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© The Rockefeller University Press,
0021-9525/2000//1 $5.00
The Journal of Cell Biology, Volume 148, Number 1,
, 2000 1-6
Mini-Review |
F-Actin Bundles Are Derivatives of Microvilli
: What Does This Tell US about How Bundles Might Form?
b Department of Biology, University of Pennsylvania, Philadelphia, Pennsylvania 19104
MS029 Brandeis University, Waltham, MA 02454.(781) 736-2405(781) 736-2494
derosier{at}brandeis.edu
© 2000 The Rockefeller University Press
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The Fruit Fly Bristle, a Thorn in Our Side |
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 Top The Fruit Fly Bristle,... The Microvillus: The Archetypal...Other Long Bundles Made...Common Features of Bundles...How Are These Two...How a Bundle Factory...References |
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To figure out the puzzle of modules and their assembly, we reexamined bundles and their assembly in a variety of cell types. (We should mention at the outset that we are defining bundles in this essay as closely packed, parallel filaments that all have the same polarity and are cross-linked by an actin-bundling protein. Thus, by the definition we are using here, stress fibers or muscle fibers are not bundles.) What we found is that all bundles share a common mechanism in morphogenesis which is related to bundle formation in microvilli. Based on our comparisons, we propose that there is a common factory inside cells that generates short bundles and that these are the building blocks out of which cells can make longer bundles.
This essay will first describe the characteristics of bundle formation in a variety of cell types and explain why we think all bundles are derived from microvilli, which in some cases are secondarily modified. We will then propose where and what we should look for in trying to understand the genesis of the bundles. At the end of this essay, we argue that although different cells make different kinds of bundles, they have a common feature, the small bundle factory.
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The Microvillus: The Archetypal Factory of an Actin Bundle |
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TopThe Fruit Fly Bristle,...The Microvillus: The Archetypal...Other Long Bundles Made...Common Features of Bundles...How Are These Two...How a Bundle Factory...References |
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The Brush Border
An astounding 15,000 microvilli extend from the apical surface of each brush-border cell in vertebrate intestinal epithelium. Each microvillus contains an actin bundle of 
20 filaments, all of which have their barbed ends facing into a small patch of dense material at the tip of each microvillus. In the intestine new epithelial cells are formed in the crypt and as they migrate out, the microvilli grow from a tiny dense patch on the plasma membrane and gradually increase in length from a fraction of a micron in the crypt to 3 or 4 µm (Fath et al. 1990). Three bundling proteins, villin, fimbrin, and espin, link together adjacent filaments (Shibayama et al. 1987; Ezzell et al. 1989; Bartles et al. 1998). Although villin appears first followed by fimbrin and then espin, microvilli of similar length and diameters are assembled even in the absence of villin (Ferrary et al. 1999).
Sea Urchin Egg Microvilli
The unfertilized sea urchin egg has on its surface tiny pimples. Each pimple seems to be the nub of a microvillus. It contains on the cytoplasmic surface of the plasma membrane some electron-dense material (Tilney and Jaffe 1980). Immediately after fertilization these pimples extend to form microvilli (Begg et al. 1982). Within each is a bundle of actin filaments that are cross-linked together by fascin. As in other microvilli, the filaments all have the same polarity with their barbed ends facing the electron-dense material. During the next 30 min the microvilli gradually elongate up to 10 µm (Begg et al. 1982).
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Other Long Bundles Made from Microvillar-like Modules |
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TopThe Fruit Fly Bristle,...The Microvillus: The Archetypal...Other Long Bundles Made...Common Features of Bundles...How Are These Two...How a Bundle Factory...References |
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Nurse Cell Struts
There is a second system in fruit flies in which long bundles are also composed of units or modules. In developing ovarian follicles the polyploid nurse cells at a late stage in oogenesis contract and in 30 min dump their contents into the oocytes via intercellular channels called ring canals. The nuclei are retained in the nurse cells and are kept from blocking the ring canals by a system of actin-containing struts that project from the plasma membrane toward the nucleus. Each strut is composed of overlapping units or modules each composed of 25 filaments cross-linked by two cross-links, fascin and villin. As dumping proceeds, the struts become progressively shorter and thicker due to the modules sliding past one another like the retraction of extension ladders when they are removed for storage (Guild et al. 1997). We have studied the formation of these struts. Each module is constructed out of a bundle derived from a microvillus (Fig. 3). The actin core of each microvillus elongates such that its base extends further into the cytoplasm. In our model for this process, the bundle is then released from its connection to the plasma membrane. A neighboring microvillus core binds to the newly released bundle. The neighboring core or elongation transports the first bundle towards the nucleus. The new bundle in turn becomes free from the membrane and the process is repeated with a third microvillus and then a fourth and so on, thereby producing a strut (Fig. 3). Since each bundle is derived from a microvillus, each module has the same polarity in the bundle with barbed ends of the filaments facing the cell surface (Guild et al. 1997) as they arose from the same kind of small patch of dense material seen in other microvilli.
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Of interest to our discussion here are the similarities in these three systems. First and most important is that long actin bundles are composed of shorter units or modules that bind to each other. Second, in all three systems these modules are derived from the core filament bundle in microvilli. Are similar strategies used in the assembly of other kinds of bundles? There are indeed obvious parallels between the bundles generated in the fruit fly with other systems. Below we enumerate a few of these.
Modified Microvilli
Some cell types also make long bundles but there is no need for modules. The two examples listed below are the result of secondary elaboration of microvilli. Other examples exist but for brevity we have just included these two.
The Stereocilium
Each stereocilium present in the hair cell of the ear is also derived from microvilli (Tilney and DeRosier 1986). Early in development, the surface of the hair cells and the adjacent supporting cells are covered with microvilli. The microvilli in the hair cells subsequently develop into stereocilia by the lateral addition of filaments to the microvillar bundle as well as elongation of the filaments in the bundle. The ends of the filaments at the stereociliary tips are embedded in a dense material (Fig. 3), and the polarity of the filaments is identical to its microvillar precursor (Tilney et al. 1983).
Acrosomal Processes of Marine Sperm
A more unusual kind of bundle assembly occurs in the production of the acrosomal bundles in marine sperm, but here again, they seem to be derivatives of microvilli.
Within the mature sperm of the edible blue mussel Mytilus edulis is a 2–5-µm-long maximally cross-linked actin bundle that contains 50 filaments (Tilney et al. 1987). Unlike the microvilli that extend from the cell surface the apical tip of this bundle is connected to the base of the acrosomal vacuole which is a secretory vacuole. Interestingly, the membrane of this vacuole will be continuous with the plasma membrane after activation. During spermiogenesis, this bundle is initiated at a small patch of dense material on the acrosomal surface and elongates posteriorly into the body of the sperm. The filaments in this bundle like those in the microvilli are unidirectionally polarized and crossbridged into a hexagonal bundle (Tilney et al. 1987).
In the sperm of the horseshoe crab Limulus there is a 60-µm-long bundle of actin filaments. The actin filaments in the bundle are stabilized and cross-linked by a unique cross-linking protein, scruin, that appears during spermiogenesis. This long bundle tapers, having 15 filaments at its tip and 85 filaments at its base. Studies on the formation of the bundle during spermiogenesis show that the basal end, containing the 85 filaments, assembles first and, as this bundle elongates basally, the number of filaments is gradually reduced, thereby producing the taper (Tilney et al. 1981). The bundle begins from a small patch of dense material that is attached to the acrosomal vacuole and then elongates. The elongation proceeds as one continuous process. It is as if the whole bundle is made as one long module. As expected, all the filaments have the same polarity with the barbed ends at the apical tip of the bundle.
From all these examples, e.g., in bristles, nurse cells, the fertilization cone, stereocilia, and the acrosomal processes, it appears that the microvillus or the microvillus-like structure initiates the formation of each bundle type. We have tried to depict these common mechanisms and their consequences in Fig. 3, which show how microvillus-like bundles are generated (see center portion), and then incorporated into other kinds of bundles that can be modified by the individual cell for its specific purpose. Thus, the microvillus seems to be the archetypal bundle factory. Accordingly we ask what are the characteristics of all these microvillus derivatives and how do they form?
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Common Features of Bundles and Bundle Production |
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TopThe Fruit Fly Bristle,...The Microvillus: The Archetypal...Other Long Bundles Made...Common Features of Bundles...How Are These Two...How a Bundle Factory...References |
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The common features of all bundles and their apparent origins as microvilli suggest that all cells use some common mechanism to construct initial bundles. Cells, however, then modify these initial bundles to make larger assemblies. For example, stereocilia elongate and widen their bundles, and bristle cells and nurse cells glue bundles together to form long cables, and in bristles modules can at a later time period incorporate additional cross-links that will change filament packing (Fig. 2 and Tilney et al. 1998). Because of these similarities, we propose that there are in all these cell types common factories that generate bundles. These bundle-making factories can be reduced to two elements: a nucleating component, which specifies location and size, and a component that controls length.
Nucleating Component
Actin filaments appear to be nucleated near the plasma membrane, and it appears that elongation of the filaments occurs by the addition of monomers to the membrane-associated (barbed) ends of the filaments. In the cases we presented, the barbed end of the filaments are attached to membranes and are inserted in an electron-dense material of unknown composition. We suggest that this dense material may be the part of the nucleating component of our bundle factories and may also control the number of filaments on the bundle.
What might be the characteristics of this nucleating component? At present, the only system in which nucleation of actin is even vaguely understood is that involving the Arp2/3 complex. In Listeria-infected cells, for example, the Arp2/3 complex binds to G actin to form a nucleus. The idea is that other actin monomers can add to this complex to produce a filament. The Arp2/3 complex remains bound to the pointed end of the filament but detaches from the ActA, a Listeria-bound protein. Thus, as the filament elongates, the Arp2/3 complex, bound to the pointed end, is moved away from the site of initiation (for reviews, see Beckerle 1998; Machesky and Insall 1999). Several groups have visualized the Arp2/3 complex, showing that it localizes at Y junctions between filaments due to its capability both to bind to the side of a filament and/or nucleate a new branch (Mullins et al. 1998; Svitkina and Borisy 1999). In the case of a gel-like pseudopod this makes sense because one wants an open structure, and the Y junction promotes this (see Mullins et al. 1998; Svitkina and Borisy 1999), whereas in a bundle one wants a parallel set of filaments, which a Y junction would defeat. Accordingly, it is no surprise that by antibody staining the Arp2/3 complex is missing on bundles such as occur in filopodia (Welch et al. 1997) and in Drosophila bristles. The implication here is that bundles may be nucleated differently from gel-like actin structures in which Arp2/3 has been implicated.
Components that Control Elongation
After nucleation, there must be an elongation phase in which the filaments in the bundle grow. In the case of the brush border microvilli, the end result is a set of bundles that are of uniform length. In the bristle, the situation is more interesting. Recall that the 10 or so bundles in each cell are made of modules, which are glued end to end. The mean length of the modules is 3 µm, but there is variation with some modules being as short as 1 µm to as long as 5 or 6 µm. There is no obvious systematic variation of module length along the bundle even though the diameter decreases with distance along the bristle. Instead, there appears to be a correlation of module length between the bundles in the same portion of the bristle. It is as if the modules assembled at the same time are the same lengths. Moreover, the sizes of the bundles vary within the same portion of the cell so that the bundles closest to the fruit fly's body are the biggest. All this suggests to us that nucleation and elongation are independent, but they must be coordinated.
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How Are These Two Processes Coordinated? |
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TopThe Fruit Fly Bristle,...The Microvillus: The Archetypal...Other Long Bundles Made...Common Features of Bundles...How Are These Two...How a Bundle Factory...References |
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One possibility is that a ruler defines length of the structure. For example, the length of the helical T4 phage tail is set by a protein, which runs up the center of the tail (Duda and Eiserling 1982). One would expect a similar mechanism to operate in muscle using nebulin to regulate thin filament length (Kruger et al. 1991). If there were a ruler, bundle length would not depend on rate of assembly or width of the bundle but the bundle length would equal the ruler length. Such a mechanism is unlikely, however, because the lengths of bundles in bristle cells vary from 1 to 5 µm. A second possibility is that random filament capping is employed to stop filament elongation. This kind of mechanism has been suggested to account for the short filaments in the tails of Listeria (Tilney et al. 1992; Mullins et al. 1997, Mullins et al. 1998). While such a mechanism could produce the variations in length seen in the short bundles comprising the bristle, it can't explain the correlation of module lengths in adjacent bundles. A third possibility is that one filament or one small bundle serves as a template for the other bundles made at about the same time. Thus, each round of bundle production begins with construction of a new template for that round. This would explain both the variation in module length and the correlation of lengths between modules made at the same time. This seems unlikely because modules made at the same time are made in different parts of the cell. A fourth possibility might involve some hanky-panky with the membrane in which the association of the bundle with the membrane somehow limits the module length. We could not think of how this might actually work nor how it would arrange that bundles made at the same time had the same length. Fifth, there may be some clock that starts and stops bundle formation. This does not explain why the rate of bristle elongation increases with bristle length whereas the module length remains unchanged. A sixth mechanism for determining bundle length involves a limitation in the concentration of the components available for assembly. Such a mechanism might work for the microvilli, but it does not account for the growth of the bristle because it does not explain why as the bundle size decreases, the module length is unaffected.
Our proposal for bundle length determination does involve a limitation in the concentration of components but it also couples the concentration of components to the concentration of nucleating sites. Thus, if the number of filaments specified in a nucleating site determines the concentration of components available for bundle formation, the average length of the bundles will be constant, independent of bundle width or rate of bristle elongation. In this sense, the bundle factory would work like the hay baler. Let us suppose for a moment that the generation of nucleating sites requires activation of a protein and that the concentration of activated protein determines the concentration of bundle components available for elongation. If the concentration of components is directly tied to the number of filaments nucleated, then the length of filaments will be constant. Thus, bundles made at the same time from the same pool of components will be the same length.
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How a Bundle Factory Works |
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TopThe Fruit Fly Bristle,...The Microvillus: The Archetypal...Other Long Bundles Made...Common Features of Bundles...How Are These Two...How a Bundle Factory...References |
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While this mechanism can explain how the average length of the bundle is independent of bundle diameter and rate of assembly in the case of the bristle, can it equally explain why bundles made at the same time are more uniform than bundles made at different times? Filaments assembled at the same time from a common pool of subunits will have lengths that are Poisson distributed. In a 3-µm-long filament, there are 1,000 actin subunits. If the average is 1,000, its standard deviation is 30, a few percent of the average. Thus, filaments assembled at the same time will have lengths within a few percent of one another. If the concentration of nucleating sites determines the concentration of components for bundle assembly, then the fluctuations in its concentration will determine the variation in the concentration of components. The number of such sites is small, and thus the fluctuations arising from the small number will be proportionately higher relative to the average. Thus we would expect the variation in lengths of bundles made at different times to be significantly greater than those made at the same time. Exactly what the actual numbers or concentrations are, and what the fluctuations are due to, requires a knowledge of the components.
We have argued for the existence of a small bundle–making factory that ties nucleation of the bundle to the activation of components for bundle assembly. We think that such a scheme can account for the common beginnings of all bundles in cells. We noted that all bundles initiate at a dense patch on a membrane. The identity of the components in such patches is completely unknown. Because microvilli typify best the components of this factory, we suggest it is time to turn our attention to identifying the components that make up the dense patch. Their identities should unlock the pathway of bundle assembly.
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Acknowledgments |
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This work is supported by grants NIH-GM26357 to David J. DeRosier and NIH-GM52857 to Lewis G. Tilney.
Submitted: 7 September 1999
Revised: 3 December 1999
Accepted: 3 December 1999
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References |
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TopThe Fruit Fly Bristle,...The Microvillus: The Archetypal...Other Long Bundles Made...Common Features of Bundles...How Are These Two...How a Bundle Factory...References |
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