A Dual Role for Actin and Microtubule Cytoskeleton in the Transport of Golgi Units from the Nurse Cells to the Oocyte Across Ring Canals

Emmanuelle Nicolas^*, Nicolas Chenouard, Jean-Christophe Olivo-Marin, and Antoine Guichet^*

*Morphogenesis and Polarity Unit, Institut Jacques Monod, 75005 Paris, France; and Quantitative Image Analysis Unit, Institut Pasteur, 75724 Paris, France

Submitted April 8, 2008; Revised October 27, 2008; Accepted October 30, 2008
Monitoring Editor: Vivek Malhotra

ABSTRACT

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Axis specification during Drosophila embryonic development requirestransfer of maternal components during oogenesis from nursecells (NCs) into the oocyte through cytoplasmic bridges. Wefound that the asymmetrical distribution of Golgi, between nursecells and the oocyte, is sustained by an active transport process.We have characterized actin basket structures that asymmetricallycap the NC side of Ring canals (RCs) connecting the oocyte.Our results suggest that these actin baskets structurally supporttransport mechanisms of RC transit. In addition, our trackinganalysis indicates that Golgi are actively transported to theoocyte rather than diffusing. We observed that RC transit ismicrotubule-based and mediated at least by dynein. Finally,we show that actin networks may be involved in RC crossing througha myosin II step process, as well as in dispatching Golgi unitsinside the oocyte subcompartments.

INTRODUCTION

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Throughout the animal kingdom, germ cells commonly develop aspart of syncytia in which cytoplasmic canals connect sistercells. Intercellular bridges represent specific types of cellularcontacts that allow the flow of cytoplasm to be shared amongsister cells in order to synchronize their division, differentiation,or hormone release (see for review Robinson and Cooley, 1996).These intercellular communications between adjacent cells arecommonly found in the developing male and female germline ofdiverse species: in mammal ovaries, in insects and mammaliansspermatocytes as well as in plants, Caenorhabditis elegans,or mammalsomatic lineages (see for review Robinson and Cooley,1996). The intercellular bridges in Drosophila oogenesis arebetter characterized and have a slightly different role thanin the male germline: it allows the transfer of maternal components,including key mRNAs that encode axis-determining proteins, intothe oocyte to support the subsequent development of the embryo.Additionally, oocyte growth also requires a supply of plasmamembrane that is provided by the secretion pathway (Janusckheet al., 2007). Thus, we were interested in understanding howmembrane trafficking occurs and how it is regulated during Drosophilaoogenesis.

A Drosophila egg chamber is composed of 16 germline cells encapsulatedby somatically derived follicle cells (Brown and King, 1964).This cyst of 16 germ cells is formed when cystocytes undergofour rounds of cell division without fully completing cytokinesis,giving rise to cells interconnected by cytoplasmic bridges.As development proceeds, these cytoplasmic connections are modifiedinto stable ones, ring canals (RCs). A RC is made up of twoparts: a layer of circumferentially oriented F-actin–richfilaments that form the inner rim and a thickening of the plasmamembrane, originally derived from the arrested cleavage furrowforming the outer rim (Hime et al., 1996).

Among these 16 cells, only one differentiates into a matureoocyte, whereas the other 15 become polyploïd cells callednurse cells (NCs). The Drosophila oocyte is transcriptionallyinactive throughout much of oogenesis, therefore the majorityof nutrients (mRNA, proteins, and organelles) required for itsdevelopment are synthesized in the NC and transported into theoocyte through the RC in a slow process of cytoplasmic transfer(Clark et al., 2007; Theurkauf and Hazelrigg, 1998). A key questionconcerns the mechanism by which this cytoplasmic transport isachieved. There is growing evidence for the importance of microtubule(MT) cytoskeleton and its associated motor proteins, kinesin(Brendza et al., 2002; Januschke et al., 2002) and dynein (Chaet al., 2002; Clark et al., 2007, Januschke et al., 2002) inactive transport of organelles (Januschke et al., 2007). Lessis known concerning the role of the actin cytoskeleton and itsassociated proteins during this process. However, studies haveshown the involvement of myosins in the transport of vesicles/organellesin vertebrates neurons (DePina and Langford, 1999) and the transientassociation of MyoVI with mitochondria during their RC transitin the Drosophila egg chamber (Bohrmann and Schill, 1997), suggestinga role for the actin network in organelle transport.

The mechanism of cellular organelle transport through RCs remainspoorly understood. It is not known for instance how the selectionof what gets into the oocyte occurs or whether the secretionpathway sustains it by means of specific motors and cytoskeletaltracks. To address this issue, we focused on the regulationof transport of Golgi units from NCs to the oocyte. In mammaliancells, Golgi is a discrete organelle that contains dozens ofstacked cisternae linked together by tubules which form a singlelarge structure capping the nucleus (Mellman and Warren, 2000).In Drosophila, the Golgi apparatus does not always exhibit amorphology of stacked cisternae. But, when stacks are present,they do not form a single copy organelle. Instead, they remainscattered throughout the cytoplasm (Kondylis and Rabouille,2003; Herpers and Rabouille, 2004), an organization that issimilar to that in yeast (Rossanese et al., 1999). Whateverthe morphology of the Golgi apparatus, they are in proximityto tER sites (trans-endoplasmic reticulum). The resulting structure(one tERsite and one Golgi complex) is called tER-Golgi unit(Kondylis and Rabouille, 2003).

To understand the regulation of cytoplasmic transport of Golgito the oocyte through RCs, we have analyzed the movement ofparticles expressing a Golgi marker, in living Drosophila eggchambers. We show that they are actively transported to theRCs, where they accumulate before a subset transits throughthe cytoplasmic bridges at a much slower speed. Mechanisms oftransport through RCs seem to be structurally sustained by thepresence of an asymmetric basket-like actin structure cappingthe NC side of RCs. In addition, we show that MTs are requiredfor the integrity of these baskets and that the transport towardand through RCs is dynein- and MyoII-dependant.

MATERIALS AND METHODS

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Fly Stocks
w¹¹¹⁸ was used as wild type, GalT (A. Debec, Institut JacquesMonod, Paris, France) as a Golgi marker (Januschke et al., 2007),Rab6-GFP (Januschke et al., 2002), Ph-GFP (L. Gervais InstitutJacques Monod) to visualize plasma membrane and tub-GFP-Dmn/CyOto visualize MTs. Overexpression of dynamitin was performedas described previously in Januschke et al. (2002), with thefollowing stocks: tub-gal4/UAS-hDmn. Germline clones were generatedby FRT/FLP-mediated recombination (Chou and Perrimon, 1992)by crossing y w sqh¹ sn³ FRT101/FM7 females to ovoD1, FRT101/Y;hs-flipF38 males. Twenty-four-hour pulses of egg were allowedto develop to second or early third instar larvae before a 2-hheat shock at 37°C.

Immunostaining of Whole Mount Egg Chambers
Egg chambers were dissected in phosphate-buffered saline (PBS)–0.,1%Triton X-100 and fixed in 4% paraformaldehyde (PFA) in PBS.Primary antibody staining was performed overnight at 4°C.To visualize the actin basket, egg chambers were fixed as describedabove and incubated 1 h 30 min in a 1/20 rhodamine-conjugatedphalloïdin (Molecular Probes, Eugene, OR) dilution andsubsequently imaged on a spinning-disk confocal microscope.Green fluorescent protein (GFP)-expressing strains were fixed5 min in 4% PFA if no additional antibody staining was requiredand imaged either on a spinning-disk confocal microscope oran Apotome system. Image J (http://rsbweb.nih.gov/ij/) and Photoshop(Adobe Photosystems, San Jose, CA) were used to process images.

Time-Lapse Imaging
To keep egg chambers alive during several hours, we used a POCchamber system (Leica, Deerfield, IL). Living egg chambers wereseparated form each other directly on a coverslip in a 15-µldrop of M3 medium supplemented with 2% fetal bovine serum (FBS,Sigma, St. Louis, MO), 0.24 µl insulin (Sigma), 0.01 µg/mljuvenile hormone (Sigma), and 50 µg/ml penicillin/streptomycinsolution (Sigma). To prevent evaporation, samples were coveredby a special FoilCover (Leica), which is gas permeable CultFoil.Time-lapse videomicroscopy was performed with an inverted spinning-diskconfocal microscope CSU 10 (Perkin Elmer-Cetus, Norwalk, CT)connected to a Coolsnap HQL camera (Photometrics, Tucson, AZ)with a 40x/1.25 NA or a 63x/1.4 NA objective lens. To followparticles that moved along the Z-axis, three Z-positions wereselected at each time point, with a step size of 0.5 µm.Given that 4D visualization is not possible yet, trails of particleswere generated by a Z-projection. Speed of particles is shownas average speed ± SE.

Particle Tracking in a Noisy Biological Environment
A dedicated program was developed to detect and track fluorescentlylabeled Golgi particles visualized in 3D with a spinning diskmicroscope. Spot detection was performed automatically by amultiresolution algorithm based on wavelet decomposition ofthe image, correlation analysis ofwavelet coefficients, andthresholding the output binary masks for each detected object(Olivo-Marin, 2002). Once particles have been detected in theimage sequences, a Bayesian tracking algorithm is used to linkthem. Associations between existing tracks and detections ata given time were selected on the basis of the maximizationof their kinetic likelihood. This likelihood was computed usingthe Interacting Multiple Model (Genovesio et al., 2006) estimatorthat makes an adaptive weighted mixture of three models of motion:Brownian motion, directed motion, and curvilinear motion. Becausethe weights of these models are automatically updated, changesin type of motion are automatically taken into account. Onceall the tracks were determined, motions of particles in theovocyte and the ring canal were characterized by their meanSDs and velocities.

Inhibitor Treatment
Colchicine. Flies were fed with colchicines as described in Januschke etal. (2002).

Latrunculin B. Directly after dissection in PBS + 0.1% Triton X-100, egg chamberswere incubated for 5 min in 150 mM or 300 mM latrunculin B (LatB;Sigma) and fixed 20 min in 4% PFA. Stainings were subsequentlyperformed as described in the Immunostaining of Whole MountEgg Chambers. For live imaging, the drug was diluted in M3 medium+hormones (see Time Lapse Imaging) and washed away after 5 minof incubation. For live imaging, we worked at a 150 mM concentrationto prevent chambers from blowing up as soon as the permeablemembrane was in contact with them.

RESULTS

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Golgi Units Are Asymmetrically Distributed within the Drosophila Egg Chamber
Unlike mammalian cells in which Golgi units are found closeto the nucleus, Drosophila egg chambers present Golgi dispersedboth throughout the NC and the oocyte cytoplasm (Herpers andRabouille, 2004). Its correct distribution is essential forthe proper development of the oocyte (Januschke et al., 2007;Coutelis and Ephrussi, 2007), but the process controlling thetransport of Golgi to the oocyte has not been addressed. Toinvestigate the way the subcellular distribution of Golgi iscontrolled, we took advantage of a GFP-trap strain, GalT (Morinet al., 2001), in which a GFP-tag is inserted into a gene encodingUDP galactosyl:beta-N-acetylglucosamine beta-1,3-galactosyltransferase,a resident enzyme of Golgi stacks in mammals (Elhammer and Kornfeld1984). In Drosophila, this protein copurifies with Golgi fractionsand colocalizes with Golgi markers (Janushcke et al., 2007).We chose to focus our analysis on stages 7-10A, before cytoplasmicstreaming occurs (Gutzeit, 1986). During these developmentalsteps, transport of proteins and lipids to the plasma membraneare required for subsequent oocyte growth, presumably involvingGolgi stacks and secretion vesicles to ensure the process.

We observed that, during the early phases of development, eventhough dispersed throughout NCs and oocyte cytoplasm, Golgiunits were present with a much higher density in the oocyteas shown in Figure 1, B–D. Indeed, we observed that GalT-containingdots gradually accumulated in the oocyte as development progressed.First, at stage 6, the Golgi was found evenly distributed betweenNCs and the oocyte (data not shown), but as soon as the nucleusmigrated to the anteroposterior region of the oocyte (stage7), the Golgi started to accumulate in the oocyte (Figure 1B).At stage 8 it was distributed throughout the entire oocyte,although less abundantly at the anterior margin (Figure 1C).Finally, by stage 10, GalT-containing vesicles were uniformlyscattered within the oocyte (Figure 1D). We interpreted theaccumulation of the Golgi in the oocyte as an indication ofactive transport of Golgi into the oocyte against a concentrationgradient. In Drosophila egg chamber, the Golgi is observed inclose vicinity of ER-exit sites and forms functional units called"tER-Golgi units" (Kondylis and Rabouille, 2003; Herpers andRabouille, 2004). To discriminate the transport that we werefollowing, either Golgi vesicles or tER-Golgi units, we performeda double labeling with a dCOG5-GFP transgene, which labels ER-exitsites (Herpers and Rabouille, 2004), and a lectin wheat germagglutinin (WGA), which distribution is similar to GalT (Januschkeet al., 2007). We observed that 45% of the WGA signal is associatedwith the dCOG5 labeling, either at the vicinity or inside RCs(Supplemental Figure S1), indicating that whole tER-Golgi unitswere transported into the oocyte. The WGA signal that did notcolocalize with dCOG5 may correspond to membrane vesicles thathave left the tER-Golgi units. In the this article, we willuse the term "Golgi units" when referring to tER-Golgi units.

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Figure 1. Asymmetrical distribution of Golgi units between NC and the oocyte. (A) Actin distribution at the plasma membrane cortex and in ring canals (RCs) connecting adjacent nurse cells (NCs) or between NCs and the oocyte (Oo). (B–D) Golgi units labeled with galT-GFP gradually accumulate in the oocyte from stage 7 to stage10 egg chambers. Scale bars, 38 µm.

Golgi Units Are Transported toward and through the RCs in a Three-Step Process
To elucidate the Golgi unit transport mechanism from the NCto the oocyte, we studied their movement at both high magnificationand time resolution in living egg chambers using a spinningdisk confocal microscope. Speed measure of Golgi units allowedus to demonstrate sequential events and distinct mechanismsof transport during RC approach and crossing. We used a computerprogram for automated 4D tracking of fluorescent particles,which allows the quantification of intracellular movements ofvesicles relative to the mass center of the cell nucleus (seeMaterials and Methods). First, in the NC cytoplasm, we observedtwo categories of movements (Figure 2A): 1) "random" movementsconsisting of sequences of discrete zigzag steps, previouslydescribed as Brownian movement (Doob, 1957

); 2) linear and rapidmovements interrupted from time to time by short stops or backwardshifts, trajectories that would be compatible with directedtransport along cytoskeleton tracks (Figure 2A, yellow arrow).Among these linear paths, we focused on a subset heading towardthe oocyte and more specifically to the RC (Figure 2, B, yellowarrow, E, left part of the panel, and E', AT; Supplemental MovieS1). We managed to track Golgi units moving toward RCs and calculatedan average velocity of 0.190 ± 0.024 µm/s duringRC approach.

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Figure 2. Golgi units move in a direct path toward and across the oocyte. (A–D) Trails of Golgi units were obtained by superimposing time-lapse snapshots taken every 5 s, during approximately 2 min. (A and C) and 9 min (D). (A) In NCs, Golgi units exhibited either Brownian movements (labeled as B) or directional trajectories (yellow arrow). (B) Trail of a Golgi unit approaching the RC (yellow arrow). Others linger at the RC front (red line). Blue stars point to the RC rims. (C) Transit of Golgi units across the RCs. (D) Golgi units leaving the RCs. Scale bar, 9 µm. n = number of egg chambers; p = number of Golgi units. (E-E'') Tracks of Golgi units while approaching and transiting across an RC were calculated by a computer program (see Material and methods). (E) Trajectories of Golgi units were recorded during 15 min. Snapshots were taken at 6-s intervals. Arrival, pausing, and crossing are shown together with a different color for each tracked particle. GalT cortical accumulation (delineated in green) highlights the RC rims. NC, nurse cell; Oo, oocyte. (E') A close- up of the RC entrance showing four trajectories selected in E. AT, Golgi units actively transported toward the RC; B, Golgi units pausing at the RC entrance. They exhibited short back-and-forth movements, presumably Brownian movements. (E'') Close-up at the RC crossing. Time-point calculation and trajectory analysis suggest that Golgi units are either actively transported AT or transit to the oocyte by successive Brownian and directed movements AT+B. (F) Graph of Golgi unit velocity during RC transit. Time point 0 corresponds to the RC entrance. Time point 10 corresponds to the RC exit. According to their location within the RC, Golgi units exhibited speed differences during RC transit. In the center (blue line) they crossed the RC with a constant speed, and when close to the rim (pink line), they exhibited acceleration and deceleration phases.

In front of the RCs, no subsequent direct translocation intothe oocyte was observed; instead, Golgi units paused and clusteredat the RC entrance (Figure 2B, red bracket). This second stepwas characterized by short Brownian movements (Figure 2E', Blabel). Then in a third step, a subset of Golgi units detachedfrom lingering clusters and translocated through RC into theoocyte (Figure 2, C and E''), suggesting that the transit throughRCs might be selective. Indeed, we scored only 17% of the Golgiunits arriving at the RCs transiting through them (see SupplementalMovie S1: eight particles crossed out of 47 that were lingeringoutside the RC). Interestingly, speed calculation revealed aswitch from fast motion during the approach (0.190 ±0.024 µm/s) to slower movement during RC transit (0.110± 0.026 µm/s), suggesting that different molecularmotors might be required for RC approach and transit. To furthercharacterize RC crossing, trajectories and speed parametersfor each Golgi units were calculated at each time point (Figure 2,E–E''; Supplemental Movie S2). It enabled us to distinguishtwo types of directional trajectories during RC transit dependingon where Golgi units crossed (Figure 2E''). Transit in the middleof the RC exhibited straight trajectories (Figure 2E'', AT label)and a continuous motion (Figure 2F, blue line), which are featuresof active transport. On the other hand Golgi units crossingclose to the canal rim displayed more complex trajectories ofacceleration and short stops together (Figure 2F, pink line),with slight deflections from linear (Figure 2E'', AT+B label),suggesting sequences of successive Brownian movements and activemotion. Finally, Golgi, units that managed to get into the oocyteleft the RC vicinity with a slow motion along straight trajectories(Figure 2D).

Altogether these data suggest that Golgi units are transportedin a three-step process into the oocyte through RCs, characterizedby a switch from fast motion during approach, to a slow movementduring RC transit, interrupted in between by a pause at theRC entrance. In addition, we pointed out a selective processthat sort out Golgi units in front of RC.

A Basket-like Actin Structure Associated with RCs
To gain insight into the regulation of cytoplasmic transportfrom NCs to the oocyte, we analyzed the detailed structure ofRCs themselves. These bridges, interconnecting either NCs orlinking NCs with the oocyte (Figure 1A), are derived from thecontractile rings of the incomplete cytokinesis that characterizescystocyte mitosis (Riparbelli and Callaini, 1995). To labelRCs, we used rhodamine-conjugated phalloidin, which mainly stainsthe inner rim (Tilney et al., 1996). These canals consist ofa layer of circumferentially oriented actin filaments, the innerrim and an outer region containing subcortical actin filamentsforming a crown radiating from the inner rim (Figure 3A). Thisouter domain is attached to a thickening of the plasma membrane(Tilney et al., 1996; see review Robinson and Cooley, 1996),as shown by a double labeling with actin and pleckstrin homologydomain of the phospholipase C fused to GFP (Ph-GFP) that specificallylabels the plasma membrane (Varnai and Balla, 1998; Figure 3,B and C). Under the standard staining protocol, cytoplasmicactin filament bundles are weakly stained. However, we wereable to detect actin cytoplasmic structures composed of bundlesof filaments that extended in the NC cytoplasm from the externalmargin of the outer rim. They had an overall shape like a conicalbasket (Figure 3, D and E) asymmetrically distributed on theNC side of the RCs, connecting the oocyte with its four neighboringNCs. Such actin baskets were also observed on RCs connectingadjacent NCs (Figure 3, F and F'), with the difference thatthey were present on both sides of the RCs. The asymmetricalactin baskets were detected from stages 6–7, and graduallyincreased in size until stage 9–10, in term of lengthand number of filaments. By stage 10B, its identification wasmade difficult by the appearance of cytoplasmic actin filamentbundles radiating from the plasma membrane, which preventedthe nucleus to physically block RCs during the dumping process(Guild et al., 1997). The identification of this actin basketbetween NCs and the oocyte raised the possibility that thisasymmetrical structure might have a function at the RC entrance.

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Figure 3. An actin-based structure capping RCs. (A–C) RCs are composed of an inner rim (In), which corresponds to bundles of actin filaments organized into a ring, and an outer rim (Ou) containing actin filaments that radiate from the inner rim. (C) This crown of actin filaments is embedded in a thickening of the plasma membrane as shown by the double-labeling with a membrane marker, PH-GFP. Although these actin baskets are asymmetrically present on the NC side of the four RC connecting the oocyte (D and E), they cap both sides of RC that connect neighboring NC (F and F'). Ba, actin basket; In, inner rim; Ou, outer rim. Scale bar, 8 µm. (G) Diagram of an actin basket–like structure capping a RC.

Actin Network and MyoII Are Involved in the RC Crossing Efficiency and the Golgi Redistribution within the Egg Chamber
In the Drosophila egg chamber, there are at least three setsof actin filaments in the NCs: a subcortical layer associatedwith the cortical region of NC membrane, actin filaments liningthe RCs and a network of cytoplasmic actin bundles that extendin the cytoplasm (Guild et al., 1997

). Because actin filamentsare involved in the maintenance of the Golgi structure (seefor review Egea et al., 2006

), we asked whether the actin networkcould also be involved specifically in the transport of Golgiunits from the NCs to the oocyte in Drosophila egg chambers.We chose to focus on myosins, because they have been found tobe involved in the transport and steady-state localization ofcytoplasmic particles or organelles in several systems (Mermallet al., 1994

, Bohrmann and Schill, 1997

). At first, we observedthe expression of a sqh-GFP construct in the RCs (Figure 4A).The spaghetti squash (sqh) gene encodes the regulatory lightchain of nonmuscle myosin II (MyoII) without which myosin isnonfunctional (Karess et al., 1991

). Then, to assess the requirementfor MyoII in the Golgi units cytoplasmic transport, we inducedhomozygous germline clones of the hypomorphic mutation sqh¹.In 14% (n = 65) of sqh¹ egg chambers, movements were detected:Brownian motion in 7% of the chambers and directional trajectoriesin the other 7% (see Table 2). However present, rectilineartrajectories toward RCs were slowed down by a factor 4 in asqh¹ mutant background (0.052 ± 0.010 µm/s) comparedwith wild type (wt; 0.190 ± 0.024 µm/s; Table 1),suggesting a role of MyoII in the Golgi unit transport to RCs.Interestingly, at the RC vicinity, we noticed an abnormal lingeringof the Golgi units along filaments of the actin baskets. Indeed,the transient pause observed in wt egg chambers lasted muchlonger in sqh mutants (data not shown). This observation gaveus a first hint of the MyoII requirement during RC transit.Consistently, we also noticed an unusual accumulation of Golgiunits clusters either in front of the RCs (23%; Figure 4B) orinside the RCs (18%; Figure 4C; Table 2), which reinforced thehypothesis for which MyoII may be required during RC transit.However, transport of Golgi units to the oocyte did not seemto be completely abolished in the absence of MyoII. Indeed,the Golgi gradient was still present in sqh mutants (Figure 4B).In fact, speed calculation pointed out a fourfold slower motionthan in a wt context (0.023 ± 0.002 vs. 0.110 ±0.026 µm/s in wt). This remaining activity favors thehypothesis for which it is a complex of molecular motors thataccount for the transit process, rather than a single partner.Finally, we noticed as previously reported by Jordan and Karess(1997)

, a delay in oocyte growth (Figure 4, D compared withE, wt). In sqh background, the size of the oocyte was reducedin stage 10A egg chamber (borders cells contact the anteriormargin, Figure 4, D and E, yellow arrowhead). This phenotypemay reflect a defect in membrane trafficking across RC. Altogether,these sets of data suggest that actin filaments network maycontribute to RC transit through MyoII activity.

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Figure 4. Actin network is involved in RC crossing and in Golgi unit redistribution within the oocyte. (A) MyoII is present in the RC inner rim. (B and C) Snapshots of sqh ovoD living egg chambers. Golgi units cluster at the RC entrance (B) or are clogged inside the RC (C). (D and E) The development of the oocyte is frequently delayed in sqh mutants (D), compared with wt (E): the oocyte is much smaller in sqh mutant egg chambers, whereas the border cells have already reached the anterior margin (white arrowhead). n, number of egg chambers; p, number of Golgi units. Scale bars, (A)6 µm; (B, C, and D–G') 38 µm. (F–G') Snapshots of one time point of wt (F and F') or LatB-treated (G and G') living egg chambers. (G–G', arrowhead) Upon actin filaments depolymerization, Golgi units cluster at the RC exit. Scale bars, 6 µm.

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Table 1. Velocity of Golgi unit transport in control, UAS-Dmn–overexpressing, and sqh living egg chambers

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Table 2. Quantification of defects in control, UAS-Dmn–overexpressing, and sqh living egg chambers

Next, we analyzed Golgi units trajectories in the presence ofLatB, an inhibitor of actin filament assembly (Spector et al.,1983

). In extreme cases, in which no cortical actin remained,treatment with LatB eliminated all particle movements (datanot shown). In less affected egg chambers with partial disassemblyof the actin scaffold, some Golgi units still managed to reachthe RC vicinity. However, they did not accumulate in front ofthe RCs (Figure 4, G and G'), which correlates well with thedisappearance of the actin basket in 100% of the chambers (datanot shown) and its putative role as a selective barrier. Onthe other hand, we observed in four of six LatB-treated eggchambers a large cluster of Golgi units at the RC exit (Figure 4,G and G', arrowhead) compared with wt (Figure 4, F and F').These observations suggest that an actin-dependent process mightbe involved in dispatching Golgi units to the oocyte subcellularcompartments where they are required. This is also consistentwith data from other systems implicating actin networks in aspectsof vesicle sorting and distribution (Lantz et al., 1998

; seefor review Buss et al., 2002

; Rogers and Gelfand, 2000

Microtubules Inhibitors Prevent Golgi Transportation to the Oocyte and Disassemble the RC Actin Baskets
Given that MTs are required for subcellular localization ofseveral mRNAs and Rab6 transport (Theurkauf and Hazelrigg 1998;Clark et al., 2007; Januschke et al., 2007), we next checkedwhether they could also be involved in the cytoplasmic transportof Golgi units. MTs are enriched at the RC entrance (Griederand Hazelrigg, 2000; Moon and Hazelrigg, 2004; Clark et al.,2007; Mische et al., 2007). They concentrate and converge towardthe cytoplasmic bridges (Figure 5, A and B), and some extendthrough them (Figure 5B), suggesting that MTs might serve astracks along which Golgi units could be towed.

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Figure 5. Alteration of Golgi unit transport toward and through RCs upon MTs depletion. (A) MTs are visualized with a ${alpha}$ tub84-GFP or (B) a Dmn-GFP construct (green). Phalloidin (red) labels actin at the RCs and at the plasma membrane cortex. MTs converge toward RCs. Some seem to extend through it. Arrowheads point to the RC hedges (A). Scale bar, 40 µm. (C and D) MT depletion upon colchicine treatment (D) induces the redistribution of Golgi units between NCs and the oocyte as well as their clustering in big aggregates compared with untreated (C). Scale bar, 40 µm. (E–H') Successive snapshots taken at different time intervals in colchicine-treated living egg chambers. (E–H) Entrance: in the absence of MTs, Golgi units lying at RC vicinity enter the oocyte with a straight trajectory and at a constant and slow velocity, suggesting a switch from active transport to diffusion between NC and the oocyte. (E'–F') Exit. Unidirectional transport is abolished in absence of MTs network. Golgi units can now leave the oocyte. n, number of chambers; p, number of particles. Scale bar, 6 µm. (I–J) Fixed preparations of wt and colchicine-treated egg chambers. When the MTs network is impaired, actin baskets are not present anymore. Scale bar, 6 µm.

To address this question, we first depolymerized MTs by a colchicinetreatment (Janusckhe et al., 2002

). We particularly focusedon chambers in which the nucleus was mislocalized in the oocytecentral region, a consequence of MTs depolymerization (Kochand Spitzer, 1982

). This displacement served as an internalcontrol (Figure 5D). In these egg chambers, Golgi units formedclusters that were scattered throughout NCs and the oocyte cytoplasm(Figure 5, D compared with C, the untreated egg chamber). Inaddition, colchicine treatment abolished Golgi units accumulationat the RC entrance as well as fast directional movements, indicatingthat transport of Golgi units toward RCs along straight pathsis MT dependent. Moreover, in colchicine-treated egg chambers,the gradient of Golgi units was not present anymore; instead,Golgi units were equally distributed between the NCs and theoocyte (Figure 5D), suggesting that MTs may also be requiredfor active transport of Golgi units through RCs. Even thoughno direct transport toward the RCs occurred, we observed thatas soon as a cluster of Golgi units happened to be close tothe RCs, it was able to get into the oocyte with a differenttrajectory and velocity than in untreated conditions (Figure 5,E–H; 0.160 ± 0.020 vs. 0.194 ± 0.024 µm/sin wt; Supplemental Movie S4). No pause or selection was observed.Instead, trajectories were straight, with a constant velocityas if clusters of Golgi units were dumped in the oocyte. Importantly,we also observed clusters leaving the oocyte back toward theNCs (Figure 5E'–H'; 0.080 ± 0.018 µm/s (n= 7); Supplemental Movie S5). They moved more slowly than thoseentering the oocyte, suggesting that an MT-independent transportmechanism toward the oocyte may still remain. Altogether, theserecords suggest that active transport was switched to free exchangesbetween both compartments, which would then imply that nothingmaintained the gradient at the RCs anymore. Indeed, a closelook at the RCs after colchicine treatment confirmed that theactin baskets were no longer present at the RC entrance (Figure 5,J compared with I), suggesting that actin baskets may also playthe role of physical barriers to prevent any outflow from theoocyte.

Dynein Is Required for Golgi Unit Transport from the NCs to the Oocyte
To obtain further evidence for MTs involvement in RC transit,we sought to interfere with the MT function by blocking dynein,a minus-end–directed MT motor involved in the mRNA transportfrom the NC to the oocyte (Januschke et al., 2002; Tekotte andDavis, 2002; Duncan and Warrior, 2002; Bullock et al., 2006;Clark et al., 2007). Because null alleles of dynein heavy-chain(dhc) mutation compromise oocyte development (McGrail et al.,1995, 1997), we chose to disrupt dynein activity indirectlyby overexpressing the dynactin subunit, dynamitin (Dmn; Burkhardtet al., 1997; Duncan and Warrior, 2002; Januschke et al., 2002).In these egg chambers, the Golgi units organized into big clusters(Figure 6, B and C, white arrow) compared with wt chambers (Figure 6A),which is consistent with a role for dynein in Golgi subcellularorganization. First, we observed that the gradient of Golgiunits between the NCs and the oocyte was always conserved whendynein activity was impaired (n = 20), as well as the presenceof the actin basket (Supplemental Figure S2). Second, in chambersin which movements were not totally abolished (10 of 20 scored),we mainly observed Golgi units manifesting Brownian movements.Directional trajectories were detected in 15% of the chambers(Table 2), but the Golgi unit's velocity was substantially reduced,(0.114 ± 0.033 vs. 0.190 ± 0.024 µm/s inwt; Table 1). These results suggest that dynein actively transportsGolgi units toward RC.

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Figure 6. Dynein is required for RC crossing of Golgi units. Snapshot at one time point of wt (A) and UAS-Dmn–overexpressing (mimicking dynein loss-of-function) living egg chambers. (A'–C') Close-ups of the above pictures. (B and B') When dynein function is impaired, Golgi units cluster (white arrowhead) and accumulate in front of RCs. Most of them do not managed to cross. (C–C') However, in extreme cases, some do cross as long stretches. Those stretches manage to get to the RC exit, but with a much slower motion than in wt chambers. Scale bars, 10 µm. n, number of chambers; p, number of particles. (D–E) Distribution of MTs at the vicinity of the RC-capping actin baskets. MTs are visualized with a Dmn-GFP construct (green) and actin by a phalloidin labeling (red). A subpopulation of MTs run parallel to the actin basket filaments (D–D'', white arrowhead), whereas others connect directly to the inner rim (E–E'') or to actin filaments of the basket (D–D'', red arrowhead).

Next, we had a closer look at RC transit in egg chambers inwhich Golgi units still exhibited directional movements (Figure 6,C and C'; Supplemental Movie S6). In the absence of functionaldynein, translocation through RCs was about fourfold slowerthan in control chambers (0.025 ± 0.007 vs. 0.110 ±0.026 µm/s in wt). In extreme cases, either clusters accumulatedin front of the RCs (25%; Table 2) without crossing or did notmanaged to disassemble as soon as RC transit started (10%; Table 2;Figure 6, C and C'). Instead, they formed some sort of filamentsthat stretched out from one side of the canal to the other,before they reached the oocyte and retracted. These resultssuggest that dynein participates in the active translocationof Golgi units through RCs along MTs.

To visualize MTs in the vicinity of actin baskets, we took advantageof a transgenic strain expressing moderately a Dmn-GFP fusionprotein that decorates the MTs without perturbing the transport(Januschke et al., 2002). Labeling of both MTs and actin networksrevealed that MTs come very close to the actin baskets (Figure 6,D–E'') and could be divided into at least three populations:1) MTs running parallel to the actin filaments of the basket(see white arrowheads in Figure 6, D–D''); 2) MTs connectingeither the filaments of actin baskets (see red arrowheads inFigure 6, D–D'') or the ring itself (Figure 6, E–E'');and 3) MTs coming directly from NC cytoplasm and passing throughthe RCs as shown in Figure 5B (and mentioned by Grieder et al.,2000). Altogether, these observations suggest that each MT subgroupmight be involved specifically in different steps of the Golgitransport from the NCs to the oocyte.

DISCUSSION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

In this study, we have described the first live visualizationof the transport of Golgi units through RCs into the Drosophilaoocyte. We carried out a detailed analysis with high-resolutiontime-lapse images and functional disruption approaches thatprovided new aspects required for transport from the NC to theoocyte. We have characterized an asymmetric basket-like actinstructure capping the NC side of the four RC that connect theoocyte with its neighboring NC. We have shown that Golgi unitsare actively transported to the oocyte instead of diffusing.They move in a direct path toward the RCs where they accumulatebefore a subset transits to the oocyte. We propose that theactin baskets structurally support the Golgi units pause atthe RC entrance. We show that partial loss of either dyneinor MyoII activity reduces velocity of Golgi units, which isconsistent with a MT/actin-dependent transport from the NCsto the oocyte.

Identification of an Asymmetric Actin Basket at the RCs Connecting the NCs with the Oocyte
We have characterized a new actin structure capping every RCpresent in the Drosophila egg chamber, overall shape of whichlooks like a conical basket. These actin baskets are presenton both sides of the RCs connecting adjacent NCs but are asymmetricallydistributed on the NC side of the RCs connecting the oocytewith its four neighboring NCs. We showed that these actin basketsare sensitive to MTs depolymerization and brefeldin A treatment(E. Nicolas, personal communication). It suggests that eitherMTs may serve as a scaffold that helps maintaining the basketstructure or that MTs may sustain the addition of proteins orcomponents that participate in the anchoring or maintenanceof the actin baskets at the RC surface.

Golgi Units Transport from NCs to Oocyte Can Be Divided into Three Distinct Steps
Altogether, our observations led us to propose the followingworking model for the NC to oocyte transport (Figure 7). PanelA shows the RC approach: Golgi units associated with the dyneinmotors complex and MyoII are actively transported along MTsand actin filaments toward the RCs. Panel B shows the pause:At the RC entrance, Golgi units pause along the filaments ofthe actin baskets that decorate the NC side of the RCs. We hypothesizethat they might dissociate or/and associate with different motorsand regulators, allowing them to switch onto a second groupof MTs that cross the canal. We propose that this step enablesa specific selection of Golgi units that can get into the oocyteto prevent any occasional accidents such as direct crossingof organelles. However, the presence of MTs coming from theNC lumen and entering directly into the RC suggests that someparticles might be able to directly transit to the oocyte. Thesespecific particles might be already hooked onto the "crossing"partners. Panel C shows the RC Transit: Once associated withthe right partners, Golgi units transit through the RC. Ourdata show that dynein and MyoII are required for RC crossing.Panel D shows the distribution: Once at the RC exit side, vesiclesmay be transferred onto a third population of MTs in order tobe distributed to the subcompartments where they are required.The presence of large clusters of Golgi units at the RC exitupon LatB treatment supports the actin network role in the redistributionof secretory vesicles within the oocyte, which is consistentwith other data showing functional interactions of actin andMT networks (Lantz et al., 1998, Buss et al., 2002).

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Figure 7. Working model for Golgi units transport across RCs. Cross section of an RC is shown, capped by an actin basket (orange). Left (green) is the NC side, and right (light orange) is the oocyte (Oo). (A) Approach. Black lines are MTs and red lines are filaments of the actin network. Green circles, Golgi units; blue circles, dynein motor complex; and pink circles, MyoII. These two motors contribute to Golgi units transport toward RC. (B) Pause. Once at the RC entrance, Golgi units pause in order to associate with the right motors for transit. (C) Transit. Dynein and MyoII contribute to RC crossing, though MyoII to a lesser extend. (D) Distribution. Once in the oocyte, Golgi units redistribution onto new MTs is actin network mediated.

Actin Baskets Participates in the Transport Mechanism through RCs
The presence of actin baskets at the RC entrance led us to proposethat active transport toward the oocyte might be structurallysupported by these baskets for three reasons. 1) We observed,in living egg chambers, Golgi units organized in transient filament-likestructures that colocalize with actin baskets. 2) Upon colchicineor LatB treatment, the absence of actin baskets correlates withno net accumulation of Golgi units in front of the RC and withbidirectional RC transit (colchicine treatment only). Thesetwo observations led us to speculate that actin baskets might"force" Golgi units to pause. This stop could provide the opportunityto change motor complex composition in order to modulate parametersof RC transit. Thus, actin baskets may function as platformsupon which specific Golgi units recruit specific motors andpartners that ultimately direct them to the oocyte. 3) In sqhclones, Golgi units linger much longer on the actin basket filamentsand, in extreme cases, cluster in front of the RCs. 4) Finally,these baskets may also serve as physical barriers preventingoutflow from the oocyte, thus assuring the maintenance of thegradient as shown by the observation of Golgi units gettingout of the oocyte in colchicine-treated egg chambers.

Approach and RCs Transit Are Two Specific Processes
This study provides the following evidence for different transportmechanisms sustaining RCs approach and RCs transit: 1) Dynamicsspecificity. Vesicles arrive much more quickly (1.7-fold greater)at the RCs than they do to cross it. The association to differentmotors and/or regulators could explain this difference (Bullocket al., 2006). 2) Trajectory specificity. Although Golgi unitsexhibit straight trajectories to reach the RC entrance, transitpath characteristics depend on where the crossing occurs insidethe RCs. In the center, linear tracks correspond to active transport,whereas on the edges, Golgi units are constantly switching fromBrownian motion to active transport. 3) Velocity specificity.Transport in NCs is rapid. In contrast, Golgi units movementis significantly slower once they transit into the RCs. Thisindicates that motor dependent movement is down-regulated asGolgi units cross the RCs.

Transport of Golgi Units Is Dynein and MyoII mediated
We observed that transport of Golgi units toward and throughthe RC is colchicine sensitive. It is reduced in NCs and evenmore dramatically impaired during RC transit when dynein, aminus-end–directed motor, also known to associate withmembranes of the trans-Golgi network (Matanis et al., 2002),is absent. These observations indicate an MT-dependent mechanismfor Golgi units transport to the oocyte. In addition, we highlightedthe presence of at least three different groups of MTs relativeto their localization at the actin basket and RC vicinity. Wepropose that they may be specifically involved in the differentsteps of RC approach and transit. Indeed, MacDougal et al.,2003 have suggested that accessory factors are required to specifythe MTs subset along which dynein-mediated transport occurs.We also identified MyoII as a motor required for transport duringRC approach as well as RC transit. Surprisingly, the reductionof Sqh activity seems to have a stronger effect on Golgi unitvelocity than on the impairment of dynein activity. One canhypothesize that, in UAS-Dmn–overexpressing egg chambers,the remaining activity of dynein may be higher than what isleft of Sqh function in sqh clones. Overall, our results showthat both MTs and actin networks contribute to the regulationof Golgi units transport, as we showed that disruption of eitherMTs or actin motors impaired Golgi units transport. Comparisonof motility toward RCs and during RC transit in both mutantbackgrounds suggests that at least both dynein and MyoII arerequired, given that the absence of a single one does not completelystop the traffic. It would be interesting to determine whattheir contribution is and how it is differentially regulatedin order to better understand the cross-talk between actin filamentsand MTs. Investigating the role of cytoskeletal linkers suchas Short stop, will be interesting, given that shot mutant eggchambers have a similar phenotype to dynein associated proteinsEgalitarian and Bicaudal B (Röper and Brown, 2003, 2004).In this study, we show that Golgi units as for mRNA such asgrk (Clark et al., 2007), bcd (Mische et al., 2007), or hairy(Bullock et al., 2006), depend on dynein for transport fromNCs to the oocyte. Interestingly, the average velocity of mRNAis faster than the transport of Golgi units (1.45 ± 0.087µm/s (Clark et al., 2007) vs. 0.190 ± 0.024 µm/s,toward RC) and 0.25 ± 0.036 µm/s (Clark et al.,2007) vs. 0.110 ± 0.026 µm/s, through RCs). Thisdiscrepancy of a factor 7 and 2, respectively, suggests thatalthough a dynein-based transport is conserved, their motorpartners and/or regulators may differ. Indeed, recent observationssuggest that 1) dynein may be associated with motors of oppositepolarity, like kinesin I that acts as an antagonist of dyneinmediated-transport of Exu RNP complexes (Mische et al., 2007);and 2) cooperativity of multiple motors can regulate force andvelocity of motor complexes (Kural et al., 2005; Mallik et al.,2005; Levi et al., 2006). Thus, regulation of opposing motorsmay provide the means to control velocity of Golgi units duringthe different steps of their journey to the oocyte. Furtherexperiments will be required to characterize these specificpartners.

ACKNOWLEDGMENTS

We thank T. Piolot and C. Chamot for their technical help forimages and time-lapse acquisitions. We thank Jean-RenéHuynh, Roger Caress, and Véronique Brodu for their commentson the manuscript. This work was supported by ACI "Biologiecellulaire," "Jeune Chercheur" Grant 035117, and ANR "Blanche"(Cymempol, Grant Blan06-3-139786).

Footnotes

This was published online ahead of print in MBC in Press(http://www.molbiolcell.org/cgi/doi/10.1091/mbc.E08-04-0360)on November 12, 2008.

Address correspondence to: Emmanuelle Nicolas (nicolas{at}ijm.jussieu.fr) or Antoine Guichet (guichet{at}ijm.jussieu.fr)

Abbreviations used: MT, microtubule; NC, nurse cell; RC, ring canals.

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