial loss of dynein HC function. This screening procedure takes advantage of sensitized genetic backgrounds using conditional mutants, can be completed for one mutant in less than 5 wk, and is scalable so that many mutants can be screened in parallel. In fact, we have performed 15 such screens in different sensitized backgrounds (unpublished data). By using three dhc-1ts mutant strains, we found that strain background differences and allele specificity are minimal because most of these genes suppress all three dynein mutants when reduced in function using RNAi. Furthermore, by using two unrelated ts mutants to assay for specificity, we found that 57% of the suppressor genes suppress multiple unrelated mutant loci. Thus, it is clear that assaying the specificity of suppression is critical for evaluating the functional significance of these RNAi interactions. Eliminating the analysis of these nonspecific genes in future screens will save time and resources. Most of the specific suppressor proteins we examined appear to overlap in subcellular localization with the dynein HC, based on previous studies of DHC-1, while one nonspecific suppressor protein, STAR-2, localized to germline P-granules, where dynein is not known to function.

Many of the 20 genes that specifically suppress multiple dhc-1ts alleles are nonessential in C. elegans but well conserved nonetheless. Six of eight deletion alleles available for the 20 specific suppressor genes are homozygous viable, and six additional specific genes do not display lethal phenotypes when reduced in function by RNAi in wild-type worms [29]. Thus, our genetic screening has identified roles in an essential process for at least 12 apparently nonessential genes. Fourteen of the specific dynein suppressor genes have human orthologs as determined by best reciprocal BLAST hits (Table 1), while mop-25.2 has a conserved human homolog but also a paralog in C. elegans. Eleven of these conserved genes are nonessential in C. elegans. Interestingly, eight of the conserved genes in Table 1 have been implicated in human disease etiology, with three of them identified as the causative gene [3941]. Thus, using sensitized genetic backgrounds for genome-wide modifier screens can identify roles for nonessential but conserved genes and thereby provide insights into human disease.

Table 1
Conserved and Specific dhc-1 Suppressor Genes

Nonspecific Suppression of Conditional Mutants

We examined the predicted molecular functions of the suppressor proteins to better understand the basis for the nonspecific suppression phenomenon. Strikingly, many of the nonspecific suppressor genes encode proteins with predicted roles in mitochondrial, ribosomal, and collagen function (18 of 29 genes, or 62%), while only two such genes appeared to specifically suppress dhc-1 (2 of 20 genes or 10%). It is possible that stress produced by RNAi knockdown of these suppressor genes triggers the activity of molecular chaperones that can generally restore function to ts proteins. Indeed, mutation of dpy-10 is known to suppress three other ts mutants: glp-1, emb-5, and mup-1 [4244]. Furthermore, RNAi reduction of dpy-10, star-2, osr-1, or C50D2.1 (all suppressors of dhc-1, lit-1, and spn-4 ts alleles) induces the glycerol biosynthetic gene gpdh-2, while dpy-10 and osr-1 mutants exhibit increased glycerol levels, a condition that promotes protein stability [45]. We suggest that partial loss of central metabolic processes can invoke stress responses that nonspecifically alleviate protein-folding problems in ts proteins. Filtering out these nonspecific interactions by testing unrelated conditional mutants increases the likelihood that the remaining suppressor genes are more directly involved with dynein function. However, ts mutants likely differ in their susceptibility to nonspecific suppression mechanisms, and some apparently unrelated ts mutants might share common cofactors such that both mutants are suppressed by depletion of the same cofactor. Nevertheless, we expect that more extensive testing for specificity will prove very useful for judging the significance of modifier interactions.

Possible Relevance of Suppressor Proteins to Dynein Function

We examined the localization of a number of GFP fusions to suppressor proteins to gain insight into their functional relationship to dynein. In several cases, the subcellular distribution of the suppressor proteins overlapped in different ways with the known and nearly ubiquitous distribution of cytoplasmic dynein in the early C. elegans embryo. In fact, the only specific suppressor that did not display dynein-like localization was F10E7.8, a homolog of yeast Far11 of unknown function [46], which was nuclear. The one nonspecific suppressor protein we examined did not show any dynein-like localization patterns. The subcellular localizations of the GFP::suppressor protein fusions are intriguing. However, given the nearly ubiquitous distribution of dynein in early embryonic cells, biochemical tests for direct association are needed to address the significance of any colocalization detected using light microscopy.

We are particularly interested in suppressor proteins that localize to mitotic spindle poles: the association of the DYLT-1 and DYRB-1 predicted dynein light chains with centrosomes and spindle poles suggests that they may be components of cytoplasmic dynein in C. elegans. Localization of cytoplasmic dynein to centrosomes and spindle poles is well established [47,48], and the inhibition of dynein function prevents centrosome separation, centrosome attachment to nuclei, and the formation of bipolar spindles [6,10,49,50]. Moreover, the centrosomal localization of DHC-1, DYLT-1, and DYRB-1 are all greatly enhanced in dhc-1ts mutant embryos: this dependence of the light chain distribution on the HC further suggests they reside in the same motor complex (Figure 7 and [10]). Furthermore, roadblock light chains are well-established components of dynein, and all of the roadblock protein in mammalian liver extracts is dynein associated [51,52]. Finally, a DYLT-1 homolog in vertebrates is a stoichiometric subunit of cytoplasmic dynein [53]. The presence of these two light chains in a dynein complex is consistent with them having either positive or negative roles in the regulation of HC function (see below).

Cytoplasmic dynein is found on the nuclear envelope where it is thought to regulate nuclear membrane breakdown during mitosis [54], and dynein plays roles during the trafficking of endoplasmic reticulum components [55,56]. Therefore, the nuclear envelope/endoplasmic reticulum proteins NPP-22 and K04F10.3 could couple dynein activity to either of these structures. The anc-1 gene was also isolated in our screening and ANC-1 is localized to the nuclear envelope where it maintains nuclear positioning in postembryonic cells [57]. Reducing the function of these three genes may suppress partial loss of dynein HC mutants by reducing the need for dynein during nuclear envelope breakdown, through constitutive partial destabilization of the nuclear envelope.

The distribution of the cytoplasmic dynein HC includes sites other than spindle poles and nuclear envelopes in C. elegans, for example, at the cell cortex and at the cell division remnant called the midbody [6,10]. The MOP-25.2 protein was found at the midbody and faintly at spindle poles. The MOP-25.2 ortholog in S. pombe, Pmo25, is also present at the cell division site and on spindle poles [58]. Mammalian MOP-25.2 homologs stimulate the kinase activity of the LKB1 tumor suppressor (the C. elegans ortholog is PAR-4), which in turn activates MARK microtubule-destabilizing kinases [59,60]. The C. elegans MARK ortholog, PAR-1, controls cell polarity during embryogenesis, and orthologs have been implicated in regulation of microtubule dynamics from yeast to humans [6164].

Lastly, the two splice isoforms of EFA-6 were associated with the anterior cell cortex in late one-cell embryos. Cortically localized dynein may have important roles in applying forces to astral microtubules that influence mitotic spindle positioning and chromosome separation during anaphase [10,65,66]. EFA6 ARF guanine nucleotide exchange factors require their pleckstrin homology domain for cortical targeting, and are known to regulate cortical actin dynamics in vertebrate cells by promoting guanine nucleotide exchange on ARF6 [67,68]. Our results identifying efa-6 as a dynein HC suppressor suggest a functional linkage of the actin and microtubule cytoskeletons at the cell cortex. Interestingly, two yeast pleckstrin homology domain proteins, Num1 and mcp5+, localize to the cell cortex and direct astral microtubule and dynein function, although they do not contain a Sec7 domain like EFA-6 does [6971].

Function of Dynein Intermediate, Light Intermediate, and Light Chains

The dynein chains in C. elegans exhibit strikingly different functional requirements. The DYRB-1 roadblock light chain is required for completion of meiosis and pronuclear migration, but an at least partially functional mitotic spindle forms in the absence of DYRB-1 (Figure 8). The DLI-1 light intermediate chain is required for multiple dynein-dependent functions: pronuclear migration, centrosome separation, and meiotic and mitotic spindle function [12,34]. DLI-1 may promote nuclear envelope targeting of both centrosomes and DHC-1 by interacting with the nuclear envelope protein ZYG-12 [35]. The second worm light intermediate chain gene, xbx-1, is required for cilia function but not early embryonic development [12,72]. RNAi knockdown of DLC-1, one of three LC8 proteins in C. elegans, produces defects similar to dli-1 but knockdown of the other two LC8-related genes does not result in any phenotypes [12]. RNAi depletion of dyci-1 results in severe meiotic, pronuclear migration, and mitotic spindle assembly defects [12] and in our feeding RNAi regimen dyci-1(RNAi) produces a larval arrest phenotype similar to that observed for dhc-1. Finally, the three Tctex1 proteins in C. elegans, DYLT-1, 2, and 3, are not essential for dynein-related functions [12]. As the dyrb-1, dlc-1, and dli-1 dynein AC genes display some dhc-1-like requirements, they positively influence dynein function. However, because reducing their function suppresses dhc-1ts mutants, they may also exert negative regulation (along with dylt-1) on the heavy chain.

Negative Regulation of Dynein HC by Light Chain Subunits

Finding that reducing the function of light and light intermediate dynein chains suppressed the partial loss of HC function was a striking result. One member of each of four subunit classes can suppress the embryonic lethality associated with three dhc-1 ts mutants (Figure 5). We have considered two different models to explain how RNAi-mediated depletion of these dynein ACs can suppress reduced HC function. First, these dynein subunits could be in functional complexes with, and exert negative regulation on, the DHC-1 HC (Figure 5B). The suppression mechanism in this case proposes that removal of the suppressing ACs increases residual mutant DHC-1 activity. The other, nonsuppressing, accessory subunits might then function in nonmitotic cellular processes such as neuronal transport or organelle positioning. In support of this view, physical removal of the intermediate chains of rat cytoplasmic dynein increased HC ATPase activity by about 4-fold (light chains were not monitored in this study but were likely removed as well) [73]. Thus, at least with respect to ATPase activity, some dynein ACs do act as biochemical negative regulators of HC function.

An Assortment of Essential and Nonessential Dynein Complexes

Alternatively, an assortment of dynein complexes (with different ACs) could coexist within early embryonic cells, with only a subset required for the essential mitotic functions that require DHC-1. In this case, suppression might result from the release of DHC-1 HCs from less essential motor complexes, allowing more of the functionally compromised HCs to participate in the essential process of mitosis. We currently disfavor this hypothesis because two of the suppressing light chains (DYLT-1 and DYRB-1) can indeed localize to meiotic and mitotic spindles (Figures 6 and and7),7), sites where DHC-1 has been shown by others to localize and function. Furthermore, the distribution of DYRB-1 and DYLT-1 closely resembles the distribution of the HC in dhc-1(or195) embryos, suggesting that these two light chains associate with the HC during mitosis (Figure 7 and [10]). Finally, dhc-1-like phenotypes result from mutation or RNAi knockdown of three suppressing ACs in otherwise wild-type worms, indicating that they share at least some common and essential requirements. Regardless of the suppression mechanism, our identification of ACs that genetically interact with the DHC-1 HC provides a basis for functionally classifying the paralogs of these dynein subunit gene families, and for further investigation of dynein composition and function.

Nonessential Dynein Subunits and Negative Regulation of the HC

Some ACs are nonessential, supporting the view that some cytoplasmic dynein subunits could function by exerting negative regulation on the HC, rather than positively influencing essential HC function. For example, DYRB-1 is not absolutely required for viability because worms lacking this protein can be propagated, although they are extremely sick and do exhibit two dhc-1-like phenotypes (Figure 8). Also, homozygous dylt-1 deletion mutants appear fully viable (Figure 8). The two additional Tctex1 C. elegans genes could be functionally redundant with DYLT-1, but simultaneously reducing the function of DYLT-2 and DYLT-3 by RNAi in the dylt-1 deletion strain did not cause lethality (unpublished data). Because RNAi does not always completely reduce function, the question of redundancy in the Tctex1 C. elegans gene family remains unresolved. However, Drosophila contains only a single Tctex1 gene, Dlc90F [74,75]. A Dlc90F null allele that deletes 80% of the open reading frame is essential only for sperm production but not for viability of male or female flies, despite the wild-type protein being incorporated into dynein motors and expressed in various Drosophila tissues [74]. Thus, at least in Drosophila, the Tctex1 dynein light chain family is not required for cell division processes like the HC is. Interestingly, budding yeast does not possess genes for the Tctex1 or roadblock ACs, indicating that functional cytoplasmic dynein does not require these subunits that are conserved in many other organisms. The AC genes that yeast does posses are not required for HC motility in vitro because dynein purified from yeast with mutations in these genes remains fully active [2]. Thus, dynein function in several contexts does not require AC subunits, and we suggest that in some cases they may have negative regulatory roles. Negative regulation of cytoplasmic dynein may be redundant with other modes of HC regulation or only required during special circumstances. Further studies of subunit localization, and in vitro studies of C. elegans dynein motility, may provide further insight into the modes of AC regulation and function.

Materials and Methods

C. elegans strains and culture.

Strains were cultured according to standard procedures [28]. ts mutants were maintained at 15 °C and GFP-expressing strains in a wild-type background were maintained in a 23 °C incubator. dhc-1(or195) was outcrossed six times to the N2 Bristol wild-type strain and the or283 and or352 dhc-1 mutants were each outcrossed four times with N2. For sequencing mutant dhc-1 loci, genomic DNA was amplified as overlapping ~1-kb fragments from the start codon to the stop codon and sequenced at the University of Oregon DNA sequencing laboratory. For double mutant constructions, the dhc-1(or195) mutation was monitored by sequencing or by assaying a restriction fragment length polymorphism caused by the mutation with Hpy188I (New England Biolabs, http://www.neb.com), following PCR amplification of the mutated region. The dylt-1(ok417) and ufd-2(tm1380) alleles were monitored by PCR amplification of genomic sequence encompassing the deletions and assaying product size by agarose gel electrophoresis.

GFP imaging.

Visualization of GFP fusion protein localization was accomplished by mounting embryos on M9 + 3% agarose pads on microscope slides covered with a coverslip. Time-lapse videos were obtained on a spinning disk Nikon Eclipse TE2000-U microscope (Nikon Instruments, http://www.nikon.com) fitted with an ORCA-ER digital camera (Hamamatsu Photonics, http://www.hamamatsu.com) using a Nikon 60×, 1.4 NA Plan Apo oil objective lens. Videos were adjusted for contrast in ImageJ (National Institutes of Health, http://rsb.info.nih.gov/ij/) [76], images were adjusted for levels in Adobe Photoshop (http://www.adobe.com/).

RNAi screening.

After obtaining the E. coli RNAi library from the MRC Geneservice (Cambridge, UK) [17,19], we rearrayed it into a 48-well microplate format using a liquid-handling Qiagen BioRobot 8000 (http://www.qiagen.com). E. coli strains were thawed from −80 °C storage and inoculated into 1 ml of LB + 100 mg/ml ampicillin-containing 96-well growth plates (Whatman, http://www.whatman.com) and covered with microporous sealing film (USA Scientific, http://www.usascientific.com). Only 48 wells of the 96-well growth plates were filled with media, corresponding to the rearrayed E. coli library. After overnight shaking incubation at 37 °C, 20 μl of the cultures were dispensed with a 24-channel electronic repeating pipette (Rainin, http://www.rainin.com) onto 48-well plates (Nunc, http://www.nuncbrand.com/) containing NGM agar, 100 μg/ml ampicillin, and 1 mM IPTG and allowed to dry and induce dsRNA at 37 °C overnight. The 48-well agar plates were filled with a Wheaton Unispense peristaltic pump (http://www.wheaton.com) equipped with a custom-made adaptor (University of Oregon Technical Science Administration) that allowed simultaneous filling of eight wells with the agar solution. Approximately 15 hypochlorite-synchronized L1 mutant larvae were pipetted into each well of the 48-well plates with a multichannel pipette and allowed to produce broods. Screening for F1 viability was performed by visual examination with a dissecting microscope. Phenotypes were recorded on an Excel spreadsheet (http://www.microsoft.com) and organized in a FileMaker Pro (http://www.filemaker.com) database. We qualitatively identified 295 initial positive suppressing E. coli strains, for which we repeated the assay on 60-mm plates with E. coli again thawed from the library (not streak purified). If the observed phenotypes reproduced, the assay was performed with three streak-purified E. coli colonies, and a single isolate that again displayed the interaction was kept for further analysis.

Embryonic viability quantitation methods.

To quantitate embryonic viability we used the following procedure. Cultures of dsRNA-producing bacteria were grown overnight in LB + 100 μg/ml ampicillin. Cultures (0.2 ml) were seeded onto 60-mm NGM agar plates containing 100 μg/ml ampicillin and 1 mM IPTG and allowed to induce dsRNAs overnight at room temperature. The L4440 control vector-containing strain was used as the bacterial lawn for the experiments shown in Figures 2A and and3B.3B. Approximately 80 synchronized L1 larvae (obtained from hypochlorite-treated worms) were pipetted onto the plates and allowed to grow to young adulthood. Five gravid worms were transferred to prepared NGM agar plates supplemented with 100 μg/ml ampicillin and 1 mM IPTG containing a small RNAi bacterial lawn produced from ~5 μl of overnight E. coli culture. After producing broods, the adult worms were removed and the embryos were allowed to develop for at least 24 h. Embryos and larvae were then counted immediately or after storage at 4 °C. We considered only suppressor dsRNAs that increased embryonic viability greater than 3-fold above the background viability observed with the L4440 control vector (in the dhc-1(or195)) screen to be significant enough for continued study.

Molecular biology.

We introduced a polylinker site containing six unique restriction enzyme recognition sites into the pIC26 GFP-S protein plasmid by using phosphorylated and PAGE-purified synthetic oligonucleotides [77]. Following ligation, the new plasmid was sequence verified. The modified vector, pSO26, allows the use of additional restriction enzymes and directional cloning for inserting genes of interest (Figure S2). The SpeI site was recreated at the 5′ end of the polylinker but not at the 3′ end. We amplified N2 genomic DNA or cDNA (Invitrogen, http://www.invitrogen.com) with Pfu Turbo polymerase (Stratagene, http://www.stratagene.com), and cloned A-tailed PCR products into either pGEM-T or pGEM-T-easy shuttle vectors (Promega, http://www.promega.com). Inserted genes were sequence verified at the University of Oregon DNA sequencing laboratory prior to cleavage and ligation to pSO26 (see Table S3 for restriction sites and primer sequences used). All of the constructs used in this study were cloned as SpeI-AsiSI or AscI-AsiSI fragments, except for the STAR-2 gene, which was amplified as a SpeI fragment and cloned into pIC26.

To construct dynein subunit dsRNA-expressing plasmids not available in the RNAi library, gene fragments were amplified from N2 genomic DNA with the following primers: F41G4.1: 5′-AAGATATCACCCAAAATGGTCCAAAACAAAG-3′ and 5′-CGGATATCTCGACTGAAGCTGGTTCTGA-3′, xbx-1: 5′-AAGATATCTACGACGATGGAAGTTTGAAG-3′ and 5′-CGGATATCCGTGCCTCTGCAGC-3′, dlc-3: 5′-AAGATATCAATTTCAGGTGGACACTGGC-3′ and 5′-CGGATATCAGCACACTTGCATCATCTGAA-3′. The PCR products were cut with EcoRV, ligated to EcoRV-digested L4440, and sequence verified.

Isolation of transgenic worms.

GFP fusion plasmids were bombarded into unc-119(ed3) worms as previously described except with the following two changes [78]. Three milligrams of gold particles were used per hepta adaptor bombardment. Also, we briefly sonicated the gold particles (prior to DNA coating and while suspended in 50% glycerol) with a Branson sonifier 450 (http://www.sonifier.com/) fitted with a small tip set to power level 1, to disrupt gold aggregates. Non-Unc worms were picked to new plates and allowed to produce broods, which were assayed for GFP fluorescence with a Zeiss axioskop microscope (http://www.zeiss.com/) fitted with an X-Cite 120 illumination system (EXFO life sciences, Mississauga, Ontario, Canada). For each fluorescent line, 12 GFP-positive worms were singled to new plates to determine if the constructs were integrated or were carried as extrachromosomal arrays.

Supporting Information

Figure S1

Suppression of dhc-1 Early Embryonic Defects:

Twenty-three representative suppressor genes were tested for their effect on spindle length and cytokinesis in dhc-1 embryos. (A) Wild-type, dhc-1(or195), and dhc-1(or195); dylt-1(RNAi) embryos at early telophase and subsequent to cytokinesis. Reduction of dylt-1 function in the dhc-1 strain partially restores spindle length and cytokinesis is successful. (B) Graph of P0 spindle length and cytokinesis success for dhc-1(or195) embryos with reduced suppressor gene function (values expressed as percent of wild type). The numbers in parentheses denote the number of embryos recorded for each gene depleted with RNAi. The L4440 trial represents dhc-1(or195) animals feeding on bacteria harboring the empty RNAi vector. Genes were separated into specific and nonspecific suppressors based on Figure 4, and are sorted by spindle lengths.

(1.6 MB PDF)

Figure S2

Sequence of the New Multiple Cloning Site in pSO26:

The two oligonucleotides shown were ligated into SpeI-cut pIC26 to yield pSO26. pIC26 uses the pie-1 promoter and 3′ UTR and contains the unc-119(+) transformation marker [77]. Unique restriction sites are shown, enzymes giving blunt ends are indicated with a “b,” and enzymes with 8-base recognition sites are shown with an “8.” The translational reading frame is represented as codon triplets. The SpeI site was recreated and remains unique.

(75 KB PDF)

Table S1

Quantification of Embryonic Viability in RNAi-Treated ts Mutants:

Data was used to prepare Figure 3A and Figure 4. Number of progeny counted, embryonic viability, and embryonic viability standard deviation is shown for each RNAi assay. Numbers of progeny are not comparable. The rightmost four columns summarize information from other parts of this paper, and two dsRNAs are predicted to knock down expression of paralogous genes.

(27 KB XLS)

Table S2

Quantification of Embryonic Viability in RNAi-Treated dhc-1ts Mutants:

Data was used to prepare Figure 5A. Number of progeny counted, embryonic viability, and embryonic viability standard deviation is shown for each RNAi assay. Numbers of progeny are not comparable.

(20 KB XLS)

Table S3

GFP Fusion Protein Information:

PCR template type, cloning sites, primer sequences, and a representative C. elegans line are given for each gene.

(23 KB XLS)

Video S1

GFP::DYLT-1, Localization in Two Gastrulation-Stage Embryos:

Localization to nuclear envelopes and centrosomes. Three slices 1 μm apart were captured every 30 s and projected.

(1.0 MB MOV)

Video S2

GFP::DYRB-1, Localization to Meiotic Spindle Poles during Meiosis I and II:

Three slices 1 μm apart were captured every 30 s and projected.

(709 KB MOV)

Video S3

GFP::K04F10.3, nuclear membrane and pericentrosomal localization (similar to endoplasmic reticulum proteins)

Three slices 1 μm apart were captured every 30 s and projected.

(1.5 MB MOV)

Video S4

GFP::NPP-22, Nuclear Membrane and Pericentrosomal Localization (Similar to Endoplasmic Reticulum Proteins)

Note the appearance of “strings” in the nucleus that might represent furrows in the nuclear envelope. One slice was captured every 30 s.

(920 KB MOV)

Video S5

GFP::EFA-6.a, Localization to the Anterior Cortex in the One-Cell Embryo and Enrichment to the Boundary between the AB and P1 Cells:

Not present in four-cell embryos. Midbody localization is seen at 30 min and a polar body is seen in the 31–34.5 min frames. One slice was captured every 30 s.

(768 KB MOV)

Video S6

GFP::EFA-6.c, Similar to EFA-6.a (Video S5)

One slice was captured every 30 s.

(678 KB MOV)

Video S7

GFP::MOP-25.2, Localization to the Midbody and Weakly Nuclear:

Three slices 1 μm apart were captured every 30 s and projected.

(1.5 MB MOV)

Video S8

GFP::F10E7.8, Nuclear Localization:

The cytoplasmic signal is partially due to background autofluorescence. One slice was captured every 30 s.

(1.4 MB MOV)

Video S9

GFP::DYRB-1 in a Wild-Type Background:

Worms were grown at 15 °C and embryos were imaged on a room temperature microscope stage. Weak localization to mitotic spindle poles. Three slices 1 μm apart were captured every 30 s and projected.

(342 KB MOV)

Video S10

GFP::DYLT-1 in a Wild-Type Background:

Worms were grown at 15 °C and embryos were imaged on a room temperature microscope stage. Weak localization to mitotic spindle poles. Three slices 1 μm apart were captured every 30 s and projected.

(249 KB MOV)

Video S11

GFP::DYRB-1 in a dhc-1(or195ts) Homozygous Background:

Strain grown at 15 °C, shifted to 26 °C for 3 h and imaged on a microscope stage maintained at 26 °C. Robust localization to centrosomes. Three slices 1 μm apart were captured every 30 s and projected.

(313 KB MOV)

Video S12

GFP::DYLT-1 in a dhc-1(or195ts) homozygous background:

Strain grown at 15°C, shifted to 26°C for 5 hours and imaged on a microscope stage maintained at 26°C. Robust localization to centrosomes. Three slices 1 μm apart were captured every 30 s and projected.

(386 KB MOV)

Video S13

GFP::DYRB-1 in a dhc-1(or195ts) Heterozygous Background:

Strain grown at 15 °C and embryos were imaged on a room temperature microscope stage. Robust localization to mitotic spindle poles. Three slices 1 μm apart were captured every 30 s and projected.

(240 KB MOV)

Video S14

GFP::DYLT-1 in a dhc-1(or195ts) Heterozygous Background:

Strain were grown at 15 °C and embryos were imaged on a room temperature microscope stage. Robust localization to mitotic spindle poles. Three slices 1 μm apart were captured every 30 s and projected.

(206 KB MOV)

Accession Numbers

The National Center for Biotechnology Information (NCBI) database (http://www.ncbi.nlm.nih.gov/gquery/gquery.fcgi?itool=toolbar) accession numbers for the dhc-1 homologs discussed in this paper are C. elegans, NP_491363; Dictyostelium discoideum, XP_643185; Drosophila melanogaster, AAA60323; Homo sapiens, NP_001367; Mus musculus, NP_084514; Saccharomyces cerevisiae, NP_012980; and Schizosaccharomyces pombe, NP_001018285.

The NCBI accession numbers for the Drosophila and human DYLT-1 and DYRB-1 protein homologues, respectively, are Dlc90F, NP_477356; DYNLT3, NP_006511; DYNLRB1, NP_054902; and robl, NP_523771.

Acknowledgments

We thank I. Cruxent for help with RNAi screening and L. Saccomanno for cloning star-2. We also acknowledge J. Canman and M. Price for expert microscopy assistance and we received excellent comments on the manuscript from G. Sprague and M. Goulding. We are extremely grateful to the C. elegans Genetics Center, funded by the National Institutes of Health (NIH), the C. elegans knockout consortium, and the National Bioresource Project of Japan for strains.

Abbreviations

AC
accessory chain
dsRNA
double-stranded RNA
GFP
green fluorescent protein
HC
heavy chain
IPTG
isopropyl-beta-D-thiogalactopyranoside
RNAi
RNA interference
ts
temperature-sensitive

Footnotes

Author contributions. SMO and BB conceived and designed the experiments and wrote the paper. SMO performed the experiments and analyzed the data. MDD and JCC contributed reagents/materials/analysis tools.

Funding. This work was funded by NIH grant GM049869 (to BB). The Damon Runyon Cancer Research Foundation and the Leukemia and Lymphoma Society supported SO.

Competing interests. The authors have declared that no competing interests exist.

References

  • Vallee RB, Williams JC, Varma D, Barnhart LE. Dynein: An ancient motor protein involved in multiple modes of transport. J Neurobiol. 2004;58:189–200. [PubMed]
  • Reck-Peterson SL, Yildiz A, Carter AP, Gennerich A, Zhang N, et al. Single-molecule analysis of dynein processivity and stepping behavior. Cell. 2006;126:335–348. [PMC free article] [PubMed]
  • Pfister KK, Shah PR, Hummerich H, Russ A, Cotton J, et al. Genetic analysis of the cytoplasmic dynein subunit families. PLoS Genet. 2006. e1. doi: 10.1371/journal.pgen.0020001. [PMC free article] [PubMed]
  • Lye RJ, Wilson RK, Waterston RH. Genomic structure of a cytoplasmic dynein heavy chain gene from the nematode Caenorhabditis elegans. Cell Motil Cytoskeleton. 1995;32:26–36. [PubMed]
  • Oegema K, Hyman AA. WormBook. The C. elegans Research Community, editors. Jan 19,, 2006. Available: http://www.wormbook.org. Accessed 5 July 2007. [PubMed]
  • Gönczy P, Pichler S, Kirkham M, Hyman AA. Cytoplasmic dynein is required for distinct aspects of MTOC positioning, including centrosome separation, in the one cell stage Caenorhabditis elegans embryo. J Cell Biol. 1999;147:135–150. [PMC free article] [PubMed]
  • Hamill DR, Severson AF, Carter JC, Bowerman B. Centrosome maturation and mitotic spindle assembly in C. elegans require SPD-5, a protein with multiple coiled-coil domains. Dev Cell. 2002;3:673–684. [PubMed]
  • Mains PE, Sulston IA, Wood WB. Dominant maternal-effect mutations causing embryonic lethality in Caenorhabditis elegans. Genetics. 1990;125:351–369. [PMC free article] [PubMed]
  • Howell AM, Rose AM. Essential genes in the hDf6 region of Chromosome I in Caenorhabditis elegans. Genetics. 1990;126:583–592. [PMC free article] [PubMed]
  • Schmidt DJ, Rose DJ, Saxton WM, Strome S. Functional analysis of cytoplasmic dynein heavy chain in Caenorhabditis elegans with fast-acting temperature-sensitive mutations. Mol Biol Cell. 2005;16:1200–1212. [PMC free article] [PubMed]
  • Kamal A, Goldstein LS. Principles of cargo attachment to cytoplasmic motor proteins. Curr Opin Cell Biol. 2002;14:63–68. [PubMed]
  • Sönnichsen B, Koski LB, Walsh A, Marschall P, Neumann B, et al. Full-genome RNAi profiling of early embryogenesis in Caenorhabditis elegans. Nature. 2005;434:462–469. [PubMed]
  • Dell KR, Turck CW, Vale RD. Mitotic phosphorylation of the dynein light intermediate chain is mediated by cdc2 kinase. Traffic. 2000;1:38–44. [PubMed]
  • Niclas J, Allan VJ, Vale RD. Cell cycle regulation of dynein association with membranes modulates microtubule-based organelle transport. J Cell Biol. 1996;133:585–593. [PMC free article] [PubMed]
  • Huang CY, Chang CP, Huang CL, Ferrell JE., Jr. M phase phosphorylation of cytoplasmic dynein intermediate chain and p150(Glued) J Biol Chem. 1999;274:14262–14269. [PubMed]
  • Gunsalus KC, Ge H, Schetter AJ, Goldberg DS, Han JD, et al. Predictive models of molecular machines involved in Caenorhabditis elegans early embryogenesis. Nature. 2005;436:861–865. [PubMed]
  • Fraser AG, Kamath RS, Zipperlen P, Martinez-Campos M, Sohrmann M, et al. Functional genomic analysis of C. elegans chromosome I by systematic RNA interference. Nature. 2000;408:325–330. [PubMed]
  • Maeda I, Kohara Y, Yamamoto M, Sugimoto A. Large-scale analysis of gene function in Caenorhabditis elegans by high- throughput RNAi. Curr Biol. 2001;11:171–176. [PubMed]
  • Kamath RS, Fraser AG, Dong Y, Poulin G, Durbin R, et al. Systematic functional analysis of the Caenorhabditis elegans genome using RNAi. Nature. 2003;421:231–237. [PubMed]
  • Cho S, Rogers KW, Fay DS. The C. elegans glycopeptide hormone receptor ortholog, FSHR-1, regulates germline differentiation and survival. Curr Biol. 2007;17:203–212. [PubMed]
  • Holway AH, Hung C, Michael WM. Systematic, RNA-interference-mediated identification of mus-101 modifier genes in Caenorhabditis elegans. Genetics. 2005;169:1451–1460. [PMC free article] [PubMed]
  • Labbé JC, Pacquelet A, Marty T, Gotta M. A genomewide screen for suppressors of par-2 uncovers potential regulators of PAR protein-dependent cell polarity in Caenorhabditis elegans. Genetics. 2006;174:285–295. [PMC free article] [PubMed]
  • Withee J, Galligan B, Hawkins N, Garriga G. Caenorhabditis elegans WASP and Ena/VASP proteins play compensatory roles in morphogenesis and neuronal cell migration. Genetics. 2004;167:1165–1176. [PMC free article] [PubMed]
  • Timmons L, Court DL, Fire A. Ingestion of bacterially expressed dsRNAs can produce specific and potent genetic interference in Caenorhabditis elegans. Gene. 2001;263:103–112. [PubMed]
  • Kamath RS, Martinez-Campos M, Zipperlen P, Fraser AG, Ahringer J. Effectiveness of specific RNA-mediated interference through ingested double-stranded RNA in Caenorhabditis elegans. Genome Biol. 2000. [PMC free article] [PubMed]
  • Kulkarni MM, Booker M, Silver SJ, Friedman A, Hong P, et al. Evidence of off-target effects associated with long dsRNAs in Drosophila melanogaster cell-based assays. Nat Methods. 2006;3:833–838. [PubMed]
  • Ma Y, Creanga A, Lum L, Beachy PA. Prevalence of off-target effects in Drosophila RNA interference screens. Nature. 2006;443:359–363. [PubMed]
  • Brenner S. The genetics of Caenorhabditis elegans. Genetics. 1974;77:71–94. [PMC free article] [PubMed]
  • WormBase web site release WS167. 2006. Available: http://www.wormbase.org. Accessed 5 July 2007.
  • Meneghini MD, Ishitani T, Carter JC, Hisamoto N, Ninomiya-Tsuji J, et al. MAP kinase and Wnt pathways converge to downregulate an HMG-domain repressor in Caenorhabditis elegans. Nature. 1999;399:793–797. [PubMed]
  • Gomes JE, Encalada SE, Swan KA, Shelton CA, Carter JC, et al. The maternal gene spn-4 encodes a predicted RRM protein required for mitotic spindle orientation and cell fate patterning in early C. elegans embryos. Development. 2001;128:4301–4314. [PubMed]
  • Alber T, Sun DP, Nye JA, Muchmore DC, Matthews BW. Temperature-sensitive mutations of bacteriophage T4 lysozyme occur at sites with low mobility and low solvent accessibility in the folded protein. Biochemistry. 1987;26:3754–3758. [PubMed]
  • Vale RD. The molecular motor toolbox for intracellular transport. Cell. 2003;112:467–480. [PubMed]
  • Yoder JH, Han M. Cytoplasmic dynein light intermediate chain is required for discrete aspects of mitosis in Caenorhabditis elegans. Mol Biol Cell. 2001;12:2921–2933. [PMC free article] [PubMed]
  • Malone CJ, Misner L, Le Bot N, Tsai MC, Campbell JM, et al. The C. elegans hook protein, ZYG-12, mediates the essential attachment between the centrosome and nucleus. Cell. 2003;115:825–836. [PubMed]
  • Poteryaev D, Squirrell JM, Campbell JM, White JG, Spang A. Involvement of the actin cytoskeleton and homotypic membrane fusion in ER dynamics in Caenorhabditis elegans. Mol Biol Cell. 2005;16:2139–2153. [PMC free article] [PubMed]
  • Stavru F, Hulsmann BB, Spang A, Hartmann E, Cordes VC, et al. NDC1: A crucial membrane-integral nucleoporin of metazoan nuclear pore complexes. J Cell Biol. 2006;173:509–519. [PMC free article] [PubMed]
  • Fernandez AG, Gunsalus KC, Huang J, Chuang LS, Ying N, et al. New genes with roles in the C. elegans embryo revealed using RNAi of ovary-enriched ORFeome clones. Genome Res. 2005;15:250–259. [PMC free article] [PubMed]
  • Vulpe C, Levinson B, Whitney S, Packman S, Gitschier J. Isolation of a candidate gene for Menkes disease and evidence that it encodes a copper-transporting ATPase. Nat Genet. 1993;3:7–13. [PubMed]
  • Wang J, Hegele RA. Genomic basis of cystathioninuria (MIM 219500) revealed by multiple mutations in cystathionine gamma-lyase (CTH) Hum Genet. 2003;112:404–408. [PubMed]
  • Gros-Louis F, Dupre N, Dion P, Fox MA, Laurent S, et al. Mutations in SYNE1 lead to a newly discovered form of autosomal recessive cerebellar ataxia. Nat Genet. 2007;39:80–85. [PubMed]
  • Nishiwaki K, Miwa J. Mutations in genes encoding extracellular matrix proteins suppress the emb-5 gastrulation defect in Caenorhabditis elegans. Mol Gen Genet. 1998;259:2–12. [PubMed]
  • Maine EM, Kimble J. Identification of genes that interact with glp-1, a gene required for inductive cell interactions in Caenorhabditis elegans. Development. 1989;106:133–143. [PubMed]
  • Goh PY, Bogaert T. Positioning and maintenance of embryonic body wall muscle attachments in C. elegans requires the mup-1 gene. Development. 1991;111:667–681. [PubMed]
  • Lamitina T, Huang CG, Strange K. Genome-wide RNAi screening identifies protein damage as a regulator of osmoprotective gene expression. Proc Natl Acad Sci U S A. 2006;103:12173–12178. [PMC free article] [PubMed]
  • Kemp HA, Sprague GF., Jr. Far3 and five interacting proteins prevent premature recovery from pheromone arrest in the budding yeast Saccharomyces cerevisiae. Mol Cell Biol. 2003;23:1750–1763. [PMC free article] [PubMed]
  • Pfarr CM, Coue M, Grissom PM, Hays TS, Porter ME, et al. Cytoplasmic dynein is localized to kinetochores during mitosis. Nature. 1990;345:263–265. [PubMed]
  • Steuer ER, Wordeman L, Schroer TA, Sheetz MP. Localization of cytoplasmic dynein to mitotic spindles and kinetochores. Nature. 1990;345:266–268. [PubMed]
  • Robinson JT, Wojcik EJ, Sanders MA, McGrail M, Hays TS. Cytoplasmic dynein is required for the nuclear attachment and migration of centrosomes during mitosis in Drosophila. J Cell Biol. 1999;146:597–608. [PMC free article] [PubMed]
  • Vaisberg EA, Koonce MP, McIntosh JR. Cytoplasmic dynein plays a role in mammalian mitotic spindle formation. J Cell Biol. 1993;123:849–858. [PMC free article] [PubMed]
  • Bowman AB, Patel-King RS, Benashski SE, McCaffery JM, Goldstein LS, et al. Drosophila roadblock and Chlamydomonas LC7: A conserved family of dynein-associated proteins involved in axonal transport, flagellar motility, and mitosis. J Cell Biol. 1999;146:165–180. [PMC free article] [PubMed]
  • Nikulina K, Patel-King RS, Takebe S, Pfister KK, King SM. The Roadblock light chains are ubiquitous components of cytoplasmic dynein that form homo- and heterodimers. Cell Motil Cytoskeleton. 2004;57:233–245. [PubMed]
  • King SM, Dillman JF, 3rd, Benashski SE, Lye RJ, Patel-King RS, et al. The mouse t-complex-encoded protein Tctex-1 is a light chain of brain cytoplasmic dynein. J Biol Chem. 1996;271:32281–32287. [PubMed]
  • Salina D, Bodoor K, Eckley DM, Schroer TA, Rattner JB, et al. Cytoplasmic dynein as a facilitator of nuclear envelope breakdown. Cell. 2002;108:97–107. [PubMed]
  • Allan V. Protein phosphatase 1 regulates the cytoplasmic dynein-driven formation of endoplasmic reticulum networks in vitro. J Cell Biol. 1995;128:879–891. [PMC free article] [PubMed]
  • Presley JF, Cole NB, Schroer TA, Hirschberg K, Zaal KJ, et al. ER-to-Golgi transport visualized in living cells. Nature. 1997;389:81–85. [PubMed]
  • Starr DA, Han M. Role of ANC-1 in tethering nuclei to the actin cytoskeleton. Science. 2002;298:406–409. [PubMed]
  • Kanai M, Kume K, Miyahara K, Sakai K, Nakamura K, et al. Fission yeast MO25 protein is localized at SPB and septum and is essential for cell morphogenesis. EMBO J. 2005;24:3012–3025. [PMC free article] [PubMed]
  • Lizcano JM, Goransson O, Toth R, Deak M, Morrice NA, et al. LKB1 is a master kinase that activates 13 kinases of the AMPK subfamily, including MARK/PAR-1. EMBO J. 2004;23:833–843. [PMC free article] [PubMed]
  • Drewes G, Ebneth A, Preuss U, Mandelkow EM, Mandelkow E. MARK, a novel family of protein kinases that phosphorylate microtubule-associated proteins and trigger microtubule disruption. Cell. 1997;89:297–308. [PubMed]
  • Shulman JM, Benton R, St Johnston D. The Drosophila homolog of C. elegans PAR-1 organizes the oocyte cytoskeleton and directs oskar mRNA localization to the posterior pole. Cell. 2000;101:377–388. [PubMed]
  • Kusch J, Meyer A, Snyder MP, Barral Y. Microtubule capture by the cleavage apparatus is required for proper spindle positioning in yeast. Genes Dev. 2002;16:1627–1639. [PMC free article] [PubMed]
  • Guo S, Kemphues KJ. par-1, a gene required for establishing polarity in C. elegans embryos, encodes a putative Ser/Thr kinase that is asymmetrically distributed. Cell. 1995;81:611–620. [PubMed]
  • Cohen D, Brennwald PJ, Rodriguez-Boulan E, Musch A. Mammalian PAR-1 determines epithelial lumen polarity by organizing the microtubule cytoskeleton. J Cell Biol. 2004;164:717–727. [PMC free article] [PubMed]
  • Pecreaux J, Roper JC, Kruse K, Julicher F, Hyman AA, et al. Spindle oscillations during asymmetric cell division require a threshold number of active cortical force generators. Curr Biol. 2006;16:2111–2122. [PubMed]
  • Severson AF, Bowerman B. Myosin and the PAR proteins polarize microfilament-dependent forces that shape and position mitotic spindles in Caenorhabditis elegans. J Cell Biol. 2003;161:21–26. [PMC free article] [PubMed]
  • Derrien V, Couillault C, Franco M, Martineau S, Montcourrier P, et al. A conserved C-terminal domain of EFA6-family ARF6-guanine nucleotide exchange factors induces lengthening of microvilli-like membrane protrusions. J Cell Sci. 2002;115:2867–2879. [PubMed]
  • Franco M, Peters PJ, Boretto J, van Donselaar E, Neri A, et al. EFA6, a sec7 domain-containing exchange factor for ARF6, coordinates membrane recycling and actin cytoskeleton organization. EMBO J. 1999;18:1480–1491. [PMC free article] [PubMed]
  • Saito TT, Okuzaki D, Nojima H. Mcp5, a meiotic cell cortex protein, is required for nuclear movement mediated by dynein and microtubules in fission yeast. J Cell Biol. 2006;173:27–33. [PMC free article] [PubMed]
  • Heil-Chapdelaine RA, Oberle JR, Cooper JA. The cortical protein Num1p is essential for dynein-dependent interactions of microtubules with the cortex. J Cell Biol. 2000;151:1337–1344. [PMC free article] [PubMed]
  • Farkasovsky M, Kuntzel H. Cortical Num1p interacts with the dynein intermediate chain Pac11p and cytoplasmic microtubules in budding yeast. J Cell Biol. 2001;152:251–262. [PMC free article] [PubMed]
  • Schafer JC, Haycraft CJ, Thomas JH, Yoder BK, Swoboda P. XBX-1 encodes a dynein light intermediate chain required for retrograde intraflagellar transport and cilia assembly in Caenorhabditis elegans. Mol Biol Cell. 2003;14:2057–2070. [PMC free article] [PubMed]
  • Kini AR, Collins CA. Modulation of cytoplasmic dynein ATPase activity by the accessory subunits. Cell Motil Cytoskeleton. 2001;48:52–60. [PubMed]
  • Li MG, Serr M, Newman EA, Hays TS. The Drosophila tctex-1 light chain is dispensable for essential cytoplasmic dynein functions but is required during spermatid differentiation. Mol Biol Cell. 2004;15:3005–3014. [PMC free article] [PubMed]
  • Caggese C, Moschetti R, Ragone G, Barsanti P, Caizzi R. dtctex-1, the Drosophila melanogaster homolog of a putative murine t-complex distorter encoding a dynein light chain, is required for production of functional sperm. Mol Genet Genomics. 2001;265:436–444. [PubMed]
  • Rasband WS. ImageJ. Bethesda (Maryland): U.S. National Institutes of Health; 1997ENTITYSTART8211ENTITYEND2006. Available: http://rsb.info.nih.gov/ij/. Accessed 5 July 2007.
  • Cheeseman IM, Niessen S, Anderson S, Hyndman F, Yates JR, III, et al. A conserved protein network controls assembly of the outer kinetochore and its ability to sustain tension. Genes Dev. 2004;18:2255–2268. [PMC free article] [PubMed]
  • Praitis V, Casey E, Collar D, Austin J. Creation of low-copy integrated transgenic lines in Caenorhabditis elegans. Genetics. 2001;157:1217–1226. [PMC free article] [PubMed]

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