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Vol. 9, Issue 7, 1617-1626, July 1998
*Cell Biology and Metabolism Branch,National Institute of
Neurologicial Disorders and Stroke, National Institutes of Health,
Bethesda, Maryland 20892
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INTRODUCTION |
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Top
Introduction
References
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The organization and function of the Golgi complex has intrigued
cell biologists for many years (Farquhar and Palade, 1998
; Mazzarello
and Bentaivoglio, 1998). This is due both to the Golgi's central role
in secretory membrane traffic and sorting, and to its unique structure
and dynamics. The Golgi complex receives newly synthesized proteins and
lipid from the ER, covalently modifies them, and then repackages them
for delivery to plasma membrane, lysosomes, or secretory granules. It
also recycles membrane components back to the ER for continued use.
These diverse functions depend on small membrane-bound transport
intermediates that shuttle protein into and out of the Golgi's stack
of flattened cisternae and associated tubules and vesicles. Such
transport intermediates regulate protein and membrane flux into and out
of the Golgi complex and thereby control the steady-state size and
location of this organelle. In so doing, they ensure the proper
functioning of the Golgi complex, enabling the cell to tailor its
biosynthetic and secretory products for specific cellular needs.
The emergence of green fluorescent protein (GFP) technology has enabled
proteins to be visualized in the unperturbed environment of the living
cell (Chalfie et al., 1994). This allows direct observation
of intracellular structures, whose life history and pathways previously
have only been deduced. In the movies shown below, membrane proteins
fused to GFP were used to visualize the dynamics of the Golgi complex
and the transport intermediates that shuttle membrane proteins into and
out of this organelle. Included are time-lapse sequences that show the
formation, translocation, and fate of Golgi-targeted/ derived transport
intermediates. Also shown are movies revealing how the
distribution/morphology of the Golgi complex is affected when such
processes are perturbed. In addition, results of photobleaching
experiments characterizing the lateral mobility of proteins residing
within the Golgi complex are presented. These movies demonstrate the
dynamic, steady-state nature of the Golgi complex and provide insight
into the tubule-vesicular carriers that mediate membrane flow into and
out of this organelle.
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VIDEO MOVIES |
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Movie 1: Formation and Life History of ER-to-Golgi Transport Intermediates
The ts045 vesicular stomatis viral G (VSVG) protein misfolds
and is retained in the ER at 40°C and upon shift to 32°C moves as a
synchronous population to the Golgi complex before being transported to
the plasma membrane (Bergmann, 1989). These properties of VSVG are
preserved upon addition of GFP to the cytoplasmic tail of the protein,
allowing detailed analysis of the morphological characteristics of
ER-to-Golgi transport to be visualized in living cells (Presley
et al., 1997; Scales et al., 1997). Movie 1 (from Presley et al., 1997) (Figure 1) shows confocal images
acquired at 8.6-s time intervals after shift from 40 to 32°C in COS
cells expressing VSVG-GFP. Note that
within seconds of temperature shift, ER-localized VSVG-GFP became
concentrated within bright, fluorescent pre-Golgi intermediates that
were widely distributed at ER sites scattered throughout the cytoplasm.
Pre-Golgi structures never appeared to arise at the same site as
previous ones, which suggested they formed de novo from dynamically
generated nonfixed ER sites. Once formed, the pre-Golgi structures had
only a finite lifetime and quickly translocated as units through the
cytoplasm to the Golgi complex with no loss of fluorescent material.
During transport, the pre-Golgi intermediates often stretched into long
tubular elements as they moved along curvilinear tracks to the Golgi
complex. This indicated that they were not small vesicles but larger,
pleiomorphic structures. Because pre-Golgi intermediates and their
associated cargo translocate as discrete entities into the central
Golgi region, they may function both in membrane traffic and Golgi
biogenesis. Additional studies are required to understand how pre-Golgi
structures arise from the ER and the extent they engage in membrane
sorting and recycling processes.
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Movie 2: Translocation of Pre-Golgi Intermediates
This movie shows a confocal time-lapse sequence of VSVG-GFP
transport in COS cells incubated at 15°C for several hours before temperature shift to 32°C (from Presley et al., 1997)
(Figure 2). At 15°C, pre-Golgi
structures fail to translocate efficiently through the cytoplasm and
remain closely associated with ER exit sites where they can continue to
receive cargo (Saraste and Kuismanen, 1992). This results in the
formation of larger pre-Golgi intermediates (up to 1.5 µm in
diameter) which are more easily visualized within cells. As shown in
the movie (images collected at 3.6-s time intervals on a confocal
microscope), enlarged pre-Golgi intermediates quickly detached from ER
exit sites and translocated into the Golgi region upon warmup from
15 to 32°C. They moved in an identical fashion as the smaller
pre-Golgi intermediates observed in cells shifted directly from 40 to
32°C. In both cases, the pre-Golgi intermediates translocated as
discrete entities in a stop-and-go fashion through the cytoplasm.
Movement was unidirectional along curvilinear tracks toward the cell
center at rates of up to 1.4 µm/s. Long tubules extending in the
direction of motion of the pre-Golgi intermediates were often seen,
suggesting a motor on the tip of the tubule was pulling the pre-Golgi
structures inward toward the Golgi complex. These results indicate
pre-Golgi structures can be variable in size and still translocate
efficiently through the cytoplasm to the Golgi complex.
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Movie 3: Role of Microtubules in ER-to-Golgi Traffic
Microtubules have long been thought to play a role in ER-to-Golgi
traffic (Ho et al., 1989; Saraste and Svensson, 1991). These cytoplasmic filaments emanate from the centrosomal Golgi region in many
cells and form a polarized radial array
microtubule minus ends
converging at the cell center and plus ends scattered in the cell
periphery. This organization is ideal for directing peripheral ER-derived membrane into the Golgi region. The requirement of microtubules for translocation of pre-Golgi structures toward the
central Golgi complex is shown in Movie 3 (Figure
3). (Images were acquired at 4-min
intervals using a confocal microscope.) Here, VSVG-GFP-expressing COS
cells were treated with nocodazole to depolymerize microtubules prior
to temperature shift from 40 to 32°C. Note that soon after
temperature shift, VSVG-GFP was efficiently exported out of the ER
into peripheral pre-Golgi elements, but these structures remained at
peripheral sites. This effect of microtubule depolymerization was
reversible, with pre-Golgi structures quickly reattaching to newly
formed microtubules and translocating microtubule minus end-directed
into the Golgi region upon removal of nocodazole (Presley et
al., 1997). The microtubule motor complex of dynein/dynactin was
shown to power this transport to the Golgi complex (Burkhardt et
al., 1997; Presley et al., 1997). How dynein/dynactin
associates with pre-Golgi intermediates and how its interaction with
microtubules is regulated are important questions for future work.
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Movie 4, A and B: Fate of Pre-Golgi Intermediates upon Reaching the Golgi Complex
Targeting and fusion of pre-Golgi structures with Golgi
membranes was visualized in VSVG-GFP expressing COS cells whose
Golgi-associated fluorescence was photobleached with high-intensity
laser light at the time cells were warmed from 15 to 32°C. After
photobleaching, time-lapse images of the entire cell were collected
with low-power laser light to follow movement of pre-Golgi structures
into the Golgi region. As shown in the movie sequence 4A (from Presley et al., 1997) (Figure 4A),
pre-Golgi structures translocated inward to the Golgi complex, docked, and then delivered their contents of
VSVG-GFP into the Golgi system. These results indicate that pre-Golgi
structures are the major source of delivery of VSVG-GFP to the Golgi
complex. The fact that the entire profile of the Golgi complex refilled
with fluorescence within a short period after photobleaching (see Movie
4B [Figure 4B]) further suggested that VSVG-GFP is rapidly
transported throughout the Golgi complex after its delivery by
pre-Golgi intermediates.
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Movie 5: Intra-Golgi Traffic Revealed by Photobleaching Recovery
The detailed path followed by cargo and Golgi resident proteins
within the Golgi complex cannot easily be resolved at the light
microscopic level, because Golgi stacks are often <488 nm in depth
(e.g., the wavelength of blue light). Nevertheless, insight into the
lateral mobility of proteins within Golgi membranes can be obtained
using fluorescence recovery after photobleaching (FRAP). This technique
can help distinguish between retention and retrieval mechanisms for
Golgi protein localization (Cole et al., 1996b). In FRAP, a
small region of the cell is photobleached, and recovery of fluorescence
into the bleached region is monitored over time. The kinetics of
fluorescence recovery allow calculation of the diffusion coefficient,
D, which is a measure of the speed of protein diffusion in the
membrane, and the immobile fraction, which is the fraction of proteins
that do not recover during the time course of the experiment.
Photobleaching permanently inactivates the fluorophore, so return of
fluorescence is due only to exchange of nonfluorescent with fluorescent
proteins by lateral diffusion within the membrane.
Movie 5 shows recovery after photobleaching of the Golgi enzyme
galactosyltransferase tagged with GFP in HeLa cells (from Cole et
al., 1996b) (Figure 5). In this
experiment, the region of the Golgi complex above the dotted line was
photobleached with high-energy illumination from a confocal microscope.
Recovery of fluorescence into the photobleached region was then
followed by imaging the entire Golgi body at low-energy light at 4-s
time intervals. Note that within 1 min complete recovery of
fluorescence into the bleached box occurred. This indicates that Golgi
resident proteins such as GalTase diffuse rapidly, without constraints, through the Golgi complex. The diffusion coefficient calculated from
FRAP experiments was 5 × 10
9 cm2/s with
>90% of the proteins mobile (Cole et al.,
1996b).
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Movie 6: Protein Trafficking between Golgi Stacks
A variation of FRAP, called fluorescence loss in photobleaching
(FLIP), can be used to monitor movement of fluorescently tagged molecules between two different regions of a cell or organelle (Cole
et al., 1996b) (Figure 6). In
FLIP, fluorescence in one region of the cell is photobleached with
high-intensity illumination while another region is imaged with
illumination sufficiently low to avoid significant photobleaching. If
photobleaching one region reduces the fluorescence in the other region
as well, diffusional exchange of molecules between the two regions has
occurred. As shown in Movie 6 (from Cole et al., 1996b),
repetitive photobleaching in a small area of the Golgi complex led to
loss of GFP fluorescence from the entire Golgi complex with only
outlying Golgi elements retaining fluorescence. This result implies
that the numerous compact stacks of cisternae that constitute the Golgi
complex are extensively interconnected, allowing highly mobile proteins such as GalTase to move quickly from one part of the Golgi to another.
Movement is likely to occur by lateral diffusion of these proteins
across thin membrane tubules that in ultrastructural studies have been
shown to interconnect Golgi stacks (Rambourg and Clermont, 1990).
Interestingly, ATP depletion of cells, which blocks vesicle transport,
showed little or no effects in FLIP experiments of
GalTase-GFP-expressing cells (Cole et al., 1996b). This
result indicates that the extensive movement of Golgi enzymes observed
in FLIP experiments is not due to vesicle budding and fusion processes.
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Movie 7: Golgi Tubules: Potential Vehicles for Golgi-to-ER Retrograde Traffic
Golgi membrane tubules are known from ultrastructural studies to
be a major characteristic of Golgi morphology. Both the cis and trans face of the Golgi stack are composed of extensive
tubule networks of membrane, and tubule processes frequently
interconnect Golgi stacks (Rambourg et al., 1979; Tanaka
et al., 1986; Ladinsky et al., 1994). As shown in
Movie 7 (Figure 7), these structures may
also play a role in Golgi to ER retrograde traffic. KDEL-R, which is
known to constitutively cycle between the ER and Golgi complex (Pelham,
1991), was imaged with a confocal microscope in HeLa cells expressing a
GFP tagged version of this molecule (KDEL-R-GFP). Note that in addition
to labeling Golgi membranes, KDEL-R-GFP was found in membrane tubules
that extended out from the Golgi complex. After forming, the tubules
often broke off from the Golgi and moved at rates of 0.6 µm/s along
curvilinear tracks to the cell periphery. Microtubules were required
for the peripheral movement of Golgi tubules, suggesting that a plus
end-directed motor was associated with their surface (Sciaky et
al., 1997). After detaching from the Golgi complex and moving to
the cell periphery, Golgi tubules containing KDEL-R-GFP often
disappeared from view (possibly fusing with the ER, which extends
throughout the cytoplasm). Consistent with this possibility, KDEL-R-GFP
was never found on the plasma membrane but only in Golgi, ER, and tubule structures. Golgi tubules may therefore represent retrograde transport intermediates, whose role is to recycle membrane back to the
peripheral ER system. The molecular basis and regulation of Golgi
tubule budding and scission remains to be addressed.
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Movie 8: Effects of Brefeldin A (BFA) on Golgi Morphology and Dynamics
Golgi tubules are known to mediate retrograde membrane traffic in cells treated with BFA, a drug that prevents assembly of cytosolic coat proteins onto Golgi membranes. As shown in Movie 8A (Figure 8A), Golgi tubules resembling those of untreated cells are observed in BFA-treated cells, but they formed at a more rapid rate. Moreover, the tubules failed to detach from Golgi structures. This led to the formation of a dynamic Golgi tubule network within 5-8 min of adding the drug. When one or more of the Golgi tubules fused with the ER, Golgi membranes redistributed rapidly into the ER, leaving no Golgi structure behind. The fact that Golgi membranes redistributed unidirectionally into the ER (and not ER membrane into the Golgi) during BFA treatment suggests that the ER provides a lower free energy environment for membrane proteins and lipids than the Golgi system.
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The sequences in Movie 8A are of GalTase-GFP in HeLa cells. They were
acquired at 3-s time intervals on a cooled charge-coupled device
microscope. Note that Golgi protein redistribution into the ER occurred
within 30 s after fusion of Golgi with ER. The speed of this
redistribution has been shown by Sciaky et al. (1997) to be
too fast to be explained by simple protein diffusion. Instead, these
authors suggest it is driven by a membrane tension-driven membrane flow
(Bloom et al., 1991) that arises from chemical potential or
free energy differences between ER and Golgi membranes. This leads to
unidirectional protein transport when ER and Golgi membranes fuse
during BFA treatment.
A dramatic illustration of unidirectional membrane flow from Golgi into the ER in BFA-treated cells is shown in Movie 8B (Figure 8B). In this experiment cells were treated with nocodazole before addition of BFA. Note that upon addition of BFA to the cells no Golgi tubules formed, since microtubules are required for peripheral extension and movement of tubules. Nevertheless, the time for Golgi redistribution into the ER was extremely rapid once Golgi and ER membranes fused. This suggests that extension of Golgi tubules along microtubules serves only to increase the probability of fusion between Golgi and ER membranes. Once fusion between these two organelles takes place (which can occur in the absence of Golgi tubule extension, because ER membranes are distributed through the cell), the Golgi rapidly and completely empties into the ER.
The chemical basis for the free energy difference between ER and
Golgi membranes that underlies unidirectional absorption of Golgi into
the ER during BFA treatment is unknown. An interesting possibility is
that the work required to "pump" Golgi-destined components up in
energy is supplied by the peripheral "coat" system, which
concentrates and packages proteins exported from the ER (Balch et
al., 1994; Schekman and Orci, 1996). The fact that an immediate
target of BFA is ADP ribosylation factor, which in physical terms is an
energy-driven assembly transport system for supplying COPI to membranes
(Donaldson et al., 1992; Rothman and Wieland, 1996), is
consistent with this idea. When nucleotide exchange onto ADP
ribosylation factor is inhibited by BFA, COP I proteins are quickly
depleted from Golgi membranes. As shown in Movie 8A, Golgi tubules
proliferate and become longer in response. They also do not so readily
detach from the Golgi complex. Ultimately, fusion with the ER occurs
and Golgi membrane quickly empties into the ER. These findings suggest
that one function of COP I is to maintain the integrity of the Golgi
complex, possibly by severing potential links to other organelles.
Future work needs to address the mechanisms that regulate Golgi tubule
formation and detachment from the Golgi complex and how free energy
differences between the ER and Golgi complex arise.
Movie 9: Remodeling of the Golgi Complex in Response to Microtubule Depolymerization
The normal distribution of Golgi membranes within cells appears to
represent a dynamic balance of forward and recycling pathways connecting with the ER. Thus, inhibition of forward traffic into the
Golgi complex without a corresponding effect on recycling typically
leads to redistribution of Golgi material to the site of perturbation.
Fragmentation of the Golgi complex in nocodazole-treated cells is a
good example of this phenomenon. Microtubule disruption by nocodazole
is known to block the inward translocation of pre-Golgi intermediates
along microtubules (see Movie 3) without significant effects on Golgi
to ER traffic (Saraste and Svensson, 1991; Cole et al.,
1996a). Because Golgi enzymes constitutively cycle between the ER and
Golgi complex via these forward and reverse pathways (Cole et
al., 1998), they accumulate at ER exit sites when forward trafficking along microtubules is inhibited (Cole et al.,
1996a; Yang and Storrie, 1998). This leads to rebuilding of Golgi
stacks at ER exit sites and results in the formation of hundreds of
Golgi fragments distributed through the cell (Cole et al.,
1996; Burkhardt, 1998; Storrie and Yang, 1998). Movie 9 (Figure 9) (images collected at 1-min
intervals on a confocal microscope) shows this process in HeLa cells
expressing GalTase-GFP. Note that small Golgi fragments are generated
at significant distances from the central Golgi region within 15 min
after nocodazole treatment. These fragments do not move in any directed
fashion after their formation and resemble the fragments containing
VSVG-GFP in nocodazole-treated cells shifted from 40 to 32°C. The
exact mechanism for redistribution of Golgi enzymes to fragment sites
is still under debate (e.g., recycling through the ER or vesicle
transport through the cytoplasm) (Cole et al., 1996a;
Burkhardt, 1998; Sima et al., 1998; Storrie and Yang, 1998).
Nevertheless, these observations indicate the Golgi complex is capable
of de novo regeneration at ER exit sites and imply a fundamental
relationship between pre-Golgi structures and the Golgi complex.
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FOOTNOTES |
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1 Some of the experiments shown were performed in collaboration with Mark Terasaki and Noah Sciaky.
A Howard Hughes Medical Institute-NIH Research
Scholar.
Online version of this essay contains video information
for Figures 1-9. Online version available at
www.molbiolcell.org.
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REFERENCES |
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Top
Introduction
References
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