Transport and Turnover of Microtubules in Frog Neurons Depend on the Pattern of Axonal Growth

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The Journal of Neuroscience, February 1, 1998, 18(3):821-829

Transport and Turnover of Microtubules in Frog Neurons Depend on the Pattern of Axonal Growth
Sunghoe Chang¹, Vladimir I. Rodionov², Gary G. Borisy², and Sergey V. Popov¹
¹ Department of Physiology and Biophysics, University of Illinois at Chicago, Chicago, Illinois 60612, and ² Laboratory of Molecular Biology, University of Wisconsin, Madison, Wisconsin 53076

  ABSTRACT

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Abstract
Introduction
Materials & Methods
Results
Discussion
References

The transport of axonal microtubules in growing neurites has been a controversial issue because of clear but conflicting resultsobtained with fluorescence-marking techniques. We have attemptedto resolve the discordance via analysis of the relationship betweenapparent microtubule translocation and cell adhesion. Neuronalcultures were prepared from Xenopus embryos 1 d after injectionof Cy3-conjugated tubulin into one of the blastomeres of two-cell-stageembryos. Anterograde translocation of axonal microtubules wasobserved in neurons cultured on a laminin-coated surface, in agreementwith previously published data for Xenopus embryonic neurons.However, when neuronal cultures were prepared on a concanavalinA-treated surface, the axonal microtubules were stationary, asreported for all other neurons investigated previously. Neuronalcultures prepared on laminin- and concanavalin A-coated surfacesalso demonstrated dramatic differences in the pattern of axonalgrowth, dynamics of axonal microtubules, and response to brefeldinA treatment. Our findings suggest that transport and dynamicsof axonal microtubules may be directly affected by the mechanicaltension produced by growth cone activity.

Key words: tubulin; slow axonal transport; microtubules; photobleaching; neuronal cultures; mechanical tension

  INTRODUCTION

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Abstract
Introduction
Materials & Methods
Results
Discussion
References

A growing axon can be divided into two morphologically and functionally distinct domains, the growth cone and the axonal shaft.The actin-based growth cone is crucial for axonal growth and guidance,whereas the microtubule (MT)-based axonal shaft is specializedfor the transport of membrane and cytoskeletal components to thegrowing axon. The structural subunit of MTs, tubulin, is synthesizedin the soma and delivered to the growing axon by active transport.In early experiments using injection of radioactive amino acidsin the vicinity of neuronal cell bodies, labeled tubulin was foundto be transported in axons at a rate of 1-2 mm/d and could beobserved in the axoplasm as a coherent peak for a period of weeks(Hoffman and Lasek, 1975; Lasek and Hoffman, 1976; Black and Lasek,1980). Based on these experiments, it was suggested that tubulinis preassembled into microtubules in the cell body and transporteddown the axon in the form of MTs.

Strong evidence has been obtained both supporting and opposing the concept of transport of axonal MTs in preassembled form.The concept was most dramatically supported by the observationof anterograde vectorial movement of MTs in Xenopus neurites,as revealed by photoactivation (Reinch et al., 1991; Okabe andHirokawa, 1992) and photobleaching (Okabe and Hirokawa, 1993)techniques. Experimental evidence on the sites of MT nucleation(Baas and Joshi, 1992; Baas and Ahmad, 1993; Li and Black, 1996;Baas, 1997; Keating et al., 1997) and on the redistribution ofMTs from the cell body into distal axonal segments (Slaughteret al., 1997) is consistent with the idea that a significant populationof axonal MTs is transported down the axon in the assembled form.Conversely, photoactivation and photobleaching methods failedto detect a population of translocating MTs in the axons of sensoryneurons (Okabe and Hirokawa, 1990, 1992), pheochromocytoma (PC12)cells (Lim et al., 1990), Ti1 pioneer neurons in living grasshoppers(Sabry et al., 1995), and in living zebrafish (Takeda et al.,1995). These and other data (Bamburg et al., 1986; Funakoshi etal., 1996; Miller and Joshi, 1996) suggest that the majority ofaxonal tubulin is in the form of nontranslocating but dynamicMTs.

The conflicting results on the pattern of MT transport between Xenopus and the other neurons studied previously representa paradox needing investigation. In this paper, we show that thepattern of axonal growth as well as turnover rate and translocationof axonal MTs in growing Xenopus neurites depends on the cultureconditions. Taken together, our results suggest that criticalintrinsic aspects of axonal MT dynamics may be directly controlledby mechanical tension produced by the growth cone and by exogenousfactors such as attachment to the substrate.

  MATERIALS AND METHODS

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Abstract
Introduction
Materials & Methods
Results
Discussion
References

Preparation of Cy3-tubulin. MT protein was prepared from porcine brain by cycles of assembly and disassembly (Borisy et al.,1975). Labeling of porcine brain tubulin with Cy3 was performedas described previously (Keating et al., 1997). Details of Cy3-tubulinpreparation can be obtained from the Borisy Laboratory web site(http://borisy.bocklabs.wisc.edu). Before microinjection,a 10 µl aliquot of Cy3-tubulin was centrifuged at 15,000 × g for30 min at 4°C to remove particulate material and to reduce pipetteclogging and was stored on ice until the time of injection.

Microinjection of Cy3-tubulin into Xenopus embryos. Xenopus eggs were fertilized and dejellied in vitro as described previously(Popov and Poo, 1992). At the two cell stage, the eggs were injectedwith 10-25 nl of 10 mg/ml Cy3-tubulin using the air pressure injectorPicospritzer II (General Valve, Fairfield, NJ). The diameter ofthe pipettes used for injection ranged from 9 to 18 µm. Both injectionand subsequent incubation of injected embryos were performed in10% Ringer's solution (115 mM NaCl, 2 mM CaCl₂, 2.5 mM KCl, and10 mM HEPES, pH 7.6). The eggs were allowed to develop to stages19-24 and were then used for the preparation of neuronal cultures.

Cell cultures. Xenopus embryo neuronal cultures were prepared according to previously reported methods (Spitzer and Lamborghini,1976; Popov et al., 1993). Briefly, the neural tube of embryosat stages 19-24 was dissociated in Ca²⁺- and Mg²⁺-free solution (115 mM NaCl, 2.6 mM KCl, 10 mM HEPES, and 0.4mM EDTA, pH 7.6). Dissociated cells were plated on glass coverslipsprecoated with laminin (2-5 µg/cm²; GIBCO) or with Con A (0.1-1.0 µg/cm²; Sigma, St. Louis, MO). The cultures were kept at 20°C in a culturemedium consisting of 50% (v/v) Ringer's solution, 49% L-15 Leibovitzmedium (GIBCO), and 1% fetal bovine serum (GIBCO). The neuronswere used for experiments 6-36 hr after plating. In some experiments,neurotrophic growth factors neurotrophin 3 (NT-3), ciliary neurotrophicfactor (CNTF), and brain-derived neurotrophic factor (BDNF) (50ng/ml each) were added to the culture medium during cell culturepreparation. Brefeldin A (Sigma) was prepared as a 5 mg/ml stocksolution in methanol and stored at $-$ 20°C.

Photobleaching. The apparatus used for photobleaching has been described in detail previously (Gorbsky et al., 1987). Briefly,the beam of a 3 W argon ion laser (Spectra-Physics, Fremont, CA)was channeled into the epi-illumination system of a Carl ZeissIM-35 microscope. A 63×, 1.4 NA objective was used, and a cylindricallens was positioned to produce a focused 4 × 57 µm beam cross-sectionin the specimen plane. For the photobleaching experiments, thelaser was operated at 514 nm and 200 mW for 50-200 msec. Irradiationat this laser intensity does not disrupt MTs (Gorbsky et al.,1987; Rodionov et al., 1994; Keating et al., 1997).

Image acquisition and data analysis. A Zeiss IM-35-inverted microscope equipped with a 100 W mercury arc lamp was used forfluorescence microscopy. The light passed through ultraviolet-and infrared-blocking filters, neutral density filters, and arhodamine wide-band filter. A silicon-intensified target videocamera (Dage-MTI, Inc., Michigan City, IN) was used for focusing.Images were acquired with a charge-coupled device (CCD) camera(CH250; Photometrics, Tucson, AZ) driven by IPLab (Signal AnaliticsCorporation, Vienna, VA) imaging software. The CCD camera wasthermoelectrically cooled to $-$ 50°C to reduce the dark-currentnoise. Exposure time was 1 sec, and images were collected at 10-120sec intervals. Cells were kept at room temperature during photobleachingand observation. Images were processed with IPLab and Photoshop(Adobe Systems, Mountain View, CA). Quantitation of photobleachingdata were performed using IPLab software.

  RESULTS

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Abstract
Introduction
Materials & Methods
Results
Discussion
References

Microtubules translocate anterogradely in neurons plated on a laminin-coated surface

Cy3-conjugated tubulin was injected into one of the blastomeres of two-cell-stage Xenopus embryos. The embryos were allowedto develop for 1 d after injection, and then neuronal cultureswere prepared on laminin-coated coverslips. The first neuriteswere detected ~4 hr after plating. Although no data are availableon the differentiation of these neurites into axons and dendrites,all processes produced by Xenopus embryonic neurons in cultureare usually referred to as "axons" (Reinch et al., 1991; Okabeand Hirokawa, 1992; Popov et al., 1993), a term that we will usebelow. The average rate of axonal elongation for the period 6-16hr after plating was 49 ± 3 µm/hr (mean ± SEM; n = 54). Photobleachingexperiments were performed 6-36 hr after cell culture preparationon neurons containing fluorescently labeled MTs. A small zoneof axon was illuminated with a short (50-200 msec) flash of anargon laser, and the movement of the bleached segment was monitoredwith a cooled CCD camera. Figure 1 is an example of a typicalexperiment in which the bleached zone was placed ~40 µm behindthe growth cone. As reported previously for Xenopus neuronal culturesplated on surfaces coated with matrigel (Reinch et al., 1991)or laminin (Okabe and Hirokawa, 1992), the bleached zone rapidlymoved forward indicating anterograde vectorial movement of axonalMTs. The rate of bleached zone movement (48 µm/hr) was ~60% therate of growth cone advance (85 µm/hr). Fluorescence recoveryin the bleached zone was characteristically rapid, limiting theability to monitor its movement to 5-10 min. Thus, our resultsconfirm previous reports (Reinch et al., 1991; Okabe and Hirokawa,1992) that MTs in Xenopus neurons are transported toward the growthcone and are highly dynamic.

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Figure 1. Anterograde movement of photobleached MTs in an elongating Xenopus neurite growing on laminin-coated substrate. A-D, Fluorescentimages of a neurite captured after photobleaching. The photobleachingwas performed 16 hr after cell culture preparation. The bleachedsegment was at the distal (near the growth cone) axonal segment.Numbers indicate the time in minutes and seconds after the photobleachingpulse. The position of the center of the bleached zone is indicatedby arrows. The photobleached zone remained visible for ~6 min.Forward movement of the photobleached zone was clearly visibleduring the first few minutes after photobleaching. The rate ofbleached zone movement was ~48 µm/hr, and the rate of growth coneadvance was ~85 µm/hr. E, Fluorescence intensity profiles of anaxonal segment including the photobleached segment created fromimages A (15 sec after photobleaching, open circles) and C (8min and 15 sec after photobleaching, filled squares). The bottomof the fluorescence intensity profile (arrows) moved toward thedistal end of the neurite. Scale bars, 10 µm.

Microtubules are stationary in neurons plated on a concanavalin A-coated surface

The extension of Xenopus neurites on laminin- or matrigel-coated substrata is unusually fast with reported rates up to 200µm/hr and an average of ~50-80 µm/hr (Reinch et al., 1991; Okabeand Hirokawa, 1992; Popov et al., 1993). The fast axonal growthis likely to impose stringent demands on axonal transport systems.Therefore, it has been repeatedly suggested that the speed andcoherence of MT transport in Xenopus axons is likely to be greaterthan that of other neuronal types (Reinch et al., 1991; Sabryet al., 1995; Takeda et al., 1995; Baas, 1997; Slaughter et al.,1997). This may facilitate detection of MT transport by the photobleachingtechnique and explain why anterograde MT translocation was observedin Xenopus but not in other neuronal types. However, the growthpattern of Xenopus neurons on laminin-coated surfaces is ratherunusual. Neurites are poorly attached to the substrate, seem tobe under tension produced by the rapidly advancing growth cone,and decrease their diameter during axonal growth (Okabe and Hirokawa,1992; Popov et al., 1993). To examine whether the anterogradetranslocation of axonal MTs that we observed was dependent onadhesion of neurites to the substratum, we prepared cultures ofXenopus embryonic neurons on different surfaces, including cleanglass, poly-L-lysine, collagen, and concanavalin A (Con A). Therate of axonal growth under these culture conditions varied froma few micrometers per hour (clean glass) to ~30-40 µm/hr (ConA). For the reasons described above, we focused on rapidly growingneurites on Con A-coated coverslips. Under these culture conditions,the first neurites were detected ~4-6 hr after cell culture preparation.The average rate of axonal elongation for the period 6-16 hr afterplating was 31 ± 3 µm/hr (mean ± SEM; n = 39). Photobleachingexperiments were performed 8-36 hr after cell culture preparationon rapidly extending and relatively long (>500 µm in length) neurites.The optical system used for photobleaching and visualization ofthe bleached zone movement, as well as intensity of laser irradiationand duration of the laser flash, was identical to those used inexperiments performed on neurons growing on laminin-coated substrate.Figure 2 shows a typical example of a photobleaching experiment.During a 30 min period after photobleaching, the neurite elongatedby ~20 µm. The bleached zone was clearly visible for the durationof experiment. The position of the bleached zone remained constantrelative to the substrate throughout the experimental run, a conclusionsupported by analysis of the fluorescence profiles (Fig. 2E).We estimate that the accuracy of the measurement of position ofthe bleached zone was ~1 µm, and therefore the rate of the bleachedzone movement was <2 µm/hr.

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Figure 2. MTs remain stationary during axonal growth on Con A-coated substrate. A-D, Phase contrast (A, B) and fluorescent (C, D) imagesof a neurite 12 hr after cell culture preparation. The time afterphotobleaching is indicated in minutes and seconds in the topright corner of each panel. The bleached zone was clearly visibleduring the experiment (30 min). No obvious change in the positionof the bleached segment was observed. The neurite continued togrow and extended by ~20 µm. E, Fluorescence intensity profilesof an axonal segment including the photobleached segment createdfrom images C (20 sec after photobleaching, open circles) andD (30 min and 20 sec after photobleaching, filled squares). Thebottom of the fluorescence intensity profile (arrows) remainedstationary within experimental error (~1 µm). Scale bars, 10 µm.

Although some of the neurites on Con A-coated substrate grew rapidly (>60 µm/hr), the average rate of axonal elongation ona Con A-coated surface was significantly lower than that on laminin.To investigate whether the qualitatively different pattern ofMT translocation on laminin- and Con A-coated surfaces is directlyrelated to the difference in the rates of axonal growth, we repeatedthe photobleaching experiments on neurons plated on Con A-coatedsubstrate in the presence of a cocktail of neurotrophic growthfactors, NT-3, CNTF, and BDNF (50 ng/ml each), in the culturemedium. These neurotrophic factors are known to promote survivaland differentiation of Xenopus embryonic neurons in culture (Lohofet al., 1993; Stoop and Poo, 1995; Wang et al., 1995). In thepresence of neurotrophic factors, some of the neurites grew veryrapidly (>100 µm/hr) and 16 hr after plating exceeded 1100 µmin length. The average rate of axonal growth on Con A-coated substratewas significantly higher in the presence (57 ± 3 µm/hr, mean ±SEM; n = 57) than in the absence (31 ± 3 µm/hr, mean ± SEM; n= 39) of neurotrophins (p < 0.001, t test) and was similar tothe rate of axonal growth on laminin-coated substrate (49 ± 3µm/hr). Figure 3 shows an example of a photobleaching experimentperformed on a neurite growing rapidly in the presence of neurotrophinson a Con A-coated substrate. The length of the neurite was ~900µm. The photobleached zone was placed on the distal part of anaxon. No significant movement of the photobleached zone was observedthroughout the experimental run (Fig. 3C-E), although the axonelongated rapidly and the increase in axonal length was ~28 µmduring the 30 min observation period.

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Figure 3. MTs remain stationary in rapidly growing neurites plated on a Con A-coated surface in the presence of neurotrophic factors.A-D, Phase contrast (A, B) and fluorescent (C, D) images of aneurite growing in the presence of neurotrophic factors NT-3,BDNF, and CNTF (50 ng/ml each) in the culture medium. The photobleachingwas performed 18 hr after cell culture preparation. The time afterphotobleaching is indicated in minutes and seconds in the topright corner of each panel. The length of the neurite was ~900µm, and the rate of axonal growth was ~57 µm/hr. The photobleachedzone was clearly visible during the experiment (30 min) and remainedstationary within experimental error (~1 µm) (arrows in C andD). E, Fluorescence intensity profiles of an axonal segment includingthe pho-tobleached segment created from images C (20 sec afterphotobleaching, open circles) and D (30 min and 20 sec after photobleaching,filled squares). The bottom of the fluorescence intensity profile(arrows) remained stationary within experimental error (~1 µm).Scale bars, 10 µm.

Quantitative assessment of movement and fluorescence recovery of bleached zones

In total, we analyzed 18 photobleached zones in 15 neurites on a laminin-coated surface and 25 photobleached zones in 21 neuriteson a Con A-coated surface. The majority of the neurites (31 of36) were growing, and five were essentially stationary duringthe experimental run (typically 20-40 min). All neurites (includingthe stationary ones) were tipped with active growth cones. Neuriteschosen for photobleaching experiments grew with an average rateof 59 ± 7 µm/hr (mean ± SEM) and 32 ± 4 µm/hr (mean ± SEM) forlaminin- and Con A-coated substrata, respectively. In each experiment,we measured the rate of axonal elongation and the rate and directionof translocation of the center of the bleached segment, whichreflects net movement of tubulin polymer. In Figure 4, movementof bleached zones relative to the substrate is plotted againstaxonal growth rate. In all neurites growing on laminin-coatedsubstrate, anterograde movement of the bleached zone was observed(Fig. 4A). In general, the rate of MT movement was somewhat smallerthan that of axonal growth. The average rate of bleached zonemovement was 32 ± 5 µm/hr (mean ± SEM; n = 18). In one case (markedby an arrow), we observed rapid anterograde movement of MTs ina stationary neurite. In neurites growing on Con A-coated substrate(Fig. 4B), the bleached zones were stationary within experimentalerror regardless of the rate of axonal growth. The average rateof bleached zone movement was 0.0 ± 0.5 µm/hr (mean ± SEM; n =25), suggesting that the majority of axonal MTs in neurites growingon Con A-coated substrate are primarily stationary.

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Figure 4. Quantitative assessment of the movement of bleached zones. The rate of the movement of the center of the bleached zone relativeto the substrate is plotted as a function of neurite elongationrate. A, Neurites growing on laminin-coated substrate. The averagerate of neurite extension was 59 ± 7 µm/hr (mean ± SEM; n = 18).The bleached zone was located at the distal axonal segment (opencircles) and at the proximal segment (filled squares) in 11 and7 experiments, respectively. The average rate of bleached zonemovement was 32 ± 5 µm/hr (mean ± SEM). In each experiment, theaccuracy of the measurements of the positions of growth cone andbleached zone was ~1 µm. Detection of the MT translocation ratewas more accurate for neurites with relatively stable MTs (slowfluorescence recovery). Generally the bleached zone could be reliablytraced for a period of 10-20 min, and therefore the accuracy ofthe measurements was ~3-6 µm/hr. In seven experiments, we werenot able to measure reliably the rate of bleached zone movement.In two of these seven cases, the bleached zone was visible onlyfor a few minutes (t_1/2 of ~3 min), precluding accurate measurementsof the MT movement. In the remaining five cases, the lateral movementof the whole axonal structure was very fast, and the measurementsof the bleached zone position were meaningless. Results of theseseven experiments have been excluded from the analysis of MT movement.B, Neurites growing on Con A-coated substrate; summary of 25 differentexperiments. In five experiments (filled triangles), neurotrophicfactors NT-3, BDNF, and CNTF (50 ng/ml each) were added to theculture medium during cell culture preparation and were presentthroughout the experiment. No neurotrophic factors were addedto the culture medium in the remaining 20 experiments (open circles).The bleached zone was at the distal axonal segment in 18 experimentsand at the proximal segment in seven experiments. In the absenceof NT-3 in the culture medium, the average rate of axonal growthand the rate of bleached zone movement were 25.6 ± 3.7 and $-$ 0.4± 0.5 µm/hr, respectively (mean ± SEM; n = 20). In the presenceof NT-3, the rates of axonal growth and the bleached zone movementwere 55 ± 8 and 1.4 ± 1.2 µm/hr, respectively (mean ± SEM; n =5). The position of the bleached zone could be measured with anaccuracy of ~1 µm. Typically the movement of the bleached zonewas followed for 30-60 min. Therefore we estimate the accuracyof the measurements of the MT movement rate to be ~1-2 µm/hr.

To investigate the dynamics of axonal MTs in growing neurites, we measured the half-time of fluorescence recovery of the bleachedsegment (t_1/2), usually considered an indicator of MT turnoverrate (Okabe and Hirokawa, 1990; Edson et al., 1993). Both forlaminin- and Con A-coated substrata, the data were divided intotwo categories: (1) activation of distal axonal segments (within100 µm of the growth cone) and (2) activation of proximal segments(>300 µm from the growth cone). For the neurites growing on laminin,t_1/2 values were 21.5 ± 4.0 min (mean ± SEM; n = 7) and 9.7± 2.7 min (n = 11) for the proximal and distal axonal segments,respectively. On Con A-coated substrate, t_1/2 values were86.7 ± 16.3 min (n = 7) and 60.0 ± 5.4 min (n = 18) for the proximaland distal segments, respectively (Fig. 5). Both for distal andproximal segments, recovery of fluorescence after photobleachingwas approximately fivefold faster in neurites plated on laminin-coatedsubstrate than in those growing on Con A (p < 0.001, t test),suggesting significantly slower turnover of axonal MTs on ConA-treated substrate. In agreement with previously published data(Edson et al., 1993), recovery of photobleaching in the distalaxonal segments was significantly faster than that in the proximalsegments (p < 0.05, t test) for neuronal cultures plated on eitherlaminin or Con A, indicating slower MT turnover rates in the proximalaxonal segments. However, it should be noted that the apparentfaster rate of MT turnover in neurites growing on laminin maybe related to asynchronous translocation of MTs relative to eachother (see Discussion).

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Figure 5. Quantitative analysis of the fluorescence recovery in the bleached zones. Experiments were performed as described in Figures1-3. The bleached zones were at the proximal (black bars) or distal(hatched bars) axonal segments. In each experiment, the averagetime for 50% recovery of fluorescence (t_1/2) was calculated.For neuronal cultures growing on either laminin- or Con A-coatedsubstrate, t_1/2 values were significantly higher at the proximalsegments compared with the distal segments. Recovery of fluorescencewas approximately fivefold faster (smaller t_1/2 values) inneurites growing on laminin-coated compared with those growingon Con A-coated substrate.

In summary, axonal MTs in neurites growing on laminin- or Con A-coated substrate differ both qualitatively and quantitativelyin the pattern of their movement. In neurites growing on laminin-coatedsubstrate, MTs rapidly translocate forward with a rate comparablewith that of axonal elongation and seem to be highly dynamic.In neurites growing on Con A-coated substrate, MTs are significantlymore stable and stationary regardless of the axonal growth rate.The observed differences in the MT movement were not related tothe different axonal lengths or rates of axonal growth on thetwo substrata.

Differential pattern of axonal growth on laminin- and Con A-treated substrata

To determine whether differential behavior of axonal MTs on laminin- and Con A-coated surfaces may be related to the differentpatterns of axonal growth, we characterized the morphology ofneuronal cells on both substrata. Both on laminin- or Con A-coatedsurfaces, neurons projected long neurites tipped with highly activegrowth cones. On both surfaces, the neurites grew rapidly. Inagreement with previously published data (Reinch et al., 1991;Okabe and Hirokawa, 1992; Popov et al., 1993), we found that ona laminin-coated surface the neurites are often straight and attachedto the substrate only at the growth cone region. The attachmentsalong the axonal shaft, if any, are transient and readily disruptedduring neurite extension. In the cases in which the neurites wereattached to the substrate along their length, the shape of theaxon was changing constantly, and the position of the branchingpoints was not fixed either in relation to the substrate or inrelation to the neurite. At the later stages of growth, the neuriteswere visibly thinner than they were at the initial stages of growth,indicating stretching of the whole axonal structure (Okabe andHirokawa, 1992; Popov et al., 1993). In vitro growth rates ofthese neurons are a few fold higher than are the growth ratesof the same neurons in vivo (Jacobson and Huang, 1985).

On the contrary, when plated on a Con A-coated surface, the axons were firmly attached to the substrate. During neurite elongation,the proximal segments did not change their position relative tothe substrate, and axonal diameter did not change noticeably.The position of the branch points and the distance between thebranch points also did not change. Furthermore, the distance betweenindividual filopodia-like processes formed along the axonal shaftalso remained constant (Fig. 6, see also Figs. 2, 3). Neitherthe pattern of axonal growth on Con A-coated substrate nor axonalmorphology were affected by the presence of neurotrophic factorsin the culture medium (data not shown). The relatively stableposition of the proximal axonal segments and branch points inrelation to the substrate during axonal growth is routinely observedboth in vitro (Lim et al., 1990; Craig et al., 1995) and in vivo(Sabry et al., 1995; Takeda et al., 1995) and is likely to bea general feature of axonal growth mediated by growth cone activity.

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Figure 6. Axonal growth on Con A-coated substrate. A, B, DIC images of neurites growing on Con A-coated substrate. The image B was taken2 hr and 15 min after image A. Notice the constant position ofthe axon, branch point, and filopodia-like processes (arrows)relative to the substrate. Scale bar, 20 µm.

Differential dependence on the supply of new membrane

To study how axonal elongation in neuronal cultures plated on laminin- and Con A-coated surfaces depends on the supply ofnew membrane material synthesized in the cell body, we treatedthe cultures with Brefeldin A, a drug that blocks membrane trafficthrough the Golgi complex (Lippincott-Schwartz et al., 1989, 1990).A typical response of neurites growing on a Con A-coated substrateis illustrated in Figure 7A. After Brefeldin A (BFA) application,elongation of the neurite slowed within a few minutes, and thegrowth cone retracted within 12 min (Fig. 7A). In total, we followedthe growth of 16 neurites on Con A-coated substrate after BrefeldinA treatment. Within 1 hr after Brefeldin A application, the advanceof 14 of the 16 neurites almost completely stopped. In the twoinstances in which axonal growth persisted for >1 hr after BrefeldinA treatment, the neurites became visibly thinner (data not shown).In contrast, growth continued on laminin although at a somewhatreduced rate (Fig. 7B,C). None of the 20 neurites investigatedstopped elongating within 1 hr of the treatment. Axonal elongationon laminin-coated surfaces continued for a period of up to 8 hrwith an average duration of 275 ± 30 min (mean ± SEM). To characterizequantitatively the effects of BFA on axonal growth, we plottedthe rate of axonal growth as a function of time after the onsetof BFA application (Fig. 8). The rate of axonal elongation onCon A decreased twofold ~7 min after BFA application, and thegrowth almost completely terminated in ~60 min (Fig. 8A). Therate of axonal growth on laminin-coated substrate slowed afterBFA application and decreased twofold ~90 min after the startof BFA treatment (Fig. 8B). However, axonal elongation continuedfor a period of up to 8 hr.

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Figure 7. Effect of Brefeldin A treatment on axonal growth. A, DIC images of a neurite growing on Con A-coated substrate. Numbers indicatetime in minutes. Brefeldin A (10 µg/ml) was applied 16 min afterthe start of an experiment. Elongation of the neurite after BFAapplication visibly slowed down, and the growth cone retractedwithin 12 min after drug treatment (28 min after the start ofexperiment). B, C, Neurite growth on laminin-coated substrateafter Brefeldin A treatment. B, Phase contrast images of a neurite.Numbers indicate time in minutes after Brefeldin A (10 µg/ml)application. Axonal growth continues for at least 3 hr after drugtreatment. C, Quantitative analysis of axonal elongation; datafrom B. The growth cone position relative to the substrate isplotted in 20 min intervals (open circles). The average directionof axonal growth is indicated by a big arrow. The growth coneelongation appears to slow down within 80 min after applicationof BFA. Approximately 5 hr after drug application, the growthcone retracts. However, elongation resumed and continued for ~80min, after which the neurite retracted. Scale bars: A, 10 µm;B, C, 40 µm.

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Figure 8. Quantitative analysis of the effects of BFA on axonal growth on Con A-coated (A) and laminin-coated (B) surfaces. In eachexperiment, the average rate of axonal growth before BFA application(10 µg/ml) was determined for a period of 20-30 min. The rateof axonal elongation was measured as a function of time afterthe onset of BFA application and was normalized to that beforeBFA application. Each point represents the mean ± SEM of 14 (A)and 20 (B) different experiments. For neurites growing on ConA-coated substrate in 2 of 16 experiments, we observed a decreasein axonal diameter a few minutes after BFA application. Theseneurites continued to grow for at least 2 hr and became progressivelythinner. They were excluded from the analysis.

  DISCUSSION

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Abstract
Introduction
Materials & Methods
Results
Discussion
References

Formation and maintenance of axonal MTs depend on the transport of tubulin from the cell body to the axon. The structuralhypothesis of slow axonal transport holds that tubulin moves downthe axon in the form of MTs (Hoffman and Lasek, 1975; Lasek andHoffman, 1976; Baas, 1997). A seemingly direct way to test thishypothesis is to create a reference mark on the MTs by photobleachingor photoactivation and to determine whether the mark moves. Experimentsin various types of neuronal cells demonstrated that most axonalMTs are primarily stationary. However, in striking contrast tothese observations, rapid translocation of axonal MTs down theneurite at the rate of slow axonal transport was observed in Xenopusembryonic neurons (Reinch et al., 1991). It has been repeatedlyargued that because of the high rate of axonal growth, MT transportin Xenopus neurites may be more robust and easily detectable comparedwith that in other neuronal types. Do Xenopus embryonic neuronsreally possess a uniquely efficient system for MT transport? Resolutionof this problem is important for our understanding of the mechanismsof slow axonal transport.

Axonal growth on laminin- and Con A-coated substrata

Our results as well as previous studies (Okabe and Hirokawa, 1992; Popov et al., 1993) clearly demonstrate that Xenopus neuriteselongating on laminin are attached to the substrate primarilyat the soma and the growth cone region and become visibly thinnerduring elongation. Axonal elongation cannot rely on stretchingalone for a considerable period of time and must be supportedby a supply of new membrane from the soma. Previous quantitativeanalysis of the anterograde flow of plasma membrane lipids inXenopus neurites indicated that new membrane necessary for growthis inserted along the axons as well as at the soma (Popov et al.,1993). Therefore, elongation of Xenopus axons on laminin can beconsidered a combination of true axonal growth, which dependson the supply of new membrane, and stretching of the axon. Thismodel predicts that axonal elongation would continue for sometime (although probably at a slower rate) even in conditions whendelivery of Golgi-derived vesicles to the axon is inhibited. Resultsof our experiments with BFA are totally consistent with this prediction(Figs. 7B,C, 8B). On the contrary, neurites growing on Con A-treatedcoverslips are firmly attached to the substrate and seem to growby a more conventional mechanism, common to other neuronal types.Their growth depends on the supply of new membrane from the soma,similar to other neurons (Martenson et al., 1993; Dai and Sheetz,1995; Futerman and Banker, 1996).

Microtubule transport on laminin- and Con A-coated substrata

Our results obtained in Xenopus neurons plated on laminin-coated surfaces are in full agreement with previous reports on theanterograde movement of axonal MTs in these neurons using photobleachingor photoactivation techniques (Reinch et al., 1991; Okabe andHirokawa, 1992, 1993). Briefly, transport of axonal MTs in Xenopusneurites differed from other neuronal cell types in a few importantrespects. (1) MTs seemed to translocate anterogradely en bloc,(2) no stationary population of MTs was observed, and (3) therate of MT transport correlated with the rate of axonal growthand increased with increasing distance from the soma. One factorthat may directly contribute to the anterograde movement of MTsis poor adhesion of neurites growing on laminin to the substrate.In agreement with this hypothesis, when neuronal cultures wereprepared on Con A-coated substrate, the MTs were primarily stationary,similar to reports on the stationary nature of axonal MTs in otherneuronal types. The only difference between the series of experimentsperformed on Xenopus neurites plated on laminin- and Con A-coatedsubstrata was the nature of the substrate. All other parameterssuch as preparation of fluorescently tagged tubulin, loading oftubulin into neurons, and parameters of the optical system usedfor photobleaching and observation of MT dynamics were identical.Therefore it is likely that the differences observed in the movementof the bleached segment in neuronal cultures prepared on two differentsubstrata reflect a differential mode of MT movement under theseculture conditions, rather than an experimental artifact suchas photodamage of MTs. The simplest explanation of our data isthat anterograde translocation of axonal microtubules in Xenopusneurites growing on laminin is a direct consequence of axonalstretching and is not related to the activity of the slow axonaltransport system. The stretching of the axon, combined with aprogressive decrease in axonal diameter, is sufficient to explainthe most striking features of MT behavior on the laminin-coatedsubstrate, specifically, the translocation of MTs relative tothe substrate and the absence of a stationary population of MTs.The degree of axonal stretching is dictated by the mechanicaltension produced by the growth cone (see below) and by the attachmentof the axonal shaft to the substrate. The relatively poor correlationbetween the rates of axonal elongation and MT movement (Fig. 4)is likely to be related to the frequent changes in the patternof axonal adhesion to the substrate.

The lack of bleached zone movement in neurites growing on a Con A-coated substrate indicates that axonal MTs in Xenopus neuritesare primarily stationary regardless of axonal growth rate (Fig.4). However, a small fraction of transported MTs can escape detection,especially if movement of these MTs is asynchronous. Quantitativeanalysis of the fluorescence profiles after photoactivation demonstratedthat it is impossible to detect a moving population of MTs thatrepresents 10% or less of the MTs at a given axonal region (Sabryet al., 1995). Therefore, negative results obtained with the photobleachingmethod in our experiments on Xenopus neurons growing on Con A,as well as in a variety of other neuronal cells, do not excludethe possibility that a small fraction of tubulin is transportedin the form of MTs (Ahmad and Baas, 1995; Moritz et al., 1995;Zheng et al., 1995; Keating et al., 1997). However, these resultsimpose an upper limit on the size of this fraction.

Control of microtubule movement and dynamics by mechanical tension

Mechanical tension is an important intrinsic regulator of axonal growth and development. A case in point is de novo initiationand elongation of pre-existing neurites by experimentally appliedmechanical tension (Bray, 1984; Zheng et al., 1991), "towed" axonalgrowth. In this experimental paradigm, the rate of axonal elongationis proportional to the magnitude of mechanical tension (Lamoureuxet al., 1989), suggesting regulation of MT transport and assemblyby mechanical tension. Transport of tubulin has not been studiedin detail in these neurites. However, because large membrane-attachedparticles translocate forward during the experimental towed-growthregime (Zheng et al., 1991), it is likely that the whole neurite,including axonal MTs, is towed forward by the experimentally appliedmechanical force (Okabe and Hirokawa, 1992). Interestingly, theMT array observed in tension-induced neurites is similar to thatin neurites extending by growth cone activity and requires newMT assembly (Zheng et al., 1993). Therefore, it seems that MTtransport in this system is a combination of conventional slowaxonal transport and anterograde movement induced by stretching.Mechanically, the pattern of Xenopus axonal growth on a laminin-coatedsubstrate is identical to that of neurites growing in responseto experimentally applied mechanical tension (Bray, 1984; Zhenget al., 1991) and is likely to occur by a similar mechanism (Tanakaet al., 1995).

We observed about a fivefold difference in the rate of fluorescence recovery of the bleached zone between neurites growingon laminin and Con A. It is generally believed that the rate offluorescence recovery reflects MT turnover rate. How can thisintrinsic property of MTs be affected by an extrinsic factor,such as culture substrate? During elongation of Xenopus neuriteson laminin, mechanical force applied to the growth cone is notbalanced by the adhesion of the axonal shaft to the substrateand transduced to the proximal axonal segments. The mechanicaltension along the axonal shaft may directly affect dynamics ofaxonal MTs. The long-range transduction of cytomechanical forcesfrom the growth cone to proximal axonal regions may also affectother aspects of axonal mechanics and transport. However, it shouldbe noted that asynchronous movement of MTs relative to each othermay contribute to fluorescence recovery of the bleached zone aswell. Although this MT transport is not related to the turnoverof MTs per se, it will lead to a faster rate of fluorescence recoveryof the bleached zone.

In conditions in which neurites are firmly attached to the substrate, mechanical tension produced by the growth cone is balancedby the sufficiently strong attachment of neurites to the substrate.It remains to be established whether the long-range signalingbetween plasma membrane and cytoskeletal elements observed innon-neuronal cells (Ingber, 1997; Maniotis et al., 1997) occursin axons. However, it is tempting to speculate that mechanicaltension may serve as a general regulator of other aspects of axonalgrowth, such as axonal transport, addition of new membrane tothe growing neurite, and local assembly and disassembly dynamicsof axonal MTs.

  FOOTNOTES

Received Aug. 28, 1997; revised Oct. 23, 1997; accepted Nov. 6, 1997.

This work was supported by National Institutes of Health Grants NS 33570 to S.V.P. and GM 25062 to G.G.B. We also thank RegeneronPharmaceuticals, Inc. for generously providing NT-3, BDNF, andCNTF. We are grateful to John Peloquin for preparation of labeledtubulin and to Steve Limbach for maintenance of the digital fluorescenceand laser photobleaching system. We thank Primal de Lanerolle,Elly Tanaka, and Mark Rasenick for helpful discussion and comments.
Correspondence should be addressed to Dr. Sergey V. Popov, Department of Physiology and Biophysics (M/C 901), University ofIllinois at Chicago, 835 South Wolcott Avenue, Chicago, IL 60612.

  REFERENCES

Top
Abstract
Introduction
Materials & Methods
Results
Discussion
References

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